Bernatchez G, Talwar D, Parent L
Département de Physiologie, Membrane Transport Research Group, Université de Montréal, Montréal, Québec H3C 3J7, Canada.
Biophys J. 1998 Oct;75(4):1727-39. doi: 10.1016/S0006-3495(98)77614-3.
Calcium-dependent inactivation has been described as a negative feedback mechanism for regulating voltage-dependent calcium influx in cardiac cells. Most recent evidence points to the C-terminus of the alpha1C subunit, with its EF-hand binding motif, as being critical in this process. The EF-hand binding motif is mostly conserved between the C-termini of six of the seven alpha1 subunit Ca2+ channel genes. The role of E1537 in the C-terminus of the alpha1C calcium channel inactivation was investigated here after expression in Xenopus laevis oocytes. Whole-cell currents were measured in the presence of 10 mM Ba2+ or 10 mM Ca2+ after intracellular injection of 1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetraacetic acid. Against all expectations, our results showed a significant reduction in the rate of voltage-dependent inactivation as measured in Ba2+ solutions for all E1537 mutants, whereas calcium-dependent inactivation appeared unscathed. Replacing the negatively charged glutamate residue by neutral glutamine, glycine, serine, or alanine significantly reduced the rate of Ba2+-dependent inactivation by 1.5-fold (glutamine) to 3.5-fold (alanine). The overall rate of macroscopic inactivation measured in Ca2+ solutions was also reduced, although a careful examination of the distribution of the fast and slow time constants suggests that only the slow time constant was significantly reduced in the mutant channels. The fast time constant, the hallmark of Ca2+-dependent inactivation, remained remarkably constant among wild-type and mutant channels. Moreover, inactivation of E1537A channels, in both Ca2+ and Ba2+ solutions, appeared to decrease with membrane depolarization, whereas inactivation of wild-type channels became faster with positive voltages. All together, our results showed that E1537 mutations impaired voltage-dependent inactivation and suggest that the proximal part of the C-terminus may play a role in voltage-dependent inactivation in L-type alpha1C channels.
钙依赖性失活已被描述为一种调节心脏细胞中电压依赖性钙内流的负反馈机制。最新证据表明,具有EF手结合基序的α1C亚基的C末端在这一过程中至关重要。EF手结合基序在七个α1亚基Ca2+通道基因中的六个的C末端之间大多是保守的。本文在非洲爪蟾卵母细胞中表达后,研究了E1537在α1C钙通道失活C末端中的作用。在细胞内注射1,2-双(2-氨基苯氧基)乙烷-N,N,N',N'-四乙酸后,在10 mM Ba2+或10 mM Ca2+存在的情况下测量全细胞电流。与所有预期相反,我们的结果表明,在Ba2+溶液中测量时,所有E1537突变体的电压依赖性失活速率均显著降低,而钙依赖性失活似乎未受影响。用中性谷氨酰胺、甘氨酸、丝氨酸或丙氨酸取代带负电荷的谷氨酸残基,可使Ba2+依赖性失活速率显著降低1.5倍(谷氨酰胺)至3.5倍(丙氨酸)。在Ca2+溶液中测量的宏观失活总体速率也降低了,尽管仔细检查快速和慢速时间常数的分布表明,只有慢速时间常数在突变通道中显著降低。快速时间常数是钙依赖性失活的标志,在野生型和突变通道中保持相当恒定。此外,在Ca2+和Ba2+溶液中,E1537A通道的失活似乎随着膜去极化而降低,而野生型通道的失活在正电压下变得更快。总之,我们的结果表明E1537突变损害了电压依赖性失活,并表明C末端的近端部分可能在L型α1C通道的电压依赖性失活中起作用。
