Hematoxylin & Eosin Staining: Difference between revisions
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=== Overview of Stain === | |||
H&E stain is a general tissue stain used to initial visualization of microscopic structures. | |||
* Primary Stain: Hematoxylin | |||
** Demonstrates nuclei (blue) | |||
* Counterstain: Eosin | |||
** Demonstrates cytoplasmic materials | |||
** Red blood cells (red) | |||
** Muscle (dark pink) | |||
** Collagen (light pink) | |||
==== Staining Procedures ==== | |||
This stain may be applied either progressively or regressively. | |||
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H&E (Progressive) | |||
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|+H&E (Regressive) | |||
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!Rationale | |||
!Troubleshooting | |||
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==== Differentiation & Blueing ==== | |||
Differentiation is completed in regressive methods, where staining is gradually removed and proper colour is checked microscopically. The differentiation process uses acid alcohol. | |||
* Acid alcohol contains H+ ions that compete with the mordant for tissue. Weakly bound tissues lose stain more readily than tissues that are bound more tightly to the mordant. | |||
* This process causes discolouration (red colour) that needs to be reversed with an alkaline reagent. | |||
** Blueing process reverses this change. | |||
*** Blueing reagents include: alkaline running tap water, lithium carbonate, dilute ammonium hydroxide, and Scott's Tap Water Substitute. | |||
=== Troubleshooting === | === Troubleshooting === | ||
Nearly all steps of H&E staining can be troubleshooted as they dyes can be removed by use of acid alcohol and reapplied. | |||
==== Preventative Measures ==== | ==== Preventative Measures ==== | ||
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* Hematoxylin should appear dark burgundy-purple with no sheen | * Hematoxylin should appear dark burgundy-purple with no sheen | ||
** If metallic sheen or brown/red-brown appearance, may be over-oxidized and needs replacement | ** If metallic sheen or brown/red-brown appearance, may be over-oxidized and needs replacement | ||
** Oxidation occurs with exposure to oxygen or as reagent gets old | |||
*Filter all coloured reagents to remove precipitate | *Filter all coloured reagents to remove precipitate | ||
Latest revision as of 15:34, 8 March 2024
Overview of Stain
H&E stain is a general tissue stain used to initial visualization of microscopic structures.
- Primary Stain: Hematoxylin
- Demonstrates nuclei (blue)
- Counterstain: Eosin
- Demonstrates cytoplasmic materials
- Red blood cells (red)
- Muscle (dark pink)
- Collagen (light pink)
Staining Procedures
This stain may be applied either progressively or regressively.
| Procedure | Time | Rationale | Troubleshooting |
|---|---|---|---|
| Procedure | Time | Rationale | Troubleshooting |
|---|---|---|---|
Differentiation & Blueing
Differentiation is completed in regressive methods, where staining is gradually removed and proper colour is checked microscopically. The differentiation process uses acid alcohol.
- Acid alcohol contains H+ ions that compete with the mordant for tissue. Weakly bound tissues lose stain more readily than tissues that are bound more tightly to the mordant.
- This process causes discolouration (red colour) that needs to be reversed with an alkaline reagent.
- Blueing process reverses this change.
- Blueing reagents include: alkaline running tap water, lithium carbonate, dilute ammonium hydroxide, and Scott's Tap Water Substitute.
- Blueing process reverses this change.
Troubleshooting
Nearly all steps of H&E staining can be troubleshooted as they dyes can be removed by use of acid alcohol and reapplied.
Preventative Measures
Check reagents before use:
- Hematoxylin should appear dark burgundy-purple with no sheen
- If metallic sheen or brown/red-brown appearance, may be over-oxidized and needs replacement
- Oxidation occurs with exposure to oxygen or as reagent gets old
- Filter all coloured reagents to remove precipitate