Detection of mycoplasma contamination in cell substrates using reverse transcription-PCR assays

支原体 16S核糖体RNA 生物 微生物学 核糖体RNA 分子生物学 检出限 软体动物 聚合酶链反应 细菌 基因 色谱法 遗传学 化学
作者
M. Peredeltchouk,Selwyn A. Wilson David,Bhaskar Bhattacharya,Dmitriy V. Volokhov,Vladimir E. Chizhikov
出处
期刊:Journal of Applied Microbiology [Oxford University Press]
卷期号:110 (1): 54-60 被引量:20
标识
DOI:10.1111/j.1365-2672.2010.04853.x
摘要

To assess the limit of detection (LOD) and the feasibility of 16S rRNA-based reverse transcription-PCR (RT-PCR) assays for advanced detection of mycoplasma contamination in cell substrates.The RT-PCR approach is based on detecting the 16S rRNA molecules that, in contrast to genomic bacterial DNA, are represented by multiple copies in mycoplasma cell. The number of 16S rRNA molecules in mycoplasma cells of five species i.e. Mycoplasma arginini, Myc. fermentans, Myc. hyorhinis, Myc. orale and Acholeplasma laidlawii, all known to be frequent cell line contaminants in industrial and research laboratories, was measured using molecular methods. The results of two independently prepared mycoplasma cultures harvested at the stationary phase of their growth showed that the 16S rRNA copy number per cell varied in the range from about 400 to 2000 copies, depending on species, but stayed close between different preparations of one species. The assessment of the LOD of the in-house 16S rRNA-based RT-PCR was performed using samples of MDCK cell culture spiked with different amounts of five aforementioned mycoplasma species. To minimize the bias in methods comparison, the LOD of the RT-PCR assay was expressed in terms of genome equivalents (GEs) and compared with that determined for highly optimized 16S rDNA-based mycoplasma testing methods previously described in scientific literature.The results of the study showed that the in-house 16S rRNA-based RT-PCR assay was able to reliably detect the presence of less than one mycoplasma GE that is at least 10-fold higher of the LOD previously determined for well-optimized 16S rDNA-based assays developed and described by other researchers.The results of the study showed that rapid RT-PCR methods based on the detection of bacterial 16S rRNA are able to expedite mycoplasma testing of cell cultures (1-2 days vs 28 days) and to ensure the limits of detection comparable to that of currently used culture-based mycoplasma testing methods.

科研通智能强力驱动
Strongly Powered by AbleSci AI
科研通是完全免费的文献互助平台,具备全网最快的应助速度,最高的求助完成率。 对每一个文献求助,科研通都将尽心尽力,给求助人一个满意的交代。
实时播报
Orange应助WEAWEA采纳,获得10
刚刚
可靠白安发布了新的文献求助10
刚刚
BillyCHEN完成签到 ,获得积分10
1秒前
rubbish完成签到,获得积分20
1秒前
2秒前
2秒前
CodeCraft应助丰富的不惜采纳,获得10
2秒前
大个应助个性的元绿采纳,获得10
3秒前
乐正达完成签到,获得积分10
3秒前
懒得理完成签到 ,获得积分10
3秒前
cdercder应助唠叨的傲云采纳,获得10
5秒前
5秒前
虚幻小小发布了新的文献求助10
6秒前
sunny完成签到,获得积分10
6秒前
6秒前
7秒前
Bibu酱完成签到 ,获得积分10
7秒前
孤蚀月完成签到,获得积分10
8秒前
8秒前
sci大户发布了新的文献求助10
8秒前
Lucas应助Billyrain123采纳,获得10
9秒前
9秒前
Moment发布了新的文献求助10
9秒前
shengch0234完成签到,获得积分10
9秒前
10秒前
rubbish发布了新的文献求助10
12秒前
12秒前
12秒前
LKL林发布了新的文献求助20
13秒前
13秒前
勇度完成签到,获得积分10
13秒前
14秒前
lin发布了新的文献求助10
14秒前
风中琦发布了新的文献求助30
15秒前
15秒前
16秒前
123发布了新的文献求助10
17秒前
Moment完成签到,获得积分10
17秒前
扎克完成签到,获得积分20
17秒前
17秒前
高分求助中
Principles of Economics, 11th Edition 10000
University Physics with Modern Physics, 16th edition 10000
(应助此贴封号)【重要!!请各用户(尤其是新用户)详细阅读】【科研通的精品贴汇总】 10000
Molecular Mechanisms of Photosynthesis, 4th Edition 1000
Organic Reactions, Volume 116 1000
Matrix Methods in Data Mining and Pattern Recognition 510
Social Skills Improvement System-Rating Scales--Chinese Version 500
热门求助领域 (近24小时)
化学 材料科学 医学 生物 纳米技术 工程类 有机化学 化学工程 生物化学 计算机科学 内科学 物理 复合材料 催化作用 细胞生物学 无机化学 光电子学 物理化学 电极 基因
热门帖子
关注 科研通微信公众号,转发送积分 7254368
求助须知:如何正确求助?哪些是违规求助? 8876334
关于积分的说明 18741890
捐赠科研通 6934908
什么是DOI,文献DOI怎么找? 3200112
关于科研通互助平台的介绍 2374772
邀请新用户注册赠送积分活动 2175008