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通过反义介导果蝇中微小RNA 2和13失活导致的发育缺陷以及假定靶基因的鉴定。

Developmental defects by antisense-mediated inactivation of micro-RNAs 2 and 13 in Drosophila and the identification of putative target genes.

作者信息

Boutla Alexandra, Delidakis Christos, Tabler Martin

机构信息

Institute of Molecular Biology and Biotechnology, Foundation for Research and Technology, Hellas, PO Box 1527, GR-71110 Heraklion/Crete, Greece.

出版信息

Nucleic Acids Res. 2003 Sep 1;31(17):4973-80. doi: 10.1093/nar/gkg707.

Abstract

Micro-RNAs are a class of small non-coding regulatory RNAs that impair translation by imperfect base pairing to mRNAs. For analysis of their cellular function we injected different miRNA-specific DNA antisense oligonucleotides in Drosophila embryos. In four cases we observed severe interference with normal development, one had a moderate impact and six oligonucleotides did not cause detectable phenotypes. We further used the miR-13a DNA antisense oligonucleotide as a PCR primer on a cDNA library template. In this experimental way we identified nine Drosophila genes, which are characterised by 3' untranslated region motifs that allow imperfect duplex formation with miR-13 or related miRNAs. These genes, which include Sos and Myd88, represent putative targets for miRNA regulation. Mutagenesis of the target motif of two genes followed by transfection in Drosophila Schneider 2 (S2) cells and subsequent reporter gene analysis confirmed the hypothesis that the binding potential of miR-13 is inversely correlated with gene expression.

摘要

微小RNA是一类小的非编码调节性RNA,它们通过与信使核糖核酸(mRNA)进行不完全碱基配对来损害翻译过程。为了分析它们的细胞功能,我们在果蝇胚胎中注射了不同的微小RNA特异性DNA反义寡核苷酸。在四种情况下,我们观察到对正常发育的严重干扰,一种有中等影响,六种寡核苷酸未引起可检测到的表型。我们进一步将miR-13a DNA反义寡核苷酸用作cDNA文库模板上的PCR引物。通过这种实验方法,我们鉴定出九个果蝇基因,其特征在于3'非翻译区基序,该基序允许与miR-13或相关微小RNA形成不完全双链体。这些基因包括Sos和Myd88,代表了微小RNA调节的假定靶标。对两个基因的靶标基序进行诱变,然后转染到果蝇施耐德2(S2)细胞中并随后进行报告基因分析,证实了miR-13的结合潜力与基因表达呈负相关的假设。

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