| Literature DB >> 32873651 |
Daniel Silverman1,2, Zuying Chai1, Wendy W S Yue1, Sravani Keerthi Ramisetty3, Sowmya Bekshe Lokappa3, Kazumi Sakai4, Rikard Frederiksen5, Parinaz Bina1, Stephen H Tsang6,7, Takahiro Yamashita4, Jeannie Chen3, King-Wai Yau8,9.
Abstract
Numerous rhodopsin mutations have been implicated in night blindness and retinal degeneration, often with unclear etiology. D190N-rhodopsin (D190N-Rho) is a well-known inherited human mutation causing retinitis pigmentosa. Both higher-than-normal spontaneous-isomerization activity and misfolding/mistargeting of the mutant protein have been proposed as causes of the disease, but neither explanation has been thoroughly examined. We replaced wild-type rhodopsin (WT-Rho) in Rho D190N/WT mouse rods with a largely "functionally silenced" rhodopsin mutant to isolate electrical responses triggered by D190N-Rho activity, and found that D190N-Rho at the single-molecule level indeed isomerizes more frequently than WT-Rho by over an order of magnitude. Importantly, however, this higher molecular dark activity does not translate into an overall higher cellular dark noise, owing to diminished D190N-Rho content in the rod outer segment. Separately, we found that much of the degeneration and shortened outer-segment length of Rho D190N/WT mouse rods was not averted by ablating rod transducin in phototransduction-also consistent with D190N-Rho's higher isomerization activity not being the primary cause of disease. Instead, the low pigment content, shortened outer-segment length, and a moderate unfolded protein response implicate protein misfolding as the major pathogenic problem. Finally, D190N-Rho also provided some insight into the mechanism of spontaneous pigment excitation.Entities:
Keywords: D190N-rhodopsin; night blindness; protein misfolding; retinitis pigmentosa; spontaneous isomerization
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Year: 2020 PMID: 32873651 PMCID: PMC7502766 DOI: 10.1073/pnas.2010417117
Source DB: PubMed Journal: Proc Natl Acad Sci U S A ISSN: 0027-8424 Impact factor: 11.205