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Title: Examination%20of%20Peripheral%20Blood%20Smear

1
Examination of Peripheral Blood Smear

Dr S Homathy

Complete blood count
The most common test used in clinical medicine
Determine type and severity of blood cell
abnormalities
Nowadays, CBC is fully automated and highly
reproducible.
Correct interpretation of automated CBC can
reduce rate of unnecessary blood smear
examination
Provide useful information for provisional
diagnosis of RBC and WBC diseases

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A well Made and well Stained Smear can provide

Estimates of cell count
Proportions of the different types of WBC
Morphology

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Preparation of blood smear

There are three types of blood smears
The cover glass smear.
The wedge smear .
The spun smear.
The are two additional types of blood smear used
for specific purposes
Buffy coat smear for WBCs lt 1.0109/L
Thick blood smears for blood parasites .

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Peripheral Blood Smear

Objective
1. Specimen Collection
2. Peripheral Smear Preparation
3. Staining of Peripheral Blood Smear
4. Peripheral Smear Examination

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Specimen Collection

Venipuncture
should be collected on an EDTA (Disodium or
Tripotassium ethylene diamine tetra-acetic acid)
Tube
EDTA liquid form preferred over the powdered
form
Chelates calcium

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Specimen Collection

Advantages
Many smears can be done in just a single draw
Immediate preparation of the smear is not
necessary
Prevents platelet clumping on the glass slide

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Specimen Collection

Disadvantages
PLATELET SATELLITOSIS
causes pseudothrombocytopenia and
pseudoleukocytosis
Cause Platelet specific auto antibodies that
reacts best at room temperature

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Specimen Collection

Platelet satellitosis

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Peripheral Smear Preparation

Wedge technique
Coverslip technique
Automated Slide Making
and Staining

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Peripheral Smear Preparation

Wedge technique
Push Type wedge preparation
Pull Type wedge prepartion
Easiest to master
Most convenient and most commonly used technique

Material needed
Glass slide 3 in X 1in
Beveled/chamfered edges

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Peripheral Smear Preparation
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Peripheral Smear Preparation

Procedures
Drop 2-3 mm blood at one end of the slide
Diff safe can be used
a. Easy dropping
b. Uniform drop

Precaution
Too large drop too thick smear
Too small drop too thin smear

The pusher slide be held securely with the
dominant hand in a 30-45 deg angle.
- quick, swift and smooth gliding motion to the
other side of the slide creating a wedge smear

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

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Peripheral Smear Preparation
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Peripheral Smear Preparation

Precautions
Ensure that the whole drop of blood is picked
up and spread
Too slow a slide push will accentuate poor
leukocyte distribution, larger cells are pushed
at the end of the slide
Maintain an even gentle pressure on the slide
Keep the same angle all the way to the end of
the smear.

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Peripheral Smear Preparation

Precautions
Angle correction
1. In case of Polycythemia
high Hct
angle should be lowered
- ensure that the smear made is not to
thick
2. Too low Hct
Angle should be raised

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Feature of a Well Made Wedge Smear

Smear is 2/3 or 3/4 the entire slide
Smear is finger shaped, very slightly rounded at
the feathery edge
widest area of examination
Lateral edges of the smear visible
Should not touch any edge of the slide.

Should be margin free, except for point of
application
Smear is smooth without irregularities, holes or
streaks
When held up in light
feathery edge should show rainbow appearance
Entire whole drop of blood is picked up and spread

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Cover Slip Technique
rarely used
used for Bone marrow aspirate smears
Advantage
excellent leukocyte distribution
Disadvantage
labeling, transport, staining and storage is a
problem

22 x 27mm clean coverslip
More routinely used for bone marrow aspirate
Technique
1. A drop of marrow aspirate is placed on top
of 1 coverslip
2. Another coverslip is placed over the other
allowing the aspirate to spread.
3. One is pulled over the other to create 1
thin smears
4. Mounted on a 3x1 inch glass slide

Precautions
Very light pressure should be applied between the
index finger and the thumb
Crush preparation technique
Too much pressure causes rupture of the cells
making morphologic examination impossible
Too little pressure prevents the bone spicules
from spreading satisfactorily on the slide

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tail body head
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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.

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Common causes of a poor blood smear

Drop of blood too large or too small.
Spreader slide pushed across the slide in a jerky
manner.
Failure to keep the entire edge of the spreader
slide against the slide while making the smear.
Failure to keep the spreader slide at a 30 angle
with the slide.
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

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Biologic causes of a poor smear

Cold agglutinin
RBCs will clump together.
Warm the blood at 37 C for 5 minutes, and then
remake the smear.
Lipemia
holes will appear in the smear.
There is nothing you can do to correct this.
Rouleaux
RBCs will form into stacks resembling coins.
There is nothing you can do to correct this

Automatic Slide Making and Staining
SYSMEX 1000i

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Peripheral Smear Preparation

Drying of Smears
Fan
Heating pans
No breath blowing of smears may produce
crenated RBCs or develop water artifact (drying
artifact)

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Slide fixation and staining
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Romanowsky staining

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

Pure Wright stain or Wright Giemsa stain
Blood smears and bone marrow aspirate

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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.

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Features of a well-stained PBS

Macroscopically color should be pink to purple
Microscopically
RCS orange to salmon pink
WBC nuclei is purple to blue
cytoplasm is pink to tan
granules is lilac to violet
Eosinophil granules orange
Basophil granules dark blue to black

Optimal Assessment Area
RBCs are uniformly and singly distributed
Few RBC are touching or overlapping
Normal biconcave appearance
200 to 250 RBC per 100x OIO

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Trouble shooting

Macroscopic
Overall bluer color increased blood proteins
(multiple myeloma, rouleaux formation)
Grainy appearance RBC agglutination (cold
hemagglutinin diseases)
Holes increased lipid
Blue specks at the feathery edge Increased WBC
and Platelet counts

Microscopic
10x Objective
Assess overall quality of the smear i.e feathery
edge, quality of the color, distributin of the
cells and the lateral edges can be checked for
WBC distribution
Snow-plow effect more than 4x/cells per field on
the feathery edge Reject
Fibrin strands Reject
Rouleaux formation, large blast cell assessment

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Too acidic Suitable
Too basic
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Too Acid StainRBC too pale, WBC barely visible
insufficient staining time
prolonged buffering or washing
old stain
Correction
lengthen staining time
check stain and buffer pH
shorten buffering or wash time

Too Alkaline StainRBC gray, WBC too dark,
Eosinophil granules are gray
thick blood smear
prolonged staining
insufficient washing
alkaline pH of stain components
heparinized sample
Correction
check pH
shorten stain time
prolong buffering time

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Problem encountered during staining

Water artifact
moth eaten RBC,
heavily demarcated central pallor on the RBC
surface,
crenation,
refractory shiny blotches on the RBC

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What contributes to the problem
humidity in the air as you air dry the slides.
Water absorbed from the humid air into the
alcohol based stain
Solution
Drying the slide as quickly as possible.
Fix with pure anhydrous methanol before staining.
Use of 20 v/v methanol

AUTOMATED SLIDE STAINERS
It takes about 5-10 minutes to stain a batch of
smears
Slides are just automatically dipped in the stain
in the buffer and a series of rinses
Disadvantages
Staining process has begun, no STAT slides can be
added in the batch
Aqueous solutions of stains are stable only after
3-6 hours

QUICK STAINS
Fast, convenient and takes about 1 minute to be
accomplished
Modified Wrights-Giemsa Stain, buffer is aged
distilled water
Cost effective
Disadvantage
Quality of stains especially on color acceptance
For small laboratories and for physicians clinic
only

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Manual differential
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Principle

White Blood Cells
Check for even distribution and estimate the
number present (also, look for any gross
abnormalities present on the smear).
Perform the differential count.
Examine for morphologic abnormalities.

Red Blood Cells, Examine for
Size and shape ( Anisocytosis,Poikilocytosis
Relative hemoglobin content.
Polychromatophilia.
Inclusions.
Rouleaux formation or agglutination
Platelets.
Estimate number present.
Examine for morphologic abnormalities.

Observations Under 10X
Check to see if there are good counting areas
available free of ragged edges and cell clumps.
Check the WBC distribution over the smear.
Check that the slide is properly stained.
Check for the presence of large platelets,
platelet clumps, and fibrin strands.

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WBC estimation Under 40X

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.

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Platelet estimation Under 100X

Use the oil immersion lens estimate the number of
platelets per field.
Look at 5-6 fields and take an average.
Multiply the average by 20,000.
Note any macroplatelets.

Platelets per oil immersion field (OIF)
lt8 platelets/OIF decreased
8 to 20 platelets/OIF adequate
gt20 platelets/OIF increased

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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

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

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Determine a quantitative scale
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Left-shift non-segmented neutrophil gt 5
Increased bands Means acute infection, usually
bacterial

Right-shift hypersegmented neutrophil
Increased hypersegmented neutrophile

Leukocytosis, a WBC above 10,000, is usually due
to an increase in one of the five types of white
blood cells
Neutrophilic leukocytosis- neutrophilia
Lymphocytic leukocytosis - lymphocytosis
Eosinophilic leukocytosis - eosinophilia
Monocytic leukocytosis - monocytosis
Basophilic leukocytosis- basophilia

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Morphology of WBC

Normal blood smear

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Segmented neurophile

Diameter 12-16
Cytoplasm pink
Granules primary
secondary
Nucleus dark purple blue
dense chromatin
2-5 lobes

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Eosinophil

One eosinophil - mature. Normal blood - 100X.
Orange colour granules.
Bi-lobed nucleus

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Basophil

One mature basophil.
Blackish granules overlying the nucleus

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Normal lymphocytes

Lymphocytes are the smallest WBC.
They have large condensed nucleus, with a scanty
bluish cytoplasm.

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Normal monocyte

Monocytes are the largest WBC.
The nucleus is slightly indented .
The cytoplasm is abundant, sky blue in colour.
Some have vacuoles in the cytoplasm.

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Red cells

Normal red cells or erythrocytes show only slight
variation in size and shape.
The blood film should be examined in the area
where the red cells are touching but not often
overlapping.

In this area many red cells have an area of
central pallor which may be up to a third of the
diameter of the cell.
This is consequent on the shape of a normal red
cell, which resembles a disc that is thinner in
the centre.

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Summarizing RBC Parameters

RBC Count )RBC x 1012/L)
Hb (g/dl)
Hct (5 or L/L)
Mean Cell Volume (MCV. Fl)
Mean Cell Hb (MCH, pg)
Mean Cell Hb Concentration (MCHC. , g/dl)

RBC distribution
Morphology
Size
Shape
Inclusions
Young rbcs
Color
Arrangement

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Platelets

Normal platelets are also apparent.
They are small anuclear fragments between the red
cells containing small purple-staining granules.

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Platelet aggregates

Platelet aggregates may be
composed of
apparently intact platelets,
degranulated pale grey platelets
or a mixture of both, as in this example.
If the platelet count is low it is essential to
examine the blood film carefully for platelet
aggregates

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Platelet satellitism

Platelet satellitism describes the phenomenon of
adherence of platelets to white cells.
It is an in vitro phenomenon of no clinical
significance.
However it is important that it is detected since
the platelet count will be factitiously low.

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Staining of Peripheral Blood Smear
HEMA-TEK STAINER
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Component of automated CBC

Blood count basic parameters
Hb, Hct,RBC, WBC, platlet.
Red cell indices MCV, MCH, MCHC, RDW
WBC differentials
Cytogram or Scattergram
Reticulocyte count

Red cell parameters
Direct Measurement
Erythrocyte Concentration (RBC) x 106/ml
Mean Corpuscular Volume (MCV) Femtolitre (fl)
Hemoglobin (Hb) Gram/decilitre (g/dl)
Indirect Measurement
Hematocrit (Hct) RBC x MCV/10
Mean Corpuscular Hemoglobin (MCH) HB x 10 /
RBC (pg)
Mean Corpuscular Hemoglobin Concentration (MCHC)
Hb/Hct x 100 (g/dl)
Red Cell Distribution Width (RDW)

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Reticulocyte count

Reticulocyte
non-nucleated RBC with polyribosomal RNA
as stained by supravital stain (new methylene
blue or brilliant cresyl blue)
Polychromasia underestimates Reticulocytes
Three methods of reticulocyte Enumeration
Manual count on slide per 1,000RBC
Automated CBC with reticulocyte counter (Coulter
VCS, Cell-Dyne 4000, Technicon-H3)
Flow cytometry with fluorescent dyes

RBC disorders
Hypochromic microcytic anemia
Iron deficiency anemia
Thalassemia and hemoglobinopathy
Macrocytic anemia
Megaloblastic anemia
Non-megaloblastic macrocytic anemia

Hemolytic anemia
Immune hemolytic anemia AIHA, DHTR
Microangiopathic hemolytic anemia (MAHA)
Red cell enzymopathies G-6-PD deficiency
RBC membrane defects spherocytosis,
ovalocytosis, elliptocytosis, stomatocytosis
RBC inclusion bodies and parasites

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WBC disorders
Leukopenia
with absolute neutropenia bone marrow failure,
agranulocytosis
with atypical lymphocytes viral infection,
chronic lymphoproliferative disorders
with immature myeloid cells acute leukemia, MDS
or myelopthisis