Forward genetic screen in human podocytes identifies diphthamide biosynthesis genes as regulators of adhesion

被引:6
|
作者
Cina, Davide P. [1 ,2 ]
Ketela, Troy [3 ]
Brown, Kevin R. [3 ]
Chandrashekhar, Megha [3 ]
Mero, Patricia [3 ]
Li, Chengjin [4 ]
Onay, Tuncer [1 ,2 ]
Fu, Yulong [5 ]
Han, Zhe [5 ]
Saleem, Moin [6 ,7 ]
Moffat, Jason [3 ]
Quaggin, Susan E. [1 ,2 ]
机构
[1] Northwestern Univ, Feinberg Cardiovasc & Renal Res Inst, Feinberg Sch Med, Chicago, IL USA
[2] Northwestern Univ, Dept Med, Feinberg Sch Med, Div Nephrol & Hypertens, Chicago, IL 60611 USA
[3] Univ Toronto, Donnelly Ctr, Banting & Best Dept Med Res, Toronto, ON, Canada
[4] Univ Toronto, Tanenbaum Lunenfeld Res Inst, Toronto, ON, Canada
[5] Childrens Natl Hlth Syst, Ctr Genet Med Res, Washington, DC USA
[6] Univ Bristol, Childrens Renal Unit, Sch Clin Sci, Bristol, Avon, England
[7] Univ Bristol, Acad Renal Unit, Bristol, Avon, England
基金
美国国家卫生研究院; 加拿大健康研究院;
关键词
adhesion; diphthamide; genetic screen; glomerulus; podocyte; INTEGRIN ADHESOME; CANDIDATE GENE; MUTATIONS; NEPHROPATHY; EXPRESSION; NEPHROSIS; COMPLEX; PROTEIN; DELGEF; SYSTEM;
D O I
10.1152/ajprenal.00195.2019
中图分类号
Q4 [生理学];
学科分类号
071003 ;
摘要
Podocyte function is tightly linked to the complex organization of its cytoskeleton and adhesion to the underlying glomerular basement membrane. Adhesion of cultured podocytes to a variety of substrates is reported to correlate with podocyte health. To identify novel genes that are important for podocyte function, we designed an in vitro genetic screen based on podocyte adhesion to plates coated with either fibronectin or soluble Fms-like tyrosine kinase-1 (sFLT1)/Fc. A genome-scale pooled RNA interference screen on immortalized human podocytes identified 77 genes that increased adhesion to fibronectin, 101 genes that increased adhesion to sFLT1/Fc, and 44 genes that increased adhesion to both substrates when knocked down. Multiple shRNAs against diphthamide biosynthesis protein 1-4 (DPH1-DPH4) were top hits for increased adhesion. Immortalized human podocyte cells stably expressing these hairpins displayed increased adhesion to both substrates. We then used CRISPR-Cas9 to generate podocyte knockout cells for DPH1, DPH2, or DPH3, which also displayed increased adhesion to both fibronectin and sFLT1/Fc, as well as a spreading defect. Finally, we showed that Drosophila nephrocyte-specific knockdown of Dph1, Dph2, and Dph4 resulted in altered nephrocyte function. In summary, we report here a novel high-throughput method to identify genes important for podocyte function. Given the central role of podocyte adhesion as a marker of podocyte health, these data are a rich source of candidate regulators of glomerular disease.
引用
收藏
页码:F1593 / F1604
页数:12
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