A limited antibody panel can distinguish B-precursor acute lymphoblastic leukemia from normal B precursors with four color flow cytometry : implications for residual disease detection

A limited antibody panel can distinguish B-precursor acute lymphoblastic leukemia from normal B precursors with four color flow cytometry : implications for residual disease detection

Multiparameter flow cytometry may be used to detect minimal residual disease in acute leukemia because leukemic cells often display aberrant phenotypes when compared to normal cells. One limitation of this approach in B-precursor ALL is that leukemic phenotypes are often qualitatively similar to nor...

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Veröffentlicht in:Leukemia 1999-04, Vol.13 (4), p.558-567
Hauptverfasser: WEIR, E. G, COWAN, K, LEBEAU, P, BOROWITZ, M. J
Format: Artikel
Sprache:eng
Schlagworte:
Acute lymphoblastic leukemia
Antibodies
Antibodies, Monoclonal - immunology
Antibodies, Neoplasm - immunology
Antigen-presenting cells
Antigens
Antigens, Differentiation, B-Lymphocyte - analysis
Antigens, Neoplasm - analysis
Biological and medical sciences
Bone Marrow - pathology
CD19 antigen
CD20 antigen
CD34 antigen
CD45 antigen
CD9 antigen
Color
Disease detection
Displays
Evaluation Studies as Topic
Flow cytometry
Flow Cytometry - methods
Hematology
Humans
Immunophenotyping - methods
Investigative techniques, diagnostic techniques (general aspects)
Leukemia
Lymphatic leukemia
Malignancy
Medical sciences
Minimal residual disease
Neoplasm, Residual
Neoplastic Stem Cells - immunology
Parameters
Pathology. Cytology. Biochemistry. Spectrometry. Miscellaneous investigative techniques
Phenotypes
Precursor B-Cell Lymphoblastic Leukemia-Lymphoma - diagnosis
Precursor B-Cell Lymphoblastic Leukemia-Lymphoma - immunology
Precursor B-Cell Lymphoblastic Leukemia-Lymphoma - pathology
Precursors
Progenitor cells
Reproducibility of Results
Sensitivity and Specificity
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Zusammenfassung:Multiparameter flow cytometry may be used to detect minimal residual disease in acute leukemia because leukemic cells often display aberrant phenotypes when compared to normal cells. One limitation of this approach in B-precursor ALL is that leukemic phenotypes are often qualitatively similar to normal marrow B progenitors, though it has long been recognized that the latter show a predictable pattern of antigen expression with differentiation. In this study we used four-color flow cytometry to define precisely the patterns of normal antigen expression on a series of normal bone marrows using two different four-color combinations of antibodies: CD19-APC/CD45-perCP/CD20-PE/CD10-FITC; and CD19-APC/CD45-perCP/CD9-PE/CD34-FITC. A series of dual parameter displays were created in which normal B precursors occupied predictable regions. We then tested these antibody combinations on a series of 82 cases of B-precursor ALL and found that in 76/82 cases (93%) the first combination demonstrated an abnormal population on at least one of the dual parameter displays, and that 72/77 cases tested (94%) showed an abnormality with the second combination. When taken together, 81/82 cases (99%) showed an abnormality. When purified blasts were serially diluted into normal marrows we found a sensitivity of detection of 1 cell in 10(4) normal marrow cells provided sufficient CD19+ cells were acquired to visualize the abnormal population as a discrete cluster. Because the pattern of antigen expression in normals is very reproducible, it is possible to create a fixed set of geometrical regions to define the normal; this makes analysis of an unknown sample very straightforward. We conclude that our approach could be employed as a simple method for the detection of minimal residual disease in B-precursor ALL, and unlike many other methods should prove applicable to virtually all cases of this malignancy.
ISSN:0887-6924
1476-5551
DOI:10.1038/sj.leu.2401364