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首页> 外文期刊>Journal of industrial microbiology & biotechnology >Desulfovibrionales-related bacteria in a paper mill environment as detected with molecular techniques and culture
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Desulfovibrionales-related bacteria in a paper mill environment as detected with molecular techniques and culture

机译:分子技术和培养法检测的造纸厂环境中与脱硫弧菌有关的细菌

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摘要

The aim of the present study was to evaluate the suitability of a nested PCR-DGGE (denaturing gradient gel electrophoresis) method for the detection of Desulfovibrionales-related sulfate-reducing bacteria (SRB) from paper mill samples. The samples were also analyzed with culturing. SRB cause/enhance industrial problems, namely creation of foul-smelling gases (hydrogen sulfide) and biological corrosion, and so far there has not been a simple method to study these bacteria in paper mill laboratories. In our study, culturing was able to detect Desulfovibrionales-related bacteria from two different white waters, two different brokes, pulp, clay, and slime. Out of the isolated Desulfovibrionales, 23 enrichment cultures were further characterized with Desulfovibrionales-selective PCR-DGGE. An identical Desulfovibrio species sequence was found from paper machine I (broke I, slime, and pulp) and from paper machine II (broke II and white water II), suggesting an in-house contamination with the same strain. Desulfovibrionales-selective PCR-DGGE was also performed from DNA templates extracted directly from the paper mill samples. The DGGE profiles derived from the samples without prior enrichment were more diverse and the sequenced amplicons proved to belong to the Desulfovibrionales order. Moreover, molecular techniques were able to detect Desulfovibrionales-related bacteria from calcium carbonate samples whereas culture did not. Altogether, the nested PCR-DGGE method used in this study was suitable for the detection of Desulfovibrionales-related SRB directly from different paper mill samples and it could be used for the rapid identification of SRB-contaminated industrial sites and, when combined with sequencing, for tracing of the contamination routes.
机译:本研究的目的是评估嵌套式PCR-DGGE(变性梯度凝胶电泳)方法从造纸厂样品中检测与脱硫弧菌相关的硫酸盐还原细菌(SRB)的适用性。还通过培养分析样品。 SRB引起/增强了工业问题,即产生恶臭气体(硫化氢)和生物腐蚀,到目前为止,还没有在造纸厂实验室中研究这些细菌的简单方法。在我们的研究中,培养能够从两种不同的白水,两种不同的破损物,纸浆,黏土和粘液中检测与脱硫弧菌有关的细菌。在分离的脱硫弧菌中,用脱硫弧菌选择性PCR-DGGE进一步鉴定了23种富集培养物。从造纸机I(纸浆I,粘液和纸浆)和造纸机II(纸浆II和白水II)中发现了相同的Desulfovibrio菌种序列,表明内部有相同菌株的污染。还从直接从造纸厂样品中提取的DNA模板中进行了脱硫弧菌选择性PCR-DGGE。来自没有事先富集的样品的DGGE图谱更加多样,测序的扩增子被证明属于Desulfovibrionales顺序。此外,分子技术能够从碳酸钙样品中检测与脱硫弧菌有关的细菌,而培养则不能。总之,本研究中使用的嵌套式PCR-DGGE方法适用于直接从不同造纸厂样品中检测与脱硫弧菌有关的SRB,可用于快速鉴定受SRB污染的工业场所,并与测序结合使用,用于追踪污染路径。

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