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体内上皮细胞增殖、细胞动力学和细胞动力学的定量分析。

Quantification of epithelial cell proliferation, cell dynamics, and cell kinetics in vivo.

作者信息

Goodlad Robert A

机构信息

Centre for Pathology, Imperial College, London, UK.

出版信息

Wiley Interdiscip Rev Dev Biol. 2017 Jul;6(4). doi: 10.1002/wdev.274. Epub 2017 May 5.

DOI:10.1002/wdev.274
PMID:28474479
Abstract

The measurement of cell proliferation in vivo is usually carried out by the examination of static measures. These comprise the mitotic index or labeling indices using incorporation of DNA synthesis markers such as bromodeoxyuridine or tritiated thymidine, or intrinsic markers, such as Ki67 and proliferative cell nuclear antigen (PCNA). But static measures only provide a 'snapshot' of cell proliferation. Rate measures, including double labeling methods and the metaphase arrest method, can actually measure cell production rates but they are far less utilized at present. Transit times and migration rates can also be measured using pulse and chase labeling or by following the transit of labeled cells through the tissue. Simple indices of cell division can easily be confounded by concomitant changes in the compartment size and many alleged markers of proliferation have serious shortcomings, as the markers may be involved in multiple aspects of cell regulation. The complexities of studying proliferation in vivo are illustrated here with a focus on the gastrointestinal tract. Some of these methods can help elucidate the role of the stem cells and their relationship to label retaining cells. WIREs Dev Biol 2017, 6:e274. doi: 10.1002/wdev.274 For further resources related to this article, please visit the WIREs website.

摘要

体内细胞增殖的测量通常通过静态指标检查来进行。这些指标包括有丝分裂指数或标记指数,使用DNA合成标记物如溴脱氧尿苷或氚标记胸腺嘧啶核苷的掺入,或内在标记物如Ki67和增殖细胞核抗原(PCNA)。但静态指标仅提供细胞增殖的“快照”。速率指标,包括双标记法和中期阻断法,实际上可以测量细胞产生速率,但目前它们的应用要少得多。转运时间和迁移速率也可以使用脉冲和追踪标记法或通过追踪标记细胞在组织中的转运来测量。细胞分裂的简单指标很容易因隔室大小的伴随变化而混淆,并且许多所谓的增殖标记物存在严重缺陷,因为这些标记物可能涉及细胞调节的多个方面。本文以胃肠道为重点阐述了体内研究增殖的复杂性。其中一些方法有助于阐明干细胞的作用及其与标记保留细胞的关系。WIREs发育生物学2017年,6:e274。doi:10.1002/wdev.274 有关本文的更多资源,请访问WIREs网站。

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