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miR-9a 通过抑制果蝇 LIM 仅蛋白来防止翅膀发育中的细胞凋亡。

miR-9a prevents apoptosis during wing development by repressing Drosophila LIM-only.

机构信息

Department of Developmental Biology, Sloan-Kettering Institute, 1275 York Ave, Box 252, New York, NY 10065, USA.

出版信息

Dev Biol. 2010 Feb 1;338(1):63-73. doi: 10.1016/j.ydbio.2009.11.025. Epub 2009 Nov 26.

Abstract

Loss of Drosophila mir-9a induces a subtle increase in sensory bristles, but a substantial loss of wing tissue. Here, we establish that the latter phenotype is largely due to ectopic apoptosis in the dorsal wing primordium, and we could rescue wing development in the absence of this microRNA by dorsal-specific inhibition of apoptosis. Such apoptosis was a consequence of de-repressing Drosophila LIM-only (dLMO), which encodes a transcriptional regulator of wing and neural development. We observed cell-autonomous elevation of endogenous dLMO and a GFP-dLMO 3'UTR sensor in mir-9a mutant wing clones, and heterozygosity for dLMO rescued the apoptosis and wing defects of mir-9a mutants. We also provide evidence that dLMO, in addition to senseless, contributes to the bristle defects of the mir-9a mutant. Unexpectedly, the upregulation of dLMO, loss of Cut, and adult wing margin defects seen with mir-9a mutant clones were not recapitulated by clonal loss of the miRNA biogenesis factors Dicer-1 or Pasha, even though these mutant conditions similarly de-repressed miR-9a and dLMO sensor transgenes. Therefore, the failure to observe a phenotype upon conditional knockout of a miRNA processing factor does not reliably indicate the lack of critical roles of miRNAs in a given setting.

摘要

果蝇 miR-9a 的缺失会导致感觉刚毛轻微增加,但翅膀组织大量缺失。在这里,我们确定后一种表型主要是由于背翅原基中的异位细胞凋亡引起的,并且我们可以通过背侧特异性抑制细胞凋亡来挽救缺乏这种 miRNA 的翅膀发育。这种凋亡是去抑制果蝇 LIM 仅(dLMO)的结果,dLMO 编码翅膀和神经发育的转录调节剂。我们观察到内源 dLMO 和 GFP-dLMO 3'UTR 传感器在 mir-9a 突变体翅膀克隆中的细胞自主升高,并且 dLMO 的杂合性挽救了 mir-9a 突变体的细胞凋亡和翅膀缺陷。我们还提供了证据表明,dLMO 除了 senseless 之外,还导致了 mir-9a 突变体的刚毛缺陷。出乎意料的是,mir-9a 突变体克隆中观察到的 dLMO 上调、Cut 的缺失以及成年翅膀边缘缺陷,并没有通过 miRNA 生物发生因子 Dicer-1 或 Pasha 的克隆缺失重现,尽管这些突变条件同样去抑制了 miR-9a 和 dLMO 传感器转基因。因此,在 miRNA 加工因子条件性敲除时未能观察到表型并不可靠地表明 miRNA 在特定环境中没有关键作用。

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