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使用单激光流式细胞仪同时测量人骨髓细胞的DNA含量和细胞表面免疫荧光。

Simultaneous measurement of DNA content and cell-surface immunofluorescence of human bone marrow cells using a single laser flow cytometer.

作者信息

Brons P P, Pennings A H, Haanen C, Wessels H M, Boezeman J B

机构信息

Department of Hematology, University Hospital Nijmegen, The Netherlands.

出版信息

Cytometry. 1990;11(7):837-44. doi: 10.1002/cyto.990110710.

DOI:10.1002/cyto.990110710
PMID:1703067
Abstract

This paper describes the measurement of S phase DNA content in human bone marrow subpopulations using a single laser method for bivariate analysis of DNA content and cell-surface immunofluorescence (s-IF). Low density (less than 1.077 g/ml) bone marrow cells were labeled with a panel of unconjugated monoclonal antibodies (MoAb) for the lymphoid (CD2 + CD19), T-lymphoid (CD2), B-lymphoid (CD19), erythroid (anti-glycophorin-A), myelomonocytic (CD13, CD33; single and as cocktail) and monocytic (CD14) lineages. A fluorescein isothiocyanate (FITC)-conjugated goat anti-mouse label was used as second step. Unfixed, MoAb-labeled cells were incubated for 24 h with a hypotonic propidium iodide solution for DNA staining. Cells were analysed on a single-laser flow cytometer, operating at 488 nm. The effect of the combined staining protocol upon both s-IF and DNA stainability was evaluated. Only a slight decrease (mean: 29.0%) in s-IF intensity was observed after DNA staining. The percentages of immunofluorescent cells in the bone marrow samples of 10 normal individuals before and after DNA staining were essentially unchanged for all the MoAbs used. The DNA histograms of the immunophenotypically defined subpopulations were of excellent quality with a mean coefficient or variation of 1.8%. This procedure allows the assessment of very low levels of S-phase DNA content, as measured in normal low density blood cells of 8 healthy volunteers (mean 0.07%).(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

本文描述了使用单激光方法对DNA含量和细胞表面免疫荧光(s-IF)进行双变量分析,以测量人骨髓亚群中的S期DNA含量。用一组未结合的单克隆抗体(MoAb)标记低密度(小于1.077 g/ml)骨髓细胞,这些抗体针对淋巴细胞(CD2 + CD19)、T淋巴细胞(CD2)、B淋巴细胞(CD19)、红系(抗血型糖蛋白-A)、骨髓单核细胞系(CD13、CD33;单独及混合使用)和单核细胞(CD14)谱系。第二步使用异硫氰酸荧光素(FITC)偶联的山羊抗小鼠标记物。未固定的、MoAb标记的细胞与低渗碘化丙啶溶液孵育24小时进行DNA染色。在波长488 nm的单激光流式细胞仪上对细胞进行分析。评估了联合染色方案对s-IF和DNA染色性的影响。DNA染色后仅观察到s-IF强度略有下降(平均:29.0%)。对于所有使用的MoAb,10名正常个体骨髓样本在DNA染色前后免疫荧光细胞的百分比基本不变。免疫表型定义的亚群的DNA直方图质量极佳,平均变异系数为1.8%。该方法可评估8名健康志愿者正常低密度血细胞中极低水平的S期DNA含量(平均0.07%)。(摘要截短于250字)

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