ABC of automated CBC
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Apr 28, 2015
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About This Presentation
Automation in cell counting
Slide Content
ABC
of automated
CBC
Dr.ParthS.Kaneria
ShantiPathology Lab Junagadh
of automated
CBC
Dr.ParthS.Kaneria
ShantiPathology Lab Junagadh
Pathology in old days
Antonivan Leeuwenhoek
Antonivan Leeuwenhoek
Wallace H. Coulter an electrical engineer and businessman
while working with the US Navy in the late 1940s developed
and first applied the Coulter Principle.
Man who changed the world of counting...
while working with the US Navy in the late 1940s developed
and first applied the Coulter Principle.
Man who changed the world of counting...
Advantages
•Speed with efficient handling of large number of
samples.
•Accuracy and precision in
quantitative blood tests.
•Ability to perform multiple
tests on a single platform.
•Significant reduction of labor
requirements.
•Invaluable for accurate determination
of red cell indices.
•Speed with efficient handling of large number of
samples.
•Accuracy and precision in
quantitative blood tests.
•Ability to perform multiple
tests on a single platform.
•Significant reduction of labor
requirements.
•Invaluable for accurate determination
of red cell indices.
Disadvantages
•Flagging of a laboratory test result demands labour
intensive manual examination of a blood smear
•Comments on red cell
morphology cannot begenerated
•Platelet Clumps are counted as
single,so low count.
•Erroneously increased or
decreased results due to
interfering factors
•Expensive with high running costs
•Flagging of a laboratory test result demands labour
intensive manual examination of a blood smear
•Comments on red cell
morphology cannot begenerated
•Platelet Clumps are counted as
single,so low count.
•Erroneously increased or
decreased results due to
interfering factors
•Expensive with high running costs
TYPES OF AUTOMATED ANALYSER
Three part Five Part Seven Part
Differentiate cells
into three categories
1.Granulocytes
2.Lymphocytes
3.Monocytes/mixed
cells
Differentiatecells
into the five basic
leukocyte types
1.Neutrophils
2.Eosinophils
3.Basophils
4.Lymphocytes
5.Monocytes
In additionare able to
distinguish
1.Nucleated RBCs,
2Abnormal and
atypical cells and
immature cells
Three part Five Part Seven Part
Differentiate cells
into three categories
1.Granulocytes
2.Lymphocytes
3.Monocytes/mixed
cells
Differentiatecells
into the five basic
leukocyte types
1.Neutrophils
2.Eosinophils
3.Basophils
4.Lymphocytes
5.Monocytes
In additionare able to
distinguish
1.Nucleated RBCs,
2Abnormal and
atypical cells and
immature cells
Counting Chambers
RBC/Platelet Chamber
WBC Chamber
Differential Chamber
ReticulocyteChannel
RBC/Platelet Chamber
WBC Chamber
Differential Chamber
ReticulocyteChannel
General Principles
•Introduction to Instrumentation
–Basic principles used :
•Electronic Impedance
•Radiofrequency
•Optical Scatter
a.Laser light scatter
b. Flow cytometry
c. Chemical dye method
•Introduction to Instrumentation
–Basic principles used :
•Electronic Impedance
•Radiofrequency
•Optical Scatter
a.Laser light scatter
b. Flow cytometry
c. Chemical dye method
The Coulter Principle
•The poorly conductive blood cells are suspended in a
conductive diluent(liquid).
•The diluentis passed through an electric field created
between two electrodes.
•The liquid passes through a small aperture (hole).
•The passage of each particle through the aperture
momentarily increases the impedance (resistance) of
the electrical path between the electrodes.
•The increase in impedance creates a pulse that can be
measured.
•The number of pulses = blood cell count
•The amplitude (height) of the pulse = Volume of cell
•The poorly conductive blood cells are suspended in a
conductive diluent(liquid).
•The diluentis passed through an electric field created
between two electrodes.
•The liquid passes through a small aperture (hole).
•The passage of each particle through the aperture
momentarily increases the impedance (resistance) of
the electrical path between the electrodes.
•The increase in impedance creates a pulse that can be
measured.
•The number of pulses = blood cell count
•The amplitude (height) of the pulse = Volume of cell
Electronic Impedance:
Disrupts electrical current by displacing fluid proportional
to the size of the cell.
Disrupts electrical current by displacing fluid proportional
to the size of the cell.
Computing and generation of graph
•Each pulse is recorded as
an oscillation , the height
of which is proportional to
the volume and size of the
cell.
•These oscillations are
rearranged according to
volume interval to form a
histogram.
•Each pulse is recorded as
an oscillation , the height
of which is proportional to
the volume and size of the
cell.
•These oscillations are
rearranged according to
volume interval to form a
histogram.
Optical Scatter
Low angle scatter 2
o
-3
o
(Volume)
High angle scatter 5
o
-15
o
Forward-angle light scatter (FALS)
Illuminating beam that has been bent to a small angle from
direction of the original beam .It measures size or volume of cells
o
-3
o
(Volume)
High angle scatter 5
o
-15
o
Forward-angle light scatter (FALS)
Illuminating beam that has been bent to a small angle from
direction of the original beam .It measures size or volume of cells
Side scatter (SSC)
•The illuminating beam that is scattered by particle
to an angle of 90* from the illuminating beam.
•This depends on cell's surface texture and internal
structure as well as to its size and shape and
granularity.
•It is sometimes referred to as a granularity signalor
an orthogonal light scatter signal.
•The illuminating beam that is scattered by particle
to an angle of 90* from the illuminating beam.
•This depends on cell's surface texture and internal
structure as well as to its size and shape and
granularity.
•It is sometimes referred to as a granularity signalor
an orthogonal light scatter signal.
Forward-angle light scatter
correlates to cell volume/size
Side scatter
correlates to degree of internal
complexity (granules and nucleus)
correlates to cell volume/size
Side scatter
correlates to degree of internal
complexity (granules and nucleus)
Radiofrequency
( impedance)
Impedance -size cells
Conductivity (RF) –proportional to cell
interior density (granules and nucleus)
Five-part WBC differential
•Scatter plot (RF X DC)
•Computer cluster analysis provides
absolute counts
( impedance)
Impedance -size cells
Conductivity (RF) –proportional to cell
interior density (granules and nucleus)
Five-part WBC differential
•Scatter plot (RF X DC)
•Computer cluster analysis provides
absolute counts
ERRORS
1. Recirculation error
Cells that re circulate through the edge of an electrical
field produce an aberrant impulse, which is smaller than
cell passing through the aperture.
2. Coincidence error
Cells that pass through theaperture simultaneously, or
almost so, are counted and sized as a single large cell
called coincidence.
3. Non central flow error
Cell pass through the aperture off centre produce
aberrant impulses and appear larger than their actual size
1. Recirculation error
Cells that re circulate through the edge of an electrical
field produce an aberrant impulse, which is smaller than
cell passing through the aperture.
2. Coincidence error
Cells that pass through theaperture simultaneously, or
almost so, are counted and sized as a single large cell
called coincidence.
3. Non central flow error
Cell pass through the aperture off centre produce
aberrant impulses and appear larger than their actual size
1.Recirculation error
2. Coincidence error
3. Non central flow error
How to over come such errors ?
2. Coincidence error
3. Non central flow error
How to over come such errors ?
Hydrodynamic focusing and Laminar flow
COULTER VS FLOWCYTOMETER
•The Coulter-type volume signal is proportional
to the volume of a particle as well as to its
electrical characteristics.
•In flow cytometersignal is proportional to the
cross-sectional area of a particle as well as to
its refractive index.
•The Coulter-type volume signal is proportional
to the volume of a particle as well as to its
electrical characteristics.
•In flow cytometersignal is proportional to the
cross-sectional area of a particle as well as to
its refractive index.
PRINCIPLES
•Principles of Measurement
–Direct Measurement:
•RBC –Impedance, hydrodynamic
focusing
•WBC -Impedance, hydrodynamic
focusing
•Platelets –Impedance (2-20 fl),
hydrodynamic focusing
•Hgb–mod. Cyanmethemoglobin(525
nm)
•MCV –mean RBC volume (histogram)
–Indirect Measurement:
•Hct, MCHC, and MCH (calculations)
–RDW and MPV (CV of respective histograms)
–WBC differential
•VCS –volume, conductivity, scatter
•employs differential shrinkage
–Reticulocyte
•Supravitalstain
•Fluorescent detection
•Flags
•Principles of Measurement
–Direct Measurement:
•RBC –Impedance, hydrodynamic
focusing
•WBC -Impedance, hydrodynamic
focusing
•Platelets –Impedance (2-20 fl),
hydrodynamic focusing
•Hgb–mod. Cyanmethemoglobin(525
nm)
•MCV –mean RBC volume (histogram)
–Indirect Measurement:
•Hct, MCHC, and MCH (calculations)
–RDW and MPV (CV of respective histograms)
–WBC differential
•VCS –volume, conductivity, scatter
•employs differential shrinkage
–Reticulocyte
•Supravitalstain
•Fluorescent detection
•Flags
TWO SIDES OF INSTRUMENTS
(THREE PART INSTRUMENTS)
RBC SIDE WBC SIDE
(DILu-1:50,000) (DILu-1:500)
>30 fl size 2-30 fl size lysingreagent
RBC PLETELET
35-90 fl 90-160 fl 160-450 fl
Lymphocytes Mononuclear cells Granulocytes
Monocytes
Eosinophils Neutrophils
Basophils
(THREE PART INSTRUMENTS)
RBC SIDE WBC SIDE
(DILu-1:50,000) (DILu-1:500)
>30 fl size 2-30 fl size lysingreagent
RBC PLETELET
35-90 fl 90-160 fl 160-450 fl
Lymphocytes Mononuclear cells Granulocytes
Monocytes
Eosinophils Neutrophils
Basophils
ErythroidParameters
•Measured parameters:
Hemoglobin
RBC count
MCV
RDW
•Calculated parameters
•These are calculated values and depend on the values that go into their
calculation.
•HCT(%) = MCV x RBC concentration
•MCH(pg) = Hbconcentration / RBC concentration
•MCHC(g/dl) = Hbconcentration / HCT
•Measured parameters:
Hemoglobin
RBC count
MCV
RDW
•Calculated parameters
•These are calculated values and depend on the values that go into their
calculation.
•HCT(%) = MCV x RBC concentration
•MCH(pg) = Hbconcentration / RBC concentration
•MCHC(g/dl) = Hbconcentration / HCT
Hemoglobin Estimation
•Estimated from a part of the blood mixed with lysing
agent to lysethe RBCs.(the same can be used for
WBC counts)
Lyse treated blood
Cyanide Solution
added
Cyanmeth
hemoglobin method
Sodium LaurylSulphate
added
Sulphmethhomoglobin
method
•Estimated from a part of the blood mixed with lysing
agent to lysethe RBCs.(the same can be used for
WBC counts)
Lyse treated blood
Cyanide Solution
added
Cyanmeth
hemoglobin method
Sodium LaurylSulphate
added
Sulphmethhomoglobin
method
HGBColorimetryfor HB estimation
X axis: Volume of cells
Y axis: No. of cells
LD: 25-75 fLUD: 200-250 fL
RBC Histogram
Median =MCV
+1SD
Y axis: No. of cells
LD: 25-75 fLUD: 200-250 fL
RBC Histogram
Median =MCV
+1SD
RBC-and PLT-Histograms
1.Platelets have a size between 8 and 12 fl and are counted
between 2 and 30 fl.
2.Erythrocytes have a size of 80-100 fl and are counted
between 25 and 250 fl.
1.Platelets have a size between 8 and 12 fl and are counted
between 2 and 30 fl.
2.Erythrocytes have a size of 80-100 fl and are counted
between 25 and 250 fl.
The Size Distribution Curve should always start on
the base line and fall between the lower and the
upper discriminator.
the base line and fall between the lower and the
upper discriminator.
Histograms FLAGS Interpretation
Erythrocyte histogram Flagging
Possible causes:
•Giant platelets
•Microerythrocytes
•Fragmentocytesor dysplastic RBC
•Platelet clumps
Mark “ RL “, abnormal height at lower discriminator
LD
RBC
PLT
LD
RBC
The curve does not start at the basis line.
Possible causes:
•Giant platelets
•Microerythrocytes
•Fragmentocytesor dysplastic RBC
•Platelet clumps
Mark “ RL “, abnormal height at lower discriminator
LD
RBC
PLT
LD
RBC
The curve does not start at the basis line.
Erythrocyte histogram Flagging
Note:
All results marked with “ RL “ should be controlled.
Explanation:
RBC agglutination might cause a low incorrect RBC count and effect also the
parameter Hb, MCV, MCH and MCHC. In case of cold agglutinates warm the
sample up to 37°C.
(MCHC should drop back to normal value if the problem is solved)
Mark “ RU “, abnormal height at upper discriminator.
UD
RBC
The curve does not end at the base line.
UD
RBC
Possible causes:
•Cold agglutination
•RBC agglutination
•Rouleuxformation
Note:
All results marked with “ RL “ should be controlled.
Explanation:
RBC agglutination might cause a low incorrect RBC count and effect also the
parameter Hb, MCV, MCH and MCHC. In case of cold agglutinates warm the
sample up to 37°C.
(MCHC should drop back to normal value if the problem is solved)
Mark “ RU “, abnormal height at upper discriminator.
UD
RBC
The curve does not end at the base line.
UD
RBC
Possible causes:
•Cold agglutination
•RBC agglutination
•Rouleuxformation
Possible causes:
•Iron deficiency in recovery (therapy)
•Dimorphic picture
•Multiple RBC transfusions
•Extreme leukocytosis(> 600 x 10³/µl)
Mark “ MP “: multiple peak of RBC histogram
RBC
Note:
Parameter: RBC, MCV, RDW-SD & RDW-CV are flagged.
Explanation:
Often: Extreme anisocytosis is found. In case of anisocytosis the RBC result is not
affected.
Seldom: extreme high numbers of leukocytes may cause high incorrect RBC results.
Thereforeall RBC parameters should be controlled.
•Iron deficiency in recovery (therapy)
•Dimorphic picture
•Multiple RBC transfusions
•Extreme leukocytosis(> 600 x 10³/µl)
Mark “ MP “: multiple peak of RBC histogram
RBC
Note:
Parameter: RBC, MCV, RDW-SD & RDW-CV are flagged.
Explanation:
Often: Extreme anisocytosis is found. In case of anisocytosis the RBC result is not
affected.
Seldom: extreme high numbers of leukocytes may cause high incorrect RBC results.
Thereforeall RBC parameters should be controlled.
RDW-CV (%) = 100 x
s/µ
µ = L2 + L1 / 2
s = L2 –L1 / 2
100 %
L1µ
Turning points
Normal value: 11 -16 %
100 %
20 %
RDW-SD is calculated in
20 % of the total height of
the distribution curve.
Normal value: 37 -46 fl
Clinical relevant > 60 fl
Erythrocyte histogram Distribution width (RDW)
RDW-CV
RDW-SD
L2
Note:
RDW-CV can be used as a marker for anisocytosis
Note:
RDW-SD can be used as a marker for anisocytosis
s/µ
µ = L2 + L1 / 2
s = L2 –L1 / 2
100 %
L1µ
Turning points
Normal value: 11 -16 %
100 %
20 %
RDW-SD is calculated in
20 % of the total height of
the distribution curve.
Normal value: 37 -46 fl
Clinical relevant > 60 fl
Erythrocyte histogram Distribution width (RDW)
RDW-CV
RDW-SD
L2
Note:
RDW-CV can be used as a marker for anisocytosis
Note:
RDW-SD can be used as a marker for anisocytosis
Mark “DW “: abnormal histogram distribution (distribution width)
(only RDW-SD or RDW-CV is flagged)
RBCRBC
Explanation:
The flag “DW” is shown in case of abnormal histogram curve.
The overall height of the curve represents 100%. The width is
calculated on the 20% line of the curve. If the histogram curve does
not match the 20% line either on the lower (RL) or upper (RU)
discriminator. The flag “DW” is generatedfor RDW-SD or RDW-
CV and these results can not be calculated.
Possible causes:
•same as RL or RU
Histogram curve does not match
the 20% line twice
(only RDW-SD or RDW-CV is flagged)
RBCRBC
Explanation:
The flag “DW” is shown in case of abnormal histogram curve.
The overall height of the curve represents 100%. The width is
calculated on the 20% line of the curve. If the histogram curve does
not match the 20% line either on the lower (RL) or upper (RU)
discriminator. The flag “DW” is generatedfor RDW-SD or RDW-
CV and these results can not be calculated.
Possible causes:
•same as RL or RU
Histogram curve does not match
the 20% line twice
100 fl
100 fl
Left shift in MicrocyticAnaemia
Right shift in MacrocyticAnaemia
100 fl
Left shift in MicrocyticAnaemia
Right shift in MacrocyticAnaemia
Cold agglutinins
Because in this case erythrocytes have passed
through the detector as clusters of several cells, the
RBC, HCT,MCH, MCV, MCHC and RDW values
are abnormal. The RBC histogram shows a second
peak.
Because in this case erythrocytes have passed
through the detector as clusters of several cells, the
RBC, HCT,MCH, MCV, MCHC and RDW values
are abnormal. The RBC histogram shows a second
peak.
Calculating reported parameters
•MPV Mean of 2D-PLT Volhistogram
(Mean Platelet Volume)
•LargeP-LCR Platelets with volumes greater than 20 fL
(LargePlatelets)
The Platelet Method
•MPV Mean of 2D-PLT Volhistogram
(Mean Platelet Volume)
•LargeP-LCR Platelets with volumes greater than 20 fL
(LargePlatelets)
The Platelet Method
•The histogram curve should lay within the lower and upper
platelet discriminator (PL & PU) and start and end on the
base line.
•PLT counted between 2 fl and 30 fl.
1 flexible Discriminator PL 2 to 6 fl.
1 flexible Discriminator PU 12-30 fl.
1 fixed Discriminator at 12 fl
Thrombocyte histogram
platelet discriminator (PL & PU) and start and end on the
base line.
•PLT counted between 2 fl and 30 fl.
1 flexible Discriminator PL 2 to 6 fl.
1 flexible Discriminator PU 12-30 fl.
1 fixed Discriminator at 12 fl
Thrombocyte histogram
Parameter of the thrombocyte
histogram
MPV=mean PLT volume
reference range: 8 -12 fl
P-LCR=ratio of large platelets
Reference range 15 -35 %
Increase could be a sign
for:
•PLT Clumps
•Giant PLT
•Microerythrocytes
12 fl
LD UD
PLT P-LCR
100 %
20 %
Pct (%)
PLT (x 10
3
/µl)
MPV (fl) =
PDW= platelet distribution width
calculated at 20 % of peakheight
Reference range: 9 -14 fl
Increase could be a sign for:
•PLT Clumps
•Microerythrocytes
•Fragments
histogram
MPV=mean PLT volume
reference range: 8 -12 fl
P-LCR=ratio of large platelets
Reference range 15 -35 %
Increase could be a sign
for:
•PLT Clumps
•Giant PLT
•Microerythrocytes
12 fl
LD UD
PLT P-LCR
100 %
20 %
Pct (%)
PLT (x 10
3
/µl)
MPV (fl) =
PDW= platelet distribution width
calculated at 20 % of peakheight
Reference range: 9 -14 fl
Increase could be a sign for:
•PLT Clumps
•Microerythrocytes
•Fragments
Note :
Check blank (background check)!
Initiate auto rinse or check sample.
Explanation:
In case of high background numbers (blank), check reagent for
contamination (bacteria). Check expiry date.
In order the background check is within range, the patient
sample should be checked –platelet results might be incorrect
high due to cell fragments or bacteria's. In some cases also
platelet aggregates might cause the problem. In this case the
histogram curve would also show an abnormal distribution at
the upper discriminator. Platelet aggregation might cause low
incorrect platelet results.
Flag display: mark „PL“ is shown with higher priority than
„PU“.
Mark “ PL “, abnormal height at lower discriminator
Possible cause:
•High blank value
•Cell fragments
•High numbers of bacteria
•Contaminated reagent
•Platelet aggregation
PLT
The curve does not start at the basis line.
Thrombocyte histogram Flagging
Check blank (background check)!
Initiate auto rinse or check sample.
Explanation:
In case of high background numbers (blank), check reagent for
contamination (bacteria). Check expiry date.
In order the background check is within range, the patient
sample should be checked –platelet results might be incorrect
high due to cell fragments or bacteria's. In some cases also
platelet aggregates might cause the problem. In this case the
histogram curve would also show an abnormal distribution at
the upper discriminator. Platelet aggregation might cause low
incorrect platelet results.
Flag display: mark „PL“ is shown with higher priority than
„PU“.
Mark “ PL “, abnormal height at lower discriminator
Possible cause:
•High blank value
•Cell fragments
•High numbers of bacteria
•Contaminated reagent
•Platelet aggregation
PLT
The curve does not start at the basis line.
Thrombocyte histogram Flagging
Mark “ PU “: abnormal height at upper discriminator
Explanation:
In case of platelet aggregation, the PLT count is false low. Check EDTA incombatibility–e.g. re-
collect the sample and use citrate as anticoagulant to avoid clogging caused by EDTA.
In case of giant platelets, the PLT count might be incorrect low. PLT results should be confirmed
with alternative methods: e.g. chamber counting.
Possible Cause :
•PLT clumps
EDTA-incombatibility
Clotted sample
•Giant Platelets (False low)
•Microerythrocytes(False High)
•Fragmentocytesor dysplastic RBC
Explanation:
In case of platelet aggregation, the PLT count is false low. Check EDTA incombatibility–e.g. re-
collect the sample and use citrate as anticoagulant to avoid clogging caused by EDTA.
In case of giant platelets, the PLT count might be incorrect low. PLT results should be confirmed
with alternative methods: e.g. chamber counting.
Possible Cause :
•PLT clumps
EDTA-incombatibility
Clotted sample
•Giant Platelets (False low)
•Microerythrocytes(False High)
•Fragmentocytesor dysplastic RBC
Possible Cause:
•Platelet anisocytosis
•Recovery after
chemotherapy
•Platelet aggregation
•Platelet transfusion
Mark “ MP “: multi peaks in PLT histogram
Note:
Parameter: PLT, MPV, PDW and P-LCR is flagged.
Explanation:
In case of platelet anisocytosisthe PLT result is not affected.
Seldom: Multiple peaks can be seen in some cases of platelet aggregation (jagged
curve). In case of PLT aggregation the PLT result might be incorrect low. Therefore
recollect the sample, In case of EDTA incompatibility sodium citrate as anticoagulant
can prevent platelet clumping.
•Platelet anisocytosis
•Recovery after
chemotherapy
•Platelet aggregation
•Platelet transfusion
Mark “ MP “: multi peaks in PLT histogram
Note:
Parameter: PLT, MPV, PDW and P-LCR is flagged.
Explanation:
In case of platelet anisocytosisthe PLT result is not affected.
Seldom: Multiple peaks can be seen in some cases of platelet aggregation (jagged
curve). In case of PLT aggregation the PLT result might be incorrect low. Therefore
recollect the sample, In case of EDTA incompatibility sodium citrate as anticoagulant
can prevent platelet clumping.
WBC Histogram
The distribution curve should be within the discriminators. The curve
should start and end at the basis line.
• The LD is flexible, but can not be lower than 30 fl.
• The WBC-channel shows Leukocytes and Thrombocytes
( Erythrocytes are lysed).
• The volume of the Thrombocytsis usually between 8 -12 fl, therefore
the LD at the WBC-Histogrammseperatesthe Leukocytes from the
Thrombocytes. (Thrombocyteswere not counted).
should start and end at the basis line.
• The LD is flexible, but can not be lower than 30 fl.
• The WBC-channel shows Leukocytes and Thrombocytes
( Erythrocytes are lysed).
• The volume of the Thrombocytsis usually between 8 -12 fl, therefore
the LD at the WBC-Histogrammseperatesthe Leukocytes from the
Thrombocytes. (Thrombocyteswere not counted).
Flag “ WL “, Curve does not begin at the basis line
Possible causes :
• PLT Clumps EDTA-Incombatibilitycoagulated Sample
• High osmotic resistant (Erythrocytes not lysed)
• Erythroblasts
• Cold agglutinate
Possible causes :
• PLT Clumps EDTA-Incombatibilitycoagulated Sample
• High osmotic resistant (Erythrocytes not lysed)
• Erythroblasts
• Cold agglutinate
Flag “ WU “, Curve does not end at the base line.
High leukocyte count
High leukocyte count
T1 and T2 are valley discriminators defined by the plateau.
This discriminators separates the Leukocytes populations.
• The discriminators are flexible and will be set automatically
according the sample.
• In special cases is a separation from the valley
discriminators not possible.
This discriminators separates the Leukocytes populations.
• The discriminators are flexible and will be set automatically
according the sample.
• In special cases is a separation from the valley
discriminators not possible.
T1 could not be detected
High no. of large or atypical
lymphocytes
T1 was detected but not T2
Neutrophilichypolobation
eg. PelgerHuetand
pseudo PelgerHuetanomaly.
High no. of large or atypical
lymphocytes
T1 was detected but not T2
Neutrophilichypolobation
eg. PelgerHuetand
pseudo PelgerHuetanomaly.
This is a case of WBC agglutination, which occurs rather
rarely. The histogram does not show a clear tri-modal pattern,
with particles present in the region above 250 fl . The count of
leukocytes is likely to be falsely low. Depending on the nature
of leucocytes antibodies, agglutination may be dissolvable and
measurement may become possible upon incubation the at
37 o C or upon washing the samples with isotonic saline.
rarely. The histogram does not show a clear tri-modal pattern,
with particles present in the region above 250 fl . The count of
leukocytes is likely to be falsely low. Depending on the nature
of leucocytes antibodies, agglutination may be dissolvable and
measurement may become possible upon incubation the at
37 o C or upon washing the samples with isotonic saline.
The valley between the erythrocytes ghost area and the small
leucocytes area exceeds the limit, and WL flags are given.
NRBC are likely to contribute significantly to the population
on the WBC histogram, therefore most of them are counted as
leukocytes. corrected by the following equation:
corrected WBC Count = measured WBC Count x 100
(100 + NRBC count )
NRBC Count: The number of NRBC per 100 leukocytes.
leucocytes area exceeds the limit, and WL flags are given.
NRBC are likely to contribute significantly to the population
on the WBC histogram, therefore most of them are counted as
leukocytes. corrected by the following equation:
corrected WBC Count = measured WBC Count x 100
(100 + NRBC count )
NRBC Count: The number of NRBC per 100 leukocytes.
ABN / INDICATOR PROBABLE
CAUSE
COMMENT
WBC histogram
(lymph peak) does
not start at baseline
Giant platelets,
NRBC, Pltclumping
Review smear,
correct WBC for
NRBC
Elevation of left
portion of
granulocyte
Left Shift Review smear
Elevation of right
portion of
granulocyte peak
Neutrophilia Review smear
WBC Histogram
CAUSE
COMMENT
WBC histogram
(lymph peak) does
not start at baseline
Giant platelets,
NRBC, Pltclumping
Review smear,
correct WBC for
NRBC
Elevation of left
portion of
granulocyte
Left Shift Review smear
Elevation of right
portion of
granulocyte peak
Neutrophilia Review smear
WBC Histogram
Fivegroupsofleukocytes(stained)
What’s 5AND 7-part diff?
Neutrophil Eosinophil Basophil
Lymphocyte Monocyte
What’s 5AND 7-part diff?
Neutrophil Eosinophil Basophil
Lymphocyte Monocyte
VCS Technology
COULTER TECHNOLOGY
VOLUME
As opposed to using 0ø light loss to estimate cell
size,VCSutilizes the Coulter Principle of (DC)
Impedance to physically measure the volume that the
entire cell displaces in an isotonic diluent.
This method accurately sizes all cell types regardless
of their orientation in the light path.
As opposed to using 0ø light loss to estimate cell
size,VCSutilizes the Coulter Principle of (DC)
Impedance to physically measure the volume that the
entire cell displaces in an isotonic diluent.
This method accurately sizes all cell types regardless
of their orientation in the light path.
CONDUCTIVITY
Alternating current in the radio frequency (RF) range
short circuits the bipolar lipid layer of a cell's
membrane allowing the energy to penetrate the cell.
This powerful probe is used to collect information
about cell size and internal structure, including
chemical composition and nuclear volume.
Alternating current in the radio frequency (RF) range
short circuits the bipolar lipid layer of a cell's
membrane allowing the energy to penetrate the cell.
This powerful probe is used to collect information
about cell size and internal structure, including
chemical composition and nuclear volume.
LASER LIGHT SCATTER
When a cell is struck by the coherent light of a
LASER beam, the scattered light spreads out in all
directions.
Using a proprietary new detector, median angle light
scatter (MALS) signals, are collected to obtain
information about cellular granularity, nuclear
lobularityand cell surface structure
When a cell is struck by the coherent light of a
LASER beam, the scattered light spreads out in all
directions.
Using a proprietary new detector, median angle light
scatter (MALS) signals, are collected to obtain
information about cellular granularity, nuclear
lobularityand cell surface structure
3-D Cellular Analysis-VCS
Gate Software Technology
NORMAL DATAPLOT
DOT plot or Scattergram
Better Abnormal Cell Detection
LEUKOPENIA & THROMBOCYTOPENIA
NEW PARAMETERS
•Nucleated RBCs
•Immature granulocyte
•Haematopoiticprogenitor cells
•Immature reticulocytefraction
•RBC fragments (schistoytes)
•Reticulated platelets
•Reticulocyteindics
•Malarial parasites
•Nucleated RBCs
•Immature granulocyte
•Haematopoiticprogenitor cells
•Immature reticulocytefraction
•RBC fragments (schistoytes)
•Reticulated platelets
•Reticulocyteindics
•Malarial parasites
Newer Parameters(contd..)
•Cellular HbConcentration Mean(CHCM):
Uses Light scatter technology.
True estimate of hypochromiain IDA.
•HbDistribution Width:
Degree of variation in red cell hemoglobinization.
Range-1.82 to 2.64.
•Nucleated Red Cells:
nRBCsidentified,separated& corrected count obtained.
WBCs have high fluorescence & forward scatter.
•Cellular HbConcentration Mean(CHCM):
Uses Light scatter technology.
True estimate of hypochromiain IDA.
•HbDistribution Width:
Degree of variation in red cell hemoglobinization.
Range-1.82 to 2.64.
•Nucleated Red Cells:
nRBCsidentified,separated& corrected count obtained.
WBCs have high fluorescence & forward scatter.
Newer Parameters(contd..)
•Reticuloctes:
Various dyes & flurochromesbind with RNA
RNA content-3 Maturation stages; LFR,MFR & HFR
Immature reticulocyteFraction(IRF):
Sum of MFR & HFR.
Early and sensitive index for erythropoisis.
ReticulocyteHbEquivalent(RET-He):
Hbcontent of freshly prepared RBCs.
Real time information on Fe supply to erythropoiesis.
Early detection of Fe deficiency.
Differentiate IDA & ACD.
Monitoring of erythropoietin & Fe therapy.
•Reticuloctes:
Various dyes & flurochromesbind with RNA
RNA content-3 Maturation stages; LFR,MFR & HFR
Immature reticulocyteFraction(IRF):
Sum of MFR & HFR.
Early and sensitive index for erythropoisis.
ReticulocyteHbEquivalent(RET-He):
Hbcontent of freshly prepared RBCs.
Real time information on Fe supply to erythropoiesis.
Early detection of Fe deficiency.
Differentiate IDA & ACD.
Monitoring of erythropoietin & Fe therapy.
Newer Parameters(contd..)
•P-LCR(Platelet Large Cell Ratio):
% of platelets with a vol>12fl.
Due to platelet aggregates,microerythrocytes,giantplatelets.
•Reticulated Platelets /Immature Platelet Fraction(IPF):
Newly produced platelets that have remains of RNA in their
cytoplasm.
Reflects rate of thrombopoiesis.
•P-LCR(Platelet Large Cell Ratio):
% of platelets with a vol>12fl.
Due to platelet aggregates,microerythrocytes,giantplatelets.
•Reticulated Platelets /Immature Platelet Fraction(IPF):
Newly produced platelets that have remains of RNA in their
cytoplasm.
Reflects rate of thrombopoiesis.
WBC Research Population Data Case Study –Malaria Parasites(Normal plot and Research
Population Data compared to a patient infected with malaria type Plasmodium
falciparum. Note the increased size and variation of the lymph's and Monocyte's.)
NORMAL
Normal
Normal MO
NoralLY
Macrophage
Parasitized RBC
MALARIA
MP Positive
Reactive LY
Population Data compared to a patient infected with malaria type Plasmodium
falciparum. Note the increased size and variation of the lymph's and Monocyte's.)
NORMAL
Normal
Normal MO
NoralLY
Macrophage
Parasitized RBC
MALARIA
MP Positive
Reactive LY
Peroxide based counters:
MPO is used to count neutrophils.Lymphocytes
not stained
Fluroscencebased:
Reticand platelet count.Immatureplatlets
detected best
Immunological based:
Accurate platelet count using CD41/CD61
antibodies
MPO is used to count neutrophils.Lymphocytes
not stained
Fluroscencebased:
Reticand platelet count.Immatureplatlets
detected best
Immunological based:
Accurate platelet count using CD41/CD61
antibodies
The ReticMethod
Must to do before running the sample
•CBC specimens must be checked for clots (visually, by
applicator sticks, or by automated analyzer histogram
inspection or flags), significant in-vitro haemolysisand
interfering lipaemiabefore reporting results.
•CBC processing, either automated or manual, should
be done within 8 hours but in no case later than 24
hours of sample collection, as storage beyond 24 hours
results in erroneous data on automated / semi-
automated Haematologyanalyzers
•Blood samples must be adequately mixed before
analysis.
•CBC specimens must be checked for clots (visually, by
applicator sticks, or by automated analyzer histogram
inspection or flags), significant in-vitro haemolysisand
interfering lipaemiabefore reporting results.
•CBC processing, either automated or manual, should
be done within 8 hours but in no case later than 24
hours of sample collection, as storage beyond 24 hours
results in erroneous data on automated / semi-
automated Haematologyanalyzers
•Blood samples must be adequately mixed before
analysis.
Quality Control
Quality Assessment:
Adequate control of the pre & post analytical from
sample collection to report dispatch.
Quality Control:
Measures that must be included during each assay
run to verify the test working properly.
Proficiency Testing:
Determines the quality of results generated by lab.
Terminologies
Adequate control of the pre & post analytical from
sample collection to report dispatch.
Quality Control:
Measures that must be included during each assay
run to verify the test working properly.
Proficiency Testing:
Determines the quality of results generated by lab.
Terminologies
Accuracy & Precision
•Accuracy:
Refers to closeness to the
true value
•Precision:
Refers to reproducibility
of test
1 2
3 4
•Accuracy:
Refers to closeness to the
true value
•Precision:
Refers to reproducibility
of test
1 2
3 4
Internal Quality control:
Continuous evaluation of the reliability of the daily
works of the lab with validation of tests.
External Quality Control:
Evaluation by an outside agency of between-
laboratory & between-method comparability.
TYPES
Continuous evaluation of the reliability of the daily
works of the lab with validation of tests.
External Quality Control:
Evaluation by an outside agency of between-
laboratory & between-method comparability.
TYPES
CBC Quality Control
•Commercial Controls:
•3 levels (low, normal, high)
•Values stored in instrument computer
•Levey-Jennings graph generated and stored for each
parameter
•Delta Checks
•When the Laboratory Information System (LIS) and the
instrument are interfaced (connected) delta checks are
conducted by the LIS on selected parameters.
–Current values compared to most previous result
–Differences greater than the limits set within the LIS
are flagged
•Commercial Controls:
•3 levels (low, normal, high)
•Values stored in instrument computer
•Levey-Jennings graph generated and stored for each
parameter
•Delta Checks
•When the Laboratory Information System (LIS) and the
instrument are interfaced (connected) delta checks are
conducted by the LIS on selected parameters.
–Current values compared to most previous result
–Differences greater than the limits set within the LIS
are flagged
Controls & Calibrators
•Controls:
Substances used to check the precision.
Analyzed either daily or along each
batch.
Should have same test properties as
blood samples.
Stabilized anticoagulatedwhole blood or
pooled red cells.
3 conc.-high,normal,low
•Levey-Jennings graph generated and
stored for each parameter
•Calibrators:
Check the accuracy.
Value assigned to them by a reliable ref.
center.
•Controls:
Substances used to check the precision.
Analyzed either daily or along each
batch.
Should have same test properties as
blood samples.
Stabilized anticoagulatedwhole blood or
pooled red cells.
3 conc.-high,normal,low
•Levey-Jennings graph generated and
stored for each parameter
•Calibrators:
Check the accuracy.
Value assigned to them by a reliable ref.
center.
Levey-Jennings Chart
Mean
1 SD
2 SD
3 SD
1 SD
2 SD
3 SD
Mean
1 SD
2 SD
3 SD
1 SD
2 SD
3 SD
Control Values and Decision
Consider using WestgardControl Rules
Use premise that 95.5% of control values
should fall within ±2SD
Commonly applied when two levels of control
are used
Use in a sequential fashion
Consider using WestgardControl Rules
Use premise that 95.5% of control values
should fall within ±2SD
Commonly applied when two levels of control
are used
Use in a sequential fashion
1
2SRule= A warning to trigger careful inspection of
the control data123456789101112131415161718192021222324
Mean
Day
+1SD
+2SD
+3SD
-1SD
-2SD
-3SD
1
2Srule
violation
2SRule= A warning to trigger careful inspection of
the control data123456789101112131415161718192021222324
Mean
Day
+1SD
+2SD
+3SD
-1SD
-2SD
-3SD
1
2Srule
violation
1
3SRule= Reject the run when a single control
measurement exceeds the +3SD or -3SD control limit123456789101112131415161718192021222324
Mean
Day
+1SD
+2SD
+3SD
-1SD
-2SD
-3SD
1
3Srule
violation
3SRule= Reject the run when a single control
measurement exceeds the +3SD or -3SD control limit123456789101112131415161718192021222324
Mean
Day
+1SD
+2SD
+3SD
-1SD
-2SD
-3SD
1
3Srule
violation
2
2SRule= Reject the run when 2 consecutive control
measurements exceed the same +2SD or -2SD control limit123456789101112131415161718192021222324
Mean
Day
+1SD
+2SD
+3SD
-1SD
-2SD
-3SD
2
2Srule
violation
2SRule= Reject the run when 2 consecutive control
measurements exceed the same +2SD or -2SD control limit123456789101112131415161718192021222324
Mean
Day
+1SD
+2SD
+3SD
-1SD
-2SD
-3SD
2
2Srule
violation
10
xRule= Reject the run when 10 consecutive control
measurements fall on one side of the mean123456789101112131415161718192021222324
Mean
Day
+1SD
+2SD
+3SD
-1SD
-2SD
-3SD
10
xrule
violation
xRule= Reject the run when 10 consecutive control
measurements fall on one side of the mean123456789101112131415161718192021222324
Mean
Day
+1SD
+2SD
+3SD
-1SD
-2SD
-3SD
10
xrule
violation
What to do when Control Value is out of limit?
•In these situations, precision of routine work can be
monitored by performing duplicate tests on patient
samples.
•SD of differences between results on 20 duplicate
samples is determined and +2SD limits specified.
Subsequent duplicate values should be within these
defined limits.
•Patient data can also be used to monitor precision in a
laboratory performing >100 samples a day. Day-to-Day
variation in MCV, MCH and MCHC should be analyzed
using Bull's algorithm. This facility is available in the
software of many auto analyzers.
•The use of stable controls, however, is the method of
choice.
•In these situations, precision of routine work can be
monitored by performing duplicate tests on patient
samples.
•SD of differences between results on 20 duplicate
samples is determined and +2SD limits specified.
Subsequent duplicate values should be within these
defined limits.
•Patient data can also be used to monitor precision in a
laboratory performing >100 samples a day. Day-to-Day
variation in MCV, MCH and MCHC should be analyzed
using Bull's algorithm. This facility is available in the
software of many auto analyzers.
•The use of stable controls, however, is the method of
choice.
•OUT OF CONTROL!!!
–Repeat the assay ( One time occurrence )
–Check for trends (Delta check)
(from Levy Jennings chart)
–Check integrity of material
–Troubleshoot
–Verify instrumentation
–Repeat the assay ( One time occurrence )
–Check for trends (Delta check)
(from Levy Jennings chart)
–Check integrity of material
–Troubleshoot
–Verify instrumentation
Specimen-Related Problems
•An instrument problem is differentiated from a specimen-
related problem by running a control.
•If the control results are acceptable, the problem is
probably specimen-related.
•Check for:
–clots
–hemolysis
–lipemia
•An instrument problem is differentiated from a specimen-
related problem by running a control.
•If the control results are acceptable, the problem is
probably specimen-related.
•Check for:
–clots
–hemolysis
–lipemia
Instrument Problems
•If the control shows similar problems, it indicates an
instrument problem.
–Electronic?
–Pneumatic / Hydraulic?
–Reagent?
•Because it is easiest to detect a problem in the electronic
subsystem and hardest to detect a problem in the reagent
subsystem, the subsystems are usually checked in the
following order: electronic, pneumatic / hydraulic, reagent.
•If the control shows similar problems, it indicates an
instrument problem.
–Electronic?
–Pneumatic / Hydraulic?
–Reagent?
•Because it is easiest to detect a problem in the electronic
subsystem and hardest to detect a problem in the reagent
subsystem, the subsystems are usually checked in the
following order: electronic, pneumatic / hydraulic, reagent.
Reagent Troubleshooting
•A reagent problem can be as obvious as
precipitate in the reagent tubing.
•In the less obvious cases, the most effective
way of detecting a problem is by keeping a log
of the lot numbers with the opening and
expiration dates of the reagents in use, and
knowing how each reagent affects the data.
•Refer to the labeling information with your
reagents for details.
•A reagent problem can be as obvious as
precipitate in the reagent tubing.
•In the less obvious cases, the most effective
way of detecting a problem is by keeping a log
of the lot numbers with the opening and
expiration dates of the reagents in use, and
knowing how each reagent affects the data.
•Refer to the labeling information with your
reagents for details.
Calibration
1.It is done to compensate for any inaccuracies of the
pneumatic hydraulic and electric systems
2. Calibration fine tunes your hematology analyzer
and provides the most accurate results possible.
3. Automated Haematologyanalyzers should be
calibrated using calibrators„ that have traceability to
standard reference material or methods.
4.Controls are not used for calibration
1.It is done to compensate for any inaccuracies of the
pneumatic hydraulic and electric systems
2. Calibration fine tunes your hematology analyzer
and provides the most accurate results possible.
3. Automated Haematologyanalyzers should be
calibrated using calibrators„ that have traceability to
standard reference material or methods.
4.Controls are not used for calibration
Calibration
•Never adjust to a specific value for an
individual sample.
•For best performance, calibrate all the CBC
parameters. The WBC differential is
calibrated at the factory. They do not require
calibration in the laboratory.
•Never adjust to a specific value for an
individual sample.
•For best performance, calibrate all the CBC
parameters. The WBC differential is
calibrated at the factory. They do not require
calibration in the laboratory.
When to Calibrate
You should calibrate your instrument:
•At installation.
•After the replacement of any component
that involves dilution characteristics or
the primary measurements (such as the
apertures).
•When advised to do so by your service
representative.
You should calibrate your instrument:
•At installation.
•After the replacement of any component
that involves dilution characteristics or
the primary measurements (such as the
apertures).
•When advised to do so by your service
representative.
Blood Sample for Calibration
•4 ml specimen are obtained from three
hematological normal volunteer
in k2 edta
•4 ml specimen are obtained from three
hematological normal volunteer
in k2 edta
HbEstimation
•By Cyan meth hemoglobin method
mean value is taken
•By Cyan meth hemoglobin method
mean value is taken
ICSH Reference methods for PCV
The reference PCV is
Standard whole blood haemoglobinconcentration
-----------------------------------------------------------------
Packed red cell haemoglobinconcentration
following centrifugation in a microhaematocritcentrifuge
1.The measurement on packed red cells is performed on
cells obtained from the middle of the column of red
cells
2. where there is little trapping of plasma or white cell
contamination.
3.It therefore produces a measurement that does not
include trapped plasma.
The reference PCV is
Standard whole blood haemoglobinconcentration
-----------------------------------------------------------------
Packed red cell haemoglobinconcentration
following centrifugation in a microhaematocritcentrifuge
1.The measurement on packed red cells is performed on
cells obtained from the middle of the column of red
cells
2. where there is little trapping of plasma or white cell
contamination.
3.It therefore produces a measurement that does not
include trapped plasma.
RBC AND WBC
TOTAL COUNT
•The reference method for the RBC and
WBC employs a semi-automated
single-channel aperture-impedance
method with accurate coincidence
correction being achieved by
extrapolation from counts on serial
dilutions.
TOTAL COUNT
•The reference method for the RBC and
WBC employs a semi-automated
single-channel aperture-impedance
method with accurate coincidence
correction being achieved by
extrapolation from counts on serial
dilutions.
PLATELET
1.The platelet count can be determined by flow
cytometryusing a fluorochrome–labelled
monoclonal antibody, mixture of CD41, CD42a or
CD61,
2.That binds specifically to platelets and dilution errors
do not affect the count
4.when there is an inherited platelet membrane defect
with absence of one of the platelet glycoproteins,
5.The relevant monoclonal antibody will not bind to
platelets, hence the use of two antibodies
1.The platelet count can be determined by flow
cytometryusing a fluorochrome–labelled
monoclonal antibody, mixture of CD41, CD42a or
CD61,
2.That binds specifically to platelets and dilution errors
do not affect the count
4.when there is an inherited platelet membrane defect
with absence of one of the platelet glycoproteins,
5.The relevant monoclonal antibody will not bind to
platelets, hence the use of two antibodies
CARRY HOME MESSAGE
Automated analyzers provide rapid and useful information of the cell
count, morphology and cell function.
Automation is a supplement and not a
substitute to manual methods
Automated analyzers provide rapid and useful information of the cell
count, morphology and cell function.
Automation is a supplement and not a
substitute to manual methods
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