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Cultivation-Independent Characterization of Methylobacterium Populations in the Plant Phyllosphere by Automated Ribosomal Intergenic Spacer Analysis

机译:自动化的核糖体基因间间隔子分析技术对植物毛囊中甲基细菌种群的培养不依赖特征

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摘要

Bacteria of the genus Methylobacterium are widespread in the environment, but their ecological role in ecosystems, such as the plant phyllosphere, is not very well understood. To gain better insight into the distribution of different Methylobacterium species in diverse ecosystems, a rapid and specific cultivation-independent method for detection of these organisms and analysis of their community structure is needed. Therefore, 16S rRNA gene-targeted primers specific for this genus were designed and evaluated. These primers were used in PCR in combination with a reverse primer that binds to the tRNAAla gene, which is located upstream of the 23S rRNA gene in the 16S-23S intergenic spacer (IGS). PCR products that were of different lengths were obtained due to the length heterogeneity of the IGS of different Methylobacterium species. This length variation allowed generation of fingerprints of Methylobacterium communities in environmental samples by automated ribosomal intergenic spacer analysis. The Methylobacterium communities on leaves of different plant species in a natural field were compared using this method. The new method allows rapid comparisons of Methylobacterium communities and is thus a useful tool to study Methylobacterium communities in different ecosystems.
机译:甲基细菌属的细菌在环境中广泛分布,但是对它们在生态系统(例如植物叶序层)中的生态作用的了解还不是很清楚。为了更好地了解不同甲基菌种在不同生态系统中的分布,需要一种快速且特定于种植的方法来检测这些生物并分析其群落结构。因此,设计和评估了针对该属的16S rRNA基因靶向引物。这些引物与结合在16S-23S基因间隔区(IGS)中23S rRNA基因上游的tRNA Ala 基因的反向引物结合用于PCR。由于不同的甲基杆菌属物种的IGS的长度异质性,获得了不同长度的PCR产物。该长度变化允许通过自动核糖体基因间间隔子分析在环境样品中产生甲基细菌群落的指纹。使用此方法比较了自然田中不同植物物种的叶子上的甲基细菌群落。新方法可以快速比较甲基杆菌群落,因此是研究不同生态系统中甲基杆菌群落的有用工具。

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