Nuclear detail lost

Stainability lost

Stain precipitation

Cells coming away from basement membrane

Tumor

Placenta

Surgical

Biopsy

Are 3 cm deep

Must be labeled

Colours indicate day of week the tissue was processed

Has holes to allow the tissue to flow in an out

Functions by creating hydrogen bridges to prevent degredation

Typically shrinks, swells, and distorts tissue

Keeps bacteria and fungi viable

Allows the tissue to be stainable

Time

Density of tissue

Temperature

Type of container

Zinc

Picric Acid

Acetic Acid

Alcohol

Osmium Tetroxide

Acetic Acid

Formalin

Gluteraldehyde

55 ml

55 L

5500 ml

550 ml

2300 ml

0.23 L

2070 ml

2600 ml

It is a coagulant fixative

It is composed of liquid formaldehyde in water

Add methanol to stop the formation of paraformaldehyde

Penetrates tissue slowly but fixes quickly

Carnoy

Picric Acid

Formalin

Gluteraldehyde

Is a non-coagulant, additive fixative

Can be used to disinfect the cryostat

Can cause false positive reactions in period acid schiff

Creates methylene bridges in tissue to preserve it

Is a component in B5 fixative

Is a common fixative used in the histology lab

Mercuric pigment can be removed using alcoholic picric acid

Is a great fixative when tissue needs to be X-rayed

Fixes lipids

Used mostly for electron microscopy

Commonly a secondary fixative

Is a non-additive fixative

Is composed of picric acid, formaldehyde and mercuric chloride

Is the best preservative for glycogen

Does not stain tissue

Is commonly used as a secondary fixative

Gluteraldehyde

PAF / Zamboni

Picric Acid

Mercuric Chloride

Acetone should not be used for IHC since it destroys enzymes

Acetone is a good fixative since it does not shrink or harden tissue

Ethanol should not be used to fix frozen sections since it inhibits freezing

Ethanol should not be used to preserve glycogen as it is known to dissolve it

Carnoy's

Picric Acid

Bouin's

Acetic Acid

Tissue should be placed in fixative 10X greater than the tissue itself

Tissue should have been placed in fixative right after removal from the body

Tissue in fixative should be placed at 4 degrees Celcius

Tissue should have been frozen before fixation

Large tissue should not be fixed

Large tissue must be cut into smaller pieces

Holes must be poked in the specimen to allow fixative to penetrate

Fixative must be injected into the specimen

Uses vacuum technology to infiltrate tissues

Hematoxylin is added to tint the tissue pink for easier embedding orientation

This processor is safer since it does not use heat

This is an open system

The dehydration process begins with the highest alcohol concentration then descends

Ethyl alcohol is the best for dehydration

Butanol is a good substitution because it is quick

Alcohol dehydrates tissue by removing xylene

Tissue would smell like xylene

Tissue would be soft

Impossible to tell until staining

Tissue would be dessicated

First xylene, then several changes of alcohol, then xylene, then wax

Impossible to fix, request new specimen

First several changes of alcohol, then xylene, then wax

Several changes of wax

Improper fixation

Improper dehydration

Improper clearing

Improper infiltration

Xylene

Toluene

Benzene

Chloridine

An example is Limonene

A solution that dehydrates and clears

An example is Xylene

A solution that dehydrates and infiltrates

Increase the temperature of the wax

Remove wax with xylene, dehydrate with alcohol, then clear with xylene, then several changes of wax

Re-fix the tissue

Several changes of wax

Soft wax allows for easy ribboning

Soft wax provides the most support

Hard wax melts at 45 degrees Celsius

Hard wax should not be used if thinner sections are required

Wax should be kept at least 10 degrees over the melting point

Typical melting point is 35-48 degrees

Overexposure to wax will cause tissue hardening and shrinking

Water-bath should be kept 2 degrees above the melting point

Clearing step can be skipped

Infiltration step can be skipped

Dehydration step can be skipped

Microwaves would never be used for processing

Several small biopsies are placed together

Red dot is facing towards you when cutting

Two pieces of small bowel are orientated so that the lumens are facing eachother

Transverse cut of tubular tissue

Incorrect orientation of tissue when embedding - discard the tissue and request new specimen

Poor processing of tissues - check solutions and machine

Tissue is over-dehydrated - increase time in alcohol

NBF precipitate is found in the tubing of the processor - perform a picric acid flush

Block not chilled enough

Cutting too slowly

Dull blade

Block and knife not parallel to eachother

Tissue must be > 3 mm in order to be decalcified properly

Calcium is soluble at pH 4.5

Acid methods are usually slow

Decalcification increases stainability of bone tissue

Mechanical methods such as poking

Chemical methods such as ammonium hydroxide and ammonium oxalate which check for the precipitation of calcium oxalate

Cutting the bone tissue

Radiography

Bone was stained too long in hematoxylin

Bone was underdecalcified

Bone was improperly fixed

Bone was not stained with the correct stain

Disinfect daily with sodium hypochlorite

Use cryostat when rapid diagnosis is required or when fat or enzymes need to be demonstrated.

If a tissue with known TB requires cutting, disinfect afterwards with formaldehyde vapor

If tissue is sticking the antiroll plate may be too warm

Fluorescent microscope for Acid Fast Bacilli

Polarizing microscope for Oil Red O

Compound light microscope for Acridine Orange

Electron microscope for H&E

"Roughing in" is usually done at 20 micrometers

The clearance angle is usually set at 10 degrees

Speed of cutting has no effect on ribbon quality

In a rotary microtome, the knife moves side to side

With linear stainers, time in solution can be varied by adding more containers

With robotic stainers, the programs cannot be changed

Robotic stainers are good for progressive staining

Linear stainers are good for regressing staining

Water bath should be kept at 5 - 10 degrees above the melting point of wax

Tap water should always be used to fill water baths

Parched earth artifact can result if the water bath is too cold

Water bath should be cleaned after each ribbon

Slides for IHC were placed on a hotplate for drying.

Slides with biospy were cut using special techniques with 6 tissues per slide

Slides for neurology were placed in a 37 degree oven for drying

Slides for routine H&E were placed in a 60 degree oven for drying

Embedding

Grossing

Autopsy

Frozen sectioning

Placing used blades in the garbage

Fixing tissue that is known to be TB positive with formalin

Storing glacial acetic acid on the counter top

Fixing CJD positive tissue with formalin

metachrome

benzene ring

auxochrome

chromaphore

A method of nuclear staining is acidic dye

A method of nuclear staining is dye + metal mordant

Cytoplasmic staining occurs from the interaction of dye with neutral molecules

Lipids are stained because the dye has a greater affinity to the solution than the fat

-NH2

-COOH

-OH

-SO4

Basic dyes will have a negative auxochrome

Basic dyes will produce chloride salt

Acid dyes are cationic

Acid dyes produce magnesium salt

Modifiers will affect staining time

Sulphonics makes acidic dyes basic

Dye binding can be affected by pH

Orthochromic dye will stain a different colour than the dye colour

AFB

Mucin

Mast Cell

Amyloid

Prevent mold growth

Enhance staining

Makes the dye more acidic

Makes the dye fluorescent

Hematoxylin

Orcein

Acridine Orange

Saffron

Weak acid differentiating basic dyes ex. PTA/PMA for Biebrich Scarlet

Weak base differentiating acid dyes ex. PTA/PMA for Biebrich Scarlet

Excess mordant differentiating ex. iron alum for Verhoeff

Alcoholic differentiation ex. alcohol for eosin

Oxidize the hematoxylin with sodium iodate

Prepare hematoxylin using aluminum since it can withstand strong acids in the stain

After preparing the hematoxylin, pour directly into the coplin jar for staining

Gill's hematoxylin should be prepared for this stain

Gill's hematoxylin for use in Alcian Blue

Mayer's hematoxylin for Oil Red O

Harris hematoxylin for Masson's Trichrome

Weigert's hematoxylin for routine H&E

Hematoxylin stains indirectly

Is never a regressive stain

Cannot be used to stain bone tissue

The best substitute for eosin would be phenol red

Tissue was left in acid alcohol for 20 minutes during coffee break

Aluminum / iron was not present in the hematoxylin

The hematoxylin was not filtered properly

The hematoxylin was stored in a clear glass jar

Tissue was cut at 3 micrometers

Eosin is too concentrated

Eosin was not left in alcohol long enough

Tissue was left in eosin for too long

Places slide in Bouin's for 1 hour at 56 degrees.

Counterstain in Light Green

Places slides in Biebrich Scarlet Acid Fuchsin before PTA/PMA

Uses Mayer's Hematoxylin to stain nuclei

Collagen has stained blue

Cytoplasm has stained red

RBCs have stained red

Nucleic acids have stained red

Ensure than silver solution is neutralized with HCl before disposal

Place the slides in a thin walled coplin jar to ensure good heating in the microwave

Bleach tissue in Oxalic Acid after Potassium Permanganate

Counterstain in Light Green

Gomori Burnter - argentaffin

Grocott - argyrophilic

von Kossa - substitution

Gordon and Sweets - argyrophilic

Elastic fibers cannot easily be seen on the brain control slide so it was placed in Verhoffs stain for a longer period of time

Nuclei are not staining so a new solution of Verhoffs made and used

The stain looks very muddy so it was placed back into gold chloride for a longer time

Elastic fibers are too pale so the slide was placed back into van Gieson stain for longer

Orcein is specific for elastic fibres

Orcein will stain elastic fibres brown

Aldehyde fuchsin will stain elastic fibres green

Aldehyde fuchsin is a regressive method

Take the slides down to water before staining

Place the slides in Toludine Blue to stain for mast cells

Place the slides in Light Green as a counterstain

Differentiate with alcohol then clear and mount

Stomach tissue was used as the control

The tissue was placed in 3% acetic acid before Alcian Blue dye

The tissue was placed in Acetic Acid following Alcian Blue for 10 minutes

The pH of Alcian Blue was 6.5

Schiff's reagent was tested before use using formalin and the reaction became a deep blue colour

Grocott's method was performed earlier so the periodic acid solution was saved and used agian

Metabisulfite rinse was prepared using 100% HCl straight from the bottle

Tissues were washed for 10 minutes in water after Schiff's

Schiff's reagent is composed of Acid Fuchsin and Sulpheric Acid

Periodic acid is the secondary oxidizer

Sodium Metabisulfite rise is what brings the pink colour to the tissue

Fungi will stain pink

Metanil Yellow is the primary stain

Mucicarmine stains acid mucins

Gill's hematoxylin should not be used as the nuclear stain

Cryptococcus can also be demonstrated with this method

The technologist double checked to ensure sections were cut at 4um

The doctor would like to differentiate between primary and secondary amyloidosis so the slide was pretreated with potassium permangonate

Slides were placed in neutral red to stain for amyloid

The technologist did not know how to use the polarizing microscope so birefringence was not checked on the control

The tissue was previously fixed in formalin

A frozen section was cut for staining

Tissue was taken down to water before staining

The tissue was placed in hematoxylin after Oil Red O

Luxol Fast Blue dye is differentiated with an acid

The control tissue is cerebellum

Eosin is the counterstain

Luxol Fast Blue stains myelin

mercury

tattoo

carbon

melanin

Tissue is placed in silver nitrate and then microwaved for the appropriate time

Placenta is used as the calcium control

The tissues are placed in nuclear fast red or neutral red

The technologist decides the control passed since the calcium stained brown

Slide was placed in eosin

Patient tissue does not contain iron

Slide was taken down to distilled water

Slide was placed in HCl + Potassium Ferrocyanide

This stain is used to demonstrate argentaffin granules

Gold chloride is a fixing agent

Hematoxylin is the counterstain

Melanin cannot oxidize silver therefore a reducer such as Sodium Thiosulfate is required

Ziehl Neelson

Gram

Geimsa

Grocott

After fixation, Gram stain the tissue to detect the bacteria

Wear N-95 for frozen section

Place the specimen in Carnoy's for fixation then stain with Ziehl Neelson

After fixation, take down slides to tap water before staining

Not enough Acid Alcohol was used to decolourize the AFB

Methylene blue stain was missed

Nature of their cell wall

Because they are Gram negative

Crystal violet - stains Gram negative bacteria

Acetone / Alcohol - decololourizes Gram positive bacteria

Basic Fuchsin - stains acid fast bacteria pink

Picric Acid - stains bacteria yellow

Fungi are stained black - the slide is placed back into gold chloride for more toning until fungi are brown

Fungi, nuclei, and other tissues are staining black - the slide is good

No fungi have been stained - the wrong concentration of periodic acid was used

Fungi are brown - the slide is good

MSB stain for bile

Warthin-Starry for H. pylori

Steiner for spirochetes

Hall for fibrin

Deparaffinize and hydrate to water

apply antibody

stain nuclei with hematoxylin

counterstain with hematoxylin

Tissue must be washed with water to remove crosslinking from formalin

Proteolytic enzymes will destroy the antigen sites

Heat methods help cleave the bonds

Enzymatic methods will unfold the bonds

Picric acid in a container

Alcohol in a container

Sodium Thiosulfate down the sink

Silver Nitrate down the sink

Kidney for Masson's Trichrome

Placenta for von Kossa

Cerebrum for Luxol Fast Blue

Stomach for Alcian Blue

To prevent the blade from getting scratched

To prevent your hands from getting infected

To prevent skin cells from getting on the microscope slides

To prevent yourself from getting cut

Left in Sodium Thiosulfate for too long

Left in Ferric Chloride too long

Left in Van Gieson stain too long

Left in Verhoeff stain too long

pH of eosin is 8.0

Sections were cut at 8 micrometers

Tissue left in alcohol for too long

Tissues were rinsed in water after blueing