采用膜联蛋白-V/碘化丙啶通过流式细胞术以及改良的原位末端标记技术分析凋亡的动态过程。

The dynamic process of apoptosis analyzed by flow cytometry using Annexin-V/propidium iodide and a modified in situ end labeling technique.

作者信息

Span L F R, Pennings A H M, Vierwinden G, Boezeman J B M, Raymakers R A P, de Witte T

机构信息

Department of Hematology, University Medical Center Nijmegen, Nijmegen, The Netherlands.

出版信息

Cytometry. 2002 Jan 1;47(1):24-31.

PMID:11774346

Abstract

BACKGROUND

To study the apoptotic process in time, we used the following flow cytometric (FCM) techniques: phosphatidylserine (PS) translocation by Annexin-V (AnV), DNA fragmentation by in situ end labeling (ISEL), and propidium iodide (PI) staining. Because PS translocation is assumed to be an early feature of programmed cell death (PCD), we questioned if AnV positivity implies inevitable cell death.

METHODS

Apoptosis was induced in Jurkat cells by gamma-irradiation, incubation with camptothecin (CPT), or cytosine beta-D-arabinofuranoside (Ara-C). At different time intervals, PCD was quantified by AnV/PI and ISEL. To analyze the influence of cell handling procedures on PCD, we applied these three FCM techniques on CD34+ bone marrow (BM) stem cells after selection and after a freeze-thaw procedure. Various AnV/PI- CD34+ fractions were cultured in a single-cell single-well (SCSW) assay.

RESULTS

Jurkat cells under three different detrimental conditions showed essentially the same pattern of apoptosis in time. Initially developed AnV+/PI- cells subsequently (within 1 h) showed ISEL positivity, after which they turned into AnV+/PI++ cells with even higher levels of ISEL positivity (80-90%). Eventually, they lost some of their PI and ISEL positivity and formed the AnV+/PI+ fraction. Cell handling of CD34+ cells caused high and variable AnV+/PI- fractions (overall range 23-62%). Within total AnV+ and AnV+/PI- populations, only a minority of CD34+ cells showed ISEL positivity (range 4-8% and 0.8-6%, respectively). Different fractions of AnV+/PI- CD34+ cells did have clonogenic capacity.

CONCLUSIONS

PCD of cell suspensions in vitro can be followed accurately in time by these three FCM techniques. PS translocation is followed rapidly (within 1 h) by oligo-nucleosomal DNA fragmentation, after which cell (and nuclear) membrane leakage occurs. Detection of PS asymmetry by AnV-fluorescein isothiocyanate (FITC) is not always associated with (inevitable) apoptosis, as can be concluded from the proliferative capacity of AnV+ /PI- CD34+ cells in the SCSW assay.

摘要

背景

为及时研究细胞凋亡过程，我们采用了以下流式细胞术（FCM）技术：用膜联蛋白-V（AnV）检测磷脂酰丝氨酸（PS）易位、原位末端标记（ISEL）检测DNA片段化以及碘化丙啶（PI）染色。由于PS易位被认为是程序性细胞死亡（PCD）的早期特征，我们质疑AnV阳性是否意味着细胞必然死亡。

方法

通过γ射线照射、喜树碱（CPT）孵育或阿糖胞苷（Ara-C）诱导Jurkat细胞凋亡。在不同时间间隔，通过AnV/PI和ISEL对PCD进行定量分析。为分析细胞处理程序对PCD的影响，我们在分选后以及冻融处理后，对CD34+骨髓（BM）干细胞应用这三种FCM技术。将不同的AnV/PI-CD34+组分在单细胞单孔（SCSW）试验中进行培养。

结果

在三种不同有害条件下的Jurkat细胞，其凋亡模式在时间上基本相同。最初出现的AnV+/PI-细胞随后（1小时内）表现出ISEL阳性，之后转变为AnV+/PI++细胞，ISEL阳性水平更高（80 - 90%）。最终，它们失去部分PI和ISEL阳性，形成AnV+/PI+组分。CD34+细胞的处理导致较高且变化的AnV+/PI-组分（总体范围23 - 62%）。在总的AnV+和AnV+/PI-群体中，只有少数CD34+细胞表现出ISEL阳性（分别为4 - 8%和0.8 - 6%）。不同比例的AnV+/PI-CD34+细胞确实具有克隆形成能力。