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通过聚合酶链反应快速检测土壤中弗氏脱硫肠状菌菌株PCP-1的方法。

Rapid method for detecting Desulfitobacterium frappieri strain PCP-1 in soil by the polymerase chain reaction.

作者信息

Lévesque M J, La Boissière S, Thomas J C, Beaudet R, Villemur R

机构信息

Centre de Recherche en Microbiologie Appliquée, Institut Armand-Frappier, Laval, Québec, Canada.

出版信息

Appl Microbiol Biotechnol. 1997 Jun;47(6):719-25. doi: 10.1007/s002530051001.

Abstract

A rapid method was developed for detecting in soil Desulfitobacterium frappieri strain PCP-1, an anaerobic gram-positive bacterium, isolated from a methanogenic consortium degrading pentachlorophenol. The method involved the establishment of a protocol for extracting total DNA from soil with the least contamination, and the use of the polymerase chain reaction (PCR) to detect strain PCP-1 with primers targeted with PCP-1 16S rRNA. To optimize the DNA extraction conditions, a glass mill homogenizer and a low-salt buffer containing polyvinylpolypyrrolidone were used on a black soil rich in organic matter. Recovered DNA was further purified with phenol/chloroform extractions, ammonium acetate precipitation and a G200 Sephadex gel-filtration column. DNA was extracted from soil supplemented with different concentrations of PCP-1 cells. Detection of PCP-1 was by PCR. The limit of detection was 800 added PCP-1 cells/g dry soil. This level of detection was achieved when the T4 gene-32 protein and 1 microgram soil DNA were added to the PCR mixture followed by a nested PCR. This method is quick, sensitive, and can process several samples at the same time.

摘要

开发了一种快速方法,用于检测从降解五氯苯酚的产甲烷菌联合体中分离出的厌氧革兰氏阳性细菌——弗氏脱硫孤菌PCP - 1菌株在土壤中的存在情况。该方法包括建立一种从土壤中提取污染最少的总DNA的方案,以及使用聚合酶链反应(PCR),用针对PCP - 1 16S rRNA的引物来检测PCP - 1菌株。为了优化DNA提取条件,在富含有机质的黑土上使用玻璃研磨匀浆器和含有聚乙烯聚吡咯烷酮的低盐缓冲液。回收的DNA进一步通过苯酚/氯仿萃取、醋酸铵沉淀和G200葡聚糖凝胶过滤柱进行纯化。从添加了不同浓度PCP - 1细胞的土壤中提取DNA。通过PCR检测PCP - 1。检测限为每克干土添加800个PCP - 1细胞。当将T4基因 - 32蛋白和1微克土壤DNA添加到PCR混合物中,随后进行巢式PCR时,可达到这一检测水平。该方法快速、灵敏,并且可以同时处理多个样品。

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