首页> 美国卫生研究院文献>The Journal of Biophysical and Biochemical Cytology >Crystal structures of IFT70/52 and IFT52/46 provide insight into intraflagellar transport B core complex assembly
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Crystal structures of IFT70/52 and IFT52/46 provide insight into intraflagellar transport B core complex assembly

机译:IFT70 / 52和IFT52 / 46的晶体结构提供了鞭毛内转运B核复合体装配的见解

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摘要

Cilia are microtubule-based organelles that assemble via intraflagellar transport (IFT) and function as signaling hubs on eukaryotic cells. IFT relies on molecular motors and IFT complexes that mediate the contacts with ciliary cargo. To elucidate the architecture of the IFT-B complex, we reconstituted and purified the nonameric IFT-B core from Chlamydomonas reinhardtii and determined the crystal structures of C. reinhardtii IFT70/52 and Tetrahymena IFT52/46 subcomplexes. The 2.5-Å resolution IFT70/52 structure shows that IFT52330–370 is buried deeply within the IFT70 tetratricopeptide repeat superhelix. Furthermore, the polycystic kidney disease protein IFT88 binds IFT52281–329 in a complex that interacts directly with IFT70/IFT52330–381 in trans. The structure of IFT52C/IFT46C was solved at 2.3 Å resolution, and we show that it is essential for IFT-B core integrity by mediating interaction between IFT88/70/52/46 and IFT81/74/27/25/22 subcomplexes. Consistent with this, overexpression of mammalian IFT52C in MDCK cells is dominant-negative and causes IFT protein mislocalization and disrupted ciliogenesis. These data further rationalize several ciliogenesis phenotypes of IFT mutant strains.
机译:纤毛是基于微管的细胞器,通过鞭毛内运输(IFT)组装,并充当真核细胞上的信号传导枢纽。 IFT依靠分子马达和IFT复合物来调节与睫状货物的接触。为了阐明IFT-B复合物的体系结构,我们重构并纯化了莱茵衣藻的非异构IFT-B核心,并确定了莱茵衣藻IFT70 / 52和四膜虫IFT52 / 46亚复合物的晶体结构。 2.5Å分辨率的IFT70 / 52结构表明IFT52330–370深埋在IFT70四三肽重复超螺旋中。此外,多囊肾疾病蛋白IFT88以复合物的形式结合IFT52281-329,该复合物直接与IFT70 / IFT52330-381相互作用。解决了IFT52C / IFT46C的结构,分辨率为2.3Å,我们证明了它通过介导IFT88 / 70/52/46与IFT81 / 74/27/25/22亚复合物之间的相互作用,对于IFT-B核的完整性至关重要。与此相一致的是,MDF细胞中哺乳动物IFT52C的过度表达为显性阴性,并导致IFT蛋白错误定位并破坏了纤毛发生。这些数据进一步合理化了IFT突变菌株的几种纤毛发生表型。

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