Hematology Lab Slideset One Flashcards
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Different sizes of purple top tubes – 7ml, 3ml, 2ml, and 0.5 ml volumes. EDTA is the anticoagulant of choice for hematology specimens. Better preservation for counts and good cell morphology. Always choose the correct size tube for the sample volume.
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EDTA – Tube with small amount of blood – EDTA induced artifacts will occur if tube is not properly filled. Should be at least half-full. Improper filling will:
- Falsely decrease the PCV due to shrinkage of RBC
- Falsely increases the plasma protein reading on the refractometer.
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Making blood smear – small drop (2-3 mm diameter) of well mixed blood on one end of clean slide. Smears should be made with fresh blood.
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Pusher slide – Place the end of a second slide (“spreader”) against the surface of the first slide, holding it at a 30-45 degree angle.
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Blood spreading – as the spreader slide makes contact with the blood, the blood will spread along the edge of the spreader slide. Push the spreader slide forward with a steady, even motion making a thin blood film.
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Pushing blood across – the thickness of the blood smear should decrease from beginning to the feathered edge. The thickness depends on the size of the drop of blood, the angle of the spreader slide, and the speed with which the spreader slide is pushed.
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Finished slide – quickly air-dry or heat-fix smear to prevent artifacts. If smear is not going to be stained soon, it’s a good idea to turn the smears over so that roaches cannot dine on the blood.
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5 problems unstained smears –
- “picket fence” – hesitation while pushing the blood across the slide
- “Holey” – greasy or dirty slide
- “Half slide” – not letting blood spread entirely across the edge of the spreader
slide
- “Short slide” – angle of the spreader was too high
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Blue Foil – Romanovsky Stains
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Diff-Quik coplin jars – Diff-Quik stain is a modification of the Wright’s stain technique which allows you to stain a slide in 15 seconds. Smear is fixed in a methanol fixative solution.
- 5 one second dips
- Solution I – stains the eosinophilic (red) cellular components; 5-6 one second dips
- Solution II – stains the basophilic (blue) cellular components; 5-7 one second dips
- Coplin jars should be tightly covered when not in use
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Stained finished slides
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Artifact-stain precipitate – not commonly seen with Diff-Quik stain. More common with automated stainers.
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Artifact – water damage – in focus – result of slow drying
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Artifact – water damage – out of focus – can be mistaken for RBC abnormalities
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Artifact – Hemolyzed RBC’s – result of red cells lysing from exposure to excessive humidity. This will appear in smears that are refrigerated before staining
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Blue Foil – Microhematocrit procedure
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PCV – filing the capillary tube for PCV
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Sealing the end of the capillary tube before spinning.
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Placing capillary tube in microhematocrit centrifuge. Length of spinning dependent on the centrifuge and species. However, a 5 minute spin is generally recommended.
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PCV reader card – packed cell volume measures the volume of red blood cells expressed as a percentage of the volume of whole blood in a sample. Care should be taken that the top of the plasma column should be aligned with the 100% line and the bottom of the packed RBCs should be on the 0% line.
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Normal vs. anemic PCV – Normal plasma appearance
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Hemolyzed plasma – will increase TPP on refractometer.
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Lipemic plasma – will obscure TPP on refractometer.
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Icteric plasma
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Standard vs. Veterinary Refractometers for Total Plasma Protein (TPP) determinations.
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Scale of standard refractometer – scale for protein, urine specific gravity, and refractive index.
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Scale of Veterinary refractometer – protein scale and 2 specific gravity scales. One for cats and one for other. Reading for specific gravity goes up to 1.060.
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Blue Foil – Electronic Cell Counter