首页> 美国卫生研究院文献>Applied and Environmental Microbiology >Distribution of sulfate-reducing bacteria in a stratified fjord (Mariager Fjord Denmark) as evaluated by most-probable-number counts and denaturing gradient gel electrophoresis of PCR-amplified ribosomal DNA fragments.
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Distribution of sulfate-reducing bacteria in a stratified fjord (Mariager Fjord Denmark) as evaluated by most-probable-number counts and denaturing gradient gel electrophoresis of PCR-amplified ribosomal DNA fragments.

机译:通过PCR扩增的核糖体DNA片段的最大可能数计数和变性梯度凝胶电泳评估硫酸盐还原菌在分层峡湾(Mariager Fjord丹麦)中的分布。

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摘要

The sulfate-reducing bacterial populations of a stratified marine water column, Mariager Fjord, Denmark, were investigated by molecular and culture-dependent approaches in parallel. Denaturing gradient gel electrophoresis (DGGE) of PCR-amplified 16S rRNA and DNA encoding rRNA (rDNA) isolated from the water column indicated specific bacterial populations in different water column layers and revealed a highly differentiated pattern of rRNA- and rDNA-derived PCR amplificates, probably reflecting active and resting bacterial populations. Hybridization of DGGE patterns with rRNA probes indicated the increased presence and activity (by at least 1 order of magnitude) of sulfate-reducing bacteria within and below the chemocline. Parallel to this molecular approach, an approach involving most-probable-number (MPN) counts was used, and it found a similar distribution of cultivable sulfate-reducing bacteria in the water column of Mariager Fjord, Approximately 25 cells and 250 cells per ml above and below the chemocline, respectively, were found. Desulfovibrio- and Desulfobulbus-related strains occurred in the oxic zone. DGGE bands from MPN cultures were sequenced and compared with those obtained from nucleic acids extracted from water column samples. The MPN isolates were phylogenetically affiliated with sulfate-reducing delta subdivision proteobacteria (members of the genera Desulfovibrio, Desulfobulbus, and Desulfobacter), whereas the molecular isolates constituted an independent lineage of the delta subdivision proteobacteria. DGGE of PCR-amplified nucleic acids with general eubacterial PCR primers conceptually revealed the general bacterial population, whereas the use of culture media allowed cultivable sulfate-reducing bacteria to be selected. A parallel study of Mariager Fjord biogeochemistry, bacterial activity, and bacterial counts complementing this investigation has been presented elsewhere (N.B. Ramsing, H. Fossing, T. G. Ferdelman, F. Andersen, and B. Thamdrup, Appl. Environ.
机译:同时通过分子和文化相关的方法,对丹麦Mariager Fjord分层海水柱中的硫酸盐还原细菌种群进行了研究。 PCR扩增的16S rRNA的变性梯度凝胶电泳(DGGE)和从水柱分离出的编码rRNA(rDNA)的DNA指示了不同水柱层中的特定细菌种群,并揭示了rRNA和rDNA衍生的PCR扩增子的高度分化模式,可能反映了活跃和静止的细菌种群。 DGGE模式与rRNA探针的杂交表明,在趋化因子内部和之下,硫酸盐还原细菌的存在和活性增加了(至少1个数量级)。与这种分子方法平行,使用了涉及最大概率数(MPN)计数的方法,该方法在Mariager Fjord的水柱中发现了可培养硫酸盐还原细菌的相似分布,每毫升约有25个细胞和250个细胞分别在趋化霉素的下方和下方。与脱硫弧菌和脱硫球菌有关的菌株发生在氧化区。对来自MPN培养物的DGGE条带进行测序,并与从水柱样品中提取的核酸获得的DGGE条带进行比较。 MPN分离株与减少硫酸盐的三角洲细分菌群(Desulfovibrio,Desulfobulbus和Desulfobacter属)的系统发育相关,而分子分离株构成了三角洲细分菌群的独立谱系。使用一般的真细菌PCR引物的PCR扩增核酸的DGGE从概念上揭示了一般的细菌种群,而使用培养基可以选择可培养的硫酸盐还原菌。对Mariager Fjord生物地球化学,细菌活性和细菌计数的补充研究已对此进行了补充(N.B. Ramsing,H.Fossing,T.G。Ferdelman,F.Andersen和B.Thamdrup,Appl.Environ。

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