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森林高地和湿地土壤中亚硝酸盐还原酶(nirK和nirS)基因片段的多样性

Diversity of nitrite reductase (nirK and nirS) gene fragments in forested upland and wetland soils.

作者信息

Priemé Anders, Braker Gesche, Tiedje James M

机构信息

Center for Microbial Ecology, Department of Crop and Soil Sciences, Michigan State University, East Lansing, Michigan 48824-1325, USA.

出版信息

Appl Environ Microbiol. 2002 Apr;68(4):1893-900. doi: 10.1128/AEM.68.4.1893-1900.2002.

DOI:10.1128/AEM.68.4.1893-1900.2002
PMID:11916709
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC123828/
Abstract

The genetic heterogeneity of nitrite reductase gene (nirK and nirS) fragments from denitrifying prokaryotes in forested upland and marsh soil was investigated using molecular methods. nirK gene fragments could be amplified from both soils, whereas nirS gene fragments could be amplified only from the marsh soil. PCR products were cloned and screened by restriction fragment length polymorphism (RFLP), and representative fragments were sequenced. The diversity of nirK clones was lower than the diversity of nirS clones. Among the 54 distinct nirK RFLP patterns identified in the two soils, only one pattern was found in both soils and in each soil two dominant groups comprised >35% of all clones. No dominance and few redundant patterns were seen among the nirS clones. Phylogenetic analysis of deduced amino acids grouped the nirK sequences into five major clusters, with one cluster encompassing most marsh clones and all upland clones. Only a few of the nirK clone sequences branched with those of known denitrifying bacteria. The nirS clones formed two major clusters with several subclusters, but all nirS clones showed less than 80% identity to nirS sequences from known denitrifying bacteria. Overall, the data indicated that the denitrifying communities in the two soils have many members and that the soils have a high richness of different nir genes, especially of the nirS gene, most of which have not yet been found in cultivated denitrifiers.

摘要

利用分子方法研究了森林高地和沼泽土壤中反硝化原核生物亚硝酸还原酶基因(nirK和nirS)片段的遗传异质性。在两种土壤中均能扩增出nirK基因片段,而nirS基因片段仅能从沼泽土壤中扩增出来。对PCR产物进行克隆,并通过限制性片段长度多态性(RFLP)进行筛选,对代表性片段进行测序。nirK克隆的多样性低于nirS克隆的多样性。在两种土壤中鉴定出的54种不同的nirK RFLP模式中,仅在两种土壤中发现了一种模式,并且在每种土壤中,两个优势组占所有克隆的比例均超过35%。在nirS克隆中未发现优势现象,冗余模式也很少。对推导氨基酸进行的系统发育分析将nirK序列分为五个主要簇,其中一个簇包含了大多数沼泽克隆和所有高地克隆。只有少数nirK克隆序列与已知反硝化细菌的序列分支。nirS克隆形成了两个主要簇和几个亚簇,但所有nirS克隆与已知反硝化细菌的nirS序列的同一性均低于80%。总体而言,数据表明两种土壤中的反硝化群落有许多成员,并且土壤中不同nir基因的丰富度很高,尤其是nirS基因,其中大多数在培养的反硝化细菌中尚未发现。

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Nitrite reductase genes (nirK and nirS) as functional markers to investigate diversity of denitrifying bacteria in pacific northwest marine sediment communities.亚硝酸盐还原酶基因(nirK和nirS)作为功能标记物用于研究西北太平洋海洋沉积物群落中反硝化细菌的多样性。
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