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基因谱分析在人类细胞系鉴定中的重要作用。

Essential role for gene profiling analysis in the authentication of human cell lines.

作者信息

Yoshino Kaori, Iimura Emi, Saijo Kaoru, Iwase Shigeru, Fukami Kaoru, Ohno Tadao, Obata Yuichi, Nakamura Yukio

机构信息

Cell Engineering Division, RIKEN BioResource Center, Ibaraki, Japan.

出版信息

Hum Cell. 2006 Feb;19(1):43-8. doi: 10.1111/j.1749-0774.2005.00007.x.

DOI:10.1111/j.1749-0774.2005.00007.x
PMID:16643607
Abstract

Cross-contamination between cultured cell lines can result in the generation of erroneous scientific data. Hence, it is very important to eliminate cell lines that are of an origin different from that being claimed. Inter-species contamination can be detected by various established methods, such as karyotype and isozyme analyses. However, it has been impossible to detect intraspecies cross-contamination prior to the development of technology to detect differences between cell lines at the molecular level. Recently, profiling of short tandem repeat (STR) polymorphisms has been established as a method for the analyses of gene polymorphism. Gene profiling by STR polymorphism (STR profiling) is a simple and reliable method to identify individual cell lines. Each human cell line currently provided by the Cell Engineering Division of the RIKEN BioResource Center was analyzed by STR profiling to authenticate its identity. We found that more than 10 human cell lines out of approximately 400 were in fact identical to a different cell line deposited in the collection, and therefore had been misidentified. We conclude that STR profiling is a useful and powerful method for eliminating cell lines that have been misidentified by cross-contamination or by other causes. Hence, STR profiling of human cell lines used in published research will likely be a prerequisite for publication in the future, so that the problem of misidentification of cell lines can be eliminated.

摘要

培养的细胞系之间的交叉污染可能导致错误科学数据的产生。因此,消除来源与所宣称的不同的细胞系非常重要。种间污染可通过各种既定方法检测,如核型分析和同工酶分析。然而,在开发出在分子水平检测细胞系之间差异的技术之前,一直无法检测到种内交叉污染。最近,短串联重复序列(STR)多态性分析已被确立为一种分析基因多态性的方法。通过STR多态性进行基因分型(STR分型)是一种简单可靠的识别单个细胞系的方法。日本理化学研究所生物资源中心细胞工程部目前提供的每个人类细胞系都通过STR分型进行了分析,以验证其身份。我们发现,在大约400个细胞系中,有10多个实际上与保藏库中另一个不同的细胞系相同,因此被错误鉴定。我们得出结论,STR分型是一种有用且强大的方法,可用于消除因交叉污染或其他原因而被错误鉴定的细胞系。因此,对已发表研究中使用的人类细胞系进行STR分型可能会成为未来发表的一个先决条件,这样细胞系错误鉴定的问题就可以消除。

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Results of species-specific hemagglutination tests on "transformed," nontransformed, and primary cell cultures.“转化的”、未转化的和原代细胞培养物的种特异性血凝试验结果。
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Immunological and karyological criteria for identification of cell lines.用于细胞系鉴定的免疫学和核型分析标准。
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Short tandem repeat profiling provides an international reference standard for human cell lines.短串联重复序列分析为人类细胞系提供了国际参考标准。
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Development and Characterization of Human Primary Cholangiocarcinoma Cell Lines.原发性人胆管癌细胞系的建立和鉴定。
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Chemical alternative for cell identification and cross-contamination detection.用于细胞识别和交叉污染检测的化学替代方法。
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