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个体 microRNAs(miRNAs)表现出不同的 mRNA 靶向“规则”。

Individual microRNAs (miRNAs) display distinct mRNA targeting "rules".

机构信息

Department of Pathology, University of Kentucky Medical Center, Lexington, KY, USA.

出版信息

RNA Biol. 2010 May-Jun;7(3):373-80. doi: 10.4161/rna.7.3.11693.

Abstract

MicroRNAs (miRNAs) guide Argonaute (AGO)-containing microribonucleoprotein (miRNP) complexes to target mRNAs.It has been assumed that miRNAs behave similarly to each other with regard to mRNA target recognition. The usual assumptions, which are based on prior studies, are that miRNAs target preferentially sequences in the 3'UTR of mRNAs,guided by the 5' "seed" portion of the miRNAs. Here we isolated AGO- and miRNA-containing miRNPs from human H4 tumor cells by co-immunoprecipitation (co-IP) with anti-AGO antibody. Cells were transfected with miR-107, miR-124,miR-128, miR-320, or a negative control miRNA. Co-IPed RNAs were subjected to downstream high-density Affymetrix Human Gene 1.0 ST microarray analyses using an assay we validated previously-a "RIP-Chip" experimental design. RIP-Chip data provided a list of mRNAs recruited into the AGO-miRNP in correlation to each miRNA. These experimentally identified miRNA targets were analyzed for complementary six nucleotide "seed" sequences within the transfected miRNAs. We found that miR-124 targets tended to have sequences in the 3'UTR that would be recognized by the 5' seed of miR-124, as described in previous studies. By contrast, miR-107 targets tended to have 'seed' sequences in the mRNA open reading frame, but not the 3' UTR. Further, mRNA targets of miR-128 and miR-320 are less enriched for 6-mer seed sequences in comparison to miR-107 and miR-124. In sum, our data support the importance of the 5' seed in determining binding characteristics for some miRNAs; however, the "binding rules" are complex, and individual miRNAs can have distinct sequence determinants that lead to mRNA targeting.

摘要

微小 RNA(miRNA)指导 Argonaute(AGO)含有 microribonucleoprotein(miRNP)复合物靶向 mRNAs。人们一直认为 miRNA 在 mRNA 靶标识别方面彼此相似。通常的假设是,miRNA 优先靶向 mRNAs 3'UTR 中的序列,由 miRNA 的 5'“种子”部分引导。在这里,我们通过与抗 AGO 抗体的共免疫沉淀(co-IP)从人 H4 肿瘤细胞中分离出 AGO 和 miRNA 含有 miRNP。细胞用 miR-107、miR-124、miR-128、miR-320 或阴性对照 miRNA 转染。共免疫沉淀的 RNA 进行下游高密度 Affymetrix Human Gene 1.0 ST microarray 分析,使用我们之前验证过的一种“RIP-Chip”实验设计。RIP-Chip 数据提供了与每种 miRNA 相关的招募到 AGO-miRNP 的 mRNAs 列表。这些通过实验鉴定的 miRNA 靶标被分析是否具有转染 miRNA 中的六个互补核苷酸“种子”序列。我们发现,miR-124 的靶标倾向于在 3'UTR 中具有序列,这些序列会被 miR-124 的 5'种子识别,这与之前的研究一致。相比之下,miR-107 的靶标倾向于在 mRNA 开放阅读框中具有“种子”序列,但不在 3'UTR 中。此外,miR-128 和 miR-320 的 mRNA 靶标与 miR-107 和 miR-124 相比,6 -mer 种子序列的富集程度较低。总之,我们的数据支持 5'种子在确定一些 miRNA 结合特征方面的重要性;然而,“结合规则”很复杂,单个 miRNA 可能具有导致 mRNA 靶向的独特序列决定因素。

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