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通过同源发夹RNA的表达在模式蘑菇灰盖鬼伞(Coprinus cinereus)中进行靶向基因沉默。

Targeted gene silencing in the model mushroom Coprinopsis cinerea (Coprinus cinereus) by expression of homologous hairpin RNAs.

作者信息

Wälti Martin A, Villalba Cristina, Buser Reto M, Grünler Anke, Aebi Markus, Künzler Markus

机构信息

Institute of Microbiology, ETH Zürich, Wolfgang-Pauli-Str. 10, CH-8093 Zürich, Switzerland.

出版信息

Eukaryot Cell. 2006 Apr;5(4):732-44. doi: 10.1128/EC.5.4.732-744.2006.

Abstract

The ink cap Coprinopsis cinerea is a model organism for studying fruiting body (mushroom) formation in homobasidiomycetes. Mutant screens and expression studies have implicated a number of genes in this developmental process. Functional analysis of these genes, however, is hampered by the lack of reliable reverse genetics tools for C. cinerea. Here, we report the applicability of gene targeting by RNA silencing for this organism. Efficient silencing of both an introduced GFP expression cassette and the endogenous cgl1 and cgl2 isogenes was achieved by expression of homologous hairpin RNAs. In latter case, silencing was the result of a hairpin construct containing solely cgl2 sequences, demonstrating the possibility of simultaneous silencing of whole gene families by a single construct. Expression of the hairpin RNAs reduced the mRNA levels of the target genes by at least 90%, as determined by quantitative real-time PCR. The reduced mRNA levels were accompanied by cytosine methylation of transcribed and nontranscribed DNA at both silencing and target loci in the case of constitutive high-level expression of the hairpin RNA but not in the case of transient expression. These results suggest the presence of both posttranscriptional and transcriptional gene silencing mechanisms in C. cinerea and demonstrate the applicability of targeted gene silencing as a powerful reverse genetics approach in this organism.

摘要

墨汁鬼伞是研究同担子菌纲子实体(蘑菇)形成的模式生物。突变体筛选和表达研究表明,许多基因参与了这一发育过程。然而,由于缺乏可靠的针对墨汁鬼伞的反向遗传学工具,这些基因的功能分析受到了阻碍。在此,我们报道了RNA沉默介导的基因靶向在该生物体中的适用性。通过表达同源发夹RNA,实现了对导入的绿色荧光蛋白(GFP)表达盒以及内源性cgl1和cgl2同基因的有效沉默。在后一种情况下,沉默是由仅包含cgl2序列的发夹构建体导致的,这表明通过单个构建体同时沉默整个基因家族的可能性。通过定量实时PCR测定,发夹RNA的表达使靶基因的mRNA水平降低了至少90%。在发夹RNA组成型高水平表达的情况下,mRNA水平的降低伴随着转录和非转录DNA在沉默位点和靶位点的胞嘧啶甲基化,但在瞬时表达的情况下则没有。这些结果表明墨汁鬼伞中存在转录后和转录基因沉默机制,并证明了靶向基因沉默作为一种强大的反向遗传学方法在该生物体中的适用性。

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