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用于监测土壤细菌的毛细管电泳单链构象多态性分析

Capillary electrophoresis single-strand conformation polymorphism analysis for monitoring soil bacteria.

作者信息

King Stephanie, McCord Bruce R, Riefler R Guy

机构信息

Department of Chemistry and Biochemistry, 171 Clippinger Laboratories, Ohio University, Athens, OH 45701, USA.

出版信息

J Microbiol Methods. 2005 Jan;60(1):83-92. doi: 10.1016/j.mimet.2004.08.014.

DOI:10.1016/j.mimet.2004.08.014
PMID:15567228
Abstract

The ability to effectively monitor a microbial community is necessary to design and implement remediation strategies for contaminated soil. Single-strand conformation polymorphism (SSCP), a technique which separates DNA fragments based on their sequence, was used to analyze amplified 16S rRNA gene fragments of 12 common soil bacteria. Separation was performed using capillary electrophoresis (CE), as opposed to other common gel techniques, to eliminate the need for band analysis on gel matrices. Four different universal bacterial primer sets were used for DNA amplification: 341-534, P11-P13, Er10-Er11, and Er14-Er15 corresponding to the V3, V8, V2, and V4 regions, respectively. The forward strand of each primer was labeled with 6-carboxy fluorescein fluorescent dye. Analyses were performed on the Applied Biosystems 310 genetic analyzer using GeneScan Analysis Software version 3.5. The best results were obtained using primer 341-534, in which 6 of the 12 bacteria could be distinguished. By combining primer sets 341-534 and Er10-Er11, all 12 of the bacteria could be separated, indicating various degrees of polymorphism within the selected primer regions. When performing simultaneous amplification and analysis of all 12 species some preferential amplification occurred, as not all peaks could be observed. However, SSCP profiles obtained for pure bacterial cultures show the potential of CE-SSCP for bacterial community analysis.

摘要

有效监测微生物群落的能力对于设计和实施污染土壤修复策略至关重要。单链构象多态性(SSCP)是一种根据DNA片段序列分离DNA片段的技术,用于分析12种常见土壤细菌的扩增16S rRNA基因片段。与其他常见的凝胶技术不同,分离是使用毛细管电泳(CE)进行的,以消除在凝胶基质上进行条带分析的需要。使用四种不同的通用细菌引物对进行DNA扩增:341 - 534、P11 - P13、Er10 - Er11和Er14 - Er15,分别对应于V3、V8、V2和V4区域。每个引物的正向链都用6 - 羧基荧光素荧光染料标记。使用GeneScan Analysis Software version 3.5在Applied Biosystems 310基因分析仪上进行分析。使用引物341 - 534获得了最佳结果,其中12种细菌中的6种可以被区分。通过组合引物对341 - 534和Er10 - Er11,可以分离所有12种细菌,表明所选引物区域内存在不同程度的多态性。当对所有12个物种进行同时扩增和分析时,出现了一些优先扩增现象,因为并非所有峰都能被观察到。然而,从纯细菌培养物获得的SSCP图谱显示了CE - SSCP在细菌群落分析中的潜力。

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