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基于 DNA、rRNA 和 mRNA 的好氧甲烷营养菌在湖泊沉积物中的稳定同位素探测。

DNA-, rRNA- and mRNA-based stable isotope probing of aerobic methanotrophs in lake sediment.

机构信息

Max Planck Institute for Terrestrial Microbiology, Karl-von-Frisch Strasse, Marburg, Germany.

出版信息

Environ Microbiol. 2011 May;13(5):1153-67. doi: 10.1111/j.1462-2920.2010.02415.x. Epub 2011 Jan 24.

DOI:10.1111/j.1462-2920.2010.02415.x
PMID:21261798
Abstract

A stable isotope probing (SIP) approach was used to study aerobic methane-oxidizing bacteria (methanotrophs) in lake sediment. Oligotrophic Lake Stechlin was chosen because it has a permanently oxic sediment surface. 16S rRNA and the pmoA gene, which encodes a subunit of the methane monooxygenase enzyme, were analysed following the incubation of sediment with (13) CH(4) and the separation of (13) C-labelled DNA and RNA from unlabelled nucleic acids. The incubation with (13) CH(4) was performed over a 4-day time-course and the pmoA genes and transcripts became progressively labelled such that approximately 70% of the pmoA genes and 80% of the transcripts were labelled at 96 h. The labelling of pmoA mRNA was quicker than pmoA genes, demonstrating that mRNA-SIP is more sensitive than DNA-SIP; however, the general rate of pmoA transcript labelling was comparable to that of the pmoA genes, indicating that the incorporation of (13) C into ribonucleic acids of methanotrophs was a gradual process. Labelling of Betaproteobacteria was clearly seen in analyses of 16S rRNA by DNA-SIP and not by RNA-SIP, suggesting that cross-feeding of the (13) C was primarily detected by DNA-SIP. In general, we show that the combination of SIP approaches provided valuable information about the activity and growth of the methanotrophic populations and the cross-feeding of methanotroph metabolites by other microorganisms.

摘要

采用稳定同位素探测(SIP)方法研究了湖泊沉积物中的好氧甲烷氧化菌(甲烷营养菌)。选择贫营养的 Stechlin 湖作为研究对象,因为其沉积物表面始终保持好氧状态。在将沉积物与 13 CH4 孵育并分离 13 C 标记 DNA 和 RNA 与未标记核酸后,对 16S rRNA 和编码甲烷单加氧酶亚基的 pmoA 基因进行了分析。用 13 CH4 孵育的时间为 4 天,pmoA 基因和转录物逐渐被标记,96 小时时,大约 70%的 pmoA 基因和 80%的转录物被标记。pmoA mRNA 的标记速度快于 pmoA 基因,表明 mRNA-SIP 比 DNA-SIP 更敏感;然而,pmoA 转录物标记的总体速率与 pmoA 基因相当,表明甲烷营养菌的(13)C 掺入到核糖核酸中是一个逐渐的过程。通过 DNA-SIP 而非 RNA-SIP 分析 16S rRNA 时,明显可以看到β变形菌的标记,表明(13)C 的交叉喂养主要是通过 DNA-SIP 检测到的。总的来说,我们表明,SIP 方法的结合提供了关于甲烷营养菌种群的活性和生长以及其他微生物对甲烷营养菌代谢物的交叉喂养的有价值的信息。

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