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Analysis of denitrification genes and comparison of nosZ, cnorB and 16S rDNA from culturable denitrifying bacteria in potato cropping systems

机译:马铃薯种植系统可培养反硝化细菌反硝化基因分析及nosZ,cnorB和16S rDNA的比较

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Bacterial denitrification in agricultural soils is a major source of nitrous oxide, a potent greenhouse gas. This study examined the culturable bacterial population of denitrifiers in arable field soils in potato (Solanum tuberosum L.) production and denitrification genes (nir, nor and nos) and 16S rDNA in those isolates. Enrichments for culturable denitrifiers yielded 31 diverse isolates that were then analysed for denitrification genes. The nitrous oxide reductase (nosZ) gene was found in all isolates. The majority of isolates ( approximately 90%) contained the cnorB nitric oxide reductase gene, with the remainder containing the qnorB gene. Nitrite reductase genes (nirS and nirK) were amplifiable from most of the isolates, and were segregated between species similar to previously isolated denitrifiers. Isolated strains were preliminarily identified using fatty acid methyl ester analysis and further identified using 16S rDNA sequencing. The majority of isolates (21) were classified as Pseudomonas sp., with smaller groups of isolates being most similar to Bosea spp. (4), Achromobacter spp. (4) and two isolates closely related to Sinorhizobium/Ensifer spp. Phylogenetic trees were compared among nosZ, cnorB and 16S rDNA genes for a subset of Pseudomonas strains. The trees were mostly congruent, but some Pseudomonas sp. isolates grouped differently depending on the gene analysed, indicating potential horizontal gene transfer of denitrification genes. Although Bosea spp. are known denitrifiers, to the best of our knowledge this is the first report of isolation and sequencing of denitrification genes from this bacterial genus.
机译:农业土壤中的细菌脱氮是一氧化二氮的主要来源,一氧化二氮是一种有效的温室气体。这项研究检查了马铃薯(Solanum tuberosum L.)生产和反硝化基因(nir,nor和nos)和这些分离物中16S rDNA的可耕田土壤中反硝化菌的可培养细菌种群。可培养反硝化菌的富集产生了31种不同的分离株,然后对其进行反硝化基因分析。在所有分离物中都发现了一氧化二氮还原酶(nosZ)基因。大多数分离株(约90%)包含cnorB一氧化氮还原酶基因,其余分离株包含qnorB基因。亚硝酸还原酶基因(nirS和nirK)可从大多数分离物中扩增,并与以前分离的反硝化剂相似,在种间隔离。使用脂肪酸甲酯分析初步鉴定出分离的菌株,并使用16S rDNA测序进一步鉴定。大多数分离株(21)被归类为假单胞菌(Pseudomonas sp。),而较小的分离株组与Bosea spp最相似。 (4),无色杆菌属。 (4)和两个与中华根瘤菌/ Ensifer spp密切相关的分离株。在nosZ,cnorB和16S rDNA基因之间比较了部分假单胞菌菌株的系统发育树。树木大多是一致的,但有些假单胞菌属。分离株根据所分析的基因进行分组,表明反硝化基因的潜在水平基因转移。虽然波西奇。据我们所知,这是已知的反硝化剂,这是该细菌属中反硝化基因分离和测序的第一个报道。

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