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TRUFFLER: programs to study microbial community composition and flux from fluorescent DNA fingerprinting data

机译:TRUFFLER:从荧光DNA指纹数据研究微生物群落组成和通量的程序

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Terminal-restriction fragment length polymorphism (T-RFLP) and length heterogeneity-polymerase chain reaction (LH-PCR) are DNA fingerprinting technologies which use PCR amplification of a gene of interest e.g. small subunit rRNA gene, to study microbial community structure and dynamics. Either one or both of the forward and reverse strand primers used to amplify the gene are fluorescently labelled. The products of restriction endonuclease digestion are electrophoresed with an automated sequencer that detects only the terminal (labelled) restriction fragments (T-RFs). In LH-PCR, products are electrophoresed without digestion, with different fragment lengths being due to inherent variation in the amplified sequence. A novel software system, TRUFFLER, has been developed to mimic this process in silico allowing comparison of experimental data against databases of theoretically determined T-RFs. As a given combination of forward and reverse primers and restriction endonuclease can yield identical T-RFs across a number of species, combinations of different endonucleases (and/or primers) are typically used In addition to fragment length data, data on fluorescence levels is also available. Computationally, this can be viewed as a constraint satisfaction problem which can be solved to allow identification of the dominant members of the microbial community, often down to individual species or at least genus level, and their relative proportions.
机译:末端限制性片段长度多态性(T-RFLP)和长度异质性聚合酶链反应(LH-PCR)是DNA指纹技术,其使用感兴趣的基因(例如cDNA)进行PCR扩增。小亚基rRNA基因,研究微生物群落结构和动力学。对用于扩增基因的正向和反向链引物之一或两者进行荧光标记。限制性核酸内切酶消化的产物用自动测序仪进行电泳,该自动测序仪仅检测末端(标记的)限制性片段(T-RF)。在LH-PCR中,无需消化即可对产物进行电泳,不同的片段长度归因于扩增序列的固有差异。已开发出一种新型软件系统TRUFFLER来模拟计算机模拟此过程,从而可以将实验数据与理论上确定的T-RF的数据库进行比较。由于正向和反向引物与限制性核酸内切酶的既定组合可在许多物种中产生相同的T-RF,因此通常使用不同核酸内切酶(和/或引物)的组合。可用的。从计算上讲,这可以视为一个约束满足问题,可以解决该问题,以便确定微生物群落的主要成员(通常仅限于单个物种或至少属属水平)及其相对比例。

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