The Special Stains general reference guide provides a general overview of special stains functionality and clinical utility. The guide describes the clinical application of the various assays, the appropriate tissue controls to be used, and some technical considerations as they relate to each of the unique histochemical stains.
The BenchMark Special Stains Product Guide includes product specific information about BenchMark Special Stains kit components and reagents, a visual demonstration of the protocol options for each assay, and information about optimizing staining performance for the BenchMark Special Stains automated staining platform.
This document provides an overview of various special staining techniques used in histology, including:
1. Trichrome stains like Masson's and van Gieson's which stain nuclei, cytoplasm, muscle fibers, and collagen different colors.
2. Metal impregnation techniques like Gordon and Sweets' silver stain to demonstrate reticular fibers.
3. Carbohydrate stains like Periodic acid-Schiff to identify glycogen, mucins, and basement membranes.
4. Hematoxylin and eosin, Gram stain, and Ziehl-Neelsen to identify cells, bacteria, and acid-fast bacteria respectively.
5. Additional specialized stains for
This lecture notes is primarily prepared for medical laboratory students pursuing their studies at bachelorrate level in various universities. It can also be helpful for those graduates who are in service.
Experiment No - 3 aims to perform an Alcian blue stain to identify acid mucopolysaccharides in a fungal sample such as Cryptococcus neoformans. The Alcian blue stain uses a blue dye that binds to acid mucopolysaccharides, allowing identification of fungi containing these substances under a microscope. The process involves staining tissue sections with Alcian blue solution followed by rinsing in distilled water and dehydration using concentrated alcohol solutions to preserve the stained sample.
This document discusses tissue fixation in histopathology. It describes the various stages of histopathology including fixation, processing, embedding, sectioning and staining of tissues. It explains the importance of fixation in preventing autolysis and putrefaction of tissues. The key properties and reactions of common fixatives like formaldehyde and glutaraldehyde are outlined. Factors that can affect fixation quality including temperature, pH, concentration and duration of fixation are also summarized. Finally, different classifications of fixatives are presented based on their structural and functional properties.
This document discusses cytopreparatory techniques, including fixation of cytological samples, staining methods, and interpretation. It focuses on fixation, explaining that fixation preserves cells in a lifelike state after death by preventing autolysis and putrefaction. The key properties of a good fixative are outlined, and various fixatives are classified and examples are provided, including alcohols, formalin, and mercuric chloride, which are commonly used for cytological preparations.
This document discusses the process of tissue processing for histological examination. It involves several key steps: specimen identification and labelling, gross examination, fixation, dehydration, clearing, infiltration, embedding, sectioning, and staining. Fixation using formalin or other fixatives preserves tissue structure. Dehydration removes water and replaces it with alcohol or other solvents to allow for infiltration of paraffin wax. The wax infiltrates and impregnates the tissue, allowing it to be sectioned thinly for microscopic examination after staining. The document provides details on common fixation and processing methods and their purposes in preparing tissue for histological analysis.
The BenchMark Special Stains Product Guide includes product specific information about BenchMark Special Stains kit components and reagents, a visual demonstration of the protocol options for each assay, and information about optimizing staining performance for the BenchMark Special Stains automated staining platform.
This document provides an overview of various special staining techniques used in histology, including:
1. Trichrome stains like Masson's and van Gieson's which stain nuclei, cytoplasm, muscle fibers, and collagen different colors.
2. Metal impregnation techniques like Gordon and Sweets' silver stain to demonstrate reticular fibers.
3. Carbohydrate stains like Periodic acid-Schiff to identify glycogen, mucins, and basement membranes.
4. Hematoxylin and eosin, Gram stain, and Ziehl-Neelsen to identify cells, bacteria, and acid-fast bacteria respectively.
5. Additional specialized stains for
This lecture notes is primarily prepared for medical laboratory students pursuing their studies at bachelorrate level in various universities. It can also be helpful for those graduates who are in service.
Experiment No - 3 aims to perform an Alcian blue stain to identify acid mucopolysaccharides in a fungal sample such as Cryptococcus neoformans. The Alcian blue stain uses a blue dye that binds to acid mucopolysaccharides, allowing identification of fungi containing these substances under a microscope. The process involves staining tissue sections with Alcian blue solution followed by rinsing in distilled water and dehydration using concentrated alcohol solutions to preserve the stained sample.
This document discusses tissue fixation in histopathology. It describes the various stages of histopathology including fixation, processing, embedding, sectioning and staining of tissues. It explains the importance of fixation in preventing autolysis and putrefaction of tissues. The key properties and reactions of common fixatives like formaldehyde and glutaraldehyde are outlined. Factors that can affect fixation quality including temperature, pH, concentration and duration of fixation are also summarized. Finally, different classifications of fixatives are presented based on their structural and functional properties.
This document discusses cytopreparatory techniques, including fixation of cytological samples, staining methods, and interpretation. It focuses on fixation, explaining that fixation preserves cells in a lifelike state after death by preventing autolysis and putrefaction. The key properties of a good fixative are outlined, and various fixatives are classified and examples are provided, including alcohols, formalin, and mercuric chloride, which are commonly used for cytological preparations.
This document discusses the process of tissue processing for histological examination. It involves several key steps: specimen identification and labelling, gross examination, fixation, dehydration, clearing, infiltration, embedding, sectioning, and staining. Fixation using formalin or other fixatives preserves tissue structure. Dehydration removes water and replaces it with alcohol or other solvents to allow for infiltration of paraffin wax. The wax infiltrates and impregnates the tissue, allowing it to be sectioned thinly for microscopic examination after staining. The document provides details on common fixation and processing methods and their purposes in preparing tissue for histological analysis.
The PAS stain identifies polysaccharides, mucus substances, basement membranes, and some fungi by causing them to appear magenta under the microscope. It works by first using periodic acid to oxidize carbohydrate groups, then exposing the tissue to Schiff's reagent, which causes aldehyde groups produced in the first step to appear magenta. The PAS stain is used to identify conditions involving abnormal glycogen storage or mucus production, such as certain tumors, infections, and genetic diseases. It helps diagnose issues in tissues from the liver, kidney, lung, muscle, and other organs.
This document discusses histotechniques related to fixation and decalcification of tissues for microscopic examination. It describes the objectives and ideal properties of fixatives, as well as common fixatives used such as formaldehyde, glutaraldehyde, and picric acid. Factors that influence fixation quality like temperature, concentration, and duration are addressed. The document also covers decalcification techniques and factors that affect the decalcification process. Special considerations for fixing different tissues are outlined.
The document discusses cryostats, which are devices used to cut thin frozen sections of tissues for examination under a microscope. Cryostats contain a microtome inside a freezer unit that can rapidly freeze tissue samples and cut sections as thin as 1 micrometer at temperatures below freezing. The cryostat process allows for quick diagnosis by freezing and sectioning tissues within minutes rather than having to dehydrate, embed in paraffin, and section as with traditional microtomes.
This document discusses the process of tissue processing in histology and histopathology laboratories. [1] Tissue samples are obtained from biopsies and autopsies and undergo histotechniques to prepare them for microscopic examination. [2] The key steps include fixation, processing, embedding in paraffin wax, sectioning, staining, and mounting. [3] Automated equipment is now commonly used to improve efficiency at many steps such as tissue processing, sectioning, and staining.
This document discusses histopathology staining techniques. It defines histopathology as staining tissue samples to examine cellular and intracellular structures microscopically. The two main categories of stains are natural dyes derived from natural resources, and artificial dyes produced through chemical reactions. Hematoxylin is a commonly used natural dye that stains nuclei blue, while eosin is an artificial dye that counterstains cytoplasm pink. The document outlines hematoxylin and eosin staining as well as other histological stains and their characteristics.
This document discusses various special stains used in pathology to identify different tissue components. It describes stains for carbohydrates like Periodic acid-Schiff (PAS), mucins like Alcian blue and mucicarmine, collagen and elastic fibers like reticulin and trichrome stains, amyloid with Congo red, lipids, melanin, calcium, iron, and microorganisms. It provides details on the principles, reagents, controls, and uses of these important special stains.
Histology is the microscopic study of tissues. Key steps in processing tissues for histological examination include fixation, dehydration, clearing, embedding in paraffin wax, sectioning, and staining. Tissues are first fixed in chemicals like formaldehyde to preserve their structure. They are then dehydrated using graded alcohols to remove water. Next, tissues are cleared using solvents like xylene to make them permeable to paraffin prior to embedding. The embedded tissues can then be thinly sectioned and stained for microscopic examination. Proper tissue processing is important for high quality histological analysis.
This document provides information about exfoliative cytology and fine needle aspiration cytology (FNAC). It discusses how exfoliative cytology involves studying cells that are shed from body surfaces and explains the basic procedure. FNAC is described as using a thin needle to aspirate cells from lumps or masses and make smears for microscopic examination. The document outlines the equipment, steps, applications and advantages of both techniques, noting they are minimally invasive ways to study cells for diagnostic purposes like detecting cancer.
This document provides an overview of hematoxylin and eosin staining. It discusses the theory behind staining, including how dyes interact with tissues through various bonding mechanisms. It also describes factors that influence staining results, such as rates of dye uptake and loss, binding site affinities, and tissue modification during fixation. The document highlights how hematoxylin and eosin work as the most commonly used routine stain in histopathology.
This document provides information on various histological staining techniques used to identify different types of tissues and biomolecules. It discusses connective tissue stains like Van Gieson's stain, Masson's trichrome stain, and Verhoeff's stain used to identify collagen fibers. It also describes reticulin stains, elastic stains, carbohydrate stains like periodic acid Schiff, and mucin stains like Alcian blue to identify different components of tissues under the microscope. Procedures for each stain are outlined along with the expected results.
This document discusses tissue processing and fixation. It begins by introducing tissue fixation and its objectives, such as preventing degradation and maintaining morphology. It then describes various fixation methods and factors that affect fixation quality. Common fixatives are discussed, including formaldehyde, glutaraldehyde, Zenker's solution and Bouin's solution. Fixation protocols for specific tissues like brain, breast, lung and kidney are also reviewed. The document emphasizes the importance of proper fixation for histological examination.
Histological Techniques: Perform Fixation and Tissue ProcessingLouisaChew
This document discusses fixation and tissue processing techniques in histology. It begins by describing the aims of fixation as preventing autolysis, putrefaction, and tissue distortion. An ideal fixative is said to preserve tissue structure and chemistry without shrinkage or swelling. Fixatives are classified based on their chemical properties, effects on cells and tissues, and whether they use single or multiple chemicals. Factors that affect fixation include temperature, tissue size, fixative concentration, duration of fixation, agitation, pH, and osmolality.
The document then discusses the aims of tissue processing as removing water from tissues and making them suitable for embedding in paraffin. The key steps are dehydration, clearing, and infiltration with par
Hematoxylin and eosin staining is a common histological technique that uses hematoxylin, which stains cell nuclei blue, and eosin, which stains cytoplasm and connective tissue pink. The document describes the full H&E staining procedure, including dewaxing, hydration, staining, differentiation, dehydration, clearing and mounting of tissue sections. It also discusses the principles and properties of hematoxylin, including how it is extracted from logwood and requires oxidation or "ripening" to become an effective nuclear stain. Commonly used hematoxylin formulations including Harris's, Mayer's, and Ehrlich's are compared.
The document discusses various techniques used in histopathology sample processing including decalcification, fixation, dehydration, clearing, embedding and sectioning. It covers different chemical agents used for each step along with their properties and advantages. Various methods are described such as paraffin, celloidin and vacuum embedding for optimal tissue preservation and section quality. Automatic tissue processors and freeze drying are also mentioned as techniques to reduce processing time.
This document discusses hematoxylin and eosin stains. It provides details on:
1) Hematoxylin is extracted from logwood and oxidized to hematin, which is responsible for staining properties. It requires a mordant like aluminum or iron salts to bind to tissues.
2) Alum hematoxylin is commonly used, with potassium or ammonium alum as the mordant. Sections can be overstained and differentiated, or stained for a predetermined time.
3) After differentiation, sections are "blued" in a weak alkaline solution to convert the hematin stain from red to blue-black in the cell nuclei.
This document discusses various special stains used in pathology and their principles and results. It describes hematoxylin and eosin staining which stains cell nuclei purple and cytoplasm pink. It also discusses mucin stains like PAS, mucicarmine and Alcian blue; melanin, lipochrome, iron, fat, AFB, fungal and connective tissue stains. It provides examples of stained tissues and conditions and includes an assignment with questions.
This is a presentation covering all techniques in histopathology. Comprehensive coverage of all related aspects.. Useful for postgraduate Pathology students and practitioners.
Histopathology specimen processing involves several key steps: specimen identification and labeling, grossing and fixation, processing including dehydration and clearing, embedding, microtomy, and staining. Specimens are examined grossly, relevant sections are selected for histology based on findings, and blocks are prepared for microscopic examination. Proper grossing involves accurate description and oriented sampling to allow for histologic diagnosis.
IPQC Tests for Opthalmic Preparations.pptxSohailSheikh62
The document discusses quality control testing for ophthalmic pharmaceutical preparations. It outlines 8 key tests: 1) pH, 2) isotonicity, 3) therapeutic efficacy, 4) compatibility with the eye, 5) clarity, 6) particulate matter, 7) bacterial endotoxins, and 8) sterility. Each test is important to ensure the safety, stability and effectiveness of ophthalmic drugs. The document provides details on acceptable ranges and testing methods for each quality control parameter based on pharmacopoeial standards.
Patel college of pharmacy m sandeep mewada.ppt.pptmSANDEEP MEWADA
The document discusses various common staining techniques used in microbiology. It begins by explaining the purpose of staining and some key terms like stain, staining, and fixation. It then describes different types of stains including simple stains like methylene blue and differential stains like Gram staining. Gram staining technique and the gram positive and gram negative reactions are explained in detail. Another differential staining method discussed is acid-fast staining using Ziehl-Neelsen stain for tuberculosis diagnosis. Various staining procedures and their applications are outlined.
The PAS stain identifies polysaccharides, mucus substances, basement membranes, and some fungi by causing them to appear magenta under the microscope. It works by first using periodic acid to oxidize carbohydrate groups, then exposing the tissue to Schiff's reagent, which causes aldehyde groups produced in the first step to appear magenta. The PAS stain is used to identify conditions involving abnormal glycogen storage or mucus production, such as certain tumors, infections, and genetic diseases. It helps diagnose issues in tissues from the liver, kidney, lung, muscle, and other organs.
This document discusses histotechniques related to fixation and decalcification of tissues for microscopic examination. It describes the objectives and ideal properties of fixatives, as well as common fixatives used such as formaldehyde, glutaraldehyde, and picric acid. Factors that influence fixation quality like temperature, concentration, and duration are addressed. The document also covers decalcification techniques and factors that affect the decalcification process. Special considerations for fixing different tissues are outlined.
The document discusses cryostats, which are devices used to cut thin frozen sections of tissues for examination under a microscope. Cryostats contain a microtome inside a freezer unit that can rapidly freeze tissue samples and cut sections as thin as 1 micrometer at temperatures below freezing. The cryostat process allows for quick diagnosis by freezing and sectioning tissues within minutes rather than having to dehydrate, embed in paraffin, and section as with traditional microtomes.
This document discusses the process of tissue processing in histology and histopathology laboratories. [1] Tissue samples are obtained from biopsies and autopsies and undergo histotechniques to prepare them for microscopic examination. [2] The key steps include fixation, processing, embedding in paraffin wax, sectioning, staining, and mounting. [3] Automated equipment is now commonly used to improve efficiency at many steps such as tissue processing, sectioning, and staining.
This document discusses histopathology staining techniques. It defines histopathology as staining tissue samples to examine cellular and intracellular structures microscopically. The two main categories of stains are natural dyes derived from natural resources, and artificial dyes produced through chemical reactions. Hematoxylin is a commonly used natural dye that stains nuclei blue, while eosin is an artificial dye that counterstains cytoplasm pink. The document outlines hematoxylin and eosin staining as well as other histological stains and their characteristics.
This document discusses various special stains used in pathology to identify different tissue components. It describes stains for carbohydrates like Periodic acid-Schiff (PAS), mucins like Alcian blue and mucicarmine, collagen and elastic fibers like reticulin and trichrome stains, amyloid with Congo red, lipids, melanin, calcium, iron, and microorganisms. It provides details on the principles, reagents, controls, and uses of these important special stains.
Histology is the microscopic study of tissues. Key steps in processing tissues for histological examination include fixation, dehydration, clearing, embedding in paraffin wax, sectioning, and staining. Tissues are first fixed in chemicals like formaldehyde to preserve their structure. They are then dehydrated using graded alcohols to remove water. Next, tissues are cleared using solvents like xylene to make them permeable to paraffin prior to embedding. The embedded tissues can then be thinly sectioned and stained for microscopic examination. Proper tissue processing is important for high quality histological analysis.
This document provides information about exfoliative cytology and fine needle aspiration cytology (FNAC). It discusses how exfoliative cytology involves studying cells that are shed from body surfaces and explains the basic procedure. FNAC is described as using a thin needle to aspirate cells from lumps or masses and make smears for microscopic examination. The document outlines the equipment, steps, applications and advantages of both techniques, noting they are minimally invasive ways to study cells for diagnostic purposes like detecting cancer.
This document provides an overview of hematoxylin and eosin staining. It discusses the theory behind staining, including how dyes interact with tissues through various bonding mechanisms. It also describes factors that influence staining results, such as rates of dye uptake and loss, binding site affinities, and tissue modification during fixation. The document highlights how hematoxylin and eosin work as the most commonly used routine stain in histopathology.
This document provides information on various histological staining techniques used to identify different types of tissues and biomolecules. It discusses connective tissue stains like Van Gieson's stain, Masson's trichrome stain, and Verhoeff's stain used to identify collagen fibers. It also describes reticulin stains, elastic stains, carbohydrate stains like periodic acid Schiff, and mucin stains like Alcian blue to identify different components of tissues under the microscope. Procedures for each stain are outlined along with the expected results.
This document discusses tissue processing and fixation. It begins by introducing tissue fixation and its objectives, such as preventing degradation and maintaining morphology. It then describes various fixation methods and factors that affect fixation quality. Common fixatives are discussed, including formaldehyde, glutaraldehyde, Zenker's solution and Bouin's solution. Fixation protocols for specific tissues like brain, breast, lung and kidney are also reviewed. The document emphasizes the importance of proper fixation for histological examination.
Histological Techniques: Perform Fixation and Tissue ProcessingLouisaChew
This document discusses fixation and tissue processing techniques in histology. It begins by describing the aims of fixation as preventing autolysis, putrefaction, and tissue distortion. An ideal fixative is said to preserve tissue structure and chemistry without shrinkage or swelling. Fixatives are classified based on their chemical properties, effects on cells and tissues, and whether they use single or multiple chemicals. Factors that affect fixation include temperature, tissue size, fixative concentration, duration of fixation, agitation, pH, and osmolality.
The document then discusses the aims of tissue processing as removing water from tissues and making them suitable for embedding in paraffin. The key steps are dehydration, clearing, and infiltration with par
Hematoxylin and eosin staining is a common histological technique that uses hematoxylin, which stains cell nuclei blue, and eosin, which stains cytoplasm and connective tissue pink. The document describes the full H&E staining procedure, including dewaxing, hydration, staining, differentiation, dehydration, clearing and mounting of tissue sections. It also discusses the principles and properties of hematoxylin, including how it is extracted from logwood and requires oxidation or "ripening" to become an effective nuclear stain. Commonly used hematoxylin formulations including Harris's, Mayer's, and Ehrlich's are compared.
The document discusses various techniques used in histopathology sample processing including decalcification, fixation, dehydration, clearing, embedding and sectioning. It covers different chemical agents used for each step along with their properties and advantages. Various methods are described such as paraffin, celloidin and vacuum embedding for optimal tissue preservation and section quality. Automatic tissue processors and freeze drying are also mentioned as techniques to reduce processing time.
This document discusses hematoxylin and eosin stains. It provides details on:
1) Hematoxylin is extracted from logwood and oxidized to hematin, which is responsible for staining properties. It requires a mordant like aluminum or iron salts to bind to tissues.
2) Alum hematoxylin is commonly used, with potassium or ammonium alum as the mordant. Sections can be overstained and differentiated, or stained for a predetermined time.
3) After differentiation, sections are "blued" in a weak alkaline solution to convert the hematin stain from red to blue-black in the cell nuclei.
This document discusses various special stains used in pathology and their principles and results. It describes hematoxylin and eosin staining which stains cell nuclei purple and cytoplasm pink. It also discusses mucin stains like PAS, mucicarmine and Alcian blue; melanin, lipochrome, iron, fat, AFB, fungal and connective tissue stains. It provides examples of stained tissues and conditions and includes an assignment with questions.
This is a presentation covering all techniques in histopathology. Comprehensive coverage of all related aspects.. Useful for postgraduate Pathology students and practitioners.
Histopathology specimen processing involves several key steps: specimen identification and labeling, grossing and fixation, processing including dehydration and clearing, embedding, microtomy, and staining. Specimens are examined grossly, relevant sections are selected for histology based on findings, and blocks are prepared for microscopic examination. Proper grossing involves accurate description and oriented sampling to allow for histologic diagnosis.
IPQC Tests for Opthalmic Preparations.pptxSohailSheikh62
The document discusses quality control testing for ophthalmic pharmaceutical preparations. It outlines 8 key tests: 1) pH, 2) isotonicity, 3) therapeutic efficacy, 4) compatibility with the eye, 5) clarity, 6) particulate matter, 7) bacterial endotoxins, and 8) sterility. Each test is important to ensure the safety, stability and effectiveness of ophthalmic drugs. The document provides details on acceptable ranges and testing methods for each quality control parameter based on pharmacopoeial standards.
Patel college of pharmacy m sandeep mewada.ppt.pptmSANDEEP MEWADA
The document discusses various common staining techniques used in microbiology. It begins by explaining the purpose of staining and some key terms like stain, staining, and fixation. It then describes different types of stains including simple stains like methylene blue and differential stains like Gram staining. Gram staining technique and the gram positive and gram negative reactions are explained in detail. Another differential staining method discussed is acid-fast staining using Ziehl-Neelsen stain for tuberculosis diagnosis. Various staining procedures and their applications are outlined.
This document discusses various staining techniques used to visualize microorganisms under the microscope. It describes two main types of staining: positive staining, which colors the microorganisms, and negative staining, which colors the background. Specific staining methods covered include simple staining using single dyes, differential staining techniques like Gram staining and acid-fast staining, and special stains for structures such as endospores, capsules, flagella, and nuclei. Detailed procedures are provided for common staining methods along with labeled microscope images showing the results.
Staining is a technique used to enhance contrast in samples, generally at the microscopic level.Staining and fluorescent tagging can serve similar purposes. Biological staining is also used to mark cells in flow cytometry, and to flag proteins or nucleic acids in gel electrophoresis.
This document provides an overview of staining techniques used in dermatology. It begins by defining stains and their uses for visualizing tissue components microscopically. Common stains are then classified and examples are given, including hematoxylin and eosin, Gram, acid-fast, Giemsa, Gomori methenamine silver, and special stains. Specific protocols and applications are described for various stains. The document concludes with a discussion of immunohistochemistry stains and their diagnostic uses.
This document provides an overview of staining techniques used in dermatology. It discusses the basic principles of staining, including what a stain is and how it works. It then classifies stains based on chemical nature and type of staining technique. Common stains discussed include hematoxylin and eosin, Gram stain, acid fast stain, Giemsa stain, Gomori methenamine silver stain, and various special stains. The uses, procedures, and importance of specific stains are described. In under 3 sentences, this document summarizes different staining techniques used in dermatology to identify structures and microorganisms.
The document discusses bacterial staining techniques, specifically simple staining and Gram's staining. It begins by explaining how staining enhances contrast under the microscope since bacteria are otherwise invisible. It then describes the basic components and process of simple staining, as well as the principles and steps of Gram's staining technique. Gram's staining allows differentiation of bacteria into Gram-positive or Gram-negative categories based on differences in cell wall structure and composition. This differential staining technique is one of the most common and important in microbiology.
This document provides information on various staining techniques used to visualize bacteria and fungi under a microscope. It discusses simple staining techniques that use a single dye to highlight structures, as well as differential staining techniques like Gram staining, acid-fast staining, and Albert staining that distinguish between bacterial groups. Special staining methods are described to visualize specific structures like endospores, flagella, and capsules. Fungal staining techniques including lactophenol cotton blue, KOH, calcofluor white, and various histopathological stains used to identify fungi are also outlined. The document aims to enhance contrast and visibility of microscopic specimens through selective staining of tissues and cellular components.
1. The document describes three bacterial tests - the Indole test, Lysine Decarboxylase test, and Mannitol Fermentation test - that were performed to identify E. coli bacteria.
2. The Indole test detects the production of indole from tryptophan, the Lysine Decarboxylase test examines an enzyme's ability to break down lysine, and the Mannitol Fermentation test observes acid production from fermenting mannitol.
3. These tests can help differentiate between bacterial species like distinguishing E. coli from other Proteus or Klebsiella species.
This document describes the preparation of Sabouraud Dextrose Agar (SDA) media for isolating fungal cultures. It details the aim, introduction, principle, required materials, composition, procedure for preparation, results interpretation, and limitations of SDA media. The procedure involves suspending ingredients in water, autoclaving, cooling, pouring into plates or tubes, streaking specimens to obtain isolated colonies, and incubating plates to examine fungal growth over several weeks. Typical fungal colony morphologies on SDA include creamy yeast colonies and variously colored filamentous mold colonies.
The document summarizes the Ziehl-Neelsen stain, an acid-fast stain used to identify acid-fast bacteria such as Mycobacteria. It works by using a primary stain, carbol fuchsin, which is retained by acid-fast bacteria after a decolorizing step. This allows acid-fast bacteria to be visualized as red rods against a blue counterstained background. The document discusses the staining procedure, interpretation of results, advantages and limitations of acid-fast staining, and causes of false-positive and false-negative results.
The document describes the parts of a microscope and their functions. It includes the eyepiece lens, tube, arm, base, illuminator, stage, revolving nosepiece, objective lenses, rack stop, and condenser lens. It then discusses pharmacognosy, crude drugs, medical plants, active ingredients in plants, and differences between herbal medicine and traditional medicine. Methods for evaluating medicinal plants include organoleptic, physical, biological, and microscopic methods. The general procedures for microscopic mounting are also described.
Bacterial capsules are composed of polysaccharides or other polymers that surround the cell wall. Capsules help bacteria resist phagocytosis and play a role in pathogenicity. Various staining methods can be used to visualize capsules, which are difficult to stain due to their non-ionic nature. Anthony's capsule stain uses crystal violet and copper sulfate to differentially stain the cell wall purple and leave the decolorized capsule appearing blue against the background. Maneval's method uses Congo red and acid fuchsin to reveal white capsules against a red-blue background. Negative staining can also visualize capsules using dyes like India ink. Capsule staining reveals structures important for bacterial virulence and survival.
The document discusses methods for identifying bacteria through growth-dependent characteristics. It describes several identification methods including isolating bacteria in pure culture, examining staining reactions, colony morphology, cultural characteristics, metabolism, and biochemical properties through various tests. Challenges with traditional bacterial identification methods are that they require culturing organisms and some strains have unique biochemical profiles that do not match known species. The document provides details on specific identification tests for bacteria.
This document provides information about identification of bacteria through staining and biochemical tests. It discusses various staining techniques like simple staining, Gram staining, negative staining and acid fast staining. It explains the principles, procedures and results of these staining methods. It also describes the IMViC tests, which are used to identify Gram negative bacteria based on their ability to produce indole, change the color of methyl red, produce acetoin in Voges-Proskauer test and utilize citrate as a carbon source. Understanding these staining techniques and biochemical tests is important for identification of microbes.
Medical Microbiology Laboratory (biochemical tests - i)Hussein Al-tameemi
The document provides information on various biochemical tests used to identify bacteria, including enzymatic tests like catalase, coagulase, oxidase, and urease. It describes the basic principles, procedures, reagents, and results for each test. The catalase test detects the presence of the catalase enzyme, while the coagulase test detects coagulase production in Staphylococcus aureus. Positive and negative results are indicated by bubble or clot formation, respectively.
Preparation of large volume and small volume parenteralsangram maskar
Large volume parenterals are sterile aqueous drug products packaged in single-dose containers holding 100 mL or more. Small volume parenterals are packaged in containers holding 100 mL or less. Both are administered via intravenous, intramuscular, or subcutaneous routes. Key differences include that small volume parenterals may use preservatives and not require isotonicity, while large volume parenterals must be isotonic. Both undergo processes like cleaning, preparation, sterilization, filling, and packaging to ensure sterility. They are tested using methods like sterility testing, particulate testing, and pyrogen testing to ensure quality and safety.
The document discusses various components of typical cell culture media, including carbohydrates, amino acids, salts, buffers, vitamins and hormones, antibiotics, and serum. It describes the purposes and considerations for each component in maintaining optimal cell growth conditions and metabolism. Key factors include maintaining isotonicity, buffering pH, providing nutrients and growth factors, and preventing bacterial/fungal contamination.
Similar to VENTANA BenchMark Special Stains General Reference Guide (20)
TEST BANK For Basic and Clinical Pharmacology, 14th Edition by Bertram G. Kat...rightmanforbloodline
TEST BANK For Basic and Clinical Pharmacology, 14th Edition by Bertram G. Katzung, Verified Chapters 1 - 66, Complete Newest Version.
TEST BANK For Basic and Clinical Pharmacology, 14th Edition by Bertram G. Katzung, Verified Chapters 1 - 66, Complete Newest Version.
TEST BANK For Basic and Clinical Pharmacology, 14th Edition by Bertram G. Katzung, Verified Chapters 1 - 66, Complete Newest Version.
TEST BANK For Basic and Clinical Pharmacology, 14th Edition by Bertram G. Katzung, Verified Chapters 1 - 66, Complete Newest Version.
Cell Therapy Expansion and Challenges in Autoimmune DiseaseHealth Advances
There is increasing confidence that cell therapies will soon play a role in the treatment of autoimmune disorders, but the extent of this impact remains to be seen. Early readouts on autologous CAR-Ts in lupus are encouraging, but manufacturing and cost limitations are likely to restrict access to highly refractory patients. Allogeneic CAR-Ts have the potential to broaden access to earlier lines of treatment due to their inherent cost benefits, however they will need to demonstrate comparable or improved efficacy to established modalities.
In addition to infrastructure and capacity constraints, CAR-Ts face a very different risk-benefit dynamic in autoimmune compared to oncology, highlighting the need for tolerable therapies with low adverse event risk. CAR-NK and Treg-based therapies are also being developed in certain autoimmune disorders and may demonstrate favorable safety profiles. Several novel non-cell therapies such as bispecific antibodies, nanobodies, and RNAi drugs, may also offer future alternative competitive solutions with variable value propositions.
Widespread adoption of cell therapies will not only require strong efficacy and safety data, but also adapted pricing and access strategies. At oncology-based price points, CAR-Ts are unlikely to achieve broad market access in autoimmune disorders, with eligible patient populations that are potentially orders of magnitude greater than the number of currently addressable cancer patients. Developers have made strides towards reducing cell therapy COGS while improving manufacturing efficiency, but payors will inevitably restrict access until more sustainable pricing is achieved.
Despite these headwinds, industry leaders and investors remain confident that cell therapies are poised to address significant unmet need in patients suffering from autoimmune disorders. However, the extent of this impact on the treatment landscape remains to be seen, as the industry rapidly approaches an inflection point.
Muktapishti is a traditional Ayurvedic preparation made from Shoditha Mukta (Purified Pearl), is believed to help regulate thyroid function and reduce symptoms of hyperthyroidism due to its cooling and balancing properties. Clinical evidence on its efficacy remains limited, necessitating further research to validate its therapeutic benefits.
Local Advanced Lung Cancer: Artificial Intelligence, Synergetics, Complex Sys...Oleg Kshivets
Overall life span (LS) was 1671.7±1721.6 days and cumulative 5YS reached 62.4%, 10 years – 50.4%, 20 years – 44.6%. 94 LCP lived more than 5 years without cancer (LS=2958.6±1723.6 days), 22 – more than 10 years (LS=5571±1841.8 days). 67 LCP died because of LC (LS=471.9±344 days). AT significantly improved 5YS (68% vs. 53.7%) (P=0.028 by log-rank test). Cox modeling displayed that 5YS of LCP significantly depended on: N0-N12, T3-4, blood cell circuit, cell ratio factors (ratio between cancer cells-CC and blood cells subpopulations), LC cell dynamics, recalcification time, heparin tolerance, prothrombin index, protein, AT, procedure type (P=0.000-0.031). Neural networks, genetic algorithm selection and bootstrap simulation revealed relationships between 5YS and N0-12 (rank=1), thrombocytes/CC (rank=2), segmented neutrophils/CC (3), eosinophils/CC (4), erythrocytes/CC (5), healthy cells/CC (6), lymphocytes/CC (7), stick neutrophils/CC (8), leucocytes/CC (9), monocytes/CC (10). Correct prediction of 5YS was 100% by neural networks computing (error=0.000; area under ROC curve=1.0).
Histololgy of Female Reproductive System.pptxAyeshaZaid1
Dive into an in-depth exploration of the histological structure of female reproductive system with this comprehensive lecture. Presented by Dr. Ayesha Irfan, Assistant Professor of Anatomy, this presentation covers the Gross anatomy and functional histology of the female reproductive organs. Ideal for students, educators, and anyone interested in medical science, this lecture provides clear explanations, detailed diagrams, and valuable insights into female reproductive system. Enhance your knowledge and understanding of this essential aspect of human biology.
Rasamanikya is a excellent preparation in the field of Rasashastra, it is used in various Kushtha Roga, Shwasa, Vicharchika, Bhagandara, Vatarakta, and Phiranga Roga. In this article Preparation& Comparative analytical profile for both Formulationon i.e Rasamanikya prepared by Kushmanda swarasa & Churnodhaka Shodita Haratala. The study aims to provide insights into the comparative efficacy and analytical aspects of these formulations for enhanced therapeutic outcomes.
Does Over-Masturbation Contribute to Chronic Prostatitis.pptxwalterHu5
In some case, your chronic prostatitis may be related to over-masturbation. Generally, natural medicine Diuretic and Anti-inflammatory Pill can help mee get a cure.
3. 3
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Table of Contents
AFB
Stain basics 4
Technical notes and references 6
Alcian Blue
Stain basics 8
Technical notes and references 10
Alcian Yellow
Stain basics 12
Technical notes and references 14
Congo Red
Stain basics 16
Technical notes and references 18
Elastic
Stain basics 20
Technical notes and references 22
Giemsa
Stain basics 24
Technical notes and references 26
GMS
Stain basics 28
Technical notes and references 30
Gram
Stain basics 32
Technical notes and references 34
Iron
Stain basics 36
Technical notes and references 38
Jones H&E & Jones Light Green
Stain basics 40
Technical notes and references 42
Mucicarmine
Stain basics 44
Technical notes and references 46
PAS
PAS Stain basics 47
PAS/Diastase Stain basics 50
PAS/Alcian Blue Stain basics 53
PAS/Light Green Stain Basics 56
Technical notes and references 58
Reticulum
Stain basics 60
Technical notes and references 62
Steiner
Stain basics 64
Technical notes and references 66
Trichrome Blue
Stain basics 68
Technical notes and references 71
Trichrome Green
Stain basics 72
Technical notes and references 75
4. 4
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
AFB
Stain basics
Figure 2. AFB organisms staining on infected colon, 600x.
Expected results
• Acid-fast bacteria — bright red
• Background — light blue
Figure 1. Lung tissue infected with AFB organisms, 600x.
Purpose
The AFB stain may be used to selectively demonstrate Mycobacteria and other acid-fast organisms or components in
formalin-fixed, paraffin-embedded tissue.1
Staining principle
The staining reaction is based on the application of pararosaniline in phenol and alcohol (carbol fuchsin), which is taken up by
the microorganisms and other tissue components. Decolorizer, an acid alcohol reagent, is applied to remove the color from
all tissue elements. The organism’s waxy capsule contains a lipid component which is resistant to decolorization by the acid
solution (acid fast). The bacteria appear as red patches on lower magnification. At 100X, under oil, they appear as overlapping
rod-shaped structures2
that are sometimes described in literature as “Chinese sticks”. Some types of acid-fast bacteria may
appear pleomorphic depending on the type of organism and the plane of the section. 3
5. 5
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
AFB
Stain basics
Figure 3. Lung tissue infected with AFB organisms, 400x. Figure 4. Lung tissue infected with AFB organisms, 200x. Figure 5. Stomach tissue infected with AFB organisms, 600x.
Common utility
AFB stain may be used in the visualization of acid-fast
bacteria in diseases such as tuberculosis and leprosy.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents. Ideally, it should be representative of the
tissues it is usually used to diagnose. An example of a positive
control material would be formalin-fixed, paraffin-embedded
human tissue positive for acid-fast bacteria.3
6. 6
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Technical notes
1. When staining for microorganisms, it is important to ensure
that the water bath is scrupulously clean prior to sectioning in
order to prevent introduction of extraneous microorganisms
onto the specimen section slide. It is recommended not to use
water left standing overnight.
2. Cut sections, usually 3–5 μm, and pick the sections up on
glass slides.
3. Section thickness may affect quality and intensity of
staining. Thinner sections (2-3 μm) may produce lighter
staining, but individual bacteria may be easier to discern.
Thicker sections (4-5 μm) may produce darker staining
due the organisms being stacked upon one another, but
individual bacteria may be more difficult to discern.
References
1. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology. 2nd edition. St. Louis, MO: C.V. Mosby
Company; 1980:235-237.
2. Bancroft JD, Gamble, M. Theory and Practice of
Histological Techniques. 2nd edition. Edinburgh: Churchill-
Livingston; 1982:244.
3. Carson F, Hladik C. Histotechnology:A Self Instructional
Text 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
AFB
Technical notes and references
7. 7
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. AFB organisms staining on infected colon, 600x.
8. 8
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Expected results
• Weakly acidic mucosubstances — bright blue/turquoise
• Nuclei stain — pinkish red
• Cytoplasm — pale pink
Figure 1. Colon stained with Alcian Blue, 200x. Figure 2. Colon stained with Alcian Blue, 400x.
Alcian Blue
Stain basics
Purpose
The Alcian Blue stain may be used as a qualitative histologic stain to demonstrate weakly acidic mucopolysaccharides. At pH
2.5, alcian blue stains sulfated and carboxylated acid mucopolysaccharides and sulfated and carboxylated sialomucins and
glycoproteins in formalin-fixed, paraffin-embedded tissue.
Staining principle
Alcian dyes belong to the cuprophthalocyanine group, a group of water–soluble polyvalent basic dyes that are blue due to
the copper in the molecule. At a pH of 2.5, alcian blue reacts with compounds containing polyanionic charges with sulfuric
and carboxylic radicals. The dye appears to be bound by the formation of salt linkages with the acid groups of the acid
mucopolysaccharides.1,2
9. 9
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Alcian Blue
Stain basics
Figure 4. Stomach stained with Alcian Blue showing very weak staining
of the gastric mucosa. 200x.
Figure 5. Duodenum stained with Alcian Blue showing strong staining of
the goblet cell. 200x.
Figure 3. Umbilical cord stained with Alcian Blue. 400x.
Common diagnostic utility
Alcian Blue may be used to detect cells expressing acid
mucopolysaccharides in conditions such as Barrett’s
Esophagus or other disease processes, or the loss of such
cells in certain disease processes in the gastrointestinal
tract. The Alcian Blue stain may be helpful in detecting
genetic disorders of acid mucosubstance metabolism, and
collagen diseases where various acid mucosubstances are
increased. The presence of acid mucosubstances tends to
decline with advancing age.
Tissue controls
Known positive tissue controls should be utilized for
monitoring the correct performance of processed tissues
and test reagents. Ideally, it should be representative of the
tissues it is usually used to diagnose. Some examples of
components that stain positive with Alcian Blue are goblet
cells, hyaluronic acid (found in umbilical cord and connective
tissue in dermis), salivary glands and gastric lining cells.
Tissues containing these components would be appropriate
positive controls.
10. 10
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Alcian Blue
Technical notes and references
Technical notes
1. Section thickness may affect quality and intensity of
staining. Cut sections, usually 3–5 μm, and pick the
sections up on glass slides.
2. Alcian Blue stain is pH dependent. If the positive control
does not stain appropriately, check the quality of the water
used to prepare the wash solutions.
3. Make sure that your positive control tissue is known to
express acid mucins
References
1. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology. 2nd edition. St. Louis, MO: C.V. Mosby
Company; 1980:172-173.
2. Carson F, Hladik C. Histotechnology: A Self Instructional
Text. 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
11. 11
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Colon stained with Alcian Blue, 200x.
12. 12
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 1. Gastric tissue with H. Pylori stained with Alcian Yellow. 600x. Figure 2. Gastric tissue with H. Pylori stained with Alcian Yellow. 1000x.
Alcian Yellow
Stain basics
Purpose
Alcian Yellow is a qualitative histologic stain for Helicobacter pylori in formalin-fixed, paraffin-embedded tissue.
Staining principle
The gastric mucin is oxidized in aqueous periodic acid and then neutralized with sodium metabisulfite. This renders the
subsequent staining with Alcian Yellow (a monoazo dye similar to Alcian Blue) resistant to staining by toluidine. Aqueous
Toluidine Blue is then applied, which stains the microorganisms and other tissue components. The final result is blue bacteria
on a yellow background. Staining the H. pylori organism with standard hematoxylin and eosin techniques produces a poor
result and the special staining process can be lengthy.1
The typical staining methods for H. pylori are Steiner and Romanowski-
type stains.2
Toluidine Blue has been used as a rapid method for the demonstration of these organisms, but the contrast is
generally very poor.
Expected results
• H. pylori organisms — blue
• Background — blue
• Mucin — yellow
13. 13
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Alcian Yellow
Stain basics
Common diagnostic utility
Helicobacter pylori is a gram-negative bacterium that has
been demonstrated as the causative organism in some
gastric and duodenal ulcers. It is the most common cause
of antral gastritis, and is associated with duodenal and
gastric peptic ulcer disease, and with the development of
distal gastric carcinoma and low grade MALT-type gastric
lymphoma. The H. pylori organism has been shown to exist
in the acid environment of the stomach and is capable
of destroying the neutral mucin secreted by the surface
epithelial cells.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents.3
Ideally, it should be representative of the
tissues it is usually used to diagnose. An example of a positive
control material would be formalin-fixed, paraffin-embedded
human gastric tissue, positive for H. pylori.4
Figure 3. Gastric tissue with H. Pylori stained with Alcian Yellow. 600x. Figure 4. Gastric tissue with H. Pylori stained with Alcian Yellow. 1000x. Figure 5. Appendix tissue with micro-organisms stained with Alcian
Yellow. 600x.
14. 14
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Alcian Yellow
Technical notes and references
Technical notes
1. Section thickness may affect quality and intensity of
staining. Cut sections, usually 3–5 μm, and pick the
sections up on glass slides.
2. When staining for microorganisms, it is important
to ensure that the water bath is scrupulously clean
prior to sectioning in order to prevent introduction of
extraneous microorganisms onto the specimen section
slide. It is recommended not to use water left standing
overnight.
3. Staining intensity and distinct visualization of the
microorganisms may be greatly affected by post-
instrument time in 95% alcohol. Longer time in 95% alcohol
will result in lighter blue and/or yellow staining. This must
be tightly controlled and validated however, as over-
differentiating in 95% alcohol may result in excessively
weak or negative staining.
References
1. Leung JK, Givvon KJ, Vartanian RK. Rapid Staining method
for Helicobacter pylori in Gastric Biopsies. J Histotechnol.
1996;19(2);131-132.
2. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology, 2nd edition. St. Louis, MO: C.V. Mosby
Company; 1980.
3. Clinical and Laboratory Standards Institute (CLSI). CLSI
Web site. http://www.clsi.org/. Accessed November 3,
2011.
4. Carson F, Hladik C. Histotechnology: A Self Instructional
Text. 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
15. 15
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Gastric tissue with H. Pylori stained with Alcian Yellow. 600x.
16. 16
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Congo Red
Stain basics
Purpose
Congo Red stain is used as a qualitative histologic stain to selectively demonstrate amyloid in formalin-fixed, paraffin-
embedded tissue. 1
Staining principle
The staining reaction is based on the application of Congo red, which stains the patterns of atypical proteins (amyloid). The
beta-pleated sheets of amyloid are suitable in size and shape to accommodate the Congo red molecules, which are held in the
latticework of the beta-pleated sheets.2
Congo red may also stain unexpected structures such as keratin and elastic and dense
collagen fibers. Birefringence is an intrinsic property of the amyloid fibril Congo red complex.3,4
When examined with polarized
light, true amyloid exhibits apple-green birefringence. Without both the red staining of Congo red and the apple-green
birefringence under polarization, a definite identification cannot be made.
Expected results
• Light Microscopy:
- Amyloid — reddish pink
- Nuclei — blue
• Polarized Light:
- Amyloid — apple-green fluorscence
- Background — dark blue/black
Figure 1. Amyloid in lung stained with Congo Red, regular light microscopy, 200x. Figure 2. Amyloid in lung stained with Congo Red, polarized light
microscopy, 200x.
17. 17
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Congo Red
Stain basics
Figure 3. Amyloid in kidney stained with Congo Red, regular light
microscopy, 200x.
Figure 4. Amyloid in kidney stained with Congo Red, polarized light
microscopy, 200x.
Common diagnostic utility
Congo red stain may be used for the definitive identification
of amyloid deposits in tissues in the diagnosis of primary
(idiopathic) amyloidosis or secondary amyloidosis related to
numerous conditions characterized by extracellular protein
deposits. The extracellular protein may be localized to one
specific site or generalized throughout the body (systemic).
Amyloidosis tends to be associated with organ structures
such as: peripheral nerves, skin, tongue, joints, heart, lung,
liver, spleen, kidneys, liver and adrenals.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents.5
An appropriate control tissue for the
Congo red stain should contain amyloid deposits. Ideally, it
should be representative of the tissues it is usually used to
diagnose. The most common tissue controls are amyloid-
positive lung or kidney.6
18. 18
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Congo Red
Technical notes and references
Technical notes
1. Tissue section thickness is important and may affect
quality and intensity of staining.
2. The amyloid fibril/Congo Red complex is a large
molecular complex. Unless sections are cut at 5-10
microns, it may be very difficult to visualize the apple-
green birefringence under polarized light. This may be
especially problematic for routinely sectioned renal
biopsies which are normally cut at 3 microns.
References
1. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology. 2nd edition. St. Louis, MO: C.V. Mosby
Company; 1980.
2. Wheater PR, Burkitt HG. Basic Histopathology, 2nd edition.
New York: Churchill Livingstone; 1991.
3. Navarro A, Tolivia J, Valle E. Congo Red Method
for Demonstrating Amyloid in Paraffin Sections. J
Histotechnol. 1999;22(4):305-308.
4. Fredenburgh JL, Grizzle WE. Special Stains: Their Chemical
Mechanism. Chicago: ASCP Press; 1998.
5. Clinical and Laboratory Standards Institute (CLSI). CLSI
Web site. http://www.clsi.org/. Accessed November 3,
2011.
6. Carson F, Hladik C. Histotechnology: A Self Instructional
Text, 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
19. 19
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 5. Amyloid in lung stained with Congo Red, regular light microscopy, 200x.
20. 20
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Elastic
Stain basics
Purpose
The Elastic Staining is used to differentiate elastic fibers from collagen. It is useful in demonstrating changes in elastic fibers in
certain disease processes.1
Depending on the method used, elastic fibers are stained black/purple with the elastic stain, while
the collagen is stained red/pink and the other tissue structures are stained yellow with the counterstain.1
Staining principle
The staining reaction is based on the affinity towards elastic fibers displayed by resorcin fuchsin. Since the method is not
absolutely specific, other structures such as collagen and basal membranes might also stain. Ferric chloride is used as a
mordant which binds to elastic fibers. The resorcin-fuchsin (resorcinol and basic fuchsin solution) and the ferric chloride react
to form an iron-resorcin lake precipitate. The complex formed from the reaction of the basic fuchsin, resorcinol and ferric
chloride (an iron resorcin lake) binds to the elastic fibers, resulting in the blue-black/purple staining of the elastic fibers. The
elastic stain is then followed by a Van Gieson counterstain solution of acid fuchsin and picric acid which stains the collagen
red and the background yellow.
Expected results
• Elastic — Blue-black/purple
• Collagen — Red
• Background — yellowish
Figure 1. Artery stained with Elastic stain Figure 2. Artery in kidney stained with Elastic stain,
21. 21
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Elastic
Stain basics
Figure 3. Temporal artery stained with Elastic stain, demonstrating a
well-defined internal elastic lamina and a less distinct external elastic
lamina separated by a smooth muscle layer. 200x.
Figure 4. Elastic staining in lung showing a bronchovascular bundle
(bronchiole with a single elastic lamina and pulmonary artery containing
both internal and external elastic laminae). 200x.
Figure 5. Normal skin stained with Elastic stain, demonstrating loosely
arranged elastic fibers in the papillary and densely arranged elastic fibers
in the reticular dermis. 200x.
Common diagnostic utility
This stain is useful in demonstrating atrophy of elastic
fibers in cases of emphysema, and the thinning and loss
of elastic fibers in arteriosclerosis and other vascular
diseases.1
The elastic stain has also been used as a possible
aid in visualizing pleural effusion in the staging and patient
management in non-small cell lung cancer. 2
Elastic stain may also be used for temporal artery biopsies
where it is a standard diagnostic test for temporal arteritis. It
is used to illustrate the inflammation and deterioration of the
internal elastic lamina.3
More recent publications suggest that Elastic stain may
be helpful in assessing transmural spread by colorectal
carcinoma. Serosal invasion by colorectal carcinoma is
generally accepted to have adverse prognostic significance
but may be difficult to assess.4
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents. An example of a positive control material
for Elastic stain would be formalin-fixed, paraffin-embedded
human tissue with elastic fibers such as aorta, artery, kidney,
lung or skin.5
Ideally, it should be representative of the tissues
it is usually used to diagnose.
22. 22
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Elastic
Technical notes and references
Technical notes
1. Section thickness may affect quality and intensity of
staining. Cut sections, usually 3–5 μm, and pick the
sections up on glass slides.
2. The last step in the Elastic staining procedure is the Van
Gieson counterstain. Since this is an acidic solution,
prolonged overstaining with the counterstain can reduce
the elastic staining.
3. Both the elastic staining as well as the counterstain can
be greatly affected by post-staining run down procedures.
Prolonged time in alcohol solutions is not recommended.
References
1. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology, 2nd edition. St. Louis, MO: C.V. Mosby
Company; 1980.
2. Taube JM, Askin FB, Brock MV, Westra W. Impact of elastic
staining on the staging of peripheral lung cancers. Am J
Surg Pathol. 2007 Jun;31(6):953-6.
3. Trevor A Flood, MD; Chief Editor: Allen Patrick Burke, MD.
Temporal Arteritis Pathology. http://emedicine.medscape.
com/article/1612591-overview#a30
4. Colin J. R. Stewart, Simon Hillery, Cameron Platell and
Giacomo Puppa. Assessment of Serosal Invasion and
Criteria for the Classification of Pathological (p) T4 Staging
in Colorectal Carcinoma: Confusions, Controversies and
Criticisms. Cancers 2011, 3, 164-181
5. Carson F, Hladik C. Histotechnology: A Self Instructional
Text. 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
23. 23
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Artery in kidney stained with Elastic stain,
24. 24
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Giemsa
Stain basics
Purpose
In formalin-fixed, paraffin-embedded tissue, Giemsa is used as a qualitative histologic stain to differentiate leukocytes in bone
marrow and other hematopoietic tissue (lymph nodes). The stain can also be used to demonstrate some microorganisms,1
such as Helicobacter pylori.
Staining principle
Giemsa stain is a type of Romanowski stain, which is a polychromatic group of stains formed from the precipitate created
by the combinations of solutions of methylene blue and eosin in methanol. These stains were originally intended as a single-
step fixation and staining method for blood and bone marrow smears or touch-preps. The staining reaction is based on the
differential affinity of cell types for the dyes in the stain. Because of the high degree of dissociation, active molecules (eosin
and thiazine dyes) are absorbed by cellular structures very quickly. Differentiation in alcohol renders the staining of the various
cell types multi-colored, with the nuclear material staining in various shades of blue and the cytoplasm staining pink.3
Cellular
granules stain red or purple, depending on whether they are acidophilic or basophilic.1, 2, 6
Expected results
• Collagen, muscle, bone — pale pink
• Micro-organisms — purplish-blue
• Nuclei — dark blue
• Red blood cells — pink (or green if bone marrow fixed in
Zenkers over the weekend)
• Cytoplasm — varying light blue shades
• Basophilic granules — blue/purple
• Eosinophilic granules — red
Figure 1. Gastric biopsy stained with Giemsa demonstrating H. Pylori organisms, 600x. Figure 2. FFPE section of bone marrow clot stained with Giemsa, 600x.
25. 25
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Giemsa
Stain basics
Figure 3. Gastric biopsy stained with Giemsa demonstrating H. Pylori
organisms stained deep blue in the gastric pits.
Figure 4. FFPE section of bone marrow trephine stained with Giemsa
showing erythrocyte precursor cells with intensely blue nuclei, white
blood cell precursor stained with lighter blue nuclei and pink, gray or
bluish cytoplasm, bone staining pink, eosinophilic granules staining dark
pink/red and basophilic granules staining blue/purple.
Figure 5. Skin biopsy stained with Giemsa demonstrating dark blue/
purple granular mast cells.
Common diagnostic utility
Giemsa stain may be used to demonstrate Helicobacter
pylori or other campylobacter species in gastric biopsies, 1,5
Donovan bodies and leishmania organisms in tissue
sections. It may also be used for the demonstration of mast
cells in cutaneous mastocytosis, or for the elucidation of
hematopoietic cell lineages in bone marrow biopsies or bone
marrow aspirates in diseases involving the bone marrow.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents. Ideally, it should be representative of
the tissues it is usually used to diagnose. Examples of
appropriate Giemsa controls include human tissue such as
bone marrow, lymph node, or spleen2
or Helicobacter pylori-
positive tissue specimen.
26. 26
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Giemsa
Technical notes & references
Technical notes
1. Section thickness may affect quality and intensity of
staining. Cut sections, usually 3–5 μm, and pick the
sections up on glass slides.
2. When staining for microorganisms, it is important to
ensure that the water bath is scrupulously clean prior to
sectioning in order to prevent introduction of extraneous
microorganisms onto the specimen section slide It is
recommended not to use water left standing overnight.
3. Staining intensity and distinct visualization of the
microorganisms may be greatly affected by post-
instrument time in 95% alcohol. Extending exposure time in
alcohol dehydration bath will enhance differentiation but, if
overdone, may also decolorize the organisms. Depending
on whether staining for H. Pylori or for hematopoietic cells
in bone marrow or mast cells in skin, 15-20 seconds in each
95% alcohol bath is a recommended starting point. This
must be tightly controlled and validated however, as over-
differentiating in 95% alcohol may result in excessively
weak or negative staining.
4. Alternately, differentiating in dilute acetic acid will bring
out the metachromatic properties of the Giemsa stain.
This may be a better option for demonstration of mast
cells in skin biopsies. The acetic acid concentration
used varies by different authors but generally ranges
from 0.1 to 0.5% in deionized/distilled water. The
differentiation time will vary according to the staining
time, temperature and even section thickness, but
it is generally achieved within 30 seconds. This
differentiating method primarily removes the blue dye,
providing greater contrast for the red dye. (See images
below demonstrating differentiation in 0.1% acetic)
5. When fixatives other than neutral buffered formalin are
used, red blood cells may appear to stain grayish green.
References
1. Bancroft and Stevens. Theory and Practice of Histological
Techniques, 2nd edition. Edinburgh: Churchill-Livingston,
1982.
2. Carson F, Hladik C. Histotechnology:A Self Instructional
Text. 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
3. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology, 2nd edition. St. Louis, MO: C.V. Mosby
Company; 1980:154-156.
4. Clinical and Laboratory Standards Institute (CLSI). CLSI
Web site. http://www.clsi.org/. Accessed November 3,
2011.
5. Loffeld RJ, Stobberingh E, Flendrig JA, Arends JW.
Helicobacter pylori in gastric biopsy specimens.
Comparison of culture, modified giemsa stain, and
immunohistochemistry. A retrospective study. J Pathol.
1991 Sep;165(1):69-73.
6. Wittekind D, Schulte E, Schmidt G, Frank G., The standard
Romanowsky-Giemsa stain in histology., Biotech
Histochem. 1991;66(6):282-95.
27. 27
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Gastric biopsy stained with Giemsa demonstrating H. Pylori organisms, 600x.
28. 28
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Gram
Stain basics
Purpose
Gram stain is a qualitative histologic stain used to classify bacteria broadly into two categories, either gram-negative or gram-
positive.
Staining principle
The classification of bacteria as either Gram-positive or Gram-negative is based on the properties of the bacterial cell walls
which allow selective retention of the Gram stain. In general, the bacterial cell wall contains a layer of peptidoglycan (an
amino acid/carbohydrate polymer). The thickness of this layer is the main factor for how the bacteria will stain with the Gram
stain. The cell wall Gram-positive bacteria generally have a thick peptidoglycan layer (20 to 80 nanometers), whereas the
cell wall of Gram-negative bacteria generally have a thinner peptidoglycan layer (7 to 8 nanometers). 1
The stain consists of
applying an aqueous solution of crystal violet which permeates the peptidoglycan layer and stains both types of organisms
blue. This followed by the addition of an iodine solution which complexes with the crystal violet rendering it water insoluble.
Differentiation is achieved with the application of an organic solvent. The thinner peptidoglycan layer of the Gram-negative
organisms is more readily decolorized than the thicker layer of the Gram-positive organisms, resulting in loss of the blue dye
in the Gram-negative organisms. The differentiation step is followed by the addition of a red dye to stain the Gram-negative
organisms. 2
Expected results
• Gram-positive bacteria - blue
• Gram-negative bacteria - red
• Fungal organisms - blue
• Background - yellow (with tratrazine counterstain)
- green (with methyl green counterstain)
Figure 1. Gram stain with Tarttrazine counterstain showing a mixture of Gram-positive and Gram-negative microorganisms, 1000x. (oil) Figure 2. Gram- stain with Light Green counterstain showing a mixture of
Gram-positive and Gram-negative microorganisms, 1000x. (oil)
29. 29
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Gram
Stain basics
Figure 3. Gram stain with Tarttrazine counterstain on appendix showing
mostly gram positive microorganisms, 600x.
Figure 4. Gram stain with Light Green counterstain on appendix
showing a mixture of Gram-positive and Gram-negative
microorganisms, 1000x. (oil)
Figure 5. Rat lung engineered control with Gram-positive and Gram-
negative organisms, 1000x.
Common diagnostic utility
The Gram stain may be used to broadly demonstrate the
presence of Gram-positive or Gram-negative organisms in
miscellaneous tissue infections from various sources and
diseases. 3-5
Tissue controls
A known positive tissue controls should be utilized for
monitoring the correct performance of processed tissues
and test reagents.6
An appropriate control tissue for the
Gram stain should contain both Gram-positive and Gram-
negative microorganisms. Ideally, it should be representative
of the tissues it is usually used to diagnose. A common tissue
controls for Gram staining is appendix.
30. 30
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Gram
Technical notes, post-instrument processing and references
Technical notes
1. Section thickness may affect quality and intensity of
staining. Cut sections, usually 3–5 μm, and pick the
sections up on glass slides.
2. When staining for microorganisms, it is important to ensure
that the water bath is scrupulously clean prior to sectioning in
order to prevent introduction of extraneous microorganisms
onto the specimen section slide. It is recommended not to use
water left standing overnight.
3. Antibiotics can affect the cell wall of gram-positive
bacteria and therefore affect the staining quality of the
Gram stain.
4. Nocardia is a variable gram-positive bacteria which may
stain pink to red with some blue to purple segments. It may
be better visualized with an alternative staining method.
References
1. C.Michael Hogan. 2010. Bacteria. Encyclopedia of Earth.
eds. Sidney Draggan and C.J.Cleveland, National Council
forScience and the Environment, Washington DC (http://
www.eoearth.org/article/Bacteria?topic=49480)
2. Kiernan J.A.: Histological and histochemical methods:
theory and practice. fourth ed. Bloxham, Scion, 2007.
3. Carson F, Hladik C. Histotechnology: A Self Instructional
Text, 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
4. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology. 2nd ed. St. Louis, MO: C.V. Mosby
Company; 1980.
5. Bancroft JD, Gamble, M. Theory and Practice of
Histological Techniques. 2nd ed. Edinburgh: Churchill-
Livingston; 1982.
6. Clinical and Laboratory Standards Institute (CLSI). CLS
31. 31
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Gram stain with Tarttrazine counterstain showing a mixture of Gram-positive and Gram-negative microorganisms, 1000x. (oil)
32. 32
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
GMS
Stain basics
Purpose
Grocott Methenamine Silver (GMS) stain is intended for use as a qualitative histologic stain to demonstrate polysaccharides in
the cell walls of fungi and other opportunistic organisms in formalin-fixed, paraffin-embedded tissue.1
Staining principle
The staining reaction is based on aldehyde reduction of silver ions to metallic silver under alkaline conditions.3
Fungal and
microbial cell wall polysaccharides are oxidized to aldehyde groups by chromic acid. This also suppresses weaker background
staining of collagen fibers and basement membranes. Excess chromic acid is removed and neutralized with sodium bisulfite.
A silver nitrate in an alkaline solution provides the silver ions and alkaline conditions necessary to reduce the silver ions to
metallic silver. Subsequent application of gold chloride forms a more stable complex with the silver and removes the yellow
tones from the tissue. Sodium thiosulfate stops the reaction and removes any unreduced silver from the section. Light Green is
applied as a counterstain to provide a contrasting background.
Expected results
• Organisms — black/gray
• Background — green
Figure 1. Pneumocystus organisms in lung stained with GMS, 200x. Figure 2. Fungus organisms in testes stained with GMS, 600x.
33. 33
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 3. Cryptococcus infected tissue stained with GMS, 400x. Figure 4. Histoplasma infected tissue stained with GMS, 400x. Figure 5. Engineered Sporothrix fungus control stained with GMS, 600x.
Common diagnostic utility
This stain is primarily used to distinguish pathogenic
fungi such as Aspergillus and Blastomyces1
and other
opportunistic organisms such as Pneumocystis pneumonia
(PCP) which is caused by Pneumocystis carinii (now
reclassified as Pneumocystis jiroveci)5, 6
in tissue sections.2
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents. Ideally, it should be representative
of the tissues it is usually used to diagnose. An example
of a positive control material would be formalin-fixed,
paraffin-embedded human tissue positive for fungus or
Pneumocystis carinii (jiroveci) which may be found in lung of
immunocompromised patients.4
GMS
Stain basics
34. 34
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Technical notes
1. Section thickness may affect quality and intensity of
staining. Cut sections, usually 3–5 μm, and pick the
sections up on glass slides.
2. When staining for microorganisms, it is important to ensure
that the water bath is scrupulously clean prior to sectioning in
order to prevent introduction of extraneous microorganisms
onto the specimen section slide. It is recommended not to use
water left standing overnight.
References
1. Rimondi AP, Bianchini E, Barucchello G, and Panzavolta
R. Addison’s disease caused by adrenal blastomycosis:
A case report with fine needle aspiration (FNA) cytology.
Cytopathology. 1995;6:211-219.
2. Carson F, Hladik C. Histotechnology: A Self Instructional
Text. 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
3. Bancroft JD, Gamble, M. Theory and Practice of
Histological Techniques. 2nd ed. Edinburgh: Churchill-
Livingston; 1982.
4. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology. 2nd ed. St. Louis, MO: C.V. Mosby
Company; 1980.
5. Frenkel JK. Pneumocystis pneumonia, an
immunodeficiency-dependent disease (IDD): a critical
historical overview. J Eukaryot Microbiol 1999;46:89S–92S.
6. Stringer JR, Beard CB, Miller RF, Wakefield, AE. A New
Name (Pneumocystis jiroveci) for Pneumocystis from
Humans. Emerg Infect Dis 2002;8:891-896.
GMS
Technical notes and references
35. 35
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Pneumocystus organisms in lung stained with GMS, 200x.
36. 36
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Iron
Stain basics
Purpose
Iron stain is intended for use as a qualitative histologic stain to detect iron pigment in bone marrow, tissue with
hemochromatosis and hemosiderosis in formalin-fixed, paraffin-embedded tissue.1
Staining principle
The iron is separated from protein by hydrochloric acid. The free ferric iron reacts with the potassium ferrocyanide to form an
insoluble bright blue ferric ferrocyanide, or Prussian blue. 1, 2, 4
Expected results
• Iron — deep blue
• Nuclei — Red
• Background — pink
Figure 1. Liver with iron deposits stained with Iron Stain , 200x. Figure 2. Liver with iron deposits stained with Iron Stain , 200x.
37. 37
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Iron
Stain basics
Figure 3. Iron deposits in undecalcified FFPE section of bone marrow clot
stained with Iron stain, 200x.
Figure 4. Iron deposits in spleen stained with Iron stain, 200x.
Common diagnostic utility
Iron is absorbed through the small intestine and transported
to the bone marrow. There it is stored as hemosiderin, until
erythropoiesis, when it is incorporated into hemoglobin
molecules. During erythrocyte destruction at the end of red
cell life span, the iron is split off from the hemoglobin in the
lymphoreticular system and again stored in the bone marrow
as hemosiderin.5
In the disease states of hemochromatosis
and hemosiderosis, excessive amounts of ferric iron are
present in the liver, spleen and lymph nodes. Iron may be
found at any site where there has been local destruction of
red cells, such as hemorrhage sites, infarctions, longstanding
congestion and trauma.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents.3
Ideally, it should be representative of the
tissues it is usually used to diagnose. An example of a positive
control material would be formalin-fixed, paraffin-embedded
human tissue positive for iron, such as tissue involved in the
above-mentioned pathological processes.4
38. 38
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Technical notes
1. Acidic fixatives (including unbuffered formalin) may
solubilize the iron in the tissues and cause false negative
staining.
2. Iron deposits in the tissue may be removed by
decalcification methods. Misleading, false-negative
staining may occur. For diagnostic testing on bone
marrow samples, iron staining may be more reliable and
appropriate on smears of bone marrow aspirates rather
than bone marrow trephines.
3. Use distilled water in the water bath.
References
1. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology. 2nd ed. St. Louis, MO: C.V. Mosby
Company; 1980:215-218.
2. Bancroft and Stevens. Theory and Practice of Histological
Techniques, 2nd edition. Edinburgh: Churchill-Livingston;
1982.
3. Clinical and Laboratory Standards Institute (CLSI). CLSI
Web site. http://www.clsi.org/. Accessed November 3,
2011.
4. Carson F, Hladik C. Histotechnology: A Self Instructional
Text ,3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
5. Kong: American Society for Clinical Pathology Press;
2009. S E Stuart-Smith, D A Hughes, B J Bain. Are routine
iron stains on bone marrow trephine biopsy specimens
necessary? J Clin Pathol 2005;58:269–272. doi: 10.1136/
jcp.2004.017038
Iron
Technical notes and references
39. 39
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 5. Liver with iron deposits stained with Iron Stain , 200x.
40. 40
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Purpose
The Jones Methenamine Silver stain is intended for use as a qualitative histologic stain to demonstrate capillary basement
membrane in formalin-fixed, paraffin-embedded tissue. 1
The basement membranes appear as black ink drawn lines. The stain
is often used to examine the basement membrane of the kidney glomerulus in certain disease states.
Staining principle
The methenamine-silver complex in this stain is used to demonstrate the carbohydrate components of reticular fibers and
basement membranes.2
The periodic acid oxidizes the carbohydrate components of the basement membrane which produce
aldehydes. The released aldehydes reduce the silver to a visible metallic silver. The black basement membranes can be
counsterstained with Hematoxylin and Eosin, or with Light Green.
Expected results
• Basement membranes - black
• Nuclei — Dark Blue
• Background — pink (with H&E counterstain)
• Background — green (with Light Green counterstain)
Figure 1. Kidney stained with Jones using Hematoxylin and Eosin counterstain, 200x. H&E Figure 2. Kidney stained with Jones using Light Green counterstain, 200x.
Jones & Jones Light Green
Stain basics
41. 41
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 3. Kidney stained with Jones using Hematoxylin and Eosin
counterstain, 400x.
Figure 4. Kidney stained with Jones using Light Green counterstain,
400x.
Common diagnostic utility
The purpose of this stain is primarily to distinguish
pathological abnormalities in kidney diseases. The Jones
stain demonstrates the spiked glomerular basement
membrane (GBM), caused by subepithelial deposits,
seen in membranous nephropathy in the autoimmune
disease Goodpasture’s syndrome, where anti-glomerular
basement auto-antibodies result in damage to the basement
membrane and inflammation of the capillaries. In diabetic
glomerulosclerosis, the basement membrane becomes
thickened up to 4-5 times the normal thickness. In nephrotic
syndrome the glomerular filtration mechanism is affected,
usually in the glomerular basement membrane, causing
structural changes. Some symptoms include proteinuria,
hypoalbuminaemia, edema and hyperlipidemia.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents.3
Ideally, it should be representative of the
tissues it is usually used to diagnose. An example of a positive
control material would be formalin-fixed, paraffin-embedded
human kidney.4
Jones & Jones Light Green
Stain basics
42. 42
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Technical notes
1. Section thickness may affect quality and intensity of
staining. In order to properly visualize the glomerular
basement membrane, tissue sections should be very thin.
Cut sections preferably at 2 to 3 μm and pick the sections
up on glass slides.
References
1. Koski JP. Silver methenamine-borate (MB): Cost reduction
with technical improvement in silver nitrate-gold chloride
impregnations. J Histotechnol. 1981;4:115.
2. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology. 2nd edition. St. Louis, MO: C.V. Mosby
Company; 1980.
3. Clinical and Laboratory Standards Institute (CLSI). CLSI
Web site. http://www.clsi.org/. Accessed November 3,
2011.
4. Carson F, Hladik C. Histotechnology: A Self Instructional
Text. 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
Jones
Technical notes and references
43. 43
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 5. Kidney stained with Jones using Hematoxylin and Eosin counterstain, 200x. H&E
44. 44
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Mucicarmine
Stain basics
Purpose
Mucicarmine stain is intended for use as a qualitative histologic stain to detect acid mucopolysaccharides (mucin) in formalin-
fixed, paraffin-embedded tissue. Mucin is a secretion of acid mucopolysaccharides and other substances produced by a
variety of epithelial and connective tissue cells. In certain inflammatory processes and certain intestinal carcinomas, epithelial
cells secrete excess mucin.1
Staining principle
The staining reaction is based on the reaction of an aluminum-carmine chelate complex attached to acid groups of mucin.
Carmine and aluminum mordant combine to stain the epithelial mucin a deep rose to red color. Although the mechanism is
not completely understood, it is believed that the aluminum forms a chelate complex with carmine by dye lake formation, to
produce a net positive charge.1
The complex then attaches to the acid groups of the mucin. Tartrazine counterstain is applied
to provide a contrasting yellow background.
Expected results
• Mucin — rose red
• Nuclei — black/gray
• Background/connective tissue — yellow
Figure 1. Colon adenocarcinoma stained with Muci stain, 200x. Figure 2. Normal colon stained with Muci stain, 200x.
45. 45
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Mucicarmine
Stain basics
Figure 3. Normal colon stained with Muci stain, 100x Figure 4. Cryptococcus organisms in bowel stained with Muci stain,
200x.
Common diagnostic utility
Mucicarmine stain detects mucins of epithelial origin.
Fibroblastic or connective tissue mucins may stain poorly.2
The purpose of this stain is primarily to determine the
site of a primary tumor or to distinguish undifferentiated
mucin-negative squamous cell lesions from mucin-
positive adenocarcinomas.1
As is the case with current
manual stains, mucicarmine stain may not be appropriate
for detection of metastatic cancers of the stomach.3
The
stain may also be used as an aid in the identification of
Cryptococcus neoformans, a pathogenic fungus containing
mucin in its capsule.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents.4
An appropriate control tissue for the
Mucicarmine stain should contain sialomucins. Ideally, it
should be representative of the tissues it is usually used to
diagnose.5
The most common tissue controls are tissues
that contain normal colonic mucosa, adenocarcinomas or
Cryptococcus infected tissue.
46. 46
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Mucicarmine
Technical notes and references
Technical notes
1. Section thickness may affect quality and intensity of
staining. Cut sections, usually 3–5 μm, and pick the
sections up on glass slides.
References
1. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology. 2nd ed. St. Louis, MO: C.V. Mosby
Company; 1980.
2. Thompson SW. Selected Histochemical and
Histopathologic Methods. Springfield, IL: CC Thomas;
1966:453.
3. Silverberg SG, Delellis RA, Frable WJ. Principles and
Practice of Surgical Pathology and Cytopathology. New
York, NY: Churchill Livingstone Inc.;1997:51.
4. Clinical and Laboratory Standards Institute (CLSI). CLSI
Web site. http://www.clsi.org/. Accessed November 3,
2011.
5. Carson F, Hladik C. Histotechnology:A Self Instructional
Text 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
47. 47
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
PAS
Stain basics
Purpose
PAS stain may be used as a qualitative histologic stain in formalin-fixed, paraffin-embedded tissue to demonstrate the
presence of neutral polysaccharides in cellular substances and structures such as glycogen, starch, cellulose, glycolipids,
glycoproteins and many other carbohydrates. It is useful as a stain for basement membranes, plasma membrane stain and
carbohydrate secretions and granules.
Staining principle
The staining reaction is based on the reactivity of Schiff’s regent with aldehyde groups. Aldehyde groups are produced in
polysaccharides though the oxidation of glycol groups by periodic acid.5
This is followed by selective staining of the aldehyde
groups by a colorless Schiff’s Reagent. Schiff’s Reagent forms a colorless dialdehyde compound that is transformed to the
magenta colored final staining of the glycol-containing cellular components.5
Expected results
• Neutral polysaccharides, glycogen, fungus and basement
membrane — bright magenta
• Nuclei — dark blue
• Background and other tissue components — depend on
combination of stain used.
Figure 1. Kidney showing glomerular basement membrane stained with PAS stain Figure 2. Stomach showing intense mucosal staining with PAS stain, 200x.
48. 48
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
PAS
Stain basics
Figure 3. Duodenum showing strong mucosal staining with PAS stain,
200x.
Figure 4. Colon showing lighter mucosal staining with PAS stain, 200x. Figure 5. Section of FFPE Bone marrow clot showing PAS positive cells
staining with PAS stain, 400x.
Common diagnostic utility
PAS stain may be used to demonstrate reticular
fibers, basement membrane, fungus and
neutralmucopolysaccharides.1
PAS stain may also be
used to aid in distinguishing a PAS-positive secreting
adenocarcinoma from an undifferentiated PAS-negative
squamous cell carcinoma.2
It may also be useful for the
detection of glycogen in certain liver diseases. The basic
PAS stain may be combined with other adjunctive staining
reagents for the better elucidation of certain cellular and
tissue components.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents.4
Ideally, it should be representative of
the tissues it is usually used to diagnose.3
An example of a
positive control material would be formalin-fixed, paraffin-
embedded human kidney, a liver tissue specimen containing
containing glycogen, and marrow.
49. 49
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Kidney showing glomerular basement membrane stained with PAS stain
50. 50
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
PAS/Diastase
Stain basics
Purpose
The PAS stain in combination with enzymatic digestion with Diastase is used to aid in the differentiation of glycogen form other
neutral polyscaccharides in tissues.
Staining principle
The PAS stain may be combined with diastase reagent for the demonstration of glycogen. The PAS stain uses periodic acid
to oxidize glycols to aldehydes. Schiff’s reagent forms a colorless dialdehyde compound that is transformed to the fuschia-
colored final staining of glycol containing cellular components.1
In the combined PAS/Diastase stain, two parallel sections are run. One section is digested with diastase prior to staining with
the PAS reaction. The Diastase digests away the glycogen before PAS staining occurs. The second is stained with the PAS
reaction without digestion. The diastase removes any glycogen in the tissue thereby confirming the presence of glycogen by
its presence in the undigested section and its absence in the digested section.
Expected results
• Neutral polysaccharides, glycogen, fungus and basement
membrane - bright magenta
• Nuclei – dark blue
• Background and other tissue components – depend on
combination of stain used.
Figure 1. Glycogen storage disease in liver showing fairly strong magenta staining with PAS stain, 200 x Figure 2. Glycogen storage disease in liver showing no staining magenta
staining with PAS stain after digestion with Diastase, 200 x
51. 51
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 3. Liver with glycogen stained with PAS, 200x. Figure 4. Liver showing absence PAS (glycogen) staining following
digestion with diastase, 200x.
Common diagnostic utility
Diastase is useful as an aid in the diagnosis of glycogen
storage disease1
.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents.4
Ideally, it should be representative of
the tissues it is usually used to diagnose.3
An example of a
positive control material would be formalin-fixed, paraffin-
embedded human liver sample from glycogen storage
disease.
PAS/Diastase
Stain basics
52. 52
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 5. Glycogen storage disease in liver showing fairly strong magenta staining with PAS stain, 200 x
53. 53
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
PAS/Alcian Blue
Stain basics
Purpose
The PAS stain may be combined with Alcian Blue as a qualitative histologic stain to differentiate acid mucopolysaccharides
(mucins) from neutral mucopolysaccharides
Staining principle
The staining reaction is based on the oxidation of glycol to aldehyde followed by selective staining of the aldehyde groups by
Schiff’s reagent. The acidic Alcian Blue reagent differentially stains acid mucins and neutral mucopolysaccharides.
Expected results
• Neutral mucins - magenta with Schiff reaction from PAS
• Acid mucins - blue with Alcian Blue
• Neutral+Acid mucins - purple with both PAS and Alcian
Blue
Figure 1. Adenocarcinoma stained with PAS and Alcian Blue. Sialomucins that have acid and neutral mucopolysaccharides stain purple. Mucosa that have
only neutral mucins will stain red.
Figure 2. Bowel stained with PAS + Alcian blue, 600x
54. 54
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 3. Stomach stained with PAS/Alcian Blue, 100x. Figure 4. Colon stained with PAS/Alcian Blue, 400x. Figure 5. Colon carcinoma stained with PAS/Alcian Blue, 200x.
Common diagnostic utility
The PAS/Alcian Blue stain may be used for the discrimination
of acid mucins from neutral sialomucins in the detection of
intestinal metaplasia in chronic gastritis, Barrets Esophagus
and other GI abnormalities.
.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents.4
Ideally, it should be representative of
the tissues it is usually used to diagnose.3
An example of a
positive control material would be formalin-fixed, paraffin-
embedded GI tract tissue such as stomach and duodenum,
and small bowel.
PAS/Alcian Blue
Stain basics
55. 55
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Colon carcinoma stained with PAS/Alcian Blue, 200x.
56. 56
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
PAS/Light Green
Stain basics
Purpose
The PAS stain in combination with Light Green counterstain may be used used as qualitative histologic stain for detection of
fungus in formalin-fixed, paraffin-embedded tissue.
Staining principle
The PAS stain uses periodic acid to oxidize glycols to aldehydes. Schiff’s Reagent forms a colorless dialdehyde compound
that is transformed to the magenta-colored final staining of the glycol containing cellular components.1
The Light Green
counterstain stains the background light green providing improved contrast to magenta.
Expected results
• Fungus - magenta
• Other tissue components - medium green
• Red blood cells - bright green
• Nuclei - Blue with hematoxylin (optional)
Figure 1. Stomach showing intense mucosal staining with PAS stain, 200x. Figure 2. Bowel stained with PAS/Light green showing showing intense
magenta staining of mucin with PAS stain , 200x
57. 57
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 3. Fungus in lung stained with PAS/Light Green, 200x. Figure 4. Intestinal tissue with Cryptococcus organisms stained with PAS/
Light Green, 400x.
Figure 5. Fungal organisms in kidney stained with PAS/Light Green, 400x.
Common diagnostic utility
PAS may also be combined with light Green as a counterstain
to aid in the visualization of fungus in tissue sections.
The light green stains the connective tissue components,
combining with the PAS stain to give them a purple color. The
fungus is not staining with Light Green thus allowing better
discrimination of the organisms from the other PAS positive
tissue components.
.
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents.4
Ideally, it should be representative of
the tissues it is usually used to diagnose.3
An example of a
positive control material would be formalin-fixed, paraffin-
embedded tissue known to contain fungus or known to
contain neutral polysaccharides, such as colon.
PAS/Light Green
Stain basics
58. 58
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
PAS, PAS/Diastase, PAS/Light Green, PAS/Alcian Blue
Technical notes and references
Technical notes
1. Section thickness may affect quality and intensity of
staining. In order to properly visualize the glomerular
basement membrane in kidney biopsies, tissue sections
should be very thin. Cut sections, preferably, at 2 to 3 μm,
and pick the sections up on glass slides.
2. When staining for microorganisms, it is important to
ensure that the waterbath is scrupulously clean prior to
sectioning in order to prevent introduction of extraneous
microorganisms onto the specimen section slide.
Therefore, it is recommended not to use water left standing
overnight.
3. Alcian Blue stain is pH dependent and therefore sensitive
to fluctuations of the deionized or distilled water used
for the wash steps. Careful monitoring of water quality is
recommended.
References
1. Thompson SW. Selected Histochemical and
Histopathological Methods. Springfield; CC Thomas; 1966:
2. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology. 2nd edition. St. Louis, MO: C.V. Mosby
Company; 1980.
3. Carson F, Hladik C. Histotechnology: A Self Instructional
Text, 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
4. Clinical and Laboratory Standards Institute (CLSI). CLSI
Web site. http://www.clsi.org/. Accessed November 3,
2011.
5. Hotchkiss RD: A microchemical reaction resulting in
the staining of polysaccharide structures in fixed tissue
preparations. Arch Biochem. 1948;16:131.
59. 59
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Stomach showing intense mucosal staining with PAS stain, 200x.
60. 60
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Reticulum
Stain basics
Purpose
The Reticulum stain is intended for use as a qualitative histologic stain to demonstrate reticular fibers in formalin-fixed, paraffin-
embedded tissue. In certain tumors, reticulum is located in a characteristic position in relation to the actual tumor cells. Reticulum
stain can be used to show disease states in organs such as the liver, spleen and kidney by demonstrating reticular patterns1
not normal
to the organ. In normal liver, the fibers are well defined strands, but in necrotic or cirrhotic liver, the fibers have discontinuous patterns.
Staining principle
Reticular fiber is composed of one or more types of very thin and delicately woven strands of type III collagen. These strands
build a highly ordered cellular network and provide a supporting network. Many of these types of collagen have been combined
with carbohydrate. They are reactive with Periodic Acid-Schiff (PAS) and are also argyrophilic (affinity for silver). They react with
silver stains where they selectively reduce silver salts to metallic silver.
The carbohydrates are oxidized with an acidic solution of potassium permanganate and produce reactive aldehyde groups. This
followed by an aqueous oxalic acid solution which bleaches the brown color left by the potassium permanganate. The oxalic
acid is followed by an iron alum which impregnates the fibers and forms complexes with the aldehyde groups. Following the iron
alum, ammoniacal silver is added which replaces the complexed iron. The silver is reduced to a black precipitate by exposure to
10% neutral buffered formalin, resulting in metallic silver impregnation of the fibers. Gold chloride and sodium thiosulfate are
then used to tone the color of the fibers and remove excess silver, respectively.
Expected results
• Reticular fibers — black
• Collagen — gray
• Nuclei/background — red to pink
Figure 1. Tonsil stained with Retic stain Figure 2. Liver stained with Retic stain demonstrating continuous fine
reticular meshwork around hepatic cords in the perisinusoidal space.
61. 61
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Reticulum
Stain basics
Figure 3. Liver biopsy stained with Retic stain demonstrating reticular
fiber network.
Figure 4. Bone marrow trephine stained with Retic stain demonstrating
periendosteal reticular fibers
Figure 5. Normal spleen stained with Retic stain demonstrating the
reticular fiber network of the normal splenic architecture
Common diagnostic utility
Reticular fibers composed mainly of type III collagen form
a type of connective tissue called reticulin. It is made up
of fine fibers cross-linked to form a meshwork.4
It acts as
support system in soft tissue organs such as the spleen,
lymph nodes and tonsils, liver and bone marrow.5
Reticulum
stain may be helpful in the identification of changes in the
reticular structure in certain disease processes such as
primary hepatocellular carcinoma and liver cirrhosis. It may
also be used in the diagnosis of diseases involving the bone
marrow. Reticular fibers in the bone marrow are formed by
fibroblasts and are normally few — mainly perivascular and
periendosteal. They may be increased or reduced in many
bone marrow disease conditions. The reticulin stain has even
been helpful in identifying Cryptococcus fungus in bone
biopsies.6
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents. Ideally, it should be representative of
the tissues it is usually used to diagnose.3
An example of a
positive control material would be formalin-fixed, paraffin-
embedded human tissue with defined reticular fibers such as
liver, spleen, kidney or lymph nodes.2
62. 62
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Technical notes
1. Section thickness may affect quality and intensity of
staining. Cut sections, usually 3–5 μm, and pick the
sections up on glass slides.
References
1. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology, 2nd edition. St. Louis, MO: C.V. Mosby
Company; 1980:181-188.
2. Carson F, Hladik C. Histotechnology: A Self Instructional
Text 3rd edition. Hong Kong: American Society for Clinical
Pathology Press; 2009.
3. Clinical and Laboratory Standards Institute (CLSI). CLSI
Web site. http://www.clsi.org/. Accessed November 3,
2011.
4. Strum, Judy M.; Gartner, Leslie P.; Hiatt, James L. (2007).
Cell Biology and Histology. Hagerstwon, MD: Lippincott
Williams & Wilkins. p. 83. ISBN 0-7817-8577-4.
5. Burkitt; et al. (1993). Wheater’s Functional Histology (3rd
ed.). New York: Churchill Livinstone. p. 62. ISBN 0-443-
04691-3.
6. Jasmina Ahluwalia, Gurjeewan Garewal, Reena Das, Kim
Vaiphei. The reticulin stain in bone marrow biopsies –
beyond marrow fibrosis. British Journal of Haematology,
Volume 123, Issue 3, page 379, November-I 2003
Reticulum
Technical notes and references
63. 63
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Tonsil stained with Reticulum stain
64. 64
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Steiner
Stain basics
Purpose
Steiner stain is a qualitative histologic stain used to study specific argyrophilic microorganisms in formalin-fixed, paraffin-
embedded tissue.1
Staining principle
The ability to visualize organisms in tissue is important in the diagnosis of many diseases: however the stains routinely used
(Gram, PAS, GMS, AFB and others) are ineffective for many organisms. Silver impregnation techniques are successful in
demonstrating several of these organisms. These techniques have been reviewed by Garvey.5
The staining reaction is based on
the impregnation of microorganisms with silver nitrate and the reduction of silver ions to metallic silver by hydroquinone.2
The
microorganisms are demonstrated using a sensitizer that enables the uptake of the silver faster than the surrounding tissue.
Silver nitrate impregnates the microorganisms. The sections are exposed to the developer, which allows the silver ions to be
reduced to black metallic silver and other tissue elements to a golden yellow to tan color.
Expected results
• Organism— black Cytoplasm - pale pink
• Background — yellow/amber
Figure 1. Gastric Biopsy positive for H. pylori, 400x. Figure 2. Gastric biopsy H. pylori, 400x.
65. 65
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Steiner
Stain basics
Figure 3. Organisms stained black with Steiner stain in Legionnaire’s
disease infected tissue control, 600x.
Figure 4. Spirochetes organisms stained black with Steiner stain in
lung, 400x.
Figure 5. Cat scratch organisms stained black with Steiner stain in
infected tissue control, 400x.
Common diagnostic utility
Steiner stain may be used as a qualitative histologic silver
stain to aide in the identification of the causative organisms
of diseases such as syphilis, some gastric ulcers (H. pylori),
Lyme disease, Legionnaire’s disease, cat scratch fever and
others in formalin fixed, paraffin embedded tissue. 1,5
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents.3
Ideally, it should be representative of
the tissues it is usually used to diagnose.4
An example of a
positive control material would be formalin-fixed, paraffin-
embedded human tissue with Helicobacter pylori organisms
in gastric ulcer, or other tissue samples known to be positive
for organisms suitable for staining with Steiner.
66. 66
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Technical notes
1. Section thickness may affect quality and intensity of
staining. Cut sections, usually 3–5 μm, and pick the
sections up on glass slides.
2. When staining for microorganisms, it is important to ensure
that the water bath is scrupulously clean prior to sectioning in
order to prevent introduction of extraneous microorganisms
onto the specimen section slide. It is recommended not to use
water left standing overnight.
References
1. Lillie RD, Editor. H.J. Conn’s Biological Stains, 9th ed.
Lippincott Williams and Wilkins Company, Baltimore, 1977.
2. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology, 2nd Edition. C.V. Mosby Company, St.
Louis, 1980, p 190.
3. NCCLS documents can be obtained from NCCLS, 940
West Valley Road, Suite 1400, Wayne, PA19087-1898, or
through the web site www.nccls.org.
4. Carson FL. Histotechnology: A Self Instructional Text, 2nd
Edition. ASCP Press, Chicago, 1996.
5. Winsome Garvey, Silver Impregnation Techniques to
Identify Spirochetes and Other Bacteria. The Journal
Histotechnology. Sept 1996;19(3):203-209.
Steiner
Technical notes and references
67. 67
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 6. Gastric Biopsy positive for H. Pylori with Steiner stain, 400x.
68. 68
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Trichrome (Masson)
Stain basics
Figure 1. Kidney stained with Trichrome Blue, 200x. Figure 2. Liver stained with Trichrome Blue, 200x.
Expected results
• Nuclei — varying shades of black/gray
• Red blood cells — vibrant dark red
• Muscle — vibrant medium red
• Cytoplasm — medium shade of muted red
• Collagen — blue
Purpose
Trichrome stains are used to differentiate collagen from muscle tissue.1
Implicit in its name: the Trichrome stain uses three
colored dyes to selectively stain certain tissue components. The first color is from the black of Weigert’s iron hematoxylin
which is used to stain the nuclei. The second dye is a red acidic dye that colors the muscle cells and the cytoplasm of liver
cells, among other tissue components. The final color is a blue or green dye which is used to stain the connective tissue and
collagen.
69. 69
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Trichrome Blue
Stain basics
Staining principle
The first trichrome stain has been attributed to Mallory.1-3
It
used a solution of acid fuchsin to stain the nuclei and muscle
red, followed by a mordant (phosphomolybdic acid), and
finally a solution of Orange G and Methylene Blue to stain
erythrocytes orange and collagen blue. Modifications which
include a nuclear stain were introduced by Masson and
Gomori, and by Lillie.3
Weigert’s iron hematoxylin is used the
nuclear stain with all three modifications due to its ability
to withstand decolorization by the subsequent acid dyes.
Masson Trichrome is a multi-step trichrome stain in that the
plasma stain and the collagen stain are applied sequentially.
In Gomori’s modification, the plasma stain dye(s) and the
collagen stain dye(s) are combined and applied in a single-
step.
It is thought that Trichrome stains function based on the
principles of acid-base chemistry and dye displacement,
using the permeability and affinity of the various tissue
components for the different acid dyes to produce differential
staining of the selective tissue components.4
In the Masson Trichrome, the nuclear stain from the iron
hematoxylin is followed by staining with a red acid dye and
solution, which is used to ultimately stain the muscle and
cytoplasmic tissue components. This sometimes referred to
as the plasma stain. The plasma stain is usually made up of
one or more of the following dyes — Acid Fuchsin, Ponceau
de Xylidine and Biebrich Scarlet - in glacial acetic acid and
distilled water.
The excess red dye is washed off with a rinse in water and
is followed by “negative” staining with a polyacid; typically
phosphotungstic or phosphomolybdic acid. Although
this mechanism is not well understood, it thought that the
polyacid binds preferentially to various tissue components,
displacing the red dye. Some tissue structures retain the red
dye more strongly than others and resist decolorization with
the polyacid. In descending order, the following components
tend to resist the removal or substitution of the red dye by
phosphomolybdic or phosphotungstic acid: erythrocytes,
eosinophil granules, keratin, fibrin, muscle, cytoplasm, bone
and tendon, collagen and areolar connective tissue.4
The plasma stain is followed by the collagen (fiber) stain,
which is usually a green dye (such as Fast Green) or blue dye
(such as Aniline Blue) in a weak acetic acid solution. The fiber
stain will more easily displace the polyacid before it displaces
the plasma stain. The excess fiber stain is rinsed with a weak
acetic acid solution. This serves to accentuate the color
balance between the plasma stain and the fiber stain.
70. 70
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 3. In liver, the cytoplasm of the hepatocytes, the smooth muscle
component of the vessel walls, and the red blood cells should stain red
in increasing intensity. The collagen component of the liver triad, a small
amount of collagen in the portal tracts, and a small rim of collagen in the
luminal rim of the hepatic venules should stain blue.2
200x.
Figure 4. In kidney, the cytoplasm of the cells in the tubules, the smooth
muscle component of the vessel walls, and the red blood cells should stain
red in increasing intensity. The collagen in between the tubules, as well as
in the glomerular basement membrane should stain blue. 200x.
Figure 5. In muscle, the cytoplasm of the muscle cells should stain red
with very clear striations. The smooth muscle components of the vessel
walls and the red blood cells should stain red in increasing intensity. The
collagen in between the myocytes and the connective tissue structures
should stain blue. 200x.
Common diagnostic utility
Trichrome stains are useful for indicating fibrotic change; that
is, an increase in collagen like that which occurs in cirrhosis of
the liver and pyelonephritis. Trichrome stains can be useful for
distinguishing histologic changes that occur in neuromuscular
diseases. They are also useful for differentiating tumors
that originated in muscle cells from those that originated in
fibroblasts. Trichrome stains are included as standard practice
in diagnostic panels for renal, liver biopsies and muscle biopsies
(such as cardiac biopsies).
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents. An appropriate control tissue for the
Trichrome stain should contain collagen and smooth muscle,
such as colon, liver, esophagus or skin. Ideally, it should be
representative of the tissues it is usually used to diagnose.
The most common tissue controls are (normal) kidney,
(normal) liver and (normal) muscle.
Trichrome Blue
Stain basics
71. 71
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Technical Note
1. 10% Neutral Buffered Formalin is not the ideal fixative for
trichrome staining as it does not confer the optimal acid/
base properties to the tissue components. For this reason,
Bouin’s is applied to tissue sections as an online secondary
fixative to intensify the final coloration. If the original
fixation of the tissue was especially problematic, a Bouin’s
pretreatment is recommended.
2. Tissue section thickness is important and may affect
quality and intensity of staining. Sections cut at 5-6
microns hold the colored dyes much better than thin (2-3
micron) sections. Since renal (kidney) biopsies and liver
biopsies must be cut very thin in order to provide better
diagnostic clarity, they may stain light & pale compared to
thicker sections.
3. Trichrome Mordant is a critical factor in achieving staining
balance between the plasma stain and the fiber stain.
Reducing Trichrome Mordant time will leave more red dye
and reduce the uptake of the blue dye. Conversely, increasing
Trichrome Mordant time will differentiate the red dye and
increase the uptake of the blue dye.
4. Some tissue displays a reddish cast in the cell nucleus. This
usually stains dark brown-black with Iron Hematoxylin.
Additionally, some tissues, such as glandular epithelium
(secretory) in the uterus and in the G.I. tract can stain
decidedly reddish.
References
1. Lillie RD, Editor. H.J. Conn’s Biological Stains, 9th ed.
Lippincott Williams and Wilkins Company, Baltimore, 1977.
2. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology, 2nd Edition. C.V. Mosby Company, St.
Louis, p. 190, 1980.
3. Lillie RD. Further experiments with the Masson trichrome
modification of Mallory’s connective tissue stain. Stain
Technol 15: 82, 1940.
4. Differential Staining With Acid Dyes. Bryan D. Llewellyn.
A presentation to the Queensland Histology Group at
Caloundra, Queensland, Australia, May 2008.
5. Stephen A. Geller, Lydia M. Petrovic – Biopsy Interpretation
of the Liver, Second edition
Trichrome Blue
Technical notes and references
72. 72
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Trichrome Green
Stain basics
Purpose
Trichrome stains are used to differentiate collagen from muscle tissue.1
Implicit in its name, the Trichrome stain uses three
colored dyes to selectively stain certain tissue components. The first color is from the black of Weigert’s iron hematoxylin which
is used to stain the nuclei. The second dye is a red acidic dye that colors the muscle cells and the cytoplasm of liver cells, among
other tissue components. The final color is a blue or green dye which is used to stain the connective tissue and collagen.
Figure 1. Liver stained with Trichrome Green, 200x. Figure 2 . Liver stained with Trichrome Green, 200x.
Expected results
• Nuclei — varying shades of black/gray
• Red blood cells — vibrant dark red
• Muscle — vibrant medium red
• Cytoplasm — medium shade of muted red
• Collagen — green
73. 73
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Staining principle
The first trichrome stain has been attributed to Mallory.1-3
It
used a solution of acid fuchsin to stain the nuclei and muscle
red, followed by a mordant (phosphomolybdic acid), and
finally a solution of Orange G and Methylene Blue to stain
erythrocytes orange and collagen blue. Modifications which
include a nuclear stain were introduced by Masson and
Gomori, and by Lillie.3
Weigert’s iron hematoxylin is used as
the nuclear stain with all three modifications due to its ability
to withstand decolorization by the subsequent acid dyes.
Masson Trichrome is a multi-step trichrome stain in that the
plasma stain and the collagen stain are applied sequentially.
In Gomori’s modification, the plasma stain dye(s) and the
collagen stain dye(s) are combined and applied in a single-
step.
It is thought that Trichrome, stains function based on the
principles of acid-base chemistry and dye displacement,
using the permeability and affinity of the various tissue
components for the different acid dyes to produce differential
staining of the selective tissue components.4
In the Masson Trichrome the nuclear stain from the iron
hematoxylin is followed by staining with a red acid dye
solution, which is used to ultimately stain the muscle and
cytoplasmic tissue components. This sometimes referred to
as the plasma stain. The plasma stain is usually made up of
one or more of the following dyes — Acid Fuchsin, Ponceau
de Xylidine and Biebrich Scarlet - in glacial acetic acid and
distilled water.
The excess red dye is washed off with a rinse in water and
is followed by “negative” staining with a polyacid, typically
phosphotungstic or phosphomolybdic acid. Although
this mechanism is not well understood, it thought that the
polyacid binds preferentially to various tissue components,
displacing the red dye. Some tissue structures retain the red
dye more strongly than others and resist decolorization with
the polyacid. In descending order, the following components
tend to resist the removal or substitution of the red dye by
phosphomolybdic or phosphotungstic acid: Erythrocytes,
eosinophil granules, keratin, fibrin, muscle, cytoplasm, bone
and tendon, collagen and areolar connective tissue.4
The plasma stain is followed by the collagen (fiber) stain,
which is usually a green dye (such as Fast Green) or blue dye
(such as Aniline Blue) in a weak acetic acid solution. The fiber
stain will more easily displace the polyacid before it displaces
the plasma stain. The excess fiber stain is rinsed with a weak
acetic acid solution. This serves to accentuate the color
balance between the plasma stain and the fiber stain.
Trichrome Green
Stain basics
74. 74
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Figure 3. In liver, the cytoplasm of the hepatocytes, the smooth muscle
component of the vessel walls and the red blood cells should stain red
in increasing intensity. The collagen component of the liver triad a small
amount of collagen in the portal tracts, and a small rim of collagen in the
luminal rim of the hepatic venules should stain green.2
200x.
Figure 4. In kidney, the cytoplasm of the cells in the tubules, the smooth
muscle component of the vessel walls, and the red blood cells should stain
red in increasing intensity. The collagen in between the tubules, as well as
in the glomerular basement membrane, should stain green. 200x.
Figure 5. In muscle, the cytoplasm of the muscle cells should stain red
with very clear striations. The smooth muscle components of the vessel
walls and the red blood cells should stain red in increasing intensity. The
collagen in between the myocytes and the connective tissue structures
should stain green. 200x.
Common diagnostic utility
Trichrome stains are useful for indicating fibrotic change; that
is, an increase in collagen like that which occurs in cirrhosis of
the liver and pyelonephritis. Trichrome stains can be useful for
distinguishing histologic changes that occur in neuromuscular
diseases. They are also useful for differentiating tumors
that originated in muscle cells from those that originated in
fibroblasts. Trichrome stains are included as standard practice
in diagnostic panels for renal, liver biopsies and muscle biopsies
(such as cardiac biopsies).
Tissue controls
A known positive tissue control should be utilized for
monitoring the correct performance of processed tissues
and test reagents. An appropriate control tissue for the
Trichrome stain should contain collagen and smooth muscle,
such as colon, liver, esophagus or skin. Ideally, it should be
representative of the tissues it is usually used to diagnose.
The most common tissue controls are (normal) kidney,
(normal) liver and (normal) muscle.
Trichrome Green
Stain basics
75. 75
This field guide is intended to be an educational supplement, not a substitute for product labeling.
Refer to the package insert and operator manual for primary information regarding your special stains kits and instrument operation.
Trichrome Green
Technical notes and references
Technical notes
1. 10% Neutral Buffered Formalin is not the ideal fixative for
trichrome staining as it does not confer the optimal acid/
base properties to the tissue components. For this reason,
Bouin’s is applied to tissue sections as an online secondary
fixative to intensify the final coloration. If the original
fixation of the tissue was especially problematic and the
online fixation in Bouin’s is insufficient, off-line Bouin’s
pretreatment is recommended. It is recommended that the
Bouin’s should be preheated for 15 minutes at 60°C. Once
the slides are added to the Bouin’s reagent, incubate for
another 1 hour at 60°C.
2. Tissue section thickness is important and may affect
quality and intensity of staining. Sections cut at 5-6
microns hold the colored dyes much better than thin (2-3
micron) sections. Since renal (kidney) biopsies and liver
biopsies must be cut very thin in order to provide better
diagnostic clarity, they may stain light and pale compared
to thicker sections.
3. Trichrome Mordant is a critical factor in achieving staining
balance between the plasma stain and the fiber stain.
Reducing Trichrome Mordant time will leave more red
dye and reduce the uptake of the green dye. Conversely,
increasing Trichrome Mordant time will differentiate the
red dye and increase the uptake of the green dye.
4. Some tissue displays a reddish cast in the cell nucleus. This
usually stains dark brown-black with Iron Hematoxylin.
Additionally, some tissues, such as glandular epithelium
(secretory) in the uterus and in the G.I. tract, can stain
decidedly reddish.
References
1. Lillie RD, Editor. H.J. Conn’s Biological Stains, 9th ed.
Lippincott Williams and Wilkins Company, Baltimore, 1977.
2. Sheehan DC, Hrapchak BB. Theory and Practice of
Histotechnology, 2nd Edition. C.V. Mosby Company, St.
Louis, p. 190, 1980.
3. Lillie RD. Further experiments with the Masson trichrome
modification of Mallory’s connective tissue stain. Stain
Technol 15: 82, 1940.
4. Differential Staining With Acid Dyes. Bryan D. Llewellyn.
A presentation to the Queensland Histology Group at
Caloundra, Queensland, Australia, May 2008.
5. Stephen A. Geller, Lydia M. Petrovic – Biopsy Interpretation
of the Liver, Second edition