Histo. processes Flashcards

1
Q

Steps for preparing tissue for microscopic assesment (after surgical excision)

A
  1. Fixation: preserve cell structure
  2. Dehydration: Remove water = harden sample
  3. Support: Infiltration (wax)
  4. Microtomy: thin sections
  5. Microscopy: differential staining (nucleus & cytoplasm contrast)
  6. Seal the preparation: preserve stain
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2
Q

Purpose of fixation

A

Preserve tissue architecture (life-like). Stop degeneration

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3
Q

Causes of degeneration once tiss. removed from body

A
  • Anoxia (no O2)
  • Autolysis (self digest of cells bc release enzymes)
  • Putrefaction (bact. decomposition)
  • Dehydration
  • Pressure (e.g. bruise)
  • Osmotic injury
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4
Q

What fixation does (to stop post mortem changes)

A
  • Stops autolysis
  • Prevent bact. decomposition
  • Hardens tiss.
  • Permanent preservation
  • Stabilise tiss. to allow further treatment
  • Enhance avidity for dyes
  • Min. loss soluble cytoplasmic components
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5
Q

Factors involved in fixation

A
  • Temp.
  • Size of specimen
  • Penetration (depend on SA)
  • pH (~6-8)
  • Osmolality (slightly hypertonic)
  • Duration: preserved ASAP
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6
Q

List 3-5 features of ideal fixatives

A
  • quick & even penetration
  • life-like preservation
  • not add artefact material
  • not swell/shrink tiss.
  • safe for user & enviro.
  • convenient shelf-storage
  • economical
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7
Q

Cell structures that need to be stabilised

A
  • lipoproteins of plasmalemma
  • cytoskeleton fibrous proteins
  • fibrous glycoproteins (collagen, basement memb.)
  • globular proteins of cytoplasm & xtra cell. fluid
  • nucleic acids
  • mucosubstances (e.g. HA)
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8
Q

4 chemical fixatives

A
  • Aldehydes: formaldehyde, glutaraldehyde
  • Oxidising agents: K2Cr2O7 (dichrom.), CH3COOH
  • Protein coagulants: eth+methanol, mercuric chloride
  • Compound fixatives: combo w/ above
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9
Q

Dis+Advantage of formalin

A

Adv: preserve biomarkers, stable specimens long periods, inexpensive
Dis: oxidises when stored -> formic acid, Irritant

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10
Q

Principles of Tiss. processing (6 steps)

A
  1. Fixation
  2. Dehydration: remove H2O (w/ ethanol)
  3. Clearing: remove dehydrating agent
  4. Impregnation: remove clearing agent
  5. Embedding: support for sectioning
  6. Microtomy: thin sections
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11
Q

Purpose of staining

A

contrast diff. elements of tiss.

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12
Q

5 chemical bonds dyes bind onto elements

A

Ionic, covalent, H bond, van der waals, hydrophobic

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13
Q

Describe some common DEHYDRATION agents and their properties

A

Alcohol: *Ethanol (50, 70, 95, 100%), methanol, isopropanol
Other: Acetone (fat)
» Rapidly removes water

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14
Q

Describe some common CLEARING agents and their properties

A

Hydrocarbons: xylene, chloroform, benzene, toluene

|&raquo_space; remove dehydrating agent

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15
Q

How pH alter dye binding?

A

Acid pH (from proteins) favours anionic dyes: Hi [H+] favours ionisation of amino groups (NH2, NH3+)

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16
Q

Components of zenker’s fluid

A
  • Distilled water
  • potassium dichromate
  • Mercuric chloride
  • Glacial acetic acid
17
Q

Melting point of paraffin wax

A

~39º-69ºC but we use 56º-57ºC

18
Q

Embedding media properties

A
  • elasticity, density, plasticity, viscosity