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首页> 外文期刊>Applied and Environmental Microbiology >Development of an oligonucleotide probe targeting 16S rRNA and its application for detection and quantitation of the ruminal bacterium Synergistes jonesii in a mixed-population chemostat.
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Development of an oligonucleotide probe targeting 16S rRNA and its application for detection and quantitation of the ruminal bacterium Synergistes jonesii in a mixed-population chemostat.

机译:靶向16S rRNA的寡核苷酸探针的开发及其在混合种群恒化器中用于瘤胃细菌Synergistes jonesii的检测和定量的应用。

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Radiolabelled and fluorescent-dye-conjugated oligonucleotide probes which targeted rRNA sequences were developed for the enumeration of the ruminal bacterium Synergistes jonesii 78-1 in mixed culture. Two probes were tested, and both were highly specific for the respective complementary sequences of the target organism. Individual cells of S. jonesii in pure and mixed cultures were clearly visualized in situ by hybridization with the fluorescent-dye-conjugated probe but could not be detected in natural samples. Therefore the radiolabelled probe was used to monitor the population of S. jonesii introduced into a chemostat which simulated the rumen ecosystem. The S. jonesii probe did not hybridize to RNA extracted from the culture prior to inoculation with the target organism. After inoculation, S. jonesii rRNA represented 4.5% of the total bacterial rRNA and then rapidly declined to < 0.2% before increasing to about 1% of the total bacterial rRNA during the following 3 weeks. This study demonstrates that rRNA-targeted probes could be used for tracking organisms introduced into the rumen ecosystem.
机译:开发了靶向rRNA序列的放射性标记和荧光染料偶联的寡核苷酸探针,用于枚举瘤胃细菌Synegeristes jonesii 78-1的混合培养。测试了两种探针,并且两种探针均对靶生物的各自互补序列具有高度特异性。通过与荧光染料偶联探针的杂交,可以在原位清晰地观察纯净和混合培养物中琼脂链球菌的单个细胞,但在自然样品中无法检测到。因此,使用放射性标记的探针来监测引入到模拟瘤胃生态系统的化学恒温器中的沙门氏菌的种群。琼脂链球菌探针在接种靶生物之前未与从培养物中提取的RNA杂交。接种后,琼脂链球菌rRNA占总细菌rRNA的4.5%,然后迅速下降至<0.2%,然后在接下来的3周内增加至总细菌rRNA的约1%。这项研究表明,rRNA靶向探针可用于跟踪引入瘤胃生态系统的生物。

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