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*Akanni EO and #Palini A.
* Department of Haematology & Blood
Transfusion,College of Health Science, Ladoke Akintola
University of Technology, P.M.B 4400,OS 230001, Osogbo .
Nigeria
* olufemiakanni@yahoo.com
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# Flow Cytometry Section, Central Blood
Transfusion Centre,
Hospital San Raffaele, Milan, Italy
Introduction
Immunophenotyping describes a process used to identify cells,
based on the types of antigens or markers on the surface of the
cell. The process is used to characterize and diagnose specific
types of leukemia and lymphoma by comparing the cancer cells to
normal cells of the immune system (1). The method uses the reaction
of antibodies with cell antigens to determine a specific type of
cell in a sample of blood cells, marrow cells or lymph node cells.
The antibodies react with specific antigens on the cell. A tag is
attached to the antibody for its detection (2) which can be
identified and quantified by a flow cytometer.
Flow cytometry is used to identify a cell population of interest
by exploiting its characteristic differential light scattering and
immunofluorescence. One of the principal applications of flow
cytometry has been the identification and the quantitative analysis
of lymphocyte sub sets (3). It is therefore possible to accurately
distinguish lymphocytes from other leukocyte populations in the
peripheral blood using the combination of fluorescence associated
with CD45/CD14 and forward and orthogonal light scatter (4).
Flow cytometry has now become the preferred method for lineage
assignment, maturational characterisation of malignant cells,
detection of clonality, heterogeneity and aberrant features of the
malignant cell populations and quantitation of haematopoietic cells
(5).
Materials and Methods
Monoclonal antibodies: CD45, CD3,CD4,CD8, CD16+56, CD19 etc
conjugated to fluorescein Iso-thiocyanate (FITC), Phycoerythrin
(PE), Peridine and chlorophylprotein (Per CP), FCD, Allophycocyanin
(APC), PECY5, PECY7 obtained from various sources such as Becton
Dickinson, CA, Beckman Coulter, etc .
Cell preparation and Immunofluorescence: Blood and bone marrow
aspirates were obtained from consenting normal adult volunteers and
suitable donors serving as base line controls. Pre- and post-
transplantation blood, stem cells, and bone marrow samples were
also obtained from patients in the haematology and oncology
departments of the Hospital San Raffaele, Milan, Italy.
Aliquots of whole blood specimens were stained with
pre-determined volumes of previously tested and titred monoclonal
antibodies specific for each phenotype marker. After staining, the
red cells in each tube were lysed and the remaining cells fixed
with paraformaldehyde. The prepared specimens were analysed on a
flow cytometer.
Flow cytometry analysis: Quantitative fluorescence analysis was
performed using a multiparametric flow cytometry analyser of
Beckman-Coulter, Cytomics FC 500, Florida, and USA. Samples were
analysed as follows:
For each specimen, values were determined as cells/microlitre of
blood expressing a particular phenotype. The �single platform�
method was used to determine absolute counts. This procedure
employed an internal standard of fluorescent microbeads. The number
of cells having each phenotype was determined independently. In
addition to determining the absolute lymphocyte counts the panel of
tests contained monoclonal antibodies identifying cells bearing the
following phenotype markers: CD3, CD16/56, CD8, CD4, CD45, CD14 and
CD19.
During analysis in the flow cytometer, lymphocytes were
identified and electronically gated on light scatter and
fluorescence signals. Cells binding the relevant markers were
identified by their fluorescence signals.
Below are typical flow cytometry analysis histograms:
Figure 1. Bivariate display of CD45 � FITC fluorescence versus side
scatter. Lymphocytes that express bright CD45 are electronically
gated. All other cells are excluded from further analysis
Figure 2. Bivariate display of orthogonal (side) scatter versus
forward light scatter to determine the purity and the percentage
(or yield) of the gated lymphocytes
Figure 3 - 4. Bivariate fluorescence displays of CD3 versus CD56
and CD3 versus CD19. Integration cursors are placed to enumerate
the percentage of cells in each sub-population of lymphocytes
Figure 5. Statistics Box: Sum of Lymphocyte subsets (L-Sum) as
an internal control. Percentage of T-Cells + B-Cells + NK Cells
should add up to 90-100%
Discussion and Conclusion
The enumeration and characterization of lymphocyte subsets are
crucial in specific clinical situations; hence, strategies to
perform reliable counts are most important. Flow cytometry
therefore provides a specific means of identification and
quantitation of cell population of interest with the highest
sensitivity. The reliability of the count, however, depends on the
instrument performance, reagents and gating strategies.
Flow cytometry offers the best approach for evaluating multiple
antigens simultaneously on large numbers of cells in a short time.
In view of its requirement for a mono-dispersed cell suspension,
flow cytometric identification of antigens has had its greatest
impact in Haematology and Immunology. Several of these
applications, such as the enumuration of CD34+ haematopoietic
progenitor cells in samples that will be used for transplantation;
have proved to be of great clinical utility.
Apart from the analysis of normal cells, clinically useful
applications of flow cytometry to immunophenotyping have also
extended to the identification and study of pathologic leukocytes
and other blood cells in several different disease conditions.
Recent reports have also shown that flow cytometry
immunophenotyping is well suited for rare-event analysis; the
immunophenotypic identification, enumeration and characterisation
of human mast cells and dendritic cells.
Acknowledgement
I would like to thank the International Federation of Clinical
Chemistry (IFCC) for supporting this program and the entire staff
of the Central Blood transfusion centre /Flow cytometry section of
the Hospital San Raffaele Milan, Italy for their cooperations.
References
Cancer dictionary and Acronyms. Web definitions for
immunophenotyping. http://www.dictionary.rare-cancer.org
Chronic Lymphocytic Leukemia Research Consortium, Glossary I. http://www.cll.ucsd.edu/glossary1.htm
Loken MR: Cell surface antigen and morphological characterisation
of leukocyte populations by flow cytometry. In: Methods in
Haematology. Beverly P (ed) Churchill Livingston, London 1985,
132-144.
Loken M, Brosnan J, Bach B and Ault K. Establishing optimal
lymphocyte Gates for Immunophenotyping by flow cytometry. Cytometry
1990; 11:453-9.
European Working Group on Clinical Cell Analysis (EWGCCA).
Consensus Document on Leukemia Immunophenotyping (1996).
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