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细菌小亚基rRNA基因的计算机模拟限制性片段长度多态性分析:用于自然环境中微生物多样性研究的选定四聚体限制性内切酶的效能

A computer-simulated restriction fragment length polymorphism analysis of bacterial small-subunit rRNA genes: efficacy of selected tetrameric restriction enzymes for studies of microbial diversity in nature.

作者信息

Moyer C L, Tiedje J M, Dobbs F C, Karl D M

机构信息

Department of Oceanography, School of Ocean and Earth Science and Technology, University of Hawaii, Honolulu 96822, USA.

出版信息

Appl Environ Microbiol. 1996 Jul;62(7):2501-7. doi: 10.1128/aem.62.7.2501-2507.1996.

Abstract

An assessment of 10 tetrameric restriction enzymes (TREs) was conducted by using a computer-simulated restriction fragment length polymorphism (RFLP) analysis for over 100 proximally and distally related bacterial small-subunit (SSU) rRNA gene sequences. Screening SSU rDNA clone libraries with TREs has become an effective strategy because of logistic simplicity, commercial availability, and economy. However, the rationale for selecting the type and number of TREs has not been systematically evaluated. Our objective was to identify the optimal combination of TREs for RFLP screening of cloned SSU rRNA genes from undefined bacterial clone libraries. After computer-simulated TRE digestion, the resultant fragments were categorized on the basis of the frequency of different restriction fragment size classes. Three groups of distribution patterns for the TREs were determined and further examined via graphical exploratory data analysis. The RFLP size-frequency distribution data for each group of enzymes were then used to infer phylogenetic relationships via the neighbor-joining method. The resulting bootstrap values and the correct placement of node bifurcations were used as additional criteria to evaluate the efficacy of the selected TREs. These RFLP data were compared with known phylogenetic relationships based on SSU rRNA sequence analysis as defined by the Ribosomal Database Project. A heuristic approach testing random combinations of TREs showed that three or more TRE combinations detected > 99% of the operational taxonomic units (OTUs) within the model data set. OTUs that remained undetected after three TRE treatments had a median sequence similarity of 96.1%. Of the 10 restriction enzymes examined, HhaI, RsaI, and BstUI (group 3) were the most efficacious at detecting and differentiating bacterial SSU rRNA genes on the basis of their ability to correctly classify OTUs. Group 3 TREs are therefore recommended for screening in studies using bacterial SSU rRNA genes as descriptors of in situ microbial diversity.

摘要

通过对100多个近端和远端相关细菌小亚基(SSU)rRNA基因序列进行计算机模拟限制性片段长度多态性(RFLP)分析,对10种四聚体限制性内切酶(TRE)进行了评估。由于操作简便、商业可得性和经济性,用TRE筛选SSU rDNA克隆文库已成为一种有效的策略。然而,选择TRE的类型和数量的基本原理尚未得到系统评估。我们的目标是确定用于从未定义的细菌克隆文库中筛选克隆的SSU rRNA基因的RFLP的最佳TRE组合。在计算机模拟TRE消化后,根据不同限制性片段大小类别的频率对所得片段进行分类。确定了三组TRE的分布模式,并通过图形探索性数据分析进一步检查。然后,每组酶的RFLP大小频率分布数据用于通过邻接法推断系统发育关系。所得的自展值和节点分支的正确位置用作评估所选TRE效力的附加标准。将这些RFLP数据与基于核糖体数据库项目定义SSU rRNA序列分析的已知系统发育关系进行比较。一种测试TRE随机组合的启发式方法表明,三种或更多种TRE组合在模型数据集中检测到>99%的操作分类单元(OTU)。经过三种TRE处理后仍未检测到的OTU的中位序列相似性为96.1%。在所检查的10种限制性内切酶中,HhaI、RsaI和BstUI(第3组)基于其正确分类OTU的能力,在检测和区分细菌SSU rRNA基因方面最有效。因此,建议在使用细菌SSU rRNA基因作为原位微生物多样性描述符的研究中使用第3组TRE进行筛选。

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