Ganesan Anand N, O'Rourke Brian, Maack Christoph, Colecraft Henry, Sidor Agnieszka, Johns David C
Institute of Molecular Cardiobiology, Department of Medicine, The Johns Hopkins University, Baltimore, MD 21205, USA.
Biochem Biophys Res Commun. 2005 Apr 8;329(2):749-54. doi: 10.1016/j.bbrc.2005.02.015.
The alpha(1c) subunit of the cardiac L-type Ca(2+) channel, which contains the channel pore, voltage- and Ca(2+)-dependent gating structures, and drug binding sites, has been well studied in heterologous expression systems, but many aspects of L-type Ca(2+) channel behavior in intact cardiomyocytes remain poorly characterized. Here, we develop adenoviral constructs with E1, E3 and fiber gene deletions, to allow incorporation of full-length alpha(1c) gene cassettes into the adenovirus backbone. Wild-type (alpha(1c-wt)) and mutant (alpha(1c-D-)) Ca(2+) channel adenoviruses were constructed. The alpha(1c-D-) contained four point substitutions at amino acid residues known to be critical for dihydropyridine binding. Both alpha(1c-wt) and alpha(1c-D-) expressed robustly in A549 cells (peak L-type Ca(2+) current (I(CaL)) at 0 mV: alpha(1c-wt) -9.94+/-1.00pA/pF, n=9; alpha(1c-D-) -10.30pA/pF, n=12). I(CaL) carried by alpha(1c-D-) was markedly less sensitive to nitrendipine (IC(50) 17.1 microM) than alpha(1c-wt) (IC(50) 88 nM); a feature exploited to discriminate between engineered and native currents in transduced guinea-pig myocytes. 10 microM nitrendipine blocked only 51+/-5% (n=9) of I(CaL) in alpha(1c-D-)-expressing myocytes, in comparison to 86+/-8% (n=9) of I(CaL) in control myocytes. Moreover, in 20 microM nitrendipine, calcium transients could still be evoked in alpha(1c-D-)-transduced cells, but were largely blocked in control myocytes, indicating that the engineered channels were coupled to sarcoplasmic reticular Ca(2+) release. These alpha(1c) adenoviruses provide an unprecedented tool for structure-function studies of cardiac excitation-contraction coupling and L-type Ca(2+) channel regulation in the native myocyte background.
心脏L型Ca(2+)通道的α(1c)亚基包含通道孔、电压和Ca(2+)依赖性门控结构以及药物结合位点,已在异源表达系统中得到充分研究,但完整心肌细胞中L型Ca(2+)通道行为的许多方面仍未得到充分表征。在此,我们构建了缺失E1、E3和纤维基因的腺病毒载体,以便将全长α(1c)基因盒整合到腺病毒骨架中。构建了野生型(α(1c-wt))和突变型(α(1c-D-))Ca(2+)通道腺病毒。α(1c-D-)在已知对二氢吡啶结合至关重要的氨基酸残基处有四个点突变。α(1c-wt)和α(1c-D-)在A549细胞中均能强劲表达(0 mV时的峰值L型Ca(2+)电流(I(CaL)):α(1c-wt) -9.94±1.00 pA/pF,n = 9;α(1c-D-) -10.30 pA/pF,n = 12)。α(1c-D-)携带的I(CaL)对尼群地平的敏感性(IC(50) 17.1 μM)明显低于α(1c-wt)(IC(50) 88 nM);这一特性被用于区分转导的豚鼠心肌细胞中工程化电流和天然电流。10 μM尼群地平仅阻断α(1c-D-)表达的心肌细胞中51±5%(n = 9)的I(CaL),而对照心肌细胞中I(CaL)的阻断率为86±8%(n = 9)。此外,在20 μM尼群地平存在时,α(1c-D-)转导的细胞中仍可诱发钙瞬变,但对照心肌细胞中的钙瞬变大多被阻断,这表明工程化通道与肌浆网Ca(2+)释放偶联。这些α(1c)腺病毒为在天然心肌细胞背景下研究心脏兴奋-收缩偶联和L型Ca(2+)通道调节的结构-功能提供了前所未有的工具。
