Mycobacteriology Unit, Department of Microbiology, Institute of Tropical Medicine, Nationalestraat 155, B-2000 Antwerp, Belgium.
J Microbiol Methods. 2010 Feb;80(2):190-7. doi: 10.1016/j.mimet.2009.12.012. Epub 2010 Jan 4.
We developed a scheme for rapid identification of Mycobacterium species using an automated fluorescence capillary electrophoresis instrument. A 441-bp region of the hsp65 gene was examined using PCR-restriction analysis (PRA). The assay was initially evaluated on 38 reference strains. The observed sizes of restriction fragments were consistently smaller than the real sizes for each of the species as deduced from the sequence analysis (mean variance=7bp). Nevertheless, the obtained PRA patterns were highly reproducible and resulted in correct species identifications. A blind test was then successfully performed on 64 test isolates previously characterized by conventional biochemical methods, a commercial INNO-LiPA Mycobacteria assay and/or sequence determination of the 5' end of 16S rRNA gene. A total of 14 of 64 isolates were erroneously identified by conventional methods (78% accuracy). In contrast, PRA performed very well in comparison with the LiPA (89% concordance) and especially with DNA sequencing (93.3% of concordant results). Also, PRA identified seven isolates representing five previously unreported hsp65 alleles. We conclude that hsp65 PRA based on automated capillary electrophoresis is a rapid, simple and reliable method for identification of mycobacteria.
我们开发了一种使用自动化荧光毛细管电泳仪快速鉴定分枝杆菌种属的方案。采用 PCR-限制性分析(PRA)检测 hsp65 基因的 441 个碱基片段。该检测最初在 38 株参考菌株上进行了评估。尽管从序列分析(平均方差=7bp)推断,每个种属的实际片段大小与观察到的限制片段大小不一致,但获得的 PRA 图谱高度可重现,并且能够正确识别种属。然后,对先前通过传统生化方法、商业 INNO-LiPA 分枝杆菌检测和/或 16S rRNA 基因 5'端序列测定进行特征描述的 64 株测试分离株进行了盲法测试。与传统方法(78%的准确率)相比,共有 14 株(64 株中的 14 株)被错误识别,而 PRA 与 LiPA(89%的一致性),特别是与 DNA 测序(93.3%的一致性)相比表现非常出色。此外,PRA 鉴定了七个代表五个以前未报道的 hsp65 等位基因的分离株。我们得出结论,基于自动化毛细管电泳的 hsp65 PRA 是一种快速、简单和可靠的分枝杆菌鉴定方法。
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