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细胞培养物中的支原体检测:四种方法的比较

Mycoplasma detection in cell cultures: a comparison of four methods.

作者信息

Garner C M, Hubbold L M, Chakraborti P R

机构信息

Oncology Research Laboratory, Derby Cancer Centre, Derby City General Hospital, Uttoxeter Road, Derby DE22 3NE, UK.

出版信息

Br J Biomed Sci. 2000;57(4):295-301.

Abstract

Mycoplasma is a common contaminant of tissue culture samples. Infection is persistent, difficult to detect and diagnose, and very difficult to cure. The concentration of mycoplasma in infected cultures can be as high as 10(7) colony-forming units per mL, and their presence can change many of the cell reactions, including altering cell growth rate, inducing morphological changes or cell transformation, and mimicking virus infection. Therefore, it should be assumed that a mycoplasma-contaminated cell line may be significantly influenced in every respect, and, thus, experimental data derived from such a cell line is likely to be invalid. Contamination is not obvious, either macroscopically or microscopically; thus, routine mycoplasma testing is essential for any cell culture laboratory. Many of the testing procedures developed so far are time-consuming, expensive, inconclusive and unsuitable for screening large numbers of test specimens. This study compares DNA staining, enzyme-linked immunosorbent assay (ELISA), polymerase chain reaction (PCR) and PCR ELISA, to determine which is the best procedure for routine assessment of cell cultures. All four methods gave reproducible results with both infected and non-infected cell lines. Both ELISA methods were easy to perform, reproducible and easily interpreted.

摘要

支原体是组织培养样本中常见的污染物。感染具有持续性,难以检测和诊断,且极难治愈。受感染培养物中支原体的浓度可高达每毫升10⁷个集落形成单位,它们的存在会改变许多细胞反应,包括改变细胞生长速率、诱导形态变化或细胞转化,以及模拟病毒感染。因此,应假定受支原体污染的细胞系在各个方面都可能受到显著影响,因此,源自此类细胞系的实验数据很可能无效。污染在宏观或微观上都不明显;因此,常规支原体检测对于任何细胞培养实验室来说都是必不可少的。迄今为止开发的许多检测程序都耗时、昂贵、结果不确定且不适用于筛查大量测试样本。本研究比较了DNA染色、酶联免疫吸附测定(ELISA)、聚合酶链反应(PCR)和PCR ELISA,以确定哪种方法是细胞培养常规评估的最佳程序。所有四种方法对受感染和未受感染的细胞系都给出了可重复的结果。两种ELISA方法操作简便、可重复且易于解读。

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