Post on 15-Jan-2017
TOTAL LEUCOCYTE COUNTTOTAL DIFFERENTIAL COUNT
Dr Neha MahajanMD Pathology
Haematopoeisis
GRANULOPOEISIS
Type of WBC’sGranulocytes—have large granules in their cytoplasm
Neutrophils( 40 to 75%) Eosinophils(1 to 6%) Basophils(0 to 1%)
Types of WBC’s Agranulocytes—do not
have granules in their cytoplasm
Lymphocytes(20 to 40%) Monocytes( 2 to 10%)
Granuloctyes Neutrophils
Stain light purple with neutral dyes Granules are small and numerous—
course appearance Several lobes in nucleus 65% of WBC count Diapedesis,inflammation
Granulocytes Eosinophils or Acidophils:
Large, numerous granules Nuclei with two lobes 2-5% of WBC count Found in lining of respiratory and digestive
tracts Protections against infections caused by
parasitic worms and involvement in allergic reactions
Secrete anti-inflammatory substances in allergic reactions
Basophils Least found- 0.5 to 1% Contain histamine,serotonin,heparin—
inflammatory chemical
Agranulocytes Lymphocytes
Smallest WBC Large nuclei/small amount of
cytoplasm Account for 25% of WBC count Two types—T lymphocytes—attack an
infect or cancerous cell, B lymphocytes—produce antibodies
against specific antigens (foreign body)
Agranulocytes Monocytes
Largest of WBCs Dark kidney bean shaped nuclei Highly phagocytic
TOTAL LEUCOCYTE COUNT
WHITE CELL COUNT (WBC)
White cell count (WBC) is the total number of leukocytes in a volume of blood, expressed as thousands/µl.
WBC can be done by manual methods or by automated cell counters.
Normal Values:• Newborn 9.0-30.0 x 103/μl• 1 week 5.0-21.0 x 103/μl• 1 month 5.0-19.5 x 103/μl• 6-12 months 6.0-17.5 x 103/μl• 2 years 6.2-17.0 x 103/μl• Child/adult 4.8-10.8 x 103/μl
PRINCIPLE OF WBCS COUNT TEST
Free-flowing capillary or well-mixed anticoagulated venous blood is added to a diluent) at a specific volume in the thoma pipette.
The diluent lyses the erythrocytes but preserves leukocytes and stains the nuceli.
The diluted blood is added to the hemacytometer chamber.
Specimen: EDTA- anticoagulated blood or capillary blood is
preferred.
Reagents, supplies and equipment: White blood cells count diluting fluid
Turks' solution which is formed of: Glacial acetic acid 3 ml Crystal violet 1 ml 100 ml distilled water.
EQUIPMENT1. White blood cells count diluting
fluid2. Thoma white pipette3. Hemacytometer and coverslip4. Microscope5. Lint-free wipe6. Alcohol pads
haemocytometer chamber
Thoma white pipette
Rubber sucking tube
HEMACYTOMETER
The hemacytometer counting chamber is used for cell counting.
It is constructed so that the distance between the bottom of the coverslip and the surface of the counting area of the chamber is 0.1 mm.
The surface of the chamber contains two square ruled areas separated by an H-shaped moat.
HEMACYTOMETER
PROCEDURE
1. Draw the blood up to 0.5 mark in the thoma pipette.
2. Wipe the outside of the capillary pipette to remove excess blood that would interfere with the dilution factor.
3. Holding the pipette almost vertical place into the fluid. Draw the diluting fluid into the pipette slowly until the mixture reaches the 11 mark, while gently rotating the pipette to ensure a proper amount of mixing.
4. Place the pipette in a horizontal position and firmly hold the index finger of either hand over the opening in the tip of the pipette, detach the aspirator from the other end of the pipette now the dilution of the blood is completed
PROCEDURE
5. Mix the sample for at least 3 minutes to facilitate hemolysis of RBCs.
6. Clean the hemacytometer and its coverslip with an alcohol pad and then dry with a wipe.
7. Before filling the chamber, discard the first four to five drops of the mixture on apiece of gauze to expel the diluent from the stem.
PROCEDURE
8. Carefully charge hemacytometer with diluted blood by gently squeezing sides of reservoir to expel contents until chamber is properly filled.
PROCEDURE FOR COUNTING WBC’S
1. Under 10 x magnifications, scan to ensure even distribution. Leukocytes are counted in all 4 large squares of counting chamber.
2. Count cells starting in the upper left large corner square. Move to the upper right corner square, bottom right corner square, bottom left corner square and end in the middle square.
3. Count all cells that touch any of the upper and left lines, do not count any cell that touches a lower or right line.
CALCULATIONSDilution factor 20Volume= Area x depthTLC/uL= No of WBCx Correction for Volume X
dilution No of large squares (4) = N x 20 x10 4 = N x 50
Corrected TLCDiluting fluid does not lyse nucleated
RBC`s/erythroblastsFalsely counted as WBC Corrected TLC/uL= TLC x 100 NRbc/100 Wbc+ 100
WHITE BLOOD CELL DIFFERENTIAL COUNT
DEFINITION
The relative percentage of each type of white blood cells in peripheral blood.
This experiment is a part of blood routine test.
PERIPHERAL BLOOD SMEAR A properly prepared blood smear is
essential to accurate assessment of cellular morphology
The wedge smear is the most convenient and commonly used technique for making PBS
PERIPHERAL BLOOD SMEARWedge technique of
making PBS
A. Correct angle to hold spreader slide
B. Blood spread across width of slide
C. Completed wedge smear
PERIPHERAL BLOOD SMEAR Characteristics:
It is smooth without irregularities, holes, or streaks
When the slide is held up to light, the featheredge of the smear should have a “rainbow” appearance
The whole drop is picked up and spread Well-made PBS
tail body head
PERIPHERAL BLOOD SMEAR Examples of unacceptable smears
PERIPHERAL BLOOD SMEAR Examples of unacceptable smears
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
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
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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 pinkWBC: nuclei is purple to blue
cytoplasm is pink to tan granules is lilac to violet
Eosinophil: granules orange Basophil: granules dark blue to black
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Optimal Assessment Area:1. RBCs are uniformly and singly distributed2. Few RBC are touching or overlapping3. Normal biconcave appearance
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PRINCIPLE
White Blood Cells1. 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.
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MANUAL DIFFERENTIAL
Red Blood Cells, Examine for: 1. Size and shape ( Anisocytosis,Poikilocytosis2. Relative hemoglobin content. 3. Polychromatophilia. 4. Inclusions. 5. Rouleaux formation or agglutination
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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. • To do a WBC estimate by taking the average number of
white cells and multiplying by 2000.
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PLATELET ESTIMATION UNDER 100X1. 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.
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Platelets per oil immersion field (OIF)
1) <8 platelets/OIF = decreased
2) 8 to 20 platelets/OIF = adequate
3) >20 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
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MICROSCOPIC EXAM
10× (low fold): overall smear quality, rouleaux, agglutination or parasites
100× (oil Len): WBC Diff, RBC morphology
RBC Morphology WBC- Total count Differential count Platelets Abnormal cells Parasites
Peripheral smear reporting
Normal blood smear
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NORMAL NEUTROPHIL COUNT (40 TO 75%) NEUTROPHILIA
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Absolute neutrophil count greater than 7500/uL
CausesAcute bacterial infections-
abscesses,pneumonia,meningitis,UTITissue necrosis- burns,injury,MIAcute blood lossAcute haemorrhageMyeloproliferative disordersPosisoning
NEUTROPENIA Absolute netrophil count less than 2000/uL Mild- 2000 to 1000/uL Moderate-1000 to 500/uL Severe- < 500/uLCAUSESI )Decreased or ineffective production in bone
marrow Infections- bacterial,protozoal,viral Haematologic disorders- megaloblastic
anemia,aplastic anemia,aleukemic leukemia Drugs Ionising radiation Congenital disorders
II) Increased destruction in peripheral bloodNeonatal isoimmune neutropeniaSystemic lupus erythematosusFelty`s syndromeIII) Increased sequestration in spleenHypersplenism
EOSINOPHILA
Absolute eosinophil count greater than 600/uL
CAUSES1.Allergic diseases-Asthma,rhinitis,urticaria
2.Skin diseases-Eczema,pemphigus,Dermatitis herpetiformis
3.Parasitic infections with tissue invasion- filariasis,trichinosis,echinoccocoosis
4.Hematologic disorders-MPD,Hodgkins disease,Peripheral T cell lymphoma
5.Carcinoma with necrosis6.Radiation therapy7.Lung diseases- loefflors syndrome,tropical
eosinophilia8.Hypereosinophilia syndrome
MONOCYTOSIS Increase in absolute monocyte count >
1000/uLCauses Infections-TB,SABE,Malaria,Kala Azar Recovery from neutropenia Autoimmmune disorders Hematologic diseases- MPD,Monocytic
leulemia,hodgkins disease Others-ulcerative colitis,chron`s
disease,sarcoidosis
LYMPHOCYTOSIS Absolute lymphocyte count more than upper
limit of normal for age( 4000/uL in adults,>7200/uL in adolescents,>9000/uL in children and infants)
CausesInfections-Viral- acute infectious
lymphocytosis,neoatitis,CMV,rubella,mumps,varicella
Bacterial- pertussis,TBProtozoal- toxoplasmosis
Hematological disorders-ALL, CLL, Multiple myeloma, Lymphoma Others-Serum sickness, post vaccination, drug
reactions
PLATELETS Small,1 to 3 um in diameter,purple structures
with tiny irregular projections on surface Occur in clumps Pseudothrombocytopenia Platelet sateletism
SUMMARY Normal haematopoeisis
Total leucocyte Count
Manual differential countPeripheral smearInterpretation
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