南方医科大学学报 ›› 2013, Vol. 33 ›› Issue (07): 983-.

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HL-1心肌细胞中桥粒蛋白基因表达下调对Nav1.5功能的影响

张黔桓,邓春玉,饶芳,刘晓颖,麦丽萍,朱杰宁,谭虹虹,吴书林   

  • 出版日期:2013-07-20 发布日期:2013-07-20

Desmoplakin expression silencing affects cardiac voltage-gated sodium channel Nav1.5 in HL-1 cells

  • Online:2013-07-20 Published:2013-07-20

摘要: 目的采用基因沉默技术抑制HL-1细胞的桥粒蛋白(DSP)基因表达以明确DSP与Nav1.5的结构和功能关系。方法用基
因沉默技术抑制DSP基因的表达,然后采用Western blotting检测HL-1细胞DSP和Nav1.5蛋白的表达,用双免疫荧光方法检测
DSP与Nav1.5蛋白的表达与定位情况,并用全细胞膜片钳技术检测细胞钠通道的电生理特征。结果与空白组和对照组相比,
siRNA-DSP组的DSP和Nav1.5 蛋白表达量降低。免疫荧光检测发现空白组和对照组DSP与Nav1.5蛋白存在共定位情况,而
siRNA-DSP组DSP和Cx43蛋白共定位则遭到破坏,并且膜片钳检测发现siRNA-DSP组峰值电流从(156.3±6.2)pA/pF 减少至
(41.8±3.1)pA/pF(P<0.05),电压依赖的失活曲线V0.5从-42 mV左移至-61 mV(P<0.05)和从失活恢复时间延长。结论DSP表
达抑制不仅使DSP与Nav1.5的共定位特征遭到破坏,而且还改变了Nav1.5电生理特征。

Abstract: Objective To investigate the association of desmoplakin with the distribution and function of Nav1.5 by RNA
silencing technology in HL-1 cells. Methods HL-1 cells with desmoplakin expression suppression by RNA silencing were
examined for desmoplakin and Nav1.5 protein expressions by Western blotting, and the distribution and co-location of
desmoplakin and Nav1.5 protein were detected by immunoflurescence staining. Patch-clamp recording was applied to analyze
the changes in whole-cell sodium current after desmoplakin silencing. Results Compared with the untreated group and
negative control group, the cells with desmoplakin silencing showed obviously reduced expressions of desmoplakin and
Nav1.5 proteins. Co-localization of desmoplakin and Nav1.5 was detected at cell-cell contact in untreated and control
conditions, and desmoplakin expression silencing induced a drastic redistribution of Nav1.5 with decreased peak current
density (156.3±6.2 vs 41.8±3.1, n=6, P<0.05), a shift in voltage dependence of steady-state inactivation (-42 mV vs -61 mV, n=5, P<
0.05), and prolonged time of recovery from inactivation. Conclusion Desmoplakin silencing caused redistribution of Nav1.5
protein and also changes in its electrophysiological properties in HL-1 cells.