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与细胞增殖相关的DNA氧化损伤分析。

Analysis of DNA oxidative damage related to cell proliferation.

作者信息

Villani P, Altavista P L, Castaldi L, Leter G, Cordelli E

机构信息

Section of Toxicology and Biomedical Sciences, ENEA CR Casaccia, Via Anguillarese 301, 00060, Rome, Italy.

出版信息

Mutat Res. 2000 Jan 24;464(2):229-37. doi: 10.1016/s1383-5718(99)00192-8.

Abstract

In vivo and in vitro cell populations exhibit a different sensitivity and a heterogeneous response to many genotoxic agents. Several studies have been carried out to evaluate the possibility that the different sensitivity of the cells is related to their proliferative status. In this study, the sensitivity of proliferating (P) and quiescent (Q) C3H10T1/2 cells to oxidative damage and their repair capability has been investigated by single cell gel electrophoresis (SCGE) and micronucleus test. Furthermore the possibility to simultaneously detect DNA damage and cell cycle position has been evaluated. Our results showed a dose-related increase of DNA damage in exponential and plateau phase cells treated with hydrogen peroxide (doses ranging between 2.5 and 100 microM). DNA damage was almost completely repaired within 2 h after treatment in both culture conditions. The percentage of cells in the various phases of the cell cycle has been determined by comet assay and by flow cytometry, and a good agreement between the results of the two techniques was found. Untreated exponentially growing cells in G1 phase showed a lower tail moment than S and G2/M cells. The same cell cycle dependence was evidenced in cells treated with low doses of H(2)O(2), while, at the higher doses, all cells showed a similar level of damage. These results confirm the sensitivity of the Comet Assay in assessing DNA damage, and support its usefulness in evaluating cell cycle-related differential sensitivity to genotoxic agents.

摘要

体内和体外细胞群体对许多基因毒性剂表现出不同的敏感性和异质性反应。已经开展了多项研究来评估细胞不同敏感性与其增殖状态相关的可能性。在本研究中,通过单细胞凝胶电泳(SCGE)和微核试验研究了增殖(P)和静止(Q)的C3H10T1/2细胞对氧化损伤的敏感性及其修复能力。此外,还评估了同时检测DNA损伤和细胞周期位置的可能性。我们的结果显示,用过氧化氢处理的指数生长期和平稳期细胞(剂量范围在2.5至100微摩尔之间)的DNA损伤呈剂量相关增加。在两种培养条件下,处理后2小时内DNA损伤几乎完全修复。通过彗星试验和流式细胞术确定了细胞周期各阶段的细胞百分比,发现两种技术的结果之间具有良好的一致性。处于G1期的未处理指数生长细胞的尾矩低于S期和G2/M期细胞。在用低剂量H₂O₂处理的细胞中也证实了相同的细胞周期依赖性,而在高剂量时,所有细胞都表现出相似程度的损伤。这些结果证实了彗星试验在评估DNA损伤方面的敏感性,并支持其在评估与细胞周期相关的对基因毒性剂的差异敏感性方面的有用性。

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