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Characterization of the Community Structure of a Dechlorinating Mixed Culture and Comparisons of Gene Expression in Planktonic and Biofloc-Associated “Dehalococcoides” and Methanospirillum Species▿ †

机译:脱氯混合培养物的群落结构的表征以及浮游生物和与生物絮凝物相关的“ Dehalococcoides”和甲螺菌种的基因表达比较†

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摘要

This study sought to characterize bacterial and archaeal populations in a perchloroethene- and butyrate-fed enrichment culture containing hydrogen-consuming “Dehalococcoides ethenogenes” strain 195 and a Methanospirillum hungatei strain. Phylogenetic characterization of this microbial community was done via 16S rRNA gene clone library and gradient gel electrophoresis analyses. Fluorescence in situ hybridization was used to quantify populations of “Dehalococcoides” and Archaea and to examine the colocalization of these two groups within culture bioflocs. A technique for enrichment of planktonic and biofloc-associated biomass was developed and used to assess differences in population distribution and gene expression patterns following provision of substrate. On a per-milliliter-of-culture basis, most D. ethenogenes genes (the hydrogenase gene hupL; the highly expressed gene for an oxidoreductase of unknown function, fdhA; the RNA polymerase subunit gene rpoB; and the 16S rRNA gene) showed no statistical difference in expression between planktonic and biofloc enrichments at either time point studied (1 to 2 and 6 h postfeeding). Normalization of transcripts to ribosome (16S rRNA) levels supported that planktonic and biofloc-associated D. ethenogenes had similar gene expression profiles, with one notable exception; planktonic D. ethenogenes showed higher expression of tceA relative to biofloc-associated cells at 6 h postfeeding. These trends were compared to those for the hydrogen-consuming methanogen in the culture, M. hungatei. The vast majority of M. hungatei cells, ribosomes (16S rRNA), and transcripts of the hydrogenase gene mvrD and the housekeeping gene rpoE were observed in the biofloc enrichments. This suggests that, unlike the comparable activity of D. ethenogenes from both enrichments, planktonic M. hungatei is responsible for only a small fraction of the hydrogenotrophic methanogenesis in this culture.
机译:这项研究试图在全氯乙烯和丁酸盐喂养的富集培养物中表征细菌和古细菌种群,该培养物中含有耗氢的“ Dehalococcoides ethenogenes”菌株195和Methanospirillum Hangatei菌株。通过16S rRNA基因克隆文库和梯度凝胶电泳分析完成了该微生物群落的系统发育鉴定。荧光原位杂交用于定量“ Dehalococcoides”和古细菌的种群,并检查这两个组在培养生物絮凝物中的共定位。开发了一种富集浮游生物和生物絮凝体相关生物质的技术,并用于评估提供底物后种群分布和基因表达模式的差异。在每毫升培养的基础上,大多数埃希氏假单胞菌基因(氢化酶基因hupL;功能未知的氧化还原酶的高表达基因fdhA; RNA聚合酶亚基基因rpoB;以及16S rRNA基因)均未显示在任一研究时间点(喂食后1至2和6小时)浮游生物富集和生物絮凝富集之间表达的统计学差异。转录本对核糖体(16S rRNA)水平的标准化支持浮游生物和与生物絮凝物相关的D. ethenogenes具有相似的基因表达谱,但有一个显着例外。浮游后的D. ethenogenes在喂食后6 h相对于与生物絮凝体相关的细胞显示出较高的tceA表达。将这些趋势与培养物中的M. Hangatei耗氢产甲烷菌的趋势进行了比较。在生物絮凝富集中观察到了绝大多数的饥饿支原体细胞,核糖体(16S rRNA)以及氢化酶基因mvrD和管家基因rpoE的转录本。这表明,与两种富集的埃森氏菌的可比性活动不同,浮游性的匈牙利分枝杆菌仅占该培养物中氢营养性甲烷生成的一小部分。

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