Abstract
Loss-of-function mutations in the cardiac Na+ channel α-subunit Nav1.5, encoded by SCN5A, cause Brugada syndrome (BrS), a hereditary disease characterized by sudden cardiac death due to ventricular fibrillation. We previously evidenced in vitro the dominant-negative effect of the BrS Nav1.5-R104W variant, inducing retention of wild-type (WT) channels and leading to a drastic reduction of the resulting Na+ current (INa). To explore this dominant-negative effect in vivo, we created a murine model using adeno-associated viruses (AAVs).MethodsDue to the large size of SCN5A, a dual AAV vector strategy was used combining viral DNA recombination and trans-splicing. Mice were injected with two AAV serotypes capsid 9: one packaging the cardiac specific troponin-T promoter, the 5′ half of hSCN5A cDNA, a splicing donor site and a recombinogenic sequence; and another packaging the complementary recombinogenic sequence, a splicing acceptor site, the 3′ half of hSCN5A cDNA fused to the gfp gene sequence, and the SV40 polyA signal. Eight weeks after AAV systemic injection in wild-type (WT) mice, echocardiography and ECG were recorded and mice were sacrificed. The full-length hSCN5A-gfp expression was assessed by western blot and immunohistochemistry in transduced heart tissues and the Na+ current was recorded by the patch-clamp technique in isolated adult GFP-expressing heart cells.ResultsAlmost 75% of the cardiomyocytes were transduced in hearts of mice injected with hNav1.5 and ∼30% in hNav1.5-R104W overexpressing tissues. In ventricular mice cardiomyocytes expressing R104W mutant channels, the endogenous INa was significantly decreased. Moreover, overexpression of R104W channels in normal hearts led to a decrease of total Nav1.5 expression. The R104W mutant also induced a slight dilatation of mice left ventricles and a prolongation of RR interval and P-wave duration in transduced mice. Altogether, our results demonstrated an in vivo dominant-negative effect of defective R104W channels on endogenous ones.ConclusionUsing a trans-splicing and viral DNA recombination strategy to overexpress the Na+ channel in mouse hearts allowed us to demonstrate in vivo the dominant-negative effect of a BrS variant identified in the N-terminus of Nav1.5.
Highlights
Brugada syndrome (BrS) is an inherited autosomaldominant cardiac channelopathy with incomplete penetrance, characterized by a typical electrocardiographic (ECG) pattern showing an ST-segment elevation in the right precordial leads (V1–V3) and an increased risk of sudden cardiac death due to ventricular fibrillation in structurally normal hearts (Brugada et al, 2018)
Our results demonstrated that the use of associated Viruses (AAVs) to overexpress SCN5A mutants in vivo is a relevant approach to create a versatile and valuable animal model of BrS
Using the Human Splicing Finder tool1, we obtained the best score for the junction between exons 17 and 18 of SCN5A, which permitted to cut the full cDNA into two portions of equivalent size and to obtain dual hybrid AAV genomes of 4.4 and 4.7 kb, respectively
Summary
Brugada syndrome (BrS) is an inherited autosomaldominant cardiac channelopathy with incomplete penetrance, characterized by a typical electrocardiographic (ECG) pattern showing an ST-segment elevation in the right precordial leads (V1–V3) and an increased risk of sudden cardiac death due to ventricular fibrillation in structurally normal hearts (Brugada et al, 2018). It was unexpected to report Nav1.5 mutants with a dominant-negative effect on wildtype (WT) channels, as we and others did a few years ago (Keller et al, 2005; Clatot et al, 2012; Mercier et al, 2012; Hoshi et al, 2014; Pambrun et al, 2014; Wang et al, 2020) In these studies, a decrease of INa exceeding the 50% of current density expected in case of haploinsufficiency was observed when co-expressing some mutants with WT channels in a 1:1 ratio to mimic patient heterozygosity (Keller et al, 2005; Clatot et al, 2012; Hoshi et al, 2014). It was established that Nav1.5 α-subunits form dimers through an interaction site located in the domain I-II linker, and that Nav1.5 channels interact and gate as dimers (Clatot et al, 2017)
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