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Analysis of microbial diversity by pyrosequencing the small-subunit ribosomal RNAwithout PCR amplification

机译:无需PCR扩增即可通过焦磷酸测序小亚基核糖体RNA进行微生物多样性分析

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To avoid the biases associated with PCR amplification in analysis of microbial communities, a new method has been tested for direct sequencing of the cDNA of fulllength Small-subunit Ribosomal RNA withOut specific PCR amplification (SROP). In silico analysis of the SROP method demonstrated that more than 99 % of the SROP sequences could be correctly annotated. Two environmental samples(activated sludge and anaerobic sludge) with complex microbial communities were used for comparison in this study. The SROP results demonstrated that the families Rhodocyclaceae and Nitrosomonadaceae in activated sludge and the phyla Synergistetes and Spirochaetes in anaerobic sludge were underestimated by PCR-based detection. One third of the 16S ribosomal RNA (rRNA) sequences obtained by the SROP method covered the V3 amplicon region, and they are suitable for phylogenetic and diversity index analyses. The microbial diversity index calculated fromthe rRNA sequences by the SROP was much higher than that calculated by conventional PCR, particularly for the anaerobic sludge. The metatranscriptome-based SROP method will contribute to our better understanding of the diversity of complex microbial communities.
机译:为避免在微生物群落分析中与PCR扩增相关的偏见,已经测试了一种直接测序全长小亚基核糖体RNA cDNA的新方法,无需进行特异性PCR扩增(SROP)。在SROP方法的计算机分析中显示,可以正确注释超过99%的SROP序列。在本研究中,使用了两个具有复杂微生物群落的环境样品(活性污泥和厌氧污泥)进行比较。 SROP结果表明,基于PCR的检测方法低估了活性污泥中的红景天科和亚硝基菜科以及厌氧污泥中的合生菌和螺旋螺科。通过SROP方法获得的16S核糖体RNA(rRNA)序列的三分之一覆盖了V3扩增子区域,适用于系统发育和多样性指数分析。 SROP从rRNA序列计算出的微生物多样性指数比常规PCR计算的要高得多,特别是对于厌氧污泥。基于转录组的SROP方法将有助于我们更好地了解复杂微生物群落的多样性。

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