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Efficient inhibition of RNA self-primed extension by addition of competing 3 '-capture DNA-improved RNA synthesis by T7 RNA polymerase

机译:通过添加竞争3' - 通过T7 RNA聚合酶添加竞争3' - 改善RNA改善的RNA合成,高效抑制RNA自灌注延伸

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摘要

In vitro synthesized RNA is used widely in studies of RNA biology, biotechnology and RNA therapeutics. However, in vitro synthesized RNA often contains impurities, such as RNAs with lengths shorter and longer than the expected runoff RNA. We have recently confirmed that longer RNA products are formed predominantly via cis self-primed extension, in which released runoff RNA folds back on itself to prime its own RNA-templated extension. In the current work, we demonstrate that addition of a DNA oligonucleotide (capture DNA) that is complementary to the 3' end of the expected runoff RNA effectively prevents self-primed extension, even under conditions commonly used for high RNA yields. Moreover, the presence of this competing capture DNA during 'high yield' transcription, leads to an increase in the yield of expected runoff RNA by suppressing the formation of undesired longer RNA byproducts.
机译:体外合成RNA广泛用于RNA生物学,生物技术和RNA治疗剂的研究。 然而,体外合成的RNA通常含有杂质,例如长度短且长于预期的径流RNA的RNA。 我们最近证实,通过CIS自灌注延伸,较长的RNA产品主要形成,其中释放径流RNA自身折叠以使其自身的RNA模板延伸。 在当前的工作中,我们证明了与预期径流RNA的3'末端互补的DNA寡核苷酸(捕获DNA)有效地防止了自灌注延伸,即使在常用于高RNA产率的条件下也是如此。 此外,在“高收益率”转录期间存在这种竞争捕获DNA,导致预期径流RNA的产量增加,通过抑制不期望的较长RNA副产物的形成。

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