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A universal method for the rapid isolation of all known classes of functional silencing small RNAs

机译:一种普遍的方法,用于快速隔离所有已知的功能沉默小RNA

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Diverse classes of silencing small (s)RNAs operate via ARGONAUTE-family proteins within RNA-induced-silencing-complexes (RISCs). Here, we have streamlined various embodiments of a Q-sepharose-based RISC-purification method that relies on conserved biochemical properties of all ARGONAUTEs. We show, in multiple benchmarking assays, that the resulting 15-min benchtop extraction procedure allows simultaneous purification of all known classes of RISC-associated sRNAs without prior knowledge of the samples-intrinsic ARGONAUTE repertoires. Optimized under a user-friendly format, the method – coined ‘TraPR’ for Trans-kingdom, rapid, affordable Purification of RISCs – operates irrespectively of the organism, tissue, cell type or bio-fluid of interest, and scales to minute amounts of input material. The method is highly suited for direct profiling of silencing sRNAs, with TraPR-generated sequencing libraries outperforming those obtained via gold-standard procedures that require immunoprecipitations and/or lengthy polyacrylamide gel-selection. TraPR considerably improves the quality and consistency of silencing sRNA sample preparation including from notoriously difficult-to-handle tissues/bio-fluids such as starchy storage roots or mammalian plasma, and regardless of RNA contaminants or RNA degradation status of samples.
机译:不同类别的沉默沉默RNA通过RNA诱导的沉积复合物(RISC)内的Argonaute-Family蛋白操作。在这里,我们已经简化了基于Q-Sepharose的RISC纯化方法的各种实施方案,其依赖于所有Argonautes的保守生化特性。在多个基准测试中,我们展示了所得到的15 min台面提取过程,允许同时纯化所有已知的RISC相关的SRNA,而无需先验知识 - 内在的Agronaute reptoIres。根据用户友好的格式优化,该方法 - 用于跨国的“TRAPR”,RISC的快速,价格净化净化 - 无论有机体,组织,细胞类型或感兴趣的生物流体如何运作,以及分钟的尺度输入材料。该方法非常适合于沉默SRNA的直接分析,Trapr产生的测序文库优于通过需要免疫沉淀和/或冗长的聚丙烯酰胺凝胶选择的金标准方法获得的库。 Trapr显着提高了沉默的SRNA样品制剂的质量和一致性,包括难以难以处理的组织/生物液,如淀粉储存根或哺乳动物等离子体,以及无论RNA污染物或样品的RNA降解状态。

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