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HISTOPATHOLOGY
PROCEDURES
Prepared by: Anish Dhakal (Aryan)
DEFINITIONS
• Histology: Study of normal tissue at microscopic level
• Histopathology: Examination of tissues for presence or
absence of changes in their structure due to disease
processes.
Fixation
Method of preserving cells and tissues from decomposition
in life-like conditions as far as possible.
The aim of fixation is:
1. To preserve the tissue in as life like manner as possible.
2. To prevent postmortem changes like autolysis and putrefaction.
3.To preserve cells of chemical compounds so that further histochemistry
is possible (cell insensitive to hypotonic or hypertonic solutions)
4. To harden the specimen so that easy manipulation of soft tissues is
possible
5. Acts as mordant and induces optical contrast
IDEAL FIXATIVE
i. It should be cheap and easily available.
ii. It should be stable and safe to handle.
iii. It should be rapid in action.
iv. It should cause minimal loss of tissue.
v. It should not bind to the reactive groups in tissue which
are meant for dyes.
vi. It should give even penetration.
vii. It should retain normal colour of the tissue.
viii. It should not impart its own colour to the tissue.
• Tissue specimen should be placed in a container with
fixative immediately after removal to prevent drying and
autolysis
• The tissue should be fully immersed in fixative
• Tissue should be kept for adequate time. No refrigeration is
needed.
• Large masses fix optimally if incised or sectioned,
although this might compromise assessment of margins.
FORMALIN
• Saturated solution of formaldehyde in gas (40% by w/v)
• 10% formalin is used for routine fixation
• Acts by polymerization of cellular proteins forming
methylene bridges
• Merits of formalin:
Rapidly penetrates the tissues
Normal colour of tissues is retained
Cheap and easily available
Best fixative for neurological tissue
• Demerits of formalin:
Causes excessive hardening of tissues.
Causes irritation of skin, mucous membranes and
conjunctiva.
Leads to formation of formalin pigment in tissues having
excessive blood at an acidic pH which can be
by treatment of section with alcoholic picric
acid.
OTHER FIXATIVES
Glutaraldehyde Electron microscopy
Expensive
Penetrates tissues slowly
Bouin’s fluid (Picric acid) Renal & testicular needle biopsies
Stains tissue yellow, Glycogen
Makes tissues harder & brittle
Causes lysis of RBCs
Carnoy’s fixative (Alcohol) Cytological smears and endometrial
curettings
Good fixative for glycogen
Dissolves fat
Osmium tetraoxide CNS tissues
Electron microscopy
Good fixative for lipids
Imparts black colour to tissues
DEHYDRATION
• Process in which water from cells and tissues is removed – so
wax can take subsequent space.
• Passing series ascending grades of alcohol – 70%, 80%, 95%
and absolute alcohol
• Alternative of ethyl alcohol – methyl alcohol, isopropyl
alcohol or acetone
CLEARING
• process in which alcohol from tissues and cells is removed
and replaced by a fluid which is miscible with wax making
tissue transparent
• Xylene – commonly used clearing agent
• Other – toluene, benzene( carcinogenic), chloroform, cedar
wood (expensive and very viscous)
IMPREGNATION
• Process in which empty spaces in the tissue and cells after
removal of water are taken up by paraffin wax
• Hardening of tissue – helps in section cutting
• Done by molten paraffin wax of melting point 54-62°C
TISSUE PROCESSOR
• 12 chambered automated device
• 10 stations are steel/glass jars and two are
thermostatically controlled wax bath
For fixation in formalin: 1 jar.
 For dehydration in ascending grades of
alcohol: 6 jars, one each of 70%, 80%, 90%
and 3 for 100%.
For clearing in xylene: 3 jars.
For impregnation in molten paraffin wax: 2
wax baths.
• Tissues move automatically from one jar to next after
scheduled time, usually 1.5 hours in each jar
• Closed(Vacuum) Tissue Processor:
Tissues cassettes are placed in a single container
Processing fluids are moved in and out sequentially
according to electronically programmed cycle
No hazard of contamination by toxic fumes unlike in open
system
EMBEDDING AND
BLOCKING
• Embedding is done by molten wax
• Conventionally prepared using metallic L(Leuckhart’s)
moulds. Plastic moulds are available
• The moulds are placed over smooth surfaced glass tile
• Molten wax is pored into the cavity and allowed to solidify
• If L-moulds are used they are removed while plastic moulds
remain with the wax block carrying the tissue piece
• Can be performed in device – embedding center
• After embedding the tissue sections are available in block for
microtomy
MICROTOMY (SECTION
CUTTING)
• Microtome – equipment for cutting section
• 5 types
• Rotary (Commonly Used)
• Sliding
• Freezing
• Rocking
• Base-sledge
• Cut section by adjusting thickness 3-4 µm and picked from
knife by help of forceps and camel hair brush
• Water bath at 40-45°C then place on clean slide at 56°C
for 20-30 mins  fishing
• Coating adhesives for section like egg albumin and gelatin
can be used before hematoxylin and eosin stain
STAINING
• Sections are deparaffinised by placing in jar of xylene
for 10-15 minutes
• Sections are then rehydrated by passing through series
of descending grades of alcohol and finally to water
• Then, place slide in haematoxylin for 8-10 minutes
followed by ringing with water and differentiation
(excess dye removed by putting in 1% acid alcohol for
10 seconds)
• Blueing is done by putting section in sodium bicarbonate
and magnesium sulphate or saturated solution of lithium
carbonate for 2-10 minutes
• Counterstain with 1% aqueous eosin for 0.5-1 minute and
dip in tap water
• Sections are then dehydrated passing through a series of
ascending grades of alcohol and finally cleared in xylene, 2-3
dips in each solution
• Mount in DPX (Dextrene Polystyrene Xylene)
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Histopathology Procedures

  • 2. DEFINITIONS • Histology: Study of normal tissue at microscopic level • Histopathology: Examination of tissues for presence or absence of changes in their structure due to disease processes.
  • 3.
  • 4. Fixation Method of preserving cells and tissues from decomposition in life-like conditions as far as possible. The aim of fixation is: 1. To preserve the tissue in as life like manner as possible. 2. To prevent postmortem changes like autolysis and putrefaction. 3.To preserve cells of chemical compounds so that further histochemistry is possible (cell insensitive to hypotonic or hypertonic solutions) 4. To harden the specimen so that easy manipulation of soft tissues is possible 5. Acts as mordant and induces optical contrast
  • 5. IDEAL FIXATIVE i. It should be cheap and easily available. ii. It should be stable and safe to handle. iii. It should be rapid in action. iv. It should cause minimal loss of tissue. v. It should not bind to the reactive groups in tissue which are meant for dyes. vi. It should give even penetration. vii. It should retain normal colour of the tissue. viii. It should not impart its own colour to the tissue.
  • 6. • Tissue specimen should be placed in a container with fixative immediately after removal to prevent drying and autolysis • The tissue should be fully immersed in fixative • Tissue should be kept for adequate time. No refrigeration is needed. • Large masses fix optimally if incised or sectioned, although this might compromise assessment of margins.
  • 7. FORMALIN • Saturated solution of formaldehyde in gas (40% by w/v) • 10% formalin is used for routine fixation • Acts by polymerization of cellular proteins forming methylene bridges • Merits of formalin: Rapidly penetrates the tissues Normal colour of tissues is retained Cheap and easily available Best fixative for neurological tissue
  • 8. • Demerits of formalin: Causes excessive hardening of tissues. Causes irritation of skin, mucous membranes and conjunctiva. Leads to formation of formalin pigment in tissues having excessive blood at an acidic pH which can be by treatment of section with alcoholic picric acid.
  • 9. OTHER FIXATIVES Glutaraldehyde Electron microscopy Expensive Penetrates tissues slowly Bouin’s fluid (Picric acid) Renal & testicular needle biopsies Stains tissue yellow, Glycogen Makes tissues harder & brittle Causes lysis of RBCs Carnoy’s fixative (Alcohol) Cytological smears and endometrial curettings Good fixative for glycogen Dissolves fat Osmium tetraoxide CNS tissues Electron microscopy Good fixative for lipids Imparts black colour to tissues
  • 10. DEHYDRATION • Process in which water from cells and tissues is removed – so wax can take subsequent space. • Passing series ascending grades of alcohol – 70%, 80%, 95% and absolute alcohol • Alternative of ethyl alcohol – methyl alcohol, isopropyl alcohol or acetone
  • 11. CLEARING • process in which alcohol from tissues and cells is removed and replaced by a fluid which is miscible with wax making tissue transparent • Xylene – commonly used clearing agent • Other – toluene, benzene( carcinogenic), chloroform, cedar wood (expensive and very viscous)
  • 12. IMPREGNATION • Process in which empty spaces in the tissue and cells after removal of water are taken up by paraffin wax • Hardening of tissue – helps in section cutting • Done by molten paraffin wax of melting point 54-62°C
  • 13. TISSUE PROCESSOR • 12 chambered automated device • 10 stations are steel/glass jars and two are thermostatically controlled wax bath For fixation in formalin: 1 jar.  For dehydration in ascending grades of alcohol: 6 jars, one each of 70%, 80%, 90% and 3 for 100%. For clearing in xylene: 3 jars. For impregnation in molten paraffin wax: 2 wax baths.
  • 14. • Tissues move automatically from one jar to next after scheduled time, usually 1.5 hours in each jar • Closed(Vacuum) Tissue Processor: Tissues cassettes are placed in a single container Processing fluids are moved in and out sequentially according to electronically programmed cycle No hazard of contamination by toxic fumes unlike in open system
  • 15. EMBEDDING AND BLOCKING • Embedding is done by molten wax • Conventionally prepared using metallic L(Leuckhart’s) moulds. Plastic moulds are available • The moulds are placed over smooth surfaced glass tile • Molten wax is pored into the cavity and allowed to solidify • If L-moulds are used they are removed while plastic moulds remain with the wax block carrying the tissue piece • Can be performed in device – embedding center • After embedding the tissue sections are available in block for microtomy
  • 16.
  • 17. MICROTOMY (SECTION CUTTING) • Microtome – equipment for cutting section • 5 types • Rotary (Commonly Used) • Sliding • Freezing • Rocking • Base-sledge • Cut section by adjusting thickness 3-4 µm and picked from knife by help of forceps and camel hair brush • Water bath at 40-45°C then place on clean slide at 56°C for 20-30 mins  fishing • Coating adhesives for section like egg albumin and gelatin can be used before hematoxylin and eosin stain
  • 18. STAINING • Sections are deparaffinised by placing in jar of xylene for 10-15 minutes • Sections are then rehydrated by passing through series of descending grades of alcohol and finally to water • Then, place slide in haematoxylin for 8-10 minutes followed by ringing with water and differentiation (excess dye removed by putting in 1% acid alcohol for 10 seconds)
  • 19. • Blueing is done by putting section in sodium bicarbonate and magnesium sulphate or saturated solution of lithium carbonate for 2-10 minutes • Counterstain with 1% aqueous eosin for 0.5-1 minute and dip in tap water • Sections are then dehydrated passing through a series of ascending grades of alcohol and finally cleared in xylene, 2-3 dips in each solution • Mount in DPX (Dextrene Polystyrene Xylene)
  • 20.