Staining and Immunohistochemistry PDF

Summary

This document provides a comprehensive overview of staining methods and immunohistochemistry techniques. It details various types of staining, including direct and indirect staining, and lists common staining solutions and procedures.

Full Transcript

# STAINING

- **STAINING:** Process of applying dyes on the sections to see and study the architectural pattern of the tissue and physical characteristics of the cell.

## METHODS OF STAINING

- **Direct Staining:** Process of giving color to the sections using aqueous dye solutions.
- **Indirect Staining:** Action of dye is intensified by adding another agent or a mordant.
- **Mordant:** Serves as a bridge between tissue and the dye to make staining reaction possible.
- **Accentuator:** Accelerates the speed of staining reaction by increasing the staining power and selectivity.

- **Blueing:** Alum hematoxylin stains nuclei with red color, which is converted to the familiar blue black when the section is washed in a weak alkali solution. Tap water is usually alkaline enough to produce this color change, but occasionally alkaline solutions such as saturated lithium carbonate, 0.5% ammonia in distilled water, or Scott's tap water substitute are necessary.
- **Metallic impregnation:** Process where a specific tissue element is demonstrated by colorless solution of metallic salts which are reduced by the tissues producing an opaque, usually black deposit on the surface of the tissue.
- **Negative staining:** Stains are not taken up by their tissue targets.
- **Vital staining:** Selective staining of living cell constituents.
- **Counterstaining:** Application with a different color for contrast and background.

## STAINS AND STAINING SOLUTIONS

### Natural dyes

1. **Hematoxylin**
- Most valuable staining reagent.
- Extracted from the core wood of a Mexican tree called _Haematoxylon campechianum_.
2. **Cochineal dyes**
- Old histologic dye derived from an extract from the female cochineal bug _Dactylopius coccus costal Coccus cacti_.
3. **Orcein**
- Vegetable dye extracted from lichens.
4. **Saffron**
- Derived from the dried stigmata of _Crocus sativus_.

### Synthetic dye

- **Chromophore:** Substances that are capable of producing visible color.
- **Chromogens:** Simple benzene compounds that contain chromophores.
- **Auxochrome:** Substances added to chromogen that alters its property.
- **Dye:** It should consist of an auxochrome and a chromophore group attached to a hydrocarbon benzene ring.

## COMMON STAINING SOLUTIONS

### 1. HEMATOXYLIN

- **Aluminum (Alum) hematoxylin:**
- Ehrlich's hematoxylin
- Harris hematoxylin
- Delafield's hematoxylin
- Cole's hematoxylin
- Mayer's hematoxylin
- Gill hematoxylin
- **Iron hematoxylin:**
- Weigert's hematoxylin
- Heidenhain's hematoxylin
- Loyez hematoxylin
- Verhoeff's hematoxylin
- **Tungsten Hematoxylin:**
- Phosphotungstic acid hematoxylin
- **Copper hematoxylin**

### 2. EOSIN

- Most widely used cytoplasmic stain. Best staining with eosin occurs at pH 4.6 to 5.

### 3. ACID FUCHSIN-PICRIC ACID

- Simplest method of differential staining of collagen.

### 4. ACRIDINE ORANGE

- Most commonly used fluorochrome to demonstrate DNA and RNA.

### 5. ALCIAN BLUE

- Stains acid mucopolysaccharides by forming salt linkages with them.

### 6. ANILINE BLUE

- Cytoplasmic stain used for counterstaining of epithelial sections.

### 7. BASIC FUCHSIN

- Stains acid-fast organism, mitochondria, differentiation of smooth muscles with the use of picric acid.

### 8. BENZIDINE

- Stains hemoglobin

### 9. BISMARCK BROWN

- Stains Diphtheria organisms

### 10. MALACHITE GREEN

- Use as both decolorizer and a counterstain.

### 11. ORCEIN

- Stain for elastic fibers.

### 12. CELESTINE BLUE

- Recommended for routine staining of fixed sections.

### 13. CONGO RED

- Stain for axis cylinders in embryos.

### 14. CRYSTAL VIOLET

- Used to stain amyloid in frozen section.

### 15. IODINE

- Stains amyloid, cellulose, starch, carotenes and glycogen.

### 16. JANUS GREEN B

- Demonstration of mitochondria.

## ROUTINE H&E STAINING FOR PARAFFIN EMBEDDED SECTIONS

**PROCEDURE:**

1. Clear paraffin-embedded section in first xylene bath for 3 mins.
2. Transfer to second xylene bath for 2-3 mins.
3. Immerse in first bath of absolute ethanol for 2 mins.
4. Transfer to a bath of 95% ethanol for 1-2 mins.
5. Rinse with running water for 1 min.
6. Stain with Harris hematoxylin for 5 mins.
7. Wash with running water.
8. Decolorize using acid alcohol for 10-30 secs.
9. Rinse in tap water.
10. Blueing step (ammonia water for 5 mins. or 1% Aq. lithium carbonate until sections appear blue).
11. Wash with running water for 5 mins.
12. Counterstain with 5% Aq. Eosin for 5 mins. (Alcoholic eosin, counterstain for 30 secs, or 1 min.)
13. Dehydrate, clear, and mount.

# IMMUNOHISTOCHEMISTRY

- Use of antibodies as histological tools for identifying patterns of antigen distribution within an organism or tissue.
- Immunohistochemical techniques are now routinely used for the identification of specific or highly selective antigens/epitopes in frozen or paraffin-embedded tissues.

## POLYCLONAL ANTIBODIES:

- Produced by immunizing an animal with an immunogen that contains the antigen of interest.

## MONOCLONAL ANTIBODIES:

- Products of an individual clone of plasma cells.

## IMMUNOHISTOCHEMISTRY TECHNIQUES

- **Direct technique:** Conjugate the primarily antibody directly to the label such as fluorochrome or horseradish peroxidase.
- **Indirect technique:** Two or three-step procedure that involves application of unconjugated primary antibody, followed by a labeled antibody directed against the first antibody
- **Peroxidase-Antiperoxidase technique:** An indirect antibody enzyme-complex technique where the soluble peroxidase-antiperoxidase complex is bound to unconjugated primary antibody by a second layer of "bridging" antibody, usually a swine anti-rabbit antibody, that then binds to both the primary antibody and the rabbit PAP complex.
- **Avidin-biotin complex technique:** Basic sequence of staining consists of primary antibody, biotinylated secondary antibody followed either by preformed avidin-biotin-enzyme complex of the avidin-biotin complex technique or by labeled streptavidin.
- **Labeled streptavidin avidin biotin technique:** The staining sequence consists of primary rabbit antibody, biotinylated anti-rabbit immunoglobulin and streptavidin-enzyme conjugate. The color reaction is then developed with appropriate substrate or chromogen, such as horseradish peroxidase.

# I. CARBOHYDRATES

| Technique | Result |
|-----------------------------------------------------|----------------------------------------------------------------------------------------------------------------------------|
| PERIODIC ACID SCHIFF, BEST CARMINE | PAS+=magenta red, Nuclei=blue<br>Glycogen=bright red granules,<br>Nuclei=grayish blue/blue<br>Mucin, fibrin=weak red |
| LANGHAN'S IODINE METHOD FOR GLYCOGEN | Glycogen= mahogany brown, Tissue constituents=yellow |
| ALCIAN BLUE | Acid mucin=blue, Nuclei= red |
| METACHROMATIC TOLUIDINE BLUE | Glycosaminoglycans= red purple, Tissue background=blue |
| FLUORESCENT ACRIDINE ORANGE | Acid mucopolysaccharide=black, Fungi=greenish red fluorescence, Background=reddish orange fluorescent |
| HALE'S DIALYZED IRONE | Acid mucin= dark blue, nuclei= blue |

# II. FATS/LIPIDS

| Technique | Result |
|--------------------|--------|
| SUDAN IV | Lipids |
| OIL RED O | Dextrin |
| OSMIC ACID STAIN | Fats |

# III. NUCLEIC ACID

| Technique | Result |
|-------------------------------|-------------------------------------------------------------------|
| FEULGEN TECHNIQUE | DNA=red purple, Cytoplasm=green |
| METHYL GREEN | DNA=green/blue green, RNA= rose red |
| ACRIDINE ORANGE- FLUORESCENT | DNA= yellow green fluorescent <br> RNA= brick to orange red |

# IV. PROTEINS

| Technique | Result |
|--------------------|----------------------------------------------------------------------|
| ALKALINE FAST | Method for basic proteins |
| PERACETIC ACID | Cystine, cysteine=blue green |
| SAKAGUCHI'S TEST | Arginine= orange red |

# V. ENZYMES

| Technique | Result |
|------------------------|-------------------------------------------------------------------------------|
| GOMORI CALCIUM | ALP= brownish black, Nuclei=green |
| GOMORI LEAD | ACP=black, Nuclei=green |
| LEAD METHOD | 5' nucleotidase= blackish brown deposits |
| A-NAPHTHYL ACETATE | Esterase= reddish brown, Nuclei=green |
| INDOXYL ACETATE | Esterase activity=blue, Nuclei=red |
| TETRAZOLIUM | Monoamine oxidase=bluish black |

# VI. CONNECTIVE TISSUE

| Technique | Result |
|-------------------------------|------------------------------------------------------------------------------------------------------|
| GOMORI'S SILVER IMPREGNATION | Reticulin fiber= black |
| VAN GIESON'S | Collagen= pink/deep red, Nuclei=brownish black |
| MASSON'S TRICHROME STAIN | Muscle, RBC, keratin=red, Nuclei= blue/black |
| WEIGERT'S | Elastic fibers= dark blue or blue black on clear background |
| VERHOEFF'S | Elastic fibers= black, Nuclei= gray to black |
| ORCEIN | Elastic fiber=dark brown, Nuclei= blue |
| KAJIAN'S TECHNIQUE | Elastic fiber=bright red, Fibrin, CT=Dark blue, RBC=orange yellow |
| PTAH STAIN | Fibrin, neuroglia, muscle striation, amoeba=dark blue |
| METHYL VIOLET-CRYSTAL VIOLET | Amyloid=purplish red, Nuclei, cytoplasm, CT= shades of violet |
| KRAJIAN AMYLOID STAIN | Amyloid= red on clear background, Nuclei=blue |

# VII. CENTRAL NERVOUS SYSTEM

| Technique | Result |
|---------------------------------|----------------------------------------------------------------------------------------------|
| BIELSCHOWSKY'S TECHNIQUE | Neurofibril, axon, dendrites=black/grayish bg. |
| SEVIER-MUNGER | Neural tissues |
| CRESYL-FAST VIOLET | Paraffin sections |
| LUXOL FAST BLUE-H&E STAIN | Myelin=blue green |
| LUXOL FAST BLUE-PAS STAIN | Myelin=blue/green |
| WEIL'S METHOD | Myelin sheath-black, background=yellow |
| CAJAL'S GOLD SUBLIMATE | Astrocytes=black on a light brownish bg. |
| WEIGERT-PAL | Normal myelin sheath=blue black, cells=brown |
| KLUVER AND BARRERS LUXOL FAST BLUE | Myelin with Nissi counterstain |

# VIII. TISSUE PIGMENTS AND DEPOSITS

| Technique | Result |
|-------------------------------------------|---------------------------------------------------------------------------------|
| PERL'S PRUSSIAN BLUE | Hemosiderin and ferric salts |
| SCHMORI'S FERRIC-FERRICYANIDE | Reducing substances |
| MALLORY'S FUCHSIN STAIN | Hemofuscin pigment |
| MASSON-FONTANA | Melanin and argentaffin cell's granule |
| VON KOSSA'S SILVER NITRATE | Calcium |
| LINQUIST'S MOD. RHODANINE | Copper |
| CALCIUM DYE LAKE | Calcium salts= intense reddish orange |
| MOD. FOUCHET'S TECHNIQUE | Liver bile pigments=emerald to blue green |
| GOMORI'S ALDEHYDE FUCHSIN | Lipofuscin=purple |

# IX. MICROORGANISMS

| Technique | Result |
|---------------------------|--------------------------------------------------------------------|
| WADE-FITE | Leprosy bacilli and nocardia |
| TOLUIDINE BLUE | Helicobacter=dark blue |
| DIETERLE | Legionella pneumophila |
| LEVADITI'S MTD. | Spirochetes |
| WARTHIN-STARRY | Spirochetes |
| MOD. STEINER AND STEINER | Spirochetes |
| GROCOTT METHENAMINE SILVER | Fungi=black |
| RAPID GIEMSA STAIN | Bacteria=blue |
| ZIEHL-NEELSEN MTD. | AFB=red, Cells, nuclei=blue, RBC=pink |