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使用光裂解生物素化核苷酸合成的 RNA 大大提高了催化效率。

RNAs synthesized using photocleavable biotinylated nucleotides have dramatically improved catalytic efficiency.

机构信息

Department of Chemistry and Biochemistry, Center for Biomolecular Structure & Organization, University of Maryland, 1115 Biomolecular Sciences Bldg, College Park, MD 20742-3360, USA.

出版信息

Nucleic Acids Res. 2011 Oct;39(19):8559-71. doi: 10.1093/nar/gkr464. Epub 2011 Jul 8.

Abstract

Obtaining homogeneous population of natively folded RNAs is a crippling problem encountered when preparing RNAs for structural or enzymatic studies. Most of the traditional methods that are employed to prepare large quantities of RNAs involve procedures that partially denature the RNA. Here, we present a simple strategy using 'click' chemistry to couple biotin to a 'caged' photocleavable (PC) guanosine monophosphate (GMP) in high yield. This biotin-PC GMP, accepted by T7 RNA polymerase, has been used to transcribe RNAs ranging in size from 27 to 527 nt. Furthermore we show, using an in-gel fluorescence assay, that natively prepared 160 and 175 kDa minimal group II intron ribozymes have enhanced catalytic activity over the same RNAs, purified via denaturing conditions and refolded. We conclude that large complex RNAs prepared by non-denaturing means form a homogeneous population and are catalytically more active than those prepared by denaturing methods and subsequent refolding; this facile approach for native RNA preparation should benefit synthesis of RNAs for biophysical and therapeutic applications.

摘要

获得天然折叠的 RNA 均相群体是在准备 RNA 进行结构或酶学研究时遇到的一个难题。大多数用于制备大量 RNA 的传统方法都涉及部分使 RNA 变性的步骤。在这里,我们提出了一种使用“点击”化学将生物素偶联到“笼状”光解(PC)鸟苷一磷酸(GMP)的简单策略,产量很高。这种生物素-PCGMP 可被 T7 RNA 聚合酶接受,已用于转录大小为 27 至 527nt 的 RNA。此外,我们通过凝胶荧光分析表明,天然制备的 160 和 175 kDa 最小 II 组内含子核酶的催化活性高于通过变性条件纯化和重折叠的相同 RNA。我们得出结论,通过非变性手段制备的大复杂 RNA 形成均相群体,并且比通过变性方法和随后的重折叠制备的 RNA 具有更高的催化活性;这种简便的天然 RNA 制备方法应有利于用于生物物理和治疗应用的 RNA 的合成。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5bd7/3201860/b1e5f717e8dc/gkr464f1.jpg

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