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PERIPHERAL SMEAR
EXAMINATION
NITHIN K MATHEW
REG NO ;- 08L1308
FATHER MULLER
MEDICAL COLLEGE
PREPARATION OF BLOOD SMEAR
 There are three types of blood
smears:
1. The cover glass smear.
2. The wedge smear .
3. The spun smear.
 The are two additional types of blood
smear used for specific purposes
1. Buffy coat smear for WBCs < 1.0×109/L
2. Thick blood smears for blood parasites .
WEDGE BLOOD SMEAR
 Specimen : EDTA blood within 2 to 3
hours & collected to the mark on tube.
 Not's : May change RBCs morphology
such as Spiculated (crenated) cells if :
1. Excessive amount of anticoagulant to
specimen
2. Old blood - long standing.
3. Warm environment (room temperature)
may hasten changes.
PROCEDURE
 placing a drop of blood from mixed
sample on a clean glass slide.
 Spreader slide using another clean glass
slide at 30-40 degree angle.
 Control thickness of the smear by
changing the angle of spreader slide
 Allow the blood film to air-dry completely
before staining. (Do not blow to dry. The
moisture from your breath will cause
RBC artifact.)
large angle
low HCT
small angle
high HCT
CHARACTERISTICS OF A GOOD SMEAR
1. Thick at one end, thinning out to a smooth
rounded feather edge.
2. Should occupy 2/3 of the total slide area.
3. Should not touch any edge of the slide.
4. Should be margin free, except for point of
application.
tail body head
MORPHOLOGIC CHANGES DUE TO
AREA OF SMEAR
 Thin area- Spherocytes which are
really "spheroidocytes" or flattened
red cells. True spherocytes will be
found in other (Good) areas of
smear.
 Thick area - Rouleaux, which is
normal in such areas. Confirm by
examining thin areas. If true
rouleaux, two-three RBC's will
stick together in a "stack of coins"
fashion..
COMMON CAUSES OF A POOR BLOOD
SMEAR
1. Drop of blood too large or too small.
2. Spreader slide pushed across the slide in a jerky manner.
3. Failure to keep the entire edge of the spreader slide
against the slide while making the smear.
4. Failure to keep the spreader slide at a 30° angle with the
slide.
5. Failure to push the spreader slide completely across the
slide.
6. Irregular spread with ridges and long tail: Edge of
spreader dirty or chipped; dusty slide
7. Holes in film: Slide contaminated with fat or grease
8. Cellular degenerative changes: delay in fixing, inadequate
fixing time or methanol contaminated with water.
BIOLOGIC CAUSES OF A POOR SMEAR
1. Cold agglutinin - RBCs will clump
together. Warm the blood at 37° C
for 5 minutes, and then remake the
smear.
2. Lipemia - holes will appear in the
smear. There is nothing you can do
to correct this.
3. Rouleaux - RBC’s will form into
stacks resembling coins. There is
nothing you can do to correct this
SLIDE FIXATION &
STAINING
LEISHMAN'S STAIN
PRINCIPLE LIKE ROMANOWSKY PRINCIPLE
Leishman's stain : a polychromatic stain
 Methanol : fixes cells to slide
 methylene blue stains RNA,DNA
=== blue-grey color
 Eosin stains hemoglobin, eosin granules
=== orange-red color
 pH value of phosphate buffer is very
important
STAINING PROCEDURE
 Thin smear are air dried.
 Flood the smear with stain.
 Stain for 1-5 min. Experience will indicate
the optimum time.
 Add an equal amount of buffer solution and
mix the stain by blowing an eddy in the fluid.
 Leave the mixture on the slide for 10-15 min.
 Wash off by running water directly to the
centre of the slide to prevent a residue of
precipitated stain.
 Stand slide on end, and let dry in air.
TOO ACIDIC SUITABLE TOO BASIC
CAUSES & CORRECTION
 Too Acid Stain:
1. insufficient staining time
2. prolonged buffering or washing
3. old stain
 Correction:
1) lengthen staining time
2) check stain and buffer pH
3) shorten buffering or wash time
 Too Alkaline Stain:
1. thick blood smear
2. prolonged staining
3. insufficient washing
4. alkaline pH of stain components
 Correction :
1) check pH
2) shorten stain time
3) prolong buffering time
PERFORMING A MANUAL
DIFFERENTIAL AND ASSESSING RBC
MORPHOLOGY
PRINCIPLE
 White Blood Cells.
1. Check for even distribution and
estimate the number present (also,
look for any gross abnormalities
present on the smear).
2. Perform the differential count.
3. Examine for morphologic
abnormalities.
PRINCIPLE
 Red Blood Cells, Examine for :
1. Size and shape.
2. Relative hemoglobin content.
3. Polychromatophilia.
4. Inclusions.
5. Rouleaux formation or
agglutination
PRINCIPLE
 Platelets.
1. Estimate number present.
2. Examine for morphologic
abnormalities.
PROCEDURES
 Observations Under ×10
1. Check to see if there are good counting
areas available free of ragged edges
and cell clumps.
2. Check the WBC distribution over the
smear.
3. Check that the slide is properly
stained.
4. Check for the presence of large
platelets, platelet clumps, and fibrin
strands.
Observing direction:
Observe one field and record the number of WBC
according to the different type then turn to another field
in the snake-liked direction
*avoid repeat or miss some cells
OBSERVATIONS UNDER× 40X : WBC
ESTIMATES
 Using the × 40 high dry with no oil.
 Choose a portion of the peripheral
smear where there is only slight
overlapping of the RBCs.
 Count 10 fields, take the total number
of white cells and divide by 10.
 To do a WBC estimate by taking the
average number of white cells and
multiplying by 2000.
OBSERVATIONS UNDER × 100: PLATELET
ESTIMATES
1. Use the oil immersion lens estimate the
number of platelets per field.
2. Look at 5-6 fields and take an average.
3. Multiply the average by 20,000.
4. Note any macroplatelets.
 Platelets per oil immersion field (OIF)
1) <8 platelets/OIF = decreased
2) 8 to 20 platelets/OIF = adequate
3) >20 platelets/OIF = increased
EVALUATE WBC MORPHOLOGY
 Note if any abnormal white cell morphology is
present
o Hypersegmented poly's (5 or more lobes)
o Vacuolation of neutrophils
o Toxic granulation of neutrophils
o Dohle bodies
o Atypical Lymphocytes
o Smudge cells
MANUAL DIFFERENTIAL COUNTS
 These counts are done in the same
area as WBC and platelet estimates
with the red cells barely touching.
 This takes place under × 100 (oil)
using the zigzag method.
 Count 100 WBCs including all cell
lines from immature to mature.
 Reporting results
Absolute number of cells/µl = % of cell
type in differential x white cell count
OBSERVING AND RECORDING
NUCLEATED RED BLOOD CELLS (NRBCS)
 If 10 or more nucleated RBC's (NRBC)
are seen, correct the
 White Count using this formula:
Corrected WBC Count =
WBC x 100/( NRBC + 100)
Example : If WBC = 5000 and 10 NRBCs
have been counted
Then 5,000× 100/110 = 4545.50
The corrected white count is 4545.50.
TIPS ON DIFF'S
 Do not count cells that are disintegrating
• smudge cells
• eosinophil with no cytoplasmic membrane
and with scattered granules
• Pyknotic cell (nucleus extremely
condensed and degenerated, lobes
condensed into small, round clumps with
no filaments interconnecting).
• Basket cells
ABNORMAL DIFFERENTIALS
1. 200 Cell diff:
a. WBC > 15.0 (>20.0 for babies under 1 month and
labor unit)
b. Three or more basophils seen.
2. If more than five immature WBC's are seen (or any
blasts) let someone else diff slide and average
results.
3. Correct WBC for NRBC's if you seen ten or more
NRBCs/100 WBC.
4. Always indicate number of cells counted on diff.
5. If any cell type is extremely elevated (such as bands,
monos, or eos > 20) indicate that you are aware of
the abnormality by circling or checking on the card
next to the results.
RECORDING RBC MORPHOLOGY
1. Scan area using ×100 (oil immersion).
2. Observe 10 fields.
3. Red cells are observed for size, shape, hemoglobin content, and the
presence or absence of inclusions.
4. Abnormal morphology: Red cell morphology is assessed according
to See the following sample grading system. Note that red cell
morphology must be scanned in a good counting area.
Two questions should be asked
1. Is the morphology seen in every field?
2. Is the morphology pathologic and not artificially induced?
Table 1 & 2 represents a system derived to determine a quantitative
scale.
RED BLOOD CELL MORPHOLOGY
 A normal red blood cell should be approximately
the same size as a normal lymphocyte nucleus or
2 normal sized red blood cells should fit side by
side across a normal sized poly (not a
hypersegmented poly).
Grade Degree of
abnormality
NO. of Field/ Oil imm.
1+1-6 per oil imm. field
2+7-10 per OIF
3+11-20 per OIF
4+> 20 per OIF
REPORTING RESULTS
 Where possible use macrocytic and
microcytic, rather than simply anisocytosis
alone, when describing red cell morphology.
 Use specific cell morphology when possible,
rather than simply reporting poikilocytosis.
 When red cells are normocytic,
normochromic, report out as NORMAL.
When abnormal morphology has been noted,
DO NOT indicate normal on the report form.
 EXAMPLE: 7-10 microcytic RBC's/OIF is
reported out as: 2+ microcytosis or Moderate
microcytosis.
DETERMINE A QUANTITATIVE SCALE
1
GRADING INCLUSIONS
2
MORPHOLOGY OF WBC
IN PERIPHERAL BLOOD
Normal
NORMAL PERIPHERAL BLOOD SMEAR
STAB NEUTROPHIL
 Diameter:12-16
 Cytoplasm : pink
 Granules: primary
secondary
 Nucleus: dark purple blue
 dense chromatin
BAND NEUTROPHIL
SEGMENTED NEUTROPHIL
 Diameter: 12-16
 Cytoplasm : pink
 Granules: primary
secondary
 Nucleus: dark purple blue
dense chromatin
2-5 lobes
SEGMENTED NEUTROPHIL
EOSINOPHIL
 Diameter: 14-16
 Cytoplasm : full of granules
 Granules: large refractile, orange-red
 Nucleus: blue
dense chromatin
2 lobes like a pair of glass
EOSINOPHIL
BASOPHIL
 Diameter: 14-16
 Cytoplasm : pink
 Granules: dark blue –black
obscure nucleus
 Nucleus: blue
BASOPHIL
LYMPHOCYTE
 Diameter: small 7-9
large 12-16
 Cytoplasm: medium blue
 Granules: small agranular
large a few
primary granules
 Nucleus: dark blue round
dense chromatin
LYMPHOCYTE
MONOCYTE
 Diameter: 14-20
 Cytoplasm : grey blue
 Granules: dust-like lilac
color granules
 Nucleus: blue
large irregularly shaped
and folded
MONOCYTE
ABNORMAL CHANGES
OF WBC MORPHOLOGY
LEFT-SHIFT AND RIGHT-SHIFT OF
NEUTROPHIL:
Left-shift: non-segmented
neutrophil > 5%
Right-shift: hypersegmented
neutrophil >3%
TOXIC GRANULATION
AUER BODIES(AUER ROD)
HYPERSEGMENTATION
Anisocytosis of neutrophil
vacuolization
Degeneration of nucleus
Dohle body

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PERIPHERAL SMEAR EXAMINATION

  • 1. PERIPHERAL SMEAR EXAMINATION NITHIN K MATHEW REG NO ;- 08L1308 FATHER MULLER MEDICAL COLLEGE
  • 2. PREPARATION OF BLOOD SMEAR  There are three types of blood smears: 1. The cover glass smear. 2. The wedge smear . 3. The spun smear.  The are two additional types of blood smear used for specific purposes 1. Buffy coat smear for WBCs < 1.0×109/L 2. Thick blood smears for blood parasites .
  • 3. WEDGE BLOOD SMEAR  Specimen : EDTA blood within 2 to 3 hours & collected to the mark on tube.  Not's : May change RBCs morphology such as Spiculated (crenated) cells if : 1. Excessive amount of anticoagulant to specimen 2. Old blood - long standing. 3. Warm environment (room temperature) may hasten changes.
  • 4. PROCEDURE  placing a drop of blood from mixed sample on a clean glass slide.  Spreader slide using another clean glass slide at 30-40 degree angle.  Control thickness of the smear by changing the angle of spreader slide  Allow the blood film to air-dry completely before staining. (Do not blow to dry. The moisture from your breath will cause RBC artifact.)
  • 5. large angle low HCT small angle high HCT
  • 6.
  • 7. CHARACTERISTICS OF A GOOD SMEAR 1. Thick at one end, thinning out to a smooth rounded feather edge. 2. Should occupy 2/3 of the total slide area. 3. Should not touch any edge of the slide. 4. Should be margin free, except for point of application.
  • 9. MORPHOLOGIC CHANGES DUE TO AREA OF SMEAR  Thin area- Spherocytes which are really "spheroidocytes" or flattened red cells. True spherocytes will be found in other (Good) areas of smear.  Thick area - Rouleaux, which is normal in such areas. Confirm by examining thin areas. If true rouleaux, two-three RBC's will stick together in a "stack of coins" fashion..
  • 10. COMMON CAUSES OF A POOR BLOOD SMEAR 1. Drop of blood too large or too small. 2. Spreader slide pushed across the slide in a jerky manner. 3. Failure to keep the entire edge of the spreader slide against the slide while making the smear. 4. Failure to keep the spreader slide at a 30° angle with the slide. 5. Failure to push the spreader slide completely across the slide. 6. Irregular spread with ridges and long tail: Edge of spreader dirty or chipped; dusty slide 7. Holes in film: Slide contaminated with fat or grease 8. Cellular degenerative changes: delay in fixing, inadequate fixing time or methanol contaminated with water.
  • 11. BIOLOGIC CAUSES OF A POOR SMEAR 1. Cold agglutinin - RBCs will clump together. Warm the blood at 37° C for 5 minutes, and then remake the smear. 2. Lipemia - holes will appear in the smear. There is nothing you can do to correct this. 3. Rouleaux - RBC’s will form into stacks resembling coins. There is nothing you can do to correct this
  • 13. PRINCIPLE LIKE ROMANOWSKY PRINCIPLE Leishman's stain : a polychromatic stain  Methanol : fixes cells to slide  methylene blue stains RNA,DNA === blue-grey color  Eosin stains hemoglobin, eosin granules === orange-red color  pH value of phosphate buffer is very important
  • 14. STAINING PROCEDURE  Thin smear are air dried.  Flood the smear with stain.  Stain for 1-5 min. Experience will indicate the optimum time.  Add an equal amount of buffer solution and mix the stain by blowing an eddy in the fluid.  Leave the mixture on the slide for 10-15 min.  Wash off by running water directly to the centre of the slide to prevent a residue of precipitated stain.  Stand slide on end, and let dry in air.
  • 15. TOO ACIDIC SUITABLE TOO BASIC
  • 16. CAUSES & CORRECTION  Too Acid Stain: 1. insufficient staining time 2. prolonged buffering or washing 3. old stain  Correction: 1) lengthen staining time 2) check stain and buffer pH 3) shorten buffering or wash time
  • 17.  Too Alkaline Stain: 1. thick blood smear 2. prolonged staining 3. insufficient washing 4. alkaline pH of stain components  Correction : 1) check pH 2) shorten stain time 3) prolong buffering time
  • 18. PERFORMING A MANUAL DIFFERENTIAL AND ASSESSING RBC MORPHOLOGY
  • 19. PRINCIPLE  White Blood Cells. 1. Check for even distribution and estimate the number present (also, look for any gross abnormalities present on the smear). 2. Perform the differential count. 3. Examine for morphologic abnormalities.
  • 20. PRINCIPLE  Red Blood Cells, Examine for : 1. Size and shape. 2. Relative hemoglobin content. 3. Polychromatophilia. 4. Inclusions. 5. Rouleaux formation or agglutination
  • 21. PRINCIPLE  Platelets. 1. Estimate number present. 2. Examine for morphologic abnormalities.
  • 22. PROCEDURES  Observations Under ×10 1. Check to see if there are good counting areas available free of ragged edges and cell clumps. 2. Check the WBC distribution over the smear. 3. Check that the slide is properly stained. 4. Check for the presence of large platelets, platelet clumps, and fibrin strands.
  • 23. Observing direction: Observe one field and record the number of WBC according to the different type then turn to another field in the snake-liked direction *avoid repeat or miss some cells
  • 24. OBSERVATIONS UNDER× 40X : WBC ESTIMATES  Using the × 40 high dry with no oil.  Choose a portion of the peripheral smear where there is only slight overlapping of the RBCs.  Count 10 fields, take the total number of white cells and divide by 10.  To do a WBC estimate by taking the average number of white cells and multiplying by 2000.
  • 25. OBSERVATIONS UNDER × 100: PLATELET ESTIMATES 1. Use the oil immersion lens estimate the number of platelets per field. 2. Look at 5-6 fields and take an average. 3. Multiply the average by 20,000. 4. Note any macroplatelets.  Platelets per oil immersion field (OIF) 1) <8 platelets/OIF = decreased 2) 8 to 20 platelets/OIF = adequate 3) >20 platelets/OIF = increased
  • 26. EVALUATE WBC MORPHOLOGY  Note if any abnormal white cell morphology is present o Hypersegmented poly's (5 or more lobes) o Vacuolation of neutrophils o Toxic granulation of neutrophils o Dohle bodies o Atypical Lymphocytes o Smudge cells
  • 27. MANUAL DIFFERENTIAL COUNTS  These counts are done in the same area as WBC and platelet estimates with the red cells barely touching.  This takes place under × 100 (oil) using the zigzag method.  Count 100 WBCs including all cell lines from immature to mature.  Reporting results Absolute number of cells/µl = % of cell type in differential x white cell count
  • 28. OBSERVING AND RECORDING NUCLEATED RED BLOOD CELLS (NRBCS)  If 10 or more nucleated RBC's (NRBC) are seen, correct the  White Count using this formula: Corrected WBC Count = WBC x 100/( NRBC + 100) Example : If WBC = 5000 and 10 NRBCs have been counted Then 5,000× 100/110 = 4545.50 The corrected white count is 4545.50.
  • 29. TIPS ON DIFF'S  Do not count cells that are disintegrating • smudge cells • eosinophil with no cytoplasmic membrane and with scattered granules • Pyknotic cell (nucleus extremely condensed and degenerated, lobes condensed into small, round clumps with no filaments interconnecting). • Basket cells
  • 30. ABNORMAL DIFFERENTIALS 1. 200 Cell diff: a. WBC > 15.0 (>20.0 for babies under 1 month and labor unit) b. Three or more basophils seen. 2. If more than five immature WBC's are seen (or any blasts) let someone else diff slide and average results. 3. Correct WBC for NRBC's if you seen ten or more NRBCs/100 WBC. 4. Always indicate number of cells counted on diff. 5. If any cell type is extremely elevated (such as bands, monos, or eos > 20) indicate that you are aware of the abnormality by circling or checking on the card next to the results.
  • 31. RECORDING RBC MORPHOLOGY 1. Scan area using ×100 (oil immersion). 2. Observe 10 fields. 3. Red cells are observed for size, shape, hemoglobin content, and the presence or absence of inclusions. 4. Abnormal morphology: Red cell morphology is assessed according to See the following sample grading system. Note that red cell morphology must be scanned in a good counting area. Two questions should be asked 1. Is the morphology seen in every field? 2. Is the morphology pathologic and not artificially induced? Table 1 & 2 represents a system derived to determine a quantitative scale.
  • 32. RED BLOOD CELL MORPHOLOGY  A normal red blood cell should be approximately the same size as a normal lymphocyte nucleus or 2 normal sized red blood cells should fit side by side across a normal sized poly (not a hypersegmented poly). Grade Degree of abnormality NO. of Field/ Oil imm. 1+1-6 per oil imm. field 2+7-10 per OIF 3+11-20 per OIF 4+> 20 per OIF
  • 33. REPORTING RESULTS  Where possible use macrocytic and microcytic, rather than simply anisocytosis alone, when describing red cell morphology.  Use specific cell morphology when possible, rather than simply reporting poikilocytosis.  When red cells are normocytic, normochromic, report out as NORMAL. When abnormal morphology has been noted, DO NOT indicate normal on the report form.  EXAMPLE: 7-10 microcytic RBC's/OIF is reported out as: 2+ microcytosis or Moderate microcytosis.
  • 36. MORPHOLOGY OF WBC IN PERIPHERAL BLOOD Normal
  • 38.
  • 39. STAB NEUTROPHIL  Diameter:12-16  Cytoplasm : pink  Granules: primary secondary  Nucleus: dark purple blue  dense chromatin
  • 41. SEGMENTED NEUTROPHIL  Diameter: 12-16  Cytoplasm : pink  Granules: primary secondary  Nucleus: dark purple blue dense chromatin 2-5 lobes
  • 43. EOSINOPHIL  Diameter: 14-16  Cytoplasm : full of granules  Granules: large refractile, orange-red  Nucleus: blue dense chromatin 2 lobes like a pair of glass
  • 45. BASOPHIL  Diameter: 14-16  Cytoplasm : pink  Granules: dark blue –black obscure nucleus  Nucleus: blue
  • 47. LYMPHOCYTE  Diameter: small 7-9 large 12-16  Cytoplasm: medium blue  Granules: small agranular large a few primary granules  Nucleus: dark blue round dense chromatin
  • 49. MONOCYTE  Diameter: 14-20  Cytoplasm : grey blue  Granules: dust-like lilac color granules  Nucleus: blue large irregularly shaped and folded
  • 52. LEFT-SHIFT AND RIGHT-SHIFT OF NEUTROPHIL: Left-shift: non-segmented neutrophil > 5% Right-shift: hypersegmented neutrophil >3%