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小鼠大肠微生物群细菌人工染色体文库的构建、分析及β-葡聚糖酶筛选

Construction, analysis, and beta-glucanase screening of a bacterial artificial chromosome library from the large-bowel microbiota of mice.

作者信息

Walter Jens, Mangold Marco, Tannock Gerald W

机构信息

Department of Microbiology and Immunology, University of Otago, PO Box 56, Dunedin, New Zealand.

出版信息

Appl Environ Microbiol. 2005 May;71(5):2347-54. doi: 10.1128/AEM.71.5.2347-2354.2005.

Abstract

A metagenomic (community genomic) library consisting of 5,760 bacterial artificial chromosome clones was prepared in Escherichia coli DH10B from DNA extracted from the large-bowel microbiota of BALB/c mice. DNA inserts detected in 61 randomly chosen clones averaged 55 kbp (range, 8 to 150 kbp) in size. A functional screen of the library for beta-glucanase activity was conducted using lichenin agar plates and Congo red solution. Three clones with beta-glucanase activity were detected. The inserts of these three clones were sequenced and annotated. Open reading frames (ORF) that encoded putative proteins with identity to glucanolytic enzymes (lichenases and laminarinases) were detected by reference to databases. Other putative genes were detected, some of which might have a role in environmental sensing, nutrient acquisition, or coaggregation. The insert DNA from two clones probably originated from uncultivated bacteria because the ORF had low sequence identity with database entries, but the genes associated with the remaining clone resembled sequences reported in Bacteroides species.

摘要

从BALB/c小鼠大肠微生物群中提取的DNA,在大肠杆菌DH10B中构建了一个由5760个细菌人工染色体克隆组成的宏基因组(群落基因组)文库。在随机挑选的61个克隆中检测到的DNA插入片段平均大小为55千碱基对(范围为8至150千碱基对)。使用地衣多糖琼脂平板和刚果红溶液对该文库进行β-葡聚糖酶活性的功能筛选。检测到三个具有β-葡聚糖酶活性的克隆。对这三个克隆的插入片段进行了测序和注释。通过参考数据库,检测到与葡聚糖分解酶(地衣多糖酶和海带多糖酶)具有同源性的推定蛋白质的开放阅读框(ORF)。还检测到了其他推定基因,其中一些可能在环境感知、营养获取或共聚集方面发挥作用。来自两个克隆的插入DNA可能源自未培养的细菌,因为其ORF与数据库条目具有较低的序列同一性,但与其余克隆相关的基因类似于拟杆菌属物种中报道的序列。

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