TBC1D8B Mutations Implicate RAB11-Dependent Vesicular Trafficking in the Pathogenesis of Nephrotic Syndrome

狭缝隔膜 肾病综合征 基因沉默 足细胞 尼福林 生物 遗传学 发病机制 细胞生物学 基因 免疫学 内分泌学 蛋白尿
作者
Lina L Kampf,Ronen Schneider,Lea Gerstner,Roland Thünauer,Mengmeng Chen,Martin Helmstädter,Ali Amar,Ana C. Onuchic-Whitford,Reyner Loza Muñarriz,Afig Berdeli,Dominik Müller,Eva Schrezenmeier,Klemens Budde,Shrikant Mane,Kristen M. Laricchia,Heidi L. Rehm,Daniel G. MacArthur,Richard P. Lifton,Gerd Walz,Winfried Römer,Carsten Bergmann,Friedhelm Hildebrandt,Tobias Hermle
出处
期刊:Journal of The American Society of Nephrology 卷期号:30 (12): 2338-2353 被引量:25
标识
DOI:10.1681/asn.2019040414
摘要

Significance Statement The discovery of monogenic causes of nephrotic syndrome led to insights about the role of podocytes and the slit diaphragm in the pathogenesis of the disease. The authors describe novel mutations in TBC1D8B in five families with steroid-resistant nephrotic syndrome. TBC1D8B binds to active RAB11A and RAB11B. Silencing TBC1D8B leads to upregulation of RAB11-dependent processes suggesting TBC1D8B inhibits RAB11. TBC1D8B also interacts and colocalizes with the slit diaphragm protein nephrin. Silencing TBC1D8B in podocyte-like Drosophila nephrocytes causes mistrafficking of fly nephrin. Nephrin trafficking in Drosophila requires Rab11 , whereas overexpression of Rab11 causes a similar phenotype as TBC1D8B silencing. These findings implicate regulation of RAB11-dependent vesicular trafficking by TBC1D8B as a novel pathogenetic pathway in nephrotic syndrome. Background Mutations in about 50 genes have been identified as monogenic causes of nephrotic syndrome, a frequent cause of CKD. These genes delineated the pathogenetic pathways and rendered significant insight into podocyte biology. Methods We used whole-exome sequencing to identify novel monogenic causes of steroid-resistant nephrotic syndrome (SRNS). We analyzed the functional significance of an SRNS-associated gene in vitro and in podocyte-like Drosophila nephrocytes. Results We identified hemizygous missense mutations in the gene TBC1D8B in five families with nephrotic syndrome. Coimmunoprecipitation assays indicated interactions between TBC1D8B and active forms of RAB11. Silencing TBC1D8B in HEK293T cells increased basal autophagy and exocytosis, two cellular functions that are independently regulated by RAB11. This suggests that TBC1D8B plays a regulatory role by inhibiting endogenous RAB11. Coimmunoprecipitation assays showed TBC1D8B also interacts with the slit diaphragm protein nephrin, and colocalizes with it in immortalized cell lines. Overexpressed murine Tbc1d8b with patient-derived mutations had lower affinity for endogenous RAB11 and nephrin compared with wild-type Tbc1d8b protein. Knockdown of Tbc1d8b in Drosophila impaired function of the podocyte-like nephrocytes, and caused mistrafficking of Sns, the Drosophila ortholog of nephrin. Expression of Rab11 RNAi in nephrocytes entailed defective delivery of slit diaphragm protein to the membrane, whereas RAB11 overexpression revealed a partial phenotypic overlap to Tbc1d8b loss of function. Conclusions Novel mutations in TBC1D8B are monogenic causes of SRNS. This gene inhibits RAB11. Our findings suggest that RAB11-dependent vesicular nephrin trafficking plays a role in the pathogenesis of nephrotic syndrome.
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