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对果蝇中散乱蛋白的突变分析确定了散乱蛋白中的新结构域以及轴蛋白的新抑制等位基因。

A mutational analysis of dishevelled in Drosophila defines novel domains in the dishevelled protein as well as novel suppressing alleles of axin.

作者信息

Penton Andrea, Wodarz Andreas, Nusse Roel

机构信息

Howard Hughes Medical Institute, Department of Developmental Biology, Stanford University Medical School, Stanford, California 94305-5323, USA.

出版信息

Genetics. 2002 Jun;161(2):747-62. doi: 10.1093/genetics/161.2.747.

Abstract

Drosophila dishevelled (dsh) functions in two pathways: it is necessary to transduce Wingless (Wg) signaling and it is required in planar cell polarity. To learn more about how Dsh can discriminate between these functions, we performed genetic screens to isolate additional dsh alleles and we examined the potential role of protein phosphorylation by site-directed mutagenesis. We identified two alleles with point mutations in the Dsh DEP domain that specifically disrupt planar polarity signaling. When positioned in the structure of the DEP domain, these mutations are located close to each other and to a previously identified planar polarity mutation. In addition to the requirement for the DEP domain, we found that a cluster of potential phosphorylation sites in a binding domain for the protein kinase PAR-1 is also essential for planar polarity signaling. To identify regions of dsh that are necessary for Wg signaling, we screened for mutations that modified a GMR-GAL4;UAS-dsh overexpression phenotype in the eye. We recovered many alleles of the transgene containing missense mutations, including mutations in the DIX domain and in the DEP domain, the latter group mapping separately from the planar polarity mutations. In addition, several transgenes had mutations within a domain containing a consensus sequence for an SH3-binding protein. We also recovered second-site-suppressing mutations in axin, mapping at a region that may specifically interact with overexpressed Dsh.

摘要

果蝇的无序蛋白(Dsh)在两条信号通路中发挥作用:它是转导无翅蛋白(Wg)信号所必需的,并且在平面细胞极性中也发挥作用。为了更深入了解Dsh如何区分这些功能,我们进行了遗传筛选以分离更多的dsh等位基因,并通过定点诱变研究了蛋白质磷酸化的潜在作用。我们鉴定出两个在Dsh DEP结构域中存在点突变的等位基因,这些突变特异性地破坏了平面极性信号。当定位在DEP结构域的结构中时,这些突变彼此靠近且靠近先前鉴定出的平面极性突变。除了DEP结构域的需求外,我们还发现蛋白激酶PAR-1结合结构域中的一组潜在磷酸化位点对于平面极性信号传导也至关重要。为了鉴定Wg信号传导所必需的dsh区域,我们筛选了能改变眼内GMR-GAL4;UAS-dsh过表达表型的突变。我们获得了许多含有错义突变的转基因等位基因,包括DIX结构域和DEP结构域中的突变,后一组与平面极性突变的定位不同。此外,几个转基因在一个含有SH3结合蛋白共有序列的结构域内存在突变。我们还在轴蛋白中获得了第二位点抑制突变,其定位在一个可能与过表达的Dsh特异性相互作用的区域。

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