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无需样品制备,通过环介导等温扩增检测芽孢杆菌炭疽从孢子和细胞。

Detection of Bacillus anthracis from spores and cells by loop-mediated isothermal amplification without sample preparation.

机构信息

Biosciences and Biotechnology Division, Physics and Life Sciences Directorate, Lawrence Livermore National Laboratory, Livermore, CA 94550, United States.

出版信息

J Microbiol Methods. 2012 Sep;90(3):280-4. doi: 10.1016/j.mimet.2012.05.022. Epub 2012 Jun 5.

Abstract

Loop-mediated isothermal amplification (LAMP) is a technique capable of rapidly amplifying specific nucleic acid sequences without specialized thermal cycling equipment. In addition, several detection methods that include dye fluorescence, gel electrophoresis, turbidity and colorimetric change, can be used to measure or otherwise detect target amplification. To date, publications have described the requirement for some form of sample nucleic acid extraction (boiling, lysis, DNA purification, etc.) prior to initiating a LAMP reaction. We demonstrate here, the first LAMP positive results obtained from vegetative cells and spores of Bacillus anthracis without nucleic acid extraction. Our data show that the simple addition of cells or spores to the reaction mixture, followed by heating at 63°C is all that is required to reproducibly amplify and detect target plasmid and chromosomal DNA via colorimetric change. The use of three primer sets targeting both plasmids and the chromosome of B. anthracis allows for the rapid discrimination of non-pathogenic bacteria from pathogenic bacteria within 30 min of sampling. Our results indicate that direct testing of B. anthracis spores and cells via LAMP assay will greatly simplify and shorten the detection process by eliminating nucleic acid purification. These results may allow more rapid detection of DNA from pathogenic organisms present in field and environmental samples.

摘要

环介导等温扩增(LAMP)是一种能够快速扩增特定核酸序列的技术,而无需专门的热循环设备。此外,还可以使用几种检测方法来测量或检测目标扩增,包括染料荧光、凝胶电泳、浊度和比色变化。迄今为止,已有文献描述了在开始 LAMP 反应之前需要对样品核酸进行某种形式的提取(煮沸、裂解、DNA 纯化等)。我们在此证明,无需核酸提取,即可从炭疽杆菌的营养细胞和孢子中获得第一个 LAMP 阳性结果。我们的数据表明,只需将细胞或孢子简单地添加到反应混合物中,然后在 63°C 下加热,即可通过比色变化可靠地扩增和检测目标质粒和染色体 DNA。使用针对炭疽杆菌质粒和染色体的三组引物,可以在采样后 30 分钟内快速区分非致病性细菌和致病性细菌。我们的结果表明,通过 LAMP 检测直接检测炭疽杆菌孢子和细胞将通过消除核酸纯化极大地简化和缩短检测过程。这些结果可能允许更快速地检测现场和环境样本中存在的致病性生物的 DNA。

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