A genome-wide CRISPR screen identifies CALCOCO2 as a regulator of beta cell function influencing type 2 diabetes risk

Author:

Rottner Antje K.ORCID,Ye YingyingORCID,Navarro-Guerrero Elena,Rajesh Varsha,Pollner Alina,Bevacqua Romina J.,Yang JingORCID,Spigelman Aliya F.,Baronio Roberta,Bautista Austin,Thomsen Soren K.,Lyon James,Nawaz Sameena,Smith Nancy,Wesolowska-Andersen Agata,Fox Jocelyn E. Manning,Sun HanORCID,Kim Seung K.ORCID,Ebner Daniel,MacDonald Patrick E.,Gloyn Anna L.ORCID

Abstract

AbstractIdentification of the genes and processes mediating genetic association signals for complex diseases represents a major challenge. As many of the genetic signals for type 2 diabetes (T2D) exert their effects through pancreatic islet-cell dysfunction, we performed a genome-wide pooled CRISPR loss-of-function screen in a human pancreatic beta cell line. We assessed the regulation of insulin content as a disease-relevant readout of beta cell function and identified 580 genes influencing this phenotype. Integration with genetic and genomic data provided experimental support for 20 candidate T2D effector transcripts including the autophagy receptor CALCOCO2. Loss of CALCOCO2 was associated with distorted mitochondria, less proinsulin-containing immature granules and accumulation of autophagosomes upon inhibition of late-stage autophagy. Carriers of T2D-associated variants at the CALCOCO2 locus further displayed altered insulin secretion. Our study highlights how cellular screens can augment existing multi-omic efforts to support mechanistic understanding and provide evidence for causal effects at genome-wide association studies loci.

Funder

Wellcome Trust

U.S. Department of Health & Human Services | NIH | National Institute of Diabetes and Digestive and Kidney Diseases

Publisher

Springer Science and Business Media LLC

Subject

Genetics

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