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Phylogeny of γ-proteobacteria inferred from comparisons of 3’ end 16S rRNA gene and 5’ end 16S-23S ITS nucleotide sequences

机译:从3'末端16S rRNA基因和5'末端16S-23S ITS核苷酸序列的比较推断出γ-变形细菌的系统发生

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The phylogeny of γ-proteobacteria was inferred from nucleotide sequence comparisons of a short 232 nucleotide sequence marker. A total of 64 γ-proteobacterial strains from 13 Orders, 22 families, 40 genera and 59 species were analyzed. The short 232 nucleotide sequence marker used here was a combination of a 157 nucleotide sequence at the 3’ end of the 16S rRNA gene and a 75 nucleotide sequence at the 5’ end of the 16S-23S Internal Transcribed Spacer (ITS) sequence. Comparative analyses of the 3’ end of the 16S rRNA gene nucleotide sequence showed that the last 157 bp were conserved among strains from same species and less conserved in more distantly related species. This 157 bp sequence was selected as the first part in the construction of our nucleotide sequence marker. A bootstrapped neighbor-joining tree based on the alignment of this 157 bp was constructed. This 157 bp could distinguish γ-proteobacterial species from different genera from same family. Closely related species could not be distinguished. Next, an alignment of the 16S-23S ITS nucleotide sequences of alleles from same bacterial strain was performed. The first 75 bp at the 5’ end of the 16S-23S ITS was highly conserved at the intra-strain level. It was selected as the second part in the construction of our nucleotide sequence marker. Finally, a bootstrapped neighbor-joining tree based on the alignment of this 232 bp sequence was constructed. Based on the topology of the neighbour-joining tree, four major Groups, Group I to IV, were revealed with several sub-groups and clusters. Our results, based on the 232 bp sequence were, in general, in agreement with the phylogeny of γ-proteobacteria based on the 16S rRNA gene. The use of this 232 bp sequence as a phylogenetic marker presents several advantages over the use of the entire 16S rRNA gene or the generation of extensive phenotypic and genotypic data in phylogenetic analyses. First, this marker is not allele-dependant. Second, this 232 bp marker contains 157 bp from the 3’ end of the 16S rRNA gene and 75 bp from the 5’ end of the 16S-23S ITS. The 157 bp allows discrimination among distantly related species. Owing to its higher rate of nucleotide substitutions, the 75 bp adds discriminating power among closely related species from same genus and closely related genera from same family. Because of its higher percentage of nucleotide sequence divergence than the 16S rRNA gene, the 232 bp marker can better discriminate among closely related γ-proteobacterial species. Third, the method is simple, rapid, suited to large screening programs and easily accessible to most laboratories. Fourth, this marker can also reveal γ-proteobacterial species which may appear misassigned and for which additional characterization appear warranted.
机译:从短232个核苷酸序列标记的核苷酸序列比较中可以推断出γ-变形细菌的系统发育。共分析了来自13个科,22科,40属和59种的64种γ-变形杆菌菌株。此处使用的短232个核苷酸序列标记是16S rRNA基因3'端的157个核苷酸序列和16S-23S内部转录间隔区(ITS)序列的5'端的75个核苷酸序列的组合。对16S rRNA基因核苷酸序列3'端的比较分析表明,在相同物种的菌株中,最后157 bp是保守的,而在远缘相关物种中则不那么保守。选择这个157 bp的序列作为构建我们的核苷酸序列标记的第一部分。基于此157 bp的比对,构建了一个自举邻居邻接树。这157bp可以区分来自同一家族的不同属的γ-蛋白酶。不能区分密切相关的物种。接下来,对来自同一细菌菌株的等位基因的16S-23S ITS核苷酸序列进行比对。 16S-23S ITS 5'末端的前75 bp在菌株内水平上高度保守。选择它作为构建我们的核苷酸序列标记的第二部分。最终,基于该232 bp序列的比对构建了自举邻居邻接树。基于邻居加入树的拓扑,显示了四个主要组,即组I至IV,其中包含几个子组和群集。我们基于232 bp序列的研究结果总体上与基于16S rRNA基因的γ-变形杆菌的系统发育一致。与整个16S rRNA基因的使用或系统发育分析中广泛的表型和基因型数据的产生相比,使用该232 bp序列作为系统发育标记具有多个优势。首先,该标记不是等位基因依赖性的。其次,这个232 bp的标记在16S rRNA基因的3'末端包含157 bp,在16S-23S ITS的5'末端包含75 bp。 157 bp可以区分远缘物种。由于其较高的核苷酸取代率,其75 bp增加了来自同一属的密切相关物种和来自同一家族的密切相关属之间的区分能力。由于它的核苷酸序列差异百分比比16S rRNA基因更高,因此232 bp标记可以更好地区分紧密相关的γ-变形杆菌物种。第三,该方法简单,快速,适用于大型筛查程序,并且大多数实验室均可轻松使用。第四,该标记物还可以揭示可能出现分配错误并需要进一步表征的γ-变形细菌。

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