Title: Dr'R'Thamilselvi, MD',
1- Dr.R.Thamilselvi, MD.,
- Associate Professor,
- VMKVMC
2Haematology
- Study of the formed cellular blood elements
- Blood is composed of a Liquid called Plasma of
cellular elements (RBCS, WBCS Platelets)
3Blood plasma is the liquid component of blood, in
which the blood cells are suspended.
4Blood serum is blood plasma without fibrinogen
or the other clotting factors.
5How to approach
- Medical history Physical examination
- Select appropriate tests
- Cost- effective
- Specific test
6To diagnose various disorders
- Disorder of blood cells
- RBC Eg anemia, polycythemia
- WBC Eg leukemia,leukopenia
- Platelets Eg thrombocytopenia, thrombocytosis
- Disorder of clotting factors
- Infections
- Malaria
- Babesiosis
- Microfilaria
7Specimen collection
- Phlebotomy
- Anticoagulants
- EDTA (Lavender)-CBC
- Sodium citrate- (light blue) - Coagulation
Profile - Heparin (Green) Osmotic fragility
8Collection of Blood
9Ethylene diamine Tetra-acetic Acid (EDTA )
- This is the anticoagulant of choice for the FBC.
- di-Na and di-K salts are solids and tri-Na is the
liquid form. - Action - EDTA chelates calcium ions to form a
soluble complex - Uses
- Haematology Profile
- EDTA blood smears
- Concentration1.5mg/mL /- 0.35mg/mL
- Disadvantages
- EDTA cannot be used for coagulation studies (as
it chelates calcium) - Platelets can sometimes be seen to satellite
neutrophils
10Sodium Citrate
- This is a liquid anticoagulant.Mode of
ActionRemoves calcium ions by forming a soluble
calcium citrate complex.Uses - Coagulation studies  91 - bloodcitrate
- ESR Â 41 - bloodcitrate
- Reticulocyte count
- Heinz body detection
- Acts as both a diluent and an anticoagulant
- Concentration0.109mg/mL
- Disadvantages
- Cannot use for FBC because of the dilution factor
11Heparin
- This anticoagulant is an acid mucopolysaccharide
- Action- Prevents the formation of thrombin from
prothrombin therefore stopping formation of
fibrin from fibrinogen - Uses
- Enzyme studies
- Cell cultures
- Osmotic fragility testing
- Concentration15IU/mL /- 2.5IU/mLDisadvantages
- Relatively Expensive
- Can give a blue background to blood films
- Platelet aggregation
12Bedside Lab Tests
- Hb
- CBC
- Total WBC Count
- Total RBC Count
- Differential Count
- Platelet count
- Hematocrit
- Red cell Indices
- ESR
- Reticulocyte count
- Peripheral smear Examination
13In cases of bleeding disorder
- Screening tests
- 1. Platelet count
- 2.Bleeding Time
- 3. Clotting Time
- Special tests
- 1. Prothrombin Time (PT)
- 2. Activated Partial Thromboplatsin Time (APTT)
- 3. Thrombin Time (TT)
- 3. Factor assay
14Haemoglobin estimation
- Physical Based on Specific gravity
- Chemical Based on Iron content of Hb
- Gasometric-Based on O2 combining capacity of Hb
- Calorimetric-Based on colour
- Photoelectric Cynmethhemoglobin method
- Automated methods
15Sahlis Haemoglobinometer
16Procedure
- Take N/10 HCL in the tube up to lowest mark.
- Fill the Hb pipette with 0.02ml of blood wipe
off the excess blood at nozzle and transfer it to
the tube. - Mix the acid and blood by shaking the tube well
with stirrer - Allow it to stand for 10 minutes to allow brown
colour to develop (acid haematin) - Now dilute the solution with distilled water
adding few drops. - Mix the solution well and match the colour with
the comparator. - The lower meniscus is noted and reading on the
tube is read as gm/dl.
17Cyanmethaemoglobin methodPRINCIPLE
- Blood is diluted in a solution of potassium
ferricyanide and potassium cyanide. The
ferricyanide oxidizes haemoglobin to
methaemoglobin. - Potassium cyanide provides cyanide ions to form
Cyanmethaemoglobin. - The absorbance of the solution is then measured
in a spectrophotometer at a wavelength of 540 nm
or in a colorimeter using a yellow-green filter.
18Procedure
- Take 20 microlitres of well mixed anticoagulated
venous blood in a glass tube and to this add 5ml
of Drabkins solution. Stopper the tube, invert
it several times to mix well. Allow it to stand
at room temperature for 3-10minutes - Absorbance is measured against reagent blank at
540nm either in a spectrophotometer or in a
photoelectric colorimeter with suitable filter. - Hicn standard after bringing it to room
temperature is taken and the absorbance measured
using the same instrument.
19Photoelectric colorimeter withgreen filter or at
a wavelength of 540nm
20RESULT
- Calculated by using the formulae
- Hb gm/dl
- ABSORBANCE OF TEST / ABSORBANCE OF STANDARD X
CONC. OF STANDARD. - ADVANTAGES
- All forms of Hb except SHb are readily converted
to HiCN. - Direct comparison with HiCN standard possible.
- Easy to perform the test.
- Reagents are readily available.
- The standard is stable.
21DISADVANTAGES
- Increased absorbance not due to hemoglobin may be
turbidity due to abnormal plasma proteins,
hyperlipaemia, high WBC count or fat. - Potassium cyanide in the solutions is poisonous,
though it is present only in a low concentration
hence the reagent is not handled carefully. - Explosion can occur if undiluted reagents are
poured in the sink. Hydrogen cyanide is released
by acidification and the gas if it accumulates
can result in explosion.
22Total WBC count
- Visual haemocytometric method
- Electronic method
- Instruments WBCpipette, Neubauerchamber,Lancet,
cotton, Micro-scope, Cover slip and WBC diluting
fluid (Turkes fluid)
23Total WBC count
- Composition - Turks fluid
- Glacial acetic acid - 3ml to lyse RBCs
- 1Gentian violet - 2ml to stain the WBC
nuclei - Water - 100ml
24Procedure- Total WBC count
- Suck the blood from finger prick or
anticoagulated blood up to 0.5 in WBC pipette - Wipe tip and outside the pipette
- Draw diluting fluid up to mark 11 in the WBC
pipette - Mix well by rotating the pipette for 2-3 minutes
- Discard 2 drops of the mixture from the WBC
pipette - Charge the Neubauer chamber
25Procedure-
26Neubauer Chamber - Total WBC count -Counting
areas (Blue)
27Calculation-
- No. of WBCs in 4 large squares N
- Dilution 1 in 20 or 1/20 (11-1/0.5)
- Depth 0.1mm or 1/10
- No.of WBC's in 1 cu.mm Nx20x10
- 4
- Nx200
/ 4
- Nx50
- NORMAL VALUES
- Adults ? 4,000 to 11,000 cells/cu.mm
- At birth ? 10,000 to 26,000 cells/cu.mm
- Childhood ? 6,000 to 15,000 cells/cu.mm
28 Causes Aplastic anaemia Typhoid Drugs R
adiation therapy Cytotoxic therapy Subleukemic
leukemia
Causes Exercise Leukemoid reaction
Bacterial
and viral infection Infectious mononucleosis
29Total RBC count
- Instruments
- RBC pipette, Neubauer chamber, Microscope,
cotton, lancet, spirit, RBC diluting fluid
(Hayems fluid) - Hayems Fluid
- Mercuric chloride 0.25gm
? Antiseptic - Sodium chloride 0.5 gm
? provides correct osmotic pressure - Sodium sulphate 2.5 gm
? provides correct osmotic pressure - Distilled water
100ml ?Solvent
30Procedure
- Methods -Visual haemocytometric method
- -Electronic method
- Draw the blood from finger prick or
anticoagulated blood up to 0.5 in RBC pipette - Draw diluting fluid up to mark 101 in the RBC
pipette - Mix well by rotating the pipette for 2-3 minutes
- Charge the Neubauers chamber after discarding
few drops (Diluting fluid is not mixed with
blood) - Allow the cells to settle down for 2 minutes.
- Count RBCs under high power in counting squares
in the centre of the chamber.
31Neubauer Chamber - Total RBC count -Counting
areas (Orange)
32Calculations
- Number of cells/cu.mm No.of cells counted
-
----------------------- -
Dilution x chamber depth x chamber area - Cells counted N
- Dilution 1/200 (101-1/0.5)
- Chamber depth 1/10 mm
- Area counted 80 / 400 1/5 sq.mm
- N
- Total RBCs/cu.mm --------------------
-
1/200x1/10x1/5 -
20x10x5N10,000 N - Area of central large square 1 sq.mm
- Area of a medium sized square -1/25 sq.mm
- Area of the 5square used in counting RBC is
1/25x51/5sq.mm
33SOURCES OF ERROR
- I.False high counts
- Inadequate wiping of excess of blood from the tip
- Blood drawn above the mark 0.5
- Diluting fluid not drawn upto mark 101
- Improper mixing
- II.False low counts
- Blood not drawn up to the mark 0.5
- Diluting fluid drawn above the mark 101
- Undue delay in counting of cells
- Faulty technique of counting
34Normal Values
- Adult male 4.5 to 5.5 million/cu.mm
- Adult female 3.8 to 5.2 million/cu.mm
- At birth 4.0 to 6.0million/cu.mm
- Increased cell count
- Physiological -At birth
- Pathological Haemoconcentration
Diarrhea
Dehydration - Cyanotic heart
diseases - Chronic lung
diseases - Polycythemia vera
- Decreased cell count
- -Anaemia
- -Haemodilution
35Differential count
- First clean the finger with cotton and spirit.
- Puncture the pulp of the index finger.
- Wipe the first drop because it will contain
tissue fluid. - Keep one drop of blood in the end of a glass
slide. Now spread the blood in to a thin smear
with a spreader slide and keeping the spreader
slide at 45
36Differential count
37Differential count
- Dry the smear and stain with Leishman stain.
- A good smear must be tongue shape, should be
evenly spread, should occupy one third of the
slide (it should not be too long or too short)
38Staining procedure
- Take leishman Stain and Pour drop by drop and
cover the smear. - Wait for 2 minutes for fixation of smear by
Methyl alcohol. - Fixation means the methyl alcohol in the smear
denatures the proteins and prevents haemolysis
when the smear comes in contact with water and
makes the smear stick to glass slide while
washing with distilled water. - Wait for two minutes, add equal amount of
distilled water and wait for 5-10 mins. - Wash the slide with distilled water or tap water
try the smear and examine it under oil immersion
objective.
39Differential count
40Normal values
- Neutrophils 50- 75
- Lymphocytes 25 45
- Monocytes 3-8
- Eosinophils 1-6
- Basophils 0-1
41Haematocrit (PCV)
- Percentage of erythrocytes in a known volume of
whole blood - Useful Anaemia Polcythaemia
- Wintrobes tube filled with anticoagulated blood
centrifuged at 3500rpm for 30 minutes. - The volume occupied by the erythrocytes is
expressed as a percentage of the total volume.
42Centrifuge - PCV
43Centrifuge - PCV
Plasma colour Clear -
Normal Yellow-Indirect
jaundice Pink
-Haemolysis Turbid
Hyperlipediamias
44PCV
- Normal values
- Males 40 to 55
- Females 35 to 48
- Infants 45 to 60
- Clinical significance
- Increase PCV Polycythemia, dehydration,
burns, and shock. - Decrease PCV Anaemia, pregnancy.
- Sources of error
- Sample
- -Increased amount of EDTA
- -Inadequate mixing of blood
- Tubes
- -Variation in the bore size
- -Improper filling of the tube
45Red cell indices
- MCV
- MCH
- MCHC
- Useful for Morphological classification of
Anaemias
46The Three Derived Indicies
MCV Hct RBC x 10 90 fl MCH Hb RBC x
10 30 pg MCHC Hb Hct x 100 33
47- Normal values
- Â MCV - 81 to 85 flÂ
- MCH - 29 to 32 pgÂ
- MCHC - 31 to 33
48Erythrocyte Sedimentation Rate
- The rate at which the RBCs settle from the
plasma. - Stage I- Rouleaux formation(Aggregation)
- RBCs come together like piles of coins, last for
10 mts. - Stage II- Stage of sedimentation
- RBCs settle at a constant rate-last for 30 mts.
- Stages III -Stage of packing
- Packing of RBCs occurs last for 10 mts.
- Methods Westergren Wintrobes
49Erythrocyte Sedimentation Rate
50Procedure
- Take 1.6ml of blood in a vial
- Add 0.4ml of anticoagulant and mix
- Draw the blood up to the 0 mark in the tube
- The tube is set up in the rack perfectly
vertical. - Start a stop watch or clock and take reading
- The reading corresponding to the upper layer of
the RBC column in the pipette is taken. - Normal
- Male 0-10mm/hr
- Female 0-20mm/hr
51Factors Influencing ESR
- Rouleaux formation -? ESR
- Ratio of red cells to plasma
- When plasma is more - ? ESR
- When plasma is less - ? ESR
- Length of the tube-
- If length of the tube is more ESR low
- If length of the tube is short -ESR ?
- Bore of the tube
- If the bore of the tube is more ? ESR will be
more - If the bore of the tube is less ? ESR will be
less - Position of the tube
- Deviation from vertical position ? ESR
- ? Plasma globulin and Fibrinogen ? ESR
- ?Plasma globulin and Fibrinogen decreased ?ESR
52Interpretation -
- This is not a specific test.
- An increase in ESR usually seen in chronic
inflammatory conditions like tuberculosis,
rheumatoid arthritis or malignancy. - The test is useful in following disease activity
or response to treatment once a diagnosis is
made.
53Platelet count
- Venous blood(Avoid finger prick blood),RBC
Pipette , Neubauer Chamber Microscope ,
Disposable syringe, Spirit , Cotton,Cover slip - Diluting Fluid for Platelet Count
- 3 sodium citrate containing 1 formalin also can
be used as diluting fluid. It, however, does not
lyse the red blood cells.
54Rees Ecker Diluting Fluid Composition
- S No Chemical Amount Use of the Chemical
- 1.Trisodium Citrate3.gms- Anticoagulant
- 2.Neutral Formaldehyde0.2 ml - Fixes the Platelet
- 3.Brilliant Cresyl Blue0.1 Gm - Stains the
Platelet and Gives background - 4.Deionised water100ml - Dissolves the chemicals
- The other diluting fluid which lyses the red
cells is 1 (w/v) ammonium oxalate.
55Calculations
- Platelets per cu mm (µl) (Number of platelets
counted x Dilution) / (Volume of fluid) - Where,
- a) Dilution 200
- b) Depth of the chamber 0.1
- c) Volume of fluid 1 x 0.1 0.1 cu mm
- d) Platelets per cu mm (µl) (Number of
platelets x 200) / 0.1 - Number of platelets x 2000
56Abnormalities Of Platelet Count
- Normal 1,50,000 4,00,000/cu mm (µl).
- Increased Platelet count
- Chronic Myeloid leukaemia
- Acute hemorrhage
- Decreased Platelet Count
- ITP , DIC
- Autoimmune disease like Systemic Lupus
Erythematosis - Viral infecton
57Peripheral Smear
- First clean the finger with cotton and spirit.
- Puncture the pulp of the index finger.
- Wipe the first drop because it will contain
tissue fluid. - Keep one drop of blood in the end of a glass
slide. - Now spread the blood into a thin smear with a
spreader slide and keeping the spreader slide at
45 - Dry the smear and stain with Leishman stain.
- A good smear must be tongue shape, should be
evenly spread, should occupy one third of the
slide
58PS
59Staining procedure
- Take leishman Stain and Pour drop by drop and
cover the smear. - Wait for 2 minutes for fixation of smear by
Methyl alcohol. - Wait for two minutes, add equal amount of
distilled water and wait for 5-10 mins. - Wash the slide with distilled water or tap water
try the smear and examine it under oil immersion
objective.
60- A Normal mature Lymphocyte is seen on the left
compared to a segmented PMN on the right. An RBC
is seen to be about 2/3 the size of a normal
lymphocyte
61- Identify the Segmented Neutrophil, Band
Neutrophil, Lymphocyte, Monocyte, Eosinophil,
Basophil, and Platelet in the image below
62- The RBC's in the background appear normal. The
important finding here is the presence of many
PMN's. An elevated WBC count with mainly
neutrophils suggests inflammation or infection. A
very high WBC count (gt50,000) that is not a
leukemia is known as a "leukemoid reaction". This
reaction can be distinguished from malignant
WBC's by the presence of large amounts of
leukocyte alkaline phosphatase (LAP) in the
normal neutrophils.
63- The RBC's here have stacked together in long
chains. This is known as "rouleaux formation" and
it happens with increased serum proteins,
particularly fibrinogen and globulins. Such long
chains of RBC's sediment more readily. This is
the mechanism for the sedimentation rate, which
increases non-specifically with inflammation and
increased "acute phase" serum proteins.
64RBC MORPHOLOGICAL ABNORMALITIESSICKLE CELLS
- MorphologySickle shaped red cells
- Found inHb-S disease
65RBC MORPHOLOGICAL ABNORMALITIESTEAR DROP CELLS
- MorphologyRed cells shaped like a tear drop or
pear - Found inBone marrow fibrosisMegaloblastic
anaemiaIron deficiencyThalassaemia
66RBC MORPHOLOGICAL ABNORMALITIESMALARIAL PARASITE
(P. falciparum)
- MorphologyRing form of Pl falciparum in red
cells. Delicate rings with 1 or 2 chromatin dots.
Often more than one ring in a red cell. Accolé
forms are found. - Found inMalaria
67- The RBC's here are smaller than normal and have
an increased zone of central pallor. This is
indicative of a hypochromic (less hemoglobin in
each RBC) microcytic (smaller size of each RBC)
anemia. There is also increased anisocytosis
(variation in size) and poikilocytosis (variation
in shape).
68- This Hypersegmented Neutrophil is present along
with Macro-ovalocytes in a case of pernicious
anemia. Compare the size of the RBC's to the
lymphocyte at the lower left center.
69- There are numerous fragmented RBC's seen here.
Some of the irregular shapes appear as "helmet"
cells. Such fragmented RBC's are known as
"schistocytes" and they are indicative of a
Microangiopathic hemolytic anemia (MAHA) or other
cause for intravascular hemolysis. This finding
is typical for disseminated intravascular
coagulopathy (DIC).
70- The WBC's seen here are "atypical" lymphocytes.
They are atypical because they are larger (more
cytoplasm) and have nucleoli in their nuclei. The
cytoplasm tends to be indented by surrounding
RBC's. Such atypical lymphocytes are often
associated with Infectious Mononucleosis.
71- Here is another example of Sickled Erythrocytes
in a patient with Hgb SS who presented with
severe abdominal pain in sickle crisis. The
sickled cells are prone to stick together,
plugging smaller vessels and leading to decreased
blood flow with ischemia.
72WBC MORPHOLOGICAL ABNORMALITIESTOXIC GRANULATION
- MorphologyIncreased granulation. Granulation
more basophilic and larger than normal. - Found inSevere bacterial infectionNon specific
finding - seen in tissue damage of various
types.Normal pregnancyTherapy with cytokines
73WBC MORPHOLOGICAL ABNORMALITIESDOHLE BODIES
- MorphologySmall pale blue cytoplasmic
inclusions, often in the periphery of the cell. - Found inInfective and inflammatory
statesSevere burnsTuberculosisPost
chemotherapyPregnancy
74- ACUTE LYMPHOBLASTIC LEUKEMIA L1
75- These mature lymphocytes are increased markedly
in number. They are indicative of Chronic
Lymphocytic Leukemia, a disease most often seen
in older adults. This disease responds poorly to
treatment, but it is indolent.
76ACUTE MYELOID LEUKEMIA
77- There are numerous granulocytic forms seen here,
including immature myeloid cells and bands. This
condition is one of the Myeloproliferative states
and is known as chronic myelogenous leukemia
(CML) that is most prevalent in middle-aged
adults. A useful test to help distinguish this
disease is the leukocyte alkaline phosphatase
(LAP) score, which should be low with CML and
high with a leukemoid reaction.
78PLATELET MORPHOLOGICAL ABNORMALITIESGIANT
PLATELETS
- MorphologyPlatelet larger than a normal red
cell. - Found inIncreased platelet turnoverMyeloprolife
rative disordersMyelodysplastic disorders
79Anaemia First Test
- Fragments of nuclear material
- RNA strands which stain blue
- New Methylene Blue or Brilliant cresyl Blue
Normal Less than 2
80Reticulocyte
No definite nucleus Reticulum of RNA Deep blue
staining Light blue cytoplasm Cell size about 10 µ
81Reticulocytes
Leishmans
Supravital
82Reticulocyte Production Index
- For example the RPI is calculated as follows
- Reticulocyte count 9
- Hb content 7.5 g
- Correction for Anaemia
- 9 x (7.5 15) 9 x 0.5 4.5
- Correction for increased life span
- 4.5 2 2.25
- 3. Thus, the RPI is 2.25
83Reticulocytes
Reticulocyte
84RETICULOCYTOSIS
85Types of Anaemia
86Causes of Anaemia
- Decreased production of Red Cells
- - Hypo proliferative, marrow failure
- Increased destruction of Red Cells
- - Hemolysis (decreased survival of RBC)
- Loss of Red Cells due to bleeding
- - Acute / chronic blood loss (hemorrhagic)
87Hypoproliferative Anaemias
88Anaemia
Hb lt 12, Hct lt 38
Hemolytic
Hypoproliferative
RPI lt 2
RPI gt 2
89Workup Second Test
- The next step is What is the size of RBC ?
- MCV indicates the Red cell volume (size)
- Both the MCH MCHC tell Hb content of RBC
- If the RPI is 2 or less
- We are dealing with either
- Hypoproliferative anaemia (lack of raw material)
- Maturation defect with less production
- Bone marrow suppression (primary/ secondary)
90Red Cell Size
91Mean Cell Volume (MCV)
- RBC volume (rather) is measured by
- The Mean Cell Volume or MCV and RDW
92Anaemia Workup - MCV
93Anaemia Workup 3rd TestPeripheral Smear Study
- Are all RBC of the same size ?
- Are all RBC of the same normal discoid shape ?
- How is the colour (Hb content) saturation ?
- Are all the RBC of same colour/ multi coloured ?
- Are there any RBC inclusions ?
- Are intra RBC there any hemo-parasites ?
- Are leucocytes normal in number and D.C ?
- Is platelet distribution adequate ?
94Coulter counter
95Principle of Coulter
96- This is Normal data from a complete blood count
as performed on an automated instrument,
including an automated WBC differential count.
97- Here is data from a CBC in a person with Iron
Deficiency Anemia. Note the low hemoglobin (HGB).
Microcytosis is indicated by the low MCV (mean
corpuscular volume). Hypochromia correlates here
with the low MCH (mean corpuscular hemoglobin).
98- The CBC here shows a markedly increased MCV,
typical for megaloblastic anemia. The MCV can be
mildly increased in persons recovering from blood
loss or hemolytic anemia, because the newly
released RBC's, the reticulocytes, are increased
in size over normal RBC's, which decrease in size
slightly with aging.
99- The CBC of a patient with Microangiopathic
Hemolytic Anemia (MAHA) demonstrates a markedly
increased RDW (red cell distribution width) due
to the marked variation in size and shape of the
RBC population.
100- Here is the CBC of a person with a severe anemia
who underwent transfusion. This accounts for the
dual RBC population as seen in the graph at the
lower left. A reticulocytosis in response to
anemia has also increased the MCV.
101What is Anaemia ?
- Important to remember
- Anemia is a clinical sign of disease
- It is not a single disease by itself
- Need to look for the underlying cause !
- Will we ignore a fever without investigation ?
- Its diagnosis is not that simple !! Well make it
- Its very common and imp. in our practice
- Drug Rx. depends on the cause
102Definition of Anaemia
- Decrease in the number of circulating red blood
cell mass or Low Hb and there by O2 carrying
capacity - Most common hematological disorder
- Almost always a secondary disorder
- As such, critical for all practitioners to know
how to evaluate / determine its cause / treat
103(No Transcript)
104Bleeding time
- Is the duration of bleeding from a standard
puncture wound in the skin to stop bleeding. - It is a measure of platelet count, platelet
function, as well as integrity of vessel wall. - This is one of the common preoperative
investigations done before surgery. - DUKES METHOD
- A small cut is made with a lancet in the Ear
lobe or finger tip. Blood flow from the puncture
is and the time taken for the bleeding to stop is
measures with a stop watch which is taken as
BLEEDING TIME
105 Uses Diagnosis of Bleeding Disorder. Before
Surgery. Before any tooth extraction Before
Liver or pleural or Bone marrow Puncture
Bleeding time-Dukes , IVYs Template md
106Bleeding time
- Normal BT - 1-6 mints.
- Above 10 mints is abnormal
- Prolonged bleeding time
- Thrombocytopenia ( Decreased Platelet count)
- Defect in platelet function( Thromboasthenia)
- Drugs heparin and Aspirin
- Other method - IVYS METHOD
107Clotting time
- The time taken for the given blood to clot is
called Clotting time. - It is a measure of plasma clotting factors.
- It is a screening test for coagulation disorders.
- Methods - 1. Capillary tube method of Wright
- 2. Lee White Method
108Capillary tube method of Wright
- Materials RequiredCapillary tube,Spirit,Cotton
,LancetStop Watch - Procedure
- First clean the pulp of the finger
- Prick the Finger
- Once bleeding starts start the stop watch and
note the time. - Collect the bleeding blood in capillary tubes.
- Seal the ends of the capillary tubes with
plasticine - Once in every 30 seconds break one capillary tube
until a thread like clot is seen between the
broken ends. - Now note the time and this gives the CLOTTING
TIME - Normal Value for this method 5-10 mins
109Lee White Method
- Sprit,Cotton ,Lancet,Stop Watch,Test tubes,Water
bathDisposable syringe - Principle- Intravenous blood when collected and
kept out side the body in a test tube it forms a
solid clot. The time taken to form solid clot is
measured as CLOTTING TIME.
110Lee Whites Method
- Take three test tubes .and put 1ml of blood in
each test tube - Place the test tube in a stand for 10 mins.
(Waterbath at 37degree) - After 10 mins take the first tube and gently tap
every 30 seconds to test for clotting - Once the blood in the first tube is found to be
clotted, note the time - Now take the second tube and start tapping every
30 seconds, till the blood clots - Then repeat the same with the third tube. Note
the time. - The time interval is taken as clotting time
111Lee Whites Method
112Normal (4 11 minutes)
- PROLONGED CLOTTING TIME
- Hemophilia
- VonWillibrand Disease.
- Vit K Deficiency
- DECREASED CLOTTING TIME
- Corticosteroid treatment
- Drugs like epinephrine
113THANK YOU