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首页> 外文期刊>Journal of Microbiological Methods >RNA-conjugated template-switching RT-PCR method for generating an Escherichia coli cDNA library for small RNAs
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RNA-conjugated template-switching RT-PCR method for generating an Escherichia coli cDNA library for small RNAs

机译:RNA缀合的模板切换RT-PCR方法用于生成小型RNA的大肠杆菌cDNA文库

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摘要

The cDNA conversion of RNA molecules is a prerequisite for their analysis. In the case of prokaryotic RNAs, cDNA conversion is difficult due to a lack of the long poly(A) tails that are found in eukaryotic mRNAs. The full cDNAs for eukaryotic mRNAs can be amplified by the reverse transcription polymerase chain reaction (RT-PCR) using the template-switching method together with an oligo(dT) primer. To amplify the full cDNAs for prokaryotic RNAs, we modified the template-switching RT-PCR method by adopting an RNA linker at the 3' end of the target RNAs. Using this method, which we named as RNA-conjugated template-switching RT-PCR (RC/TS RT-PCR), we constructed a cDNA library for small RNAs from cold-shock-treated Escherichia coli cells. To confirm that the cDNAs were amplified by RC/TS RT-PCR without a loss of sequence information, clones carrying the 6S RNA sequence were analyzed from the cDNA library for small RNAs ranging from 130 to 350 nt. We found that the 6S RNA sequences were fully converted into the corresponding cDNAs, confirming that RC/TS RT-PCR is a useful method for constructing a cDNA library for small RNAs in E. coli. This method can be also used to construct a cDNA library for non-poly(A)-containing RNAs from eukaryotic cells.
机译:RNA分子的cDNA转化是它们分析的先决条件。在原核RNA的情况下,由于缺乏真核mRNA中的长聚(a)尾部,CDNA转化率困难。用逆转录聚合酶链反应(RT-PCR)与寡核苷酸(DT)引物一起通过逆转录聚合酶链反应(RT-PCR)来扩增真核mRNA的完整CDNA。为了扩增原核RNA的完整CDNA,我们通过采用靶RNA的3'末端采用RNA接头来修复模板切换RT-PCR方法。使用这种方法,我们将其命名为RNA缀合的模板切换RT-PCR(RC / TERT-PCR),我们构建了来自冷休克治疗的大肠杆菌细胞的小RNA的cDNA文库。为了确认CDNA通过RC / TER RT-PCR扩增而不丧失序列信息,从CDNA文库中分析携带6S RNA序列的克隆,用于小RNA,范围为130至350nt。我们发现将6S RNA序列完全转化为相应的CDNA,证实RC / TERT-PCR是在大肠杆菌中构建小RNA的cDNA文库的一种有用方法。该方法还可用于构建来自真核细胞的非聚(a)癌RNA的cDNA文库。

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