Gemel Joanna, Simon Adria R, Patel Dakshesh, Xu Qin, Matiukas Arvydas, Veenstra Richard D, Beyer Eric C
Department of Pediatrics, University of Chicago, Chicago, IL 60637, USA.
Department of Pharmacology, SUNY Upstate Medical University, Syracuse, NY 13210, USA.
J Mol Cell Cardiol. 2014 Sep;74:330-9. doi: 10.1016/j.yjmcc.2014.06.010. Epub 2014 Jun 25.
Several Cx40 mutants have been identified in patients with atrial fibrillation (AF). We have been working to identify physiological or cell biological abnormalities of several of these human mutants that might explain how they contribute to disease pathogenesis. Wild type (wt) Cx40 or four different mutants (P88S, G38D, V85I, and L229M) were expressed by the transfection of communication-deficient HeLa cells or HL-1 cardiomyocytes. Biophysical channel properties and the sub-cellular localization and protein levels of Cx40 were characterized. Wild type Cx40 and all mutants except P88S formed gap junction plaques and induced significant gap junctional conductances. The functional mutants showed only modest alterations of single channel conductances or gating by trans-junctional voltage as compared to wtCx40. However, immunoblotting indicated that the steady state levels of G38D, V85I, and L229M were reduced relative to wtCx40; most strikingly, G38D was only 20-31% of wild type levels. After the inhibition of protein synthesis with cycloheximide, G38D (and to a lesser extent the other mutants) disappeared much faster than wtCx40. Treatment with the proteasomal inhibitor, epoxomicin, greatly increased levels of G38D and restored the abundance of gap junctions and the extent of intercellular dye transfer. Thus, G38D, V85I, and L229M are functional mutants of Cx40 with small alterations of physiological properties, but accelerated degradation by the proteasome. These findings suggest a novel mechanism (protein instability) for the pathogenesis of AF due to a connexin mutation and a novel approach to therapy (protease inhibition).
在心房颤动(AF)患者中已鉴定出几种Cx40突变体。我们一直在努力确定其中几种人类突变体的生理或细胞生物学异常,这可能解释它们如何导致疾病发病机制。通过转染缺乏通讯功能的HeLa细胞或HL-1心肌细胞来表达野生型(wt)Cx40或四种不同的突变体(P88S、G38D、V85I和L229M)。对Cx40的生物物理通道特性、亚细胞定位和蛋白质水平进行了表征。野生型Cx40和除P88S之外的所有突变体均形成了间隙连接斑并诱导了显著的间隙连接电导。与wtCx40相比,功能性突变体仅显示单通道电导或跨结电压门控的适度改变。然而,免疫印迹表明,相对于wtCx40,G38D、V85I和L229M的稳态水平降低;最显著的是,G38D仅为野生型水平的20-31%。在用环己酰亚胺抑制蛋白质合成后,G38D(以及程度较轻的其他突变体)比wtCx40消失得快得多。用蛋白酶体抑制剂环氧霉素处理后,G38D的水平大大增加,并恢复了间隙连接的丰度和细胞间染料转移的程度。因此,G38D、V85I和L229M是Cx40的功能性突变体,其生理特性仅有微小改变,但被蛋白酶体加速降解。这些发现提示了一种由于连接蛋白突变导致AF发病机制的新机制(蛋白质不稳定性)和一种新的治疗方法(蛋白酶抑制)。