首页> 外文期刊>Diagnostic microbiology and infectious disease >Evaluation of four DNA extraction methods for the detection of Mycobacterium avium subsp. paratuberculosis by polymerase chain reaction.
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Evaluation of four DNA extraction methods for the detection of Mycobacterium avium subsp. paratuberculosis by polymerase chain reaction.

机译:评价四种DNA提取方法以检测鸟分枝杆菌亚种。副结核病通过聚合酶链反应。

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Polymerase chain reaction (PCR) has been widely used due to its high specificity, sensitivity, and rapid turn-around time. However, inhibitory factors may be co-extracted with the target nucleic acid that will hinder the performance of PCR. In this study, DNA extraction methods for Mycobacterium avium subsp. paratuberculosis were evaluated including rapid lysis, organic extraction, silica-based and magnetic particle-based (MagaZorb(TM)) technologies on bacterial cells, and spiked bovine feces. Efficiency of the extraction was determined by PCR end point titration with primers targeting the insertion sequence, IS900. Results of the end point titrations are identical for bacterial cells and spiked feces. Inhibition was observed in PCR with DNA isolated from spiked feces, and a 1/100 dilution was able to alleviate this problem with DNA extracted by MagaZorb(TM). A 1/1000 dilution was required for the other three methods. MagaZorb(TM) proved to be more efficient at removing inhibitory factors and required the least labor and completion time. Further evaluation is required for its utilization in other clinical specimens.
机译:聚合酶链反应(PCR)由于其高特异性,灵敏度和快速周转时间而被广泛使用。但是,抑制因子可能会与目标核酸共提取,从而阻碍PCR的进行。在这项研究中,鸟分枝杆菌亚种的DNA提取方法。对副结核病进行了评估,包括细菌细胞上的快速裂解,有机提取,基于二氧化硅和基于磁性颗粒的(MagaZorb(TM))技术,以及加标的牛粪。通过PCR终点滴定,使用靶向插入序列IS900的引物确定提取效率。细菌细胞和加标粪便的终点滴定结果相同。用从加标的粪便中分离的DNA在PCR中观察到抑制作用,用MagaZorb™提取的DNA以1/100稀释液可以缓解这一问题。其他三种方法需要1/1000的稀释度。事实证明,MagaZorb(TM)在去除抑制因子方面更有效,并且所需的劳动和完成时间最少。需要将其用于其他临床标本进行进一步评估。

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