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用于研究土壤中类硝化杆菌nxrA序列多样性的PCR-变性梯度凝胶电泳工具的开发与应用

Development and application of a PCR-denaturing gradient gel electrophoresis tool to study the diversity of Nitrobacter-like nxrA sequences in soil.

作者信息

Wertz Sophie, Poly Franck, Le Roux Xavier, Degrange Valérie

机构信息

Laboratoire d'Ecologie Microbienne, Université de Lyon, Université Lyon 1, 16 rue Dubois, Villeurbanne, France.

出版信息

FEMS Microbiol Ecol. 2008 Feb;63(2):261-71. doi: 10.1111/j.1574-6941.2007.00416.x.

DOI:10.1111/j.1574-6941.2007.00416.x
PMID:18199085
Abstract

A new PCR-denaturing gel gradient electrophoresis (DGGE) tool based on the functional gene nxrA encoding the catalytic subunit of the nitrite oxidoreductase in nitrite-oxidizing bacteria (NOB) has been developed. The first aim was to determine if the primers could target representatives of NOB genera: Nitrococcus and Nitrospira. The primers successfully amplified nxrA gene sequences from Nitrococcus mobilis, but not from Nitrospira marina. The second aim was to develop a PCR-DGGE tool to characterize NOB community structure on the basis of Nitrobacter-like partial nrxA gene sequences (Nb-nxrA). We tested (1) the ability of this tool to discriminate between Nitrobacter strains, and (2) its ability to reveal changes in the community structure of NOB harbouring Nb-nrxA sequences induced by light grazing or intensive grazing in grassland soils. The DGGE profiles clearly differed between the four Nitrobacter strains tested. Differences in the structure of NOB community were revealed between grazing regimes. Phylogenetic analysis of the sequences corresponding to different DGGE bands showed that Nb-nxrA sequences did not group in management-specific clusters. Most of the nxrA sequences obtained from soils differed from nxrA sequences of NOB strains. Along with existing tools for characterizing the community structure of nitrifiers, this new approach is a significant step forward to performing comprehensive studies on nitrification.

摘要

一种基于编码亚硝酸盐氧化细菌(NOB)中亚硝酸盐氧化还原酶催化亚基的功能基因nxrA的新型聚合酶链反应-变性凝胶梯度电泳(PCR-DGGE)工具已被开发出来。首要目标是确定这些引物是否能靶向NOB属的代表菌株:硝化球菌属和硝化螺旋菌属。这些引物成功地从运动硝化球菌中扩增出nxrA基因序列,但未从海硝化螺旋菌中扩增出该序列。第二个目标是开发一种PCR-DGGE工具,以基于类硝化杆菌属部分nrxA基因序列(Nb-nxrA)来表征NOB群落结构。我们测试了(1)该工具区分硝化杆菌菌株的能力,以及(2)其揭示草地土壤中轻度放牧或重度放牧诱导的携带Nb-nrxA序列的NOB群落结构变化的能力。在所测试的四种硝化杆菌菌株之间,DGGE图谱明显不同。放牧方式之间揭示了NOB群落结构的差异。对与不同DGGE条带对应的序列进行系统发育分析表明,Nb-nxrA序列并未聚集在特定管理的簇中。从土壤中获得的大多数nxrA序列与NOB菌株的nxrA序列不同。连同现有的用于表征硝化细菌群落结构的工具一起,这种新方法是向进行全面硝化研究迈出的重要一步。

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