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应用微核细胞阻断法检测人成纤维细胞中的环境促断剂和非整倍体剂,并结合微核中着丝粒蛋白 A 的免疫荧光染色。

Detection of environmental clastogens and aneugens in human fibroblasts by cytokinesis-blocked micronucleus assay associated with immunofluorescent staining of CENP-A in micronuclei.

机构信息

Laboratoire de Biogénotoxicologie et Mutagenèse Environnementale (EA 1784/FR CNRS 3098 ECCOREV), Aix-Marseille Université, Faculté de Médecine, Marseille, France.

出版信息

Chemosphere. 2011 Jul;84(5):676-80. doi: 10.1016/j.chemosphere.2011.03.027. Epub 2011 Apr 12.

DOI:10.1016/j.chemosphere.2011.03.027
PMID:21486675
Abstract

The cytokinesis-blocked micronucleus (CBMN) assay, in combination with fluorescent in situ hybridization (FISH) of human pan-centromeric DNA probes, or with CREST antibodies that specifically stain kinetochore proteins, is widely used on several cell types. It distinguishes micronuclei containing one or several whole chromosomes, which are positively labeled (centromere positive micronucleus, C+MN, due to aneugenic effect), or acentric chromosome fragments, which are unlabeled due to the absence of centromere (centromere negative micronucleus, C-MN, due to clastogenic effect). However, the very slight level of the centromeric signals obtained with the FISH technique on primary human fibroblasts, a cell type commonly used in environmental genetic toxicology, leads to great difficulties in distinguishing C+MN and C-MN. Furthermore, the CREST technique may lead to inappropriate results particularly with regards to variations in antibody composition between patient sera. Our results show that the in vitro CBMN, in combination with immunofluorescence staining of CENP-A (centromere protein A), efficiently screens genotoxicants for their ability to induce clastogenic and/or aneugenic effects. We propose the in vitro CBMN assay in combination with immunofluorescence staining of CENP-A as a suitable tool in environmental genotoxicity testing of primary human fibroblasts.

摘要

细胞有丝分裂阻断微核(CBMN)试验与人类着丝粒 DNA 探针的荧光原位杂交(FISH)或特异性染色动粒蛋白的 CREST 抗体联合使用,已广泛应用于多种细胞类型。它可以区分含有一个或多个完整染色体的微核,这些微核被阳性标记(由于着丝粒效应而被称为着丝粒阳性微核,C+MN),或不含着丝粒的染色体片段,由于缺乏着丝粒而未被标记(由于断裂效应而被称为着丝粒阴性微核,C-MN)。然而,在环境遗传毒理学中常用的原代人成纤维细胞等细胞类型中,FISH 技术获得的着丝粒信号非常微弱,这导致区分 C+MN 和 C-MN 非常困难。此外,CREST 技术可能会导致不适当的结果,特别是在患者血清中抗体组成的变化方面。我们的研究结果表明,体外 CBMN 试验与 CENP-A(着丝粒蛋白 A)的免疫荧光染色相结合,能够有效地筛选遗传毒物诱导断裂和/或着丝粒效应的能力。我们提出体外 CBMN 试验与 CENP-A 的免疫荧光染色相结合,作为原代人成纤维细胞环境遗传毒性测试的一种合适工具。

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