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照射淋巴细胞中的G2期检查点缺失:一种评估个体辐射敏感性和癌症易感性的新细胞遗传学方法。

G2-checkpoint abrogation in irradiated lymphocytes: A new cytogenetic approach to assess individual radiosensitivity and predisposition to cancer.

作者信息

Terzoudi Georgia I, Hatzi Vasiliki I, Barszczewska Katarzyna, Manola Kalliopi N, Stavropoulou Chryssa, Angelakis Philip, Pantelias Gabriel E

机构信息

Radiobiology and Cytogenetics, IR-RP, National Center for Scientific Research (NCSR) Demokritos, Athens, Greece.

出版信息

Int J Oncol. 2009 Nov;35(5):1223-30. doi: 10.3892/ijo_00000439.

Abstract

Increased yield of chromatid breaks, following in vitro G2-phase lymphocyte irradiation, can be a marker of individual radiosensitivity and cancer predisposing genes whose role is to respond to DNA damage. Mutations or polymorphisms of genes encoding DNA repair pathways may underlie the increased chromosomal radiosensitivity. However, genes that facilitate DNA damage recognition, using signal transduction pathways to activate cell cycle arrest and preserve genomic integrity, are perhaps the most important determinant. Based on the latter hypothesis, an individual radiosensitivity parameter (IRP) is introduced, which expresses, at individual level, the G2-checkpoint potential to facilitate DNA damage recognition and repair of radiation-induced chromosomal damage during G2 to M-phase transition. Based on this parameter a new methodology for assessment of individual radiosensitivity is proposed, which involves G2-checkpoint abrogation by caffeine to obtain the IRP values. To evaluate the proposed methodology, blood samples from 52 healthy donors were taken for inter-individual radiosensitivity analysis using both the conventional G2 chromosomal radiosensitivity assay as well as the new approach using caffeine-induced G2-checkpoint abrogation. The two assays were compared in experiments using samples from 5 hypersensitive patients, 3 AT-homozygotes, 3 AT-heterozygotes, and the GM15786, GM03188A, GM09899, HCC1937 and MCF-7 cell lines. Using the G2 chromosomal radiosensitivity assay, donors are predicted as G2 radiosensitive or normal, while according to the new approach, individuals can be classified as highly radiosensitive, radiosensitive, normal, radioresistant and highly radioresistant. Overall, the new approach provides better individual radiosensitivity discrimination and intra-experimental reproducibility. Therefore, the proposed methodology using IRP values may provide a clinically applicable predictive assay for individual radiosensitivity and predisposition to cancer.

摘要

体外G2期淋巴细胞照射后染色单体断裂产量增加,可能是个体辐射敏感性和癌症易感基因的一个标志,这些基因的作用是对DNA损伤作出反应。编码DNA修复途径的基因突变或多态性可能是染色体辐射敏感性增加的基础。然而,利用信号转导途径激活细胞周期停滞并维持基因组完整性以促进DNA损伤识别的基因,可能是最重要的决定因素。基于后一种假设,引入了个体辐射敏感性参数(IRP),该参数在个体水平上表达了G2期检查点在G2期到M期转换过程中促进DNA损伤识别和修复辐射诱导的染色体损伤的潜力。基于该参数,提出了一种评估个体辐射敏感性的新方法,该方法涉及用咖啡因消除G2期检查点以获得IRP值。为了评估所提出的方法,采集了52名健康供体的血样,使用传统的G2染色体辐射敏感性测定法以及使用咖啡因诱导的G2期检查点消除的新方法进行个体间辐射敏感性分析。在使用5名超敏患者、3名共济失调毛细血管扩张症纯合子、3名共济失调毛细血管扩张症杂合子以及GM15786、GM03188A、GM09899、HCC1937和MCF-7细胞系样本的实验中对这两种测定法进行了比较。使用G2染色体辐射敏感性测定法,可将供体预测为G2期辐射敏感或正常,而根据新方法,个体可分为高度辐射敏感、辐射敏感、正常、辐射抗性和高度辐射抗性。总体而言,新方法提供了更好的个体辐射敏感性区分和实验内再现性。因此,所提出的使用IRP值的方法可能为个体辐射敏感性和癌症易感性提供一种临床适用的预测测定法。

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