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求助 HE染色,细胞边界不清晰,胞核没有着色!

Copy from Protocol Online

Hematoxylin and Eosin (H&E) staining
lace slides containing paraffin sections in a slide holder (glass or metal)
•Deparaffinize and rehydrate sections:
3 x 3´ Xylene (blot excess xylene before going into ethanol)
3 x 3´ 100% ethanol
1 x 3´ 95% ethanol
1 x 3´ 80% ethanol
1 x 5´ deionized H2O
•While sections are in water, skim surface of hematoxalin with a Kimwipe to
remove oxidized particles. Blot excess water from slide holder before going into
hematoxalin.
•Hematoxalin staining:
1 x 3´ Hematoxalin
Rinse deionized water
1 x 5´ Tap water (to allow stain to develop)
Dip 8-12x (fast) Acid ethanol (to destain)
Rinse 2 x 1´ Tap water
Rinse 1 x 2´ Deionized water (can leave overnight at this stage)
•Blot excess water from slide holder before going into eosin.
•Eosin staining and dehydration:
1 x 30 sec Eosin (up to 45 seconds for an older batch of eosin)
3 x 5´ 95% ethanol
3 x 5´ 100% ethanol (blot excess ethanol before going into xylene)
3 x 15´ Xylene
•You can leave slides in xylene overnight to get good clearing of any water.
•Coverslip slides using Permount (xylene based).
lace a drop of Permount on the slide using a glass rod, taking care to leave
no bubbles.
•Angle the coverslip and let fall gently onto the slide. Allow the Permount to
spread beneath the coverslip, covering all the tissue.
•Dry overnight in the hood.

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