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Mouse ES cells express endogenous shRNAs siRNAs and other Microprocessor-independent Dicer-dependent small RNAs

机译:小鼠ES细胞表达内源性shRNAsiRNA和其他不依赖微处理器依赖切丁酶的小RNA

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摘要

Canonical microRNAs (miRNAs) require two processing steps: the first by the Microprocessor, a complex of DGCR8 and Drosha, and the second by a complex of TRBP and Dicer. dgcr8Δ/Δ mouse embryonic stem cells (mESCs) have less severe phenotypes than dicer1Δ/Δ mESCs, suggesting a physiological role for Microprocessor-independent, Dicer-dependent small RNAs. To identify these small RNAs with unusual biogenesis, we performed high-throughput sequencing from wild-type, dgcr8Δ/Δ, and dicer1Δ/Δ mESCs. Several of the resulting DGCR8-independent, Dicer-dependent RNAs were noncanonical miRNAs. These derived from mirtrons and a newly identified subclass of miRNA precursors, which appears to be the endogenous counterpart of shRNAs. Our analyses also revealed endogenous siRNAs resulting from Dicer cleavage of long hairpins, the vast majority of which originated from one genomic locus with tandem, inverted short interspersed nuclear elements (SINEs). Our results extend the known diversity of mammalian small RNA-generating pathways and show that mammalian siRNAs exist in cell types other than oocytes.
机译:规范的microRNA(miRNA)需要两个处理步骤:第一步是由微处理器处理,是DGCR8和Drosha的复合物,第二步是由TRBP和Dicer的复合物。 dgcr8Δ/Δ小鼠胚胎干细胞(mESCs)的表型不如dicer1Δ/ΔmESCs严重,因此暗示了微处理器无关,Dicer依赖性小RNA的生理作用。为了鉴定具有异常生物发生的这些小RNA,我们从野生型,dgcr8Δ/Δ和dicer1Δ/ΔmESCs中进行了高通量测序。所产生的不依赖DGCR8的,依赖切酶切器的RNA中的一些是非经典miRNA。这些来自mirtrons和miRNA前体的新鉴定的亚类,miRNA前体似乎是shRNA的内源对应物。我们的分析还揭示了内切siRNA是由Dicer切割长发夹而产生的,其中大部分来自一个基因组位点,具有串联,倒置的短散布的核元件(SINEs)。我们的研究结果扩展了哺乳动物小RNA产生途径的已知多样性,并表明哺乳动物siRNA存在于卵母细胞以外的其他细胞类型中。

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