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基于微流控系统的毛细管电泳替代方法:用于脑肿瘤细胞系鉴定的高效方法。

Brain tumor cell line authentication, an efficient alternative to capillary electrophoresis by using a microfluidics-based system.

机构信息

Corresponding Author: Dr. Qian An, MD, PhD, School of Pharmacy and Biomedical Sciences, University of Portsmouth, St Michael's Building, White Swan Road, Portsmouth PO1 2DT, UK.

出版信息

Neuro Oncol. 2014 Jan;16(2):265-73. doi: 10.1093/neuonc/not202. Epub 2013 Dec 12.

DOI:10.1093/neuonc/not202
PMID:24335698
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3895385/
Abstract

BACKGROUND

The current method for cell line authentication is genotyping based on short tandem repeat (STR)-PCR involving coamplification of a panel of STR loci by multiplex PCR and downstream fragment length analysis (FLA), usually performed by capillary electrophoresis. FLA by capillary electrophoresis is time-consuming and can be expensive, as the facilities are generally not accessible for many research laboratories.

METHODS

In the present study, a microfluidic electrophoresis system, the Agilent 2100 Bioanalyzer, was used to analyze the STR-PCR fragments from 10 human genomic loci of a number of human cell lines, including 6 gliomas, 1 astrocyte, 1 primary lung cancer, 1 lung brain metastatic cancer, and 1 rhabdomyosarcoma; and this was compared with the standard method, that is, capillary electrophoresis, using the Applied Biosystems 3130xl Genetic Analyzer.

RESULTS

The microfluidic electrophoresis method produced highly reproducible results with good sensitivity in sizing of multiple PCR fragments, and each cell line demonstrated a unique DNA profile. Furthermore, DNA fingerprinting of samples from 5 different passage numbers of the same cell line showed excellent reproducibility when FLA was performed with the Bioanalyzer, indicating that no cross-contamination had occurred during the culture period.

CONCLUSION

This novel application provides a straightforward and cost-effective alternative to STR-based cell line authentication. In addition, this application would be of great value for cell bank repositories to maintain and distribute precious cell lines.

摘要

背景

目前细胞系鉴定的方法是基于短串联重复序列(STR)-PCR 的基因分型,包括通过多重 PCR 共扩增一组 STR 基因座和下游片段长度分析(FLA),通常通过毛细管电泳进行。毛细管电泳的 FLA 既耗时又昂贵,因为许多研究实验室通常无法获得该设备。

方法

在本研究中,使用 Agilent 2100 Bioanalyzer 微流控电泳系统分析了来自多种人类细胞系(包括 6 个神经胶质瘤、1 个星形细胞瘤、1 个原发性肺癌、1 个肺脑转移性癌症和 1 个横纹肌肉瘤)的 10 个人类基因组基因座的 STR-PCR 片段,与标准方法(即毛细管电泳,使用 Applied Biosystems 3130xl Genetic Analyzer)进行了比较。

结果

微流控电泳方法在对多个 PCR 片段进行尺寸测定时产生了高度可重复的结果,并且每个细胞系都表现出独特的 DNA 图谱。此外,当使用 Bioanalyzer 进行 FLA 时,同一细胞系的 5 个不同传代数目的样品的 DNA 指纹图谱显示出极好的重现性,表明在培养期间没有发生交叉污染。

结论

这种新颖的应用为基于 STR 的细胞系鉴定提供了一种简单、经济有效的替代方法。此外,该应用对于细胞库存储库来说将具有重要价值,可以维护和分发宝贵的细胞系。

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