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首页> 外文期刊>Applied and Environmental Microbiology >Quantification of 16S rRNAs in Complex Bacterial Communities by Multiple Competitive Reverse Transcription-PCR in Temperature Gradient Gel Electrophoresis Fingerprints
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Quantification of 16S rRNAs in Complex Bacterial Communities by Multiple Competitive Reverse Transcription-PCR in Temperature Gradient Gel Electrophoresis Fingerprints

机译:在温度梯度凝胶电泳指纹图中通过多重竞争逆转录-PCR定量分析复杂细菌群落中的16S rRNA。

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A novel approach was developed to quantify rRNA sequences in complex bacterial communities. The main bacterial 16S rRNAs in Drentse A grassland soils (The Netherlands) were amplified by reverse transcription (RT)-PCR with bacterium-specific primers and were separated by temperature gradient gel electrophoresis (TGGE). The primer pair used (primers U968-GC and L1401) was found to amplify with the same efficiency 16S rRNAs from bacterial cultures containing different taxa and cloned 16S ribosomal DNA amplicons from uncultured soil bacteria. The sequence-specific efficiency of amplification was determined by monitoring the amplification kinetics by kinetic PCR. The primer-specific amplification efficiency was assessed by competitive PCR and RT-PCR, and identical input amounts of different 16S rRNAs resulted in identical amplicon yields. The sequence-specific detection system used for competitive amplifications was TGGE, which also has been found to be suitable for simultaneous quantification of more than one sequence. We demonstrate that this approach can be applied to TGGE fingerprints of soil bacteria to estimate the ratios of the bacterial 16S rRNAs.
机译:开发了一种新颖的方法来定量复杂细菌群落中的rRNA序列。利用细菌特异性引物通过逆转录(RT)-PCR扩增Drentse A草原土壤(荷兰)中的主要细菌16S rRNA,并通过温度梯度凝胶电泳(TGGE)进行分离。发现所使用的引物对(引物U968-GC和L1401)以相同的效率从含有不同分类群的细菌培养物中扩增出16S rRNA,并从未培养的土壤细菌中克隆了16S核糖体DNA扩增子。通过动力学PCR监测扩增动力学来确定扩增的序列特异性效率。通过竞争性PCR和RT-PCR评估引物特异性扩增效率,不同16S rRNA的相同输入量导致相同的扩增子产量。用于竞争性扩增的序列特异性检测系统是TGGE,它也被发现适用于同时定量一个以上的序列。我们证明了该方法可以应用于土壤细菌的TGGE指纹,以估计细菌16S rRNA的比率。

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