比较培养的α-卤代羧酸降解细菌中的脱卤酶基因库与环境元基因库。
Comparing the dehalogenase gene pool in cultivated alpha-halocarboxylic acid-degrading bacteria with the environmental metagene pool.
作者信息
Marchesi Julian R, Weightman Andrew J
机构信息
Cardiff School of Biosciences, Cardiff University, Cardiff CF10 3TL, United Kingdom.
出版信息
Appl Environ Microbiol. 2003 Aug;69(8):4375-82. doi: 10.1128/AEM.69.8.4375-4382.2003.
Culture-dependent and culture-independent approaches were used to determine the relationship between the dehalogenase gene pool in bacteria enriched and isolated on 2,2-dichloropropionic acid (22DCPA) and the environmental metagene pool (the collective gene pool of both the culturable and uncultured microbes) from which they were isolated. The dehalogenases in the pure-cultures isolates, which were able to degrade 22DCPA, were similar to previously described group I and II dehalogenases. Significantly, the majority of the dehalogenases isolated from activated sludge by degenerate PCR with primers specific for alpha-halocarboxylic acid dehalogenases were not closely related to the dehalogenases in any isolate. Furthermore, the dehalogenases found in the pure cultures predominated in the enrichments but were a minor component of the community used to inoculate the batch cultures. Phylogenetic analysis of the dehalogenase sequences isolated by degenerate PCR showed that the diversity of the group II deh gene was greater than that of the group I deh gene. Direct plating of the activated sludge onto minimal media supplemented with 22DCPA resulted in biomass and DNA from which dehalogenases were amplified. Analysis of the sequences revealed that they were much more closely related to the sequences found in the community used to start the enrichments. However, no pure cultures were obtained with this isolation method, and thus no pure cultures were available for identification. In this study we examined the link between genes found in pure cultures with the metagene pool from which they were isolated. The results show that there is a large bias introduced by culturing, not just in the bacteria isolated but also the degradative genes that they contain. Moreover, our findings serve as a caveat for studies involving the culturing of pure cultures of bacteria and conclusions which are drawn from analysis of these organisms.
采用依赖培养和不依赖培养的方法,来确定在2,2 - 二氯丙酸(22DCPA)上富集和分离出的细菌中的脱卤酶基因库,与从中分离出这些细菌的环境元基因库(可培养和不可培养微生物的集体基因库)之间的关系。能够降解22DCPA的纯培养分离物中的脱卤酶,与先前描述的I组和II组脱卤酶相似。值得注意的是,用针对α - 卤代羧酸脱卤酶的简并引物通过简并PCR从活性污泥中分离出的大多数脱卤酶,与任何分离物中的脱卤酶都没有密切关系。此外,在纯培养物中发现的脱卤酶在富集物中占主导地位,但却是用于接种分批培养物的群落中的次要成分。对通过简并PCR分离出的脱卤酶序列进行系统发育分析表明,II组脱卤基因的多样性大于I组脱卤基因。将活性污泥直接接种到添加了22DCPA的基本培养基上,产生了可扩增出脱卤酶的生物质和DNA。对序列的分析表明,它们与用于启动富集培养的群落中发现的序列密切得多。然而,用这种分离方法没有获得纯培养物,因此没有纯培养物可用于鉴定。在本研究中,我们研究了纯培养物中发现的基因与从中分离出它们的元基因库之间的联系。结果表明,培养引入了很大的偏差,不仅在分离出的细菌中,而且在它们所含的降解基因中。此外,我们的发现为涉及细菌纯培养物培养以及从对这些生物体的分析得出的结论的研究提供了警示。
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