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通过流式细胞术在活化的和恶性的人类淋巴细胞中观察到显著的非S期DNA合成。

Significant non-S-phase DNA synthesis visualized by flow cytometry in activated and in malignant human lymphoid cells.

作者信息

Neckers L M, Funkhouser W K, Trepel J B, Cossman J, Gratzner H G

出版信息

Exp Cell Res. 1985 Feb;156(2):429-38. doi: 10.1016/0014-4827(85)90549-x.

Abstract

The development of a monoclonal antibody to the deoxynucleoside bromodeoxyuridine (BrdU), combined with two parameter flow cytometry, has allowed us to examine large numbers of cells for non-S-phase DNA synthesis. Three human lymphoid cell populations were studied to determine the level of deoxynucleoside (dN) incorporation as a function of DNA content. In each population, non-S-phase DNA synthesis was observed. In a rapidly growing human T-lymphoblastoid cell line (CCRF-CEM), 53% of dN incorporation occurred in G0/G1 plus G2 + M. In chronic lymphocytic leukemia (CLL) cells stimulated with tetradecanoylphorbol acetate (TPA), 45% of the observed burst in thymidine incorporation was found to be localized to G0/G1 cells. Non-S-phase incorporation was not, however, limited to neoplastic cells. Normal human peripheral blood B cells treated with the Cowan strain of Staphylococcus aureus (CSA) undergo a transient burst in thymidine incorporation, but do not go on to divide in the absence of other stimuli. Flow-cytometric analysis showed that 80% of this CSA-stimulated dN incorporation was into G0/G1 cells. These data are consistent with a more dynamic state of DNA synthesis than usually envisioned. Furthermore, the data show that although thymidine incorporation levels are related to incorporation of dN into DNA, they can be unrelated to cell proliferation.

摘要

一种针对脱氧核苷溴脱氧尿苷(BrdU)的单克隆抗体的开发,结合双参数流式细胞术,使我们能够检测大量细胞的非S期DNA合成。研究了三个人类淋巴细胞群体,以确定脱氧核苷(dN)掺入水平与DNA含量的关系。在每个群体中,均观察到非S期DNA合成。在快速生长的人类T淋巴母细胞系(CCRF-CEM)中,53%的dN掺入发生在G0/G1期加上G2+M期。在用十四酰佛波醇乙酸酯(TPA)刺激的慢性淋巴细胞白血病(CLL)细胞中,观察到的胸苷掺入爆发中有45%定位于G0/G1期细胞。然而,非S期掺入并不局限于肿瘤细胞。用金黄色葡萄球菌考恩菌株(CSA)处理的正常人外周血B细胞会出现胸苷掺入的短暂爆发,但在没有其他刺激的情况下不会继续分裂。流式细胞术分析表明,这种CSA刺激的dN掺入中有80%进入G0/G1期细胞。这些数据与比通常设想的更动态的DNA合成状态一致。此外,数据表明,虽然胸苷掺入水平与dN掺入DNA有关,但它们可能与细胞增殖无关。

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