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Ribosome analysis reveals prominent activity of an uncultured member of the class Actinobacteria in grassland soils

机译:核糖体分析揭示了草原土壤中型肌动菌的未培养成员的突出活动

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Summary: A 16S rRNA-based molecular ecological study was performed to search for dominant bacterial sequences in Drentse A grassland soils (The Netherlands). In the first step, a library of 165 clones was generated from PCR-amplified 16S rDNA. By sequence comparison, clone DA079 and two other identical clones could be affiliated to a group of recently described uncultured Actinobacteria. This group contained 16S rDNA clone sequences obtained from different environments across the world. To determine whether such uncultured organisms were part of the physiologically active population in the soil, ribosomes were isolated from the environment and 16S rRNA was partially amplified via RT-PCR using conserved primers for members of the domain Bacteria. Subsequent sequence-specific separation by temperature-gradient gel electrophoresis (TGGE) generated fingerprints of the amplicons. Such community fingerprints were compared with the TGGE pattern of PCR-amplified rDNA of clone DA079 which was generated with the same set of primers. One of the dominant fingerprint bands matched with the band obtained from the actinobacterial clone. Southern blot hybridization with a probe made from clone DA079 confirmed sequence identity of clone and fingerprint band. This is the first report that a member of the novel actinobacterial group may play a physiologically active role in a native microbial community.
机译:发明内容:进行了16S的基于RRNA的分子生态学研究,以寻找Drentse Grassland土壤(荷兰)中的显性细菌序列。在第一步中,从PCR扩增的16S rDNA产生165个克隆的文库。通过序列比较,可以将克隆DA079和另外两种相同的克隆隶属于最近描述的未培养的肌动菌细菌。该组含有来自世界各地的不同环境的16S rDNA克隆序列。为了确定这些未培养的生物是土壤中生理活性群的一部分,从环境中分离出核糖体,并使用RT-PCR将16S rRNA用于域细菌的构件。通过温度梯度凝胶电泳(TGGE)产生的扩增子的指纹的后续序列特异性分离。将这种社区指纹与克隆DA079的PCR扩增的RDNA的TGGE模式进行比较,其用相同的一组引物产生。与从抗原细菌克隆获得的带匹配的主导指纹带之一。 Southern印迹杂交与由克隆DA079制成的探针证实克隆和指纹带的序列同一性。这是第一份报告,即新型肌动杆菌组的成员可能在天然微生物群落中发挥生理活跃作用。

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