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TISSUE PROCESSING
DR. UMME KULSUM MUNMUN
ASSISTANT PROFESSOR
DEPARTMENT OF PATHOLOGY
CHANDPUR MEDICAL COLLEGE
TISSUE PROCESSING
• Tissue processing is defined as the process of
preparing the tissue by - embedding it in a solid
medium that is firm enough to enable thin
cutting
• And soft enough to enable the knife to cut the
sections with little damage to the knife or the
tissue
• Tissue for study can be obtained from 1) Biopsies
and 2) Autopsies
TYPES OF BIOPSY
• Excisional biopsy
• Core / true cut biopsy
• Punch biopsy etc
STAGES OF TISSUE PROCESSING
• To fill up the requisition form properly
• Fixation
• Dehydration
• Clearing
• Impregnation
• Embedding
• Section cutting
• Staining
• Mounting
• Specimen is received with a requisition form with
adequate information regarding –
- Patient information
- Relevant clinical data
- Surgical findings, name of operation, name of
tissue
• Must be received in 10% formalin solution
• The specimens are given a number for
identification
GROSS EXAMINATION
• Describing the specimen and placing all or parts
of it into a small plastic cassette
• The cassettes are placed into a fixative
FIXATION
• Specimen received in pathology laboratory is first
adequately fixed
• Fixation is the process by which specimen is
treated with an appropriate fixative for a
particular period of time in order to preserve
tissue as in life like state as possible
• The most commonly used fixative in
histopathology laboratory is 10% formalin
• Some other fixatives: gluteraldehyde, acetic
acid, Carnoy’s fixative, Clarke’s fixative etc.
PREPARATION OF 10% FORMALIN
• Formalin is prepared by dissolving 40%
formaldehyde gas in 100 ml of distilled water
• The resultant mixture is 100% formalin
• Routinely 10% formalin is used
• 10% formalin is prepared by mixing 10 ml of
100% formalin in 90 ml of distilled water
• It forms cross links between amino acids of
protein thereby make them insoluble
DECALCIFICATION
• Is the process of removing calcium salts from the
specimen
• Done for bony specimen
• Decalcifying agents:
- Nitric acid
- hydrochloric acid
- formic acid etc
DEHYDRATION
• It is the process by which the water content in
the tissue is reduced by passing the specimen
through increasing concentrations of dehydrating
agents
• The most commonly used dehydrating agent is
ethanol
DEHYDRATION
• 70% alcohol – 1 hour
• 80% alcohol – 1 hour
• 95 % alcohol – 1 hour
• Absolute alcohol – 1 hour
• Absolute alcohol – 1 hour
• Absolute alcohol – 1 hour
CLEARING
• It is the process by which alcohol in tissue is
removed which will facilitate the paraffin wax to
be impregnated in tissue
• Commonly used clearing agent: Xylene
IMPREGNATION
• Permeating the tissue with a supporting medium
is called impregnation
• Liquid paraffin is usually used for impregnation
• Paraffin impregnation is usually carried out in a
hot air oven at 52-56 ° C
EMBEDDING
• Placing the tissue which has been cleared of
alcohol to a metallic mould filled with molten
wax
• After that it is allowed to cool and solidify
• After solidification a wax block is prepared which
is ready for cutting sections
SECTIONING
• Paraffin blocks are fixed in the microtome
machine to be sectioned and thin strips of
varying thickness are prepared
• Commonly used microtome machine: Rotary
microtome
STAINING
• Routinely used stain in histopathology laboratory
:
Hematoxillin & eosin stain
Hematoxillin (basic stain) : stains acidic structure
(nucleus): deep blue or purple
Eosin (acidic stain) : stains basic structures
(cytoplasm) : pink
SPECIAL STAIN
• Special stains are used to identify certain normal
and abnormal substances present in the cells and
tissue which cannot be identified on routine H&E
stain
PERIODIC ACID SCHIFF (PAS
STAIN)
• To demonsrate glycogen (glycogen storage
disease) and neutral mucoprotein
• To differentiate poorly differentiated
adenocarcinoma
• To demonstrate basement membrane
• To demonstrate fungi
PAS
PAS
• Mucicarmine, Alcian blue (stains mucin)
• Reticulin fibres : reticulin fibres
• Masson trichrome stain: fibrosis
• Congo red, crystal violet: amyloid – brick red in Congo-red
or Apple green birefringence on polarized microscope
• Oil red O, sudan black B: lipid
• Masson Fontana: melanin
• Von kossa: calcium
• Perl’s Prussian blue: iron
MASSON TRICHROME
STAINS FOR MICROORGANISM
• Ziehl Neelsen stain : Mycobacteria bacilli - red
• Fite Faraco / Modified Ziehl Neelsen stain : Lepra
bacilli
• Gomori methenamime silver stain : fungus
• Giemsa stain : H. Pylori
• Gram staining
ZN STAIN
FITE FARACO
GIEMSA H. PYLORI
FROZEN SECTION
• Pathologic procedure to perform rapid
microscopic analysis of specimen
• Fresh specimen is received
• Cryo-section procedure
• Produces sections without dehydrating, clearing
agents and embedding media
• Section is made in cryostat machine
• Rapid intra-operative diagnosis : malignancy,
margin clearance etc
AUTOPSY
• Medical procedure to determine the cause and
manner of death and to evaluate any disease or
injury in the dead body
• Usually performed by a pathologist
AUTOPSY
• Forensic – medico-legal purpose
• Clinical / academic
CYTOPATHOLOGY
• Abrasive - Pap’s smear , bronchial brushing
• Exfoliative – naturally shedded body fluid , ex.
Sputum, urine, plural fluid, ascitic fluid
• Imprint cytology – during frozen section , bone
marrow biopsy, core biopsy procedure, an
imprint of the specimen is done
• FNAC: routine: superficially palpable lump:
breast, thyroid, lymph node
• Guided: USG guided FNAC, CT guided FNAC
• Common fixative in cytopathology: 95% Ehanol
• Stain used in cytopathology, Papanicolaou stain,
H&E stain
• Routine stain in preparation of PBF: leishman
stain
THANK YOU

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Tissue Processing.pptx

  • 1. TISSUE PROCESSING DR. UMME KULSUM MUNMUN ASSISTANT PROFESSOR DEPARTMENT OF PATHOLOGY CHANDPUR MEDICAL COLLEGE
  • 2. TISSUE PROCESSING • Tissue processing is defined as the process of preparing the tissue by - embedding it in a solid medium that is firm enough to enable thin cutting • And soft enough to enable the knife to cut the sections with little damage to the knife or the tissue • Tissue for study can be obtained from 1) Biopsies and 2) Autopsies
  • 3. TYPES OF BIOPSY • Excisional biopsy • Core / true cut biopsy • Punch biopsy etc
  • 4. STAGES OF TISSUE PROCESSING • To fill up the requisition form properly • Fixation • Dehydration • Clearing • Impregnation • Embedding • Section cutting • Staining • Mounting
  • 5. • Specimen is received with a requisition form with adequate information regarding – - Patient information - Relevant clinical data - Surgical findings, name of operation, name of tissue • Must be received in 10% formalin solution • The specimens are given a number for identification
  • 6. GROSS EXAMINATION • Describing the specimen and placing all or parts of it into a small plastic cassette • The cassettes are placed into a fixative
  • 7.
  • 8. FIXATION • Specimen received in pathology laboratory is first adequately fixed • Fixation is the process by which specimen is treated with an appropriate fixative for a particular period of time in order to preserve tissue as in life like state as possible • The most commonly used fixative in histopathology laboratory is 10% formalin • Some other fixatives: gluteraldehyde, acetic acid, Carnoy’s fixative, Clarke’s fixative etc.
  • 9. PREPARATION OF 10% FORMALIN • Formalin is prepared by dissolving 40% formaldehyde gas in 100 ml of distilled water • The resultant mixture is 100% formalin • Routinely 10% formalin is used • 10% formalin is prepared by mixing 10 ml of 100% formalin in 90 ml of distilled water • It forms cross links between amino acids of protein thereby make them insoluble
  • 10. DECALCIFICATION • Is the process of removing calcium salts from the specimen • Done for bony specimen • Decalcifying agents: - Nitric acid - hydrochloric acid - formic acid etc
  • 11. DEHYDRATION • It is the process by which the water content in the tissue is reduced by passing the specimen through increasing concentrations of dehydrating agents • The most commonly used dehydrating agent is ethanol
  • 12. DEHYDRATION • 70% alcohol – 1 hour • 80% alcohol – 1 hour • 95 % alcohol – 1 hour • Absolute alcohol – 1 hour • Absolute alcohol – 1 hour • Absolute alcohol – 1 hour
  • 13. CLEARING • It is the process by which alcohol in tissue is removed which will facilitate the paraffin wax to be impregnated in tissue • Commonly used clearing agent: Xylene
  • 14. IMPREGNATION • Permeating the tissue with a supporting medium is called impregnation • Liquid paraffin is usually used for impregnation • Paraffin impregnation is usually carried out in a hot air oven at 52-56 ° C
  • 15. EMBEDDING • Placing the tissue which has been cleared of alcohol to a metallic mould filled with molten wax • After that it is allowed to cool and solidify • After solidification a wax block is prepared which is ready for cutting sections
  • 16.
  • 17.
  • 18. SECTIONING • Paraffin blocks are fixed in the microtome machine to be sectioned and thin strips of varying thickness are prepared • Commonly used microtome machine: Rotary microtome
  • 19.
  • 20.
  • 21. STAINING • Routinely used stain in histopathology laboratory : Hematoxillin & eosin stain Hematoxillin (basic stain) : stains acidic structure (nucleus): deep blue or purple Eosin (acidic stain) : stains basic structures (cytoplasm) : pink
  • 22.
  • 23. SPECIAL STAIN • Special stains are used to identify certain normal and abnormal substances present in the cells and tissue which cannot be identified on routine H&E stain
  • 24. PERIODIC ACID SCHIFF (PAS STAIN) • To demonsrate glycogen (glycogen storage disease) and neutral mucoprotein • To differentiate poorly differentiated adenocarcinoma • To demonstrate basement membrane • To demonstrate fungi
  • 25. PAS
  • 26. PAS
  • 27. • Mucicarmine, Alcian blue (stains mucin) • Reticulin fibres : reticulin fibres • Masson trichrome stain: fibrosis • Congo red, crystal violet: amyloid – brick red in Congo-red or Apple green birefringence on polarized microscope • Oil red O, sudan black B: lipid • Masson Fontana: melanin • Von kossa: calcium • Perl’s Prussian blue: iron
  • 29. STAINS FOR MICROORGANISM • Ziehl Neelsen stain : Mycobacteria bacilli - red • Fite Faraco / Modified Ziehl Neelsen stain : Lepra bacilli • Gomori methenamime silver stain : fungus • Giemsa stain : H. Pylori • Gram staining
  • 33. FROZEN SECTION • Pathologic procedure to perform rapid microscopic analysis of specimen • Fresh specimen is received • Cryo-section procedure • Produces sections without dehydrating, clearing agents and embedding media • Section is made in cryostat machine • Rapid intra-operative diagnosis : malignancy, margin clearance etc
  • 34. AUTOPSY • Medical procedure to determine the cause and manner of death and to evaluate any disease or injury in the dead body • Usually performed by a pathologist
  • 35. AUTOPSY • Forensic – medico-legal purpose • Clinical / academic
  • 36. CYTOPATHOLOGY • Abrasive - Pap’s smear , bronchial brushing • Exfoliative – naturally shedded body fluid , ex. Sputum, urine, plural fluid, ascitic fluid • Imprint cytology – during frozen section , bone marrow biopsy, core biopsy procedure, an imprint of the specimen is done • FNAC: routine: superficially palpable lump: breast, thyroid, lymph node • Guided: USG guided FNAC, CT guided FNAC
  • 37.
  • 38.
  • 39.
  • 40.
  • 41. • Common fixative in cytopathology: 95% Ehanol • Stain used in cytopathology, Papanicolaou stain, H&E stain • Routine stain in preparation of PBF: leishman stain