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首页> 外文期刊>Nucleic Acids Research >Inhibition of pre-mRNA splicing by synthetic branched nucleic acids
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Inhibition of pre-mRNA splicing by synthetic branched nucleic acids

机译:合成分支核酸抑制前mRNA剪接

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The cellular transformation of a precursor mRNA (pre-mRNA) into its mature or functional form proceeds by way of a splicing reaction, in which the exons are ligated to form the mature linear RNA and the introns are excised as branched or lariat RNAs. We have prepared a series of branched compounds (bRNA and bDNA), and studied the effects of such molecules on the efficiency of mammalian pre-mRNA splicing in vitro. Y-shaped RNAs containing an unnatural L-2'-deoxycytidine unit (L-dC) at the 3' termini are highly stabilized against exonuclease hydrolysis in HeLa nuclear extracts, and are potent inhibitors of the splicing pathway. A bRNA containing internal 2'-O-methyl ribopyrimidine units and L-dC at the 3' ends was at least twice as potent as the most potent of the bRNAs containing no 2' modifications, with an IC_(50) of ~5 μM. Inhibitory activity was maintained in a branched molecule containing an arabino-adenosine branchpoint which, unlike the native bRANs, resisted cleavage by the lariat-debranching enzyme. The data obtained suggest that binding and sequestering of a branch recognition factor by the branched nucleic acids is an early event, which occurs prior to the first chemical step of splicing. Probably, an early recognition element preferentially binds to the synthetic branched molecules over the native pre-mRNA. As such, synthetic bRNAs may prove to be invaluable tools for the purification and identification of the putative branchopint recognition factor.
机译:前体mRNA(pre-mRNA)的细胞转化通过剪接反应进行,在该剪接反应中,外显子被连接形成成熟的线性RNA,内含子被切成分支或套索状RNA。我们准备了一系列分支化合物(bRNA和bDNA),并研究了此类分子对哺乳动物pre-mRNA体外剪接效率的影响。在3'末端含有非天然L-2'-脱氧胞苷单元(L-dC)的Y形RNA高度稳定,可抵抗HeLa核提取物中的核酸外切酶水解,是剪接途径的有效抑制剂。含有内部2'-O-甲基核糖嘧啶单元且在3'端具有L-dC的bRNA的效力至少是不含2'修饰的bRNA的最强效力的两倍,IC_(50)约为5μM 。在含有阿拉伯-腺苷分支点的支链分子中保持抑制活性,该分支点与天然bRANs不同,抵抗套索状分支酶的切割。所获得的数据表明,分支核酸与分支识别因子的结合和螯合是一个早期事件,发生在剪接的第一个化学步骤之前。可能,早期识别元件优先于天然pre-mRNA结合至合成的分支分子。这样,合成的bRNA可能被证明是提纯和鉴定推定的braintopint识别因子的宝贵工具。

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