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表皮细胞增殖。I. 小鼠表皮片中分离的、成对的和成簇的标记细胞比例随时间的变化。

Epidermal cell proliferation. I. Changes with time in the proportion of isolated, paired and clustered labelled cells in sheets of murine epidermis.

作者信息

Potten C S, Loeffler M

机构信息

Paterson Institute for Cancer Research, Christie Hospital and Holt Radium Institute, Manchester, UK.

出版信息

Virchows Arch B Cell Pathol Incl Mol Pathol. 1987;53(5):279-85.

PMID:2889291
Abstract

A new technical approach to analysing labelled cells in sheets of epidermis is presented. The changes in the proportion of isolated single labelled cells, paired or clusters of 3, 4, or more than 4, labelled cells in sheets of epidermis from the back of the mouse have been analysed at various times up to 500 h after 3HTdR administration at either 03.00 h or 15.00 h. The technique is not dependent on the relative number of labelled cells (i.e. the labelling index) but on the spatial distribution of labelled cells. The data cannot be adequately explained on the basis of a simple homogeneous stem cell population in the basal layer but can be better understood on the basis of an hierarchical stem cell-dividing transit proliferative model. The data are consistent with an average cell cycle time of about 100 h but there are suggestions of considerable cell kinetic heterogeneity. The data also suggest that the amount of lateral cell movement within the basal layer is small. The results may suggest that some stem cells either loose label in a manner similar to that suggested by Cairns (1975) i.e. through a process of selective segregation of their DNA strands, or that they have an extremely short S phase duration as postulated earlier (Potten et al. 1982). The present data have been extensively mathematically modelled in an accompanying paper. The model which best fits all the data is an hierarchical scheme with three cell divisions in the transit population but some branches of the lineage may be prematurely terminated by the early production of post-mitotic cells.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

本文介绍了一种分析表皮片中标记细胞的新技术方法。在小鼠背部表皮片中,于03:00或15:00给予3HTdR后,在长达500小时的不同时间点,分析了孤立的单个标记细胞、成对或3个、4个或4个以上标记细胞簇在表皮片中所占比例的变化。该技术不依赖于标记细胞的相对数量(即标记指数),而是依赖于标记细胞的空间分布。基于基底层中简单的均匀干细胞群体,无法充分解释这些数据,但基于分层干细胞分裂过渡增殖模型能更好地理解这些数据。数据与约100小时的平均细胞周期时间一致,但有迹象表明存在相当大的细胞动力学异质性。数据还表明基底层内细胞的侧向移动量很小。结果可能表明,一些干细胞要么以类似于凯恩斯(1975年)所提出的方式丢失标记,即通过其DNA链的选择性分离过程,要么如先前假设的那样(波滕等人,1982年)具有极短的S期持续时间。本文的数据在一篇随附论文中进行了广泛的数学建模。最符合所有数据的模型是一种分层方案,过渡群体中有三个细胞分裂,但谱系的一些分支可能因有丝分裂后细胞的早期产生而提前终止。(摘要截取自250字)

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