Flow cytometry using annexin V can detect early apoptosis in peripheral blood stem cell harvests from patients with leukaemia and lymphoma
被引:0
作者:
RS Anthony
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机构:University of Edinburgh,Department of Haematology
RS Anthony
ND McKelvie
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机构:University of Edinburgh,Department of Haematology
ND McKelvie
AJ Cunningham
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机构:University of Edinburgh,Department of Haematology
AJ Cunningham
JIO Craig
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机构:University of Edinburgh,Department of Haematology
JIO Craig
SY Rogers
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机构:University of Edinburgh,Department of Haematology
SY Rogers
AC Parker
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机构:University of Edinburgh,Department of Haematology
AC Parker
机构:
[1] University of Edinburgh,Department of Haematology
[2] John Hughes Bennett Laboratory,undefined
[3] Western General Hospital,undefined
[4] Victoria Hospital,undefined
来源:
Bone Marrow Transplantation
|
1998年
/
21卷
关键词:
PBSC;
CD34;
apoptosis;
annexin V;
D O I:
暂无
中图分类号:
学科分类号:
摘要:
Quantifying progenitor cells in peripheral blood stem cell (PBSC) harvests by flow cytometric enumeration of CD34+ cells does not account for cell viability. Cell membrane asymmetry in early apoptosis exposes phosphatidylserine on the cell surface. This can be detected by staining with annexin V FITC. Apoptosis in 30 autologous PBSC harvests mobilised by cyclophosphamide + G-CSF or standard chemotherapy + G-CSF was analysed immediately after collection by dual-colour flow cytometry with CD34 PE and annexin V FITC. Harvests contained a median of 3.4 × 106/kg (range 0.3–91.8) CD34+ cells. Of these 87.6% (range 30–96.5) were annexin V−. In 10% of harvests more than 50% of CD34+ cells were apoptotic. Differences in PBSC mobilisation or collection could not explain the variation in annexin V binding. Cyclophosphamide + G-CSF significantly increased the yield of CD34+ cells but did not increase apoptosis. Comparison of consecutive harvests showed no difference in the numbers of CD34+ cells collected but found a significant decrease in apoptotic CD34+ cells through multiple collections. Analysis of annexin V binding in PBSC harvests is a simple flow cytometry technique which gives additional information on the status of CD34+ progenitor cells.