Ryanodine receptor ion channels (RyR1s) release Ca ions from the sarcoplasmic reticulum to regulate skeletal muscle contraction. By whole-exome sequencing, we identified the heterozygous RYR1 variant c.14767_14772del resulting in the in-frame deletion p.(Phe4923_Phe4924del) in two brothers with a lethal form of the fetal akinesia deformation syndrome (FADS). The two deleted phenylalanines (RyR1-ΔFF) are located in the S6 pore-lining helix of RyR1. Clinical features in one of the two siblings included severe hypotonia, thin ribs, swallowing inability, and respiratory insufficiency that caused early death. Functional consequences of the RyR1-ΔFF variant were determined using recombinant 2,200-kDa homotetrameric and heterotetrameric RyR1 channel complexes that were expressed in HEK293 cells and characterized by cellular, electrophysiological, and computational methods. Cellular Ca release in response to caffeine indicated that the homotetrameric variant formed caffeine-sensitive Ca conducting channels in HEK293 cells. In contrast, the homotetrameric channel complex was not activated by Ca and did not conduct Ca based on single-channel measurements. The computational analysis suggested decreased protein stability and loss of salt bridge interactions between RyR1-R4944 and RyR1-D4938, increasing the electrostatic interaction energy of Ca in a region 20 Å from the mutant site. Co-expression of wild-type and mutant RyR1s resulted in Ca-dependent channel activities that displayed intermediate Ca conductances and suggested maintenance of a reduced Ca release in the two patients. Our findings reveal that the RYR1 pore variant p.(Phe4923_Phe4924del) attenuates the flow of Ca through heterotetrameric channels, but alone was not sufficient to cause FADS, indicating additional genetic factors to be involved.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7216825PMC
http://dx.doi.org/10.1016/j.ceca.2020.102182DOI Listing

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