Abstract
Long QT syndrome type 2 is caused by mutations in the human ether-a-go-go-related gene (hERG). We previously reported that the N470D mutation is retained in the endoplasmic reticulum (ER) but can be rescued to the plasma membrane by hERG channel blocker E-4031. The mechanisms of ER retention and how E-4031 rescues the N470D mutant are poorly understood. In this study, we investigated the interaction of hERG channels with the ER chaperone protein calnexin. Using coimmunoprecipitation, we showed that the immature forms of both wild type hERG and N470D associated with calnexin. The association required N-linked glycosylation of hERG channels. Pulse-chase analysis revealed that N470D had a prolonged association with calnexin compared with wild type hERG and E-4031 shortened the time course of calnexin association with N470D. To test whether the prolonged association of N470D with calnexin is due to defective folding of mutant channels, we studied hERG channel folding using the trypsin digestion method. We found that N470D and the immature form of wild type hERG were more sensitive to trypsin digestion than the mature form of wild type hERG. In the presence of E-4031, N470D became more resistant to trypsin even when its ER-to-Golgi transport was blocked by brefeldin A. These results suggest that defective folding of N470D contributes to its prolonged association with calnexin and ER retention and that E-4031 may restore proper folding of the N470D channel leading to its cell surface expression.
Highlights
We have previously shown that the maturation of newly synthesized human ether-a-go-go-related gene (hERG) protein in the endoplasmic reticulum (ER) is under stringent surveillance by the quality control system [16]
The prolonged association of N470D with calnexin may be due to defective folding of the mutant protein as evidenced by its increased sensitivity to trypsin digestion compared with wild type hERG
Interaction of Calnexin with Wild Type hERG and the N470D Mutant— To study the mechanism of defective trafficking of the N470D mutant, we examined the interaction of calnexin with wild type hERG and the N470D mutant
Summary
We have previously shown that the maturation of newly synthesized hERG protein in the ER is under stringent surveillance by the quality control system [16]. The prolonged association of N470D with calnexin may be due to defective folding of the mutant protein as evidenced by its increased sensitivity to trypsin digestion compared with wild type hERG.
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