培养的人肿瘤细胞可以在固定期的所有周期阶段被捕获:在G1, S和G2期显示静止细胞。

B Drewinko, L Y Yang, B Barlogie, J M Trujillo
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引用次数: 59

摘要

采用营养剥夺和细胞拥挤的方法诱导6株人结肠癌细胞株进入固定生长期。在体外生长的各个阶段,依次测量所有细胞系的生长动力学参数(细胞数量、DNA分布的流式细胞分析、标记和有丝分裂指数)。我们的研究结果表明,当细胞从指数生长模式转变为平稳生长模式时,相当一部分细胞(9-18%)处于G2期。此外,通过流式细胞术测定,大量处于生长固定期的细胞具有s期DNA含量,但未能纳入放射性DNA前体(差异高达15倍)。为了证实这些发现,在固定生长阶段的细胞被诱导进入指数生长,在新鲜培养基中以较低的密度重新播种。随后观察到dna区室分布、标记和有丝分裂指数的变化,这些变化是在之前的固定阶段中在周期的不同阶段被捕获的细胞所期望的。因此,非增殖静止状态(Q),传统上位于G1期的“某处”,似乎也由可以在周期的其他阶段(Q和QG2)被捕获的细胞组成。尽管这类细胞的比例相当小,但它们对人体体内肿瘤生长动力学行为的贡献将在“招募”或“同步”临床操作后变得明显,并将阻止同步细胞形成清晰的波。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Cultured human tumour cells may be arrested in all stages of the cycle during stationary phase: demonstration of quiescent cells in G1, S and G2 phase.
Six human colon carcinoma cell lines were induced to enter stationary phase of growth by nutrient deprivation and cell crowding. Growth kinetics parameters (cell number, flow cytometric analysis of DNA distribution, and labelling and mitotic indices) were measured sequentially for all lines during the various stages of in vitro growth. Our results demonstrated that a substantial fraction of cells (9–18%) were located in G2, phase when they changed from an exponential to a stationary mode of growth. Moreover, a large number of cells in stationary phase of growth had an S‐phase DNA content, as determined by flow cytometry, but failed to incorporate radioactive DNA precursors (up to 15‐fold difference). to substantiate these findings. cells in stationary phase of growth were induced to enter exponential growth by re‐seeding in fresh medium at a lower density. Subsequently observed changes in DNA‐compartment distribution, and in labelling and mitotic indices were those expected from cells that had been arrested at different stages of the cycle during their previous stationary phase. Thus, the non‐proliferating quiescent state (Q), traditionally located ‘somewhere’ in G1, phase, appears to be composed also of cells that can be arrested at other stages of the cycle (Qs, and QG). Although the proportion of such cells is rather small, their contribution to the growth kinetics behaviour of human in vivo tumours will become apparent following ‘recruiting’ or ‘synchronizing’ clinical manoeuvres and will prevent the formation of a clear‐cut wave of synchronized cells.
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