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3 ' end additions by T7 RNA polymerase are RNA self-templated, distributive and diverse in character-RNA-Seq analyses

机译:通过T7 RNA聚合酶的3'结束添加是RNA自模塑,分配和不同于性质-RNA-SEQ分析

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摘要

Synthetic RNA is widely used in basic science, nanotechnology and therapeutics research. The vast majority of this RNA is synthesized in vitro by T7 RNA polymerase or one of its close family members. However, the desired RNA is generally contaminated with products longer and shorter than the DNA-encoded product. To better understand these undesired byproducts and the processes that generate them, we analyze in vitro transcription reactions using RNA-Seq as a tool. The results unambiguously confirm that product RNA rebinds to the polymerase and self-primes (in cis) generation of a hairpin duplex, a process that favorably competes with promoter driven synthesis under high yield reaction conditions. While certain priming modes can be favored, the process is heterogeneous, both in initial priming and in the extent of priming, and already extended products can rebind for further extension, in a distributive process. Furthermore, addition of one or a few nucleotides, previously termed 'nontemplated addition,' also occurs via templated primer extension. At last, this work demonstrates the utility of RNA-Seq as a tool for in vitro mechanistic studies, providing information far beyond that provided by traditional gel electrophoresis.
机译:合成RNA广泛用于基础科学,纳米技术和治疗研究。通过T7 RNA聚合酶或其紧密家庭成员之一,体外合成绝大多数RNA。然而,所需的RNA通常污染产物较长并且比DNA编码产物短。为了更好地了解这些不期望的副产品和产生它们的过程,我们使用RNA-SEQ作为工具分析体外转录反应。结果明确证实,产品RNA重新授予Photopin双链体的聚合酶和自素(在CIS)产生,这是在高产反应条件下与启动子驱动合成有利竞争的过程。虽然可以赞成某些启动模式,但该过程是异质的,初始引发和在引发程度上,并且已经扩展的产品可以在分配过程中重新推翻进一步的延伸。此外,通过模板底漆延伸,还通过模板底漆延伸加入预先被称为“未预期的”的核苷酸。最后,这项工作证明了RNA-SEQ作为体外机制研究的工具的效用,提供了传统凝胶电泳的信息远远超过其提供的信息。

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