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简单序列重复区间PCR在小鼠模型中的应用:癌症发生过程中基因改变的评估

Application of inter-simple sequence repeat PCR to mouse models: assessment of genetic alterations in carcinogenesis.

作者信息

Benavides Fernando, Zamisch Mónica, Flores Mónica, Campbell Marcia R, Andrew Susan E, Angel Joe M, Licchesi Julien, Sternik Gabriel, Richie Ellen R, Conti Claudio J

机构信息

Department of Carcinogenesis, The University of Texas M.D. Anderson Cancer Center, Science Park-Research Division, Smithville, Texas 78957, USA.

出版信息

Genes Chromosomes Cancer. 2002 Dec;35(4):299-310. doi: 10.1002/gcc.10129.

Abstract

Genomic instability is believed to play a significant role in cancer development by facilitating tumor progression and tumor heterogeneity. Inter-simple sequence repeat (inter-SSR) PCR has been proved to be a fast and reproducible technique for quantitation of genomic instability (amplifications, deletions, translocations, and insertions) in human sporadic tumors. However, the use of inter-SSR PCR in animal models of cancer has never been described. This new technique has been adapted in our laboratory for the analysis of spontaneous and induced mouse tumors. We established the best PCR conditions for each microsatellite-anchored primer and critically evaluated the reproducibility of the band patterns. We also studied the variation of the fingerprints between and within various inbred mouse strains, including wild-derived lines. Tumor-specific alterations were detected as gains, losses, or intensity changes in bands when compared with matched normal DNA. We quantitated the extent of alterations by dividing the number of altered bands in the tumor by the total number of bands in normal DNA (instability index). By means of inter-SSR PCR, we successfully analyzed genomic alterations in various mouse tumors, including spontaneous thymic lymphomas developed in Msh2 knockout mice as well as chemically induced squamous cell carcinomas and thymic lymphomas. Instability index values ranged between 0 and 9%, the highest levels observed in N-methyl-N-nitrosourea-induced thymic lymphomas generated in Trp53 (p53) nullizygote (-/-) mice. We report here, for the first time, the use of inter-SSR PCR to detect somatic mutations in mouse tumoral DNA, including laser-capture microdissected, methanol-fixed tissues. These PCR-based fingerprints provide a novel approach to assessing the number and onset of mutational events in mouse tumors and will help to understand better the mechanisms of carcinogenesis in mouse models.

摘要

基因组不稳定被认为通过促进肿瘤进展和肿瘤异质性在癌症发展中发挥重要作用。简单序列重复区间(inter-SSR)PCR已被证明是一种快速且可重复的技术,用于定量人类散发性肿瘤中的基因组不稳定(扩增、缺失、易位和插入)。然而,inter-SSR PCR在癌症动物模型中的应用从未被描述过。这项新技术已在我们实验室中用于分析自发和诱导的小鼠肿瘤。我们为每个微卫星锚定引物建立了最佳PCR条件,并严格评估了条带模式的可重复性。我们还研究了包括野生衍生品系在内的各种近交小鼠品系之间以及品系内部指纹图谱的变化。与匹配的正常DNA相比,肿瘤特异性改变表现为条带的增加、减少或强度变化。我们通过将肿瘤中改变条带的数量除以正常DNA中条带的总数(不稳定指数)来定量改变的程度。通过inter-SSR PCR,我们成功分析了各种小鼠肿瘤中的基因组改变,包括Msh2基因敲除小鼠中自发产生的胸腺淋巴瘤以及化学诱导的鳞状细胞癌和胸腺淋巴瘤。不稳定指数值在0%至9%之间,在Trp53(p53)纯合缺失(-/-)小鼠中由N-甲基-N-亚硝基脲诱导产生的胸腺淋巴瘤中观察到最高水平。我们首次在此报告使用inter-SSR PCR检测小鼠肿瘤DNA中的体细胞突变,包括激光捕获显微切割的、甲醇固定的组织。这些基于PCR的指纹图谱为评估小鼠肿瘤中突变事件的数量和发生提供了一种新方法,并将有助于更好地理解小鼠模型中的致癌机制。

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