Varela Diego, Niemeyer María Isabel, Cid L Pablo, Sepúlveda Francisco V
Centro de Estudios Científicos (CECS), Avenida Arturo Prat 514, Casilia 1469, Valdivia, Chile.
J Physiol. 2002 Oct 15;544(2):363-72. doi: 10.1113/jphysiol.2002.026096.
ClC-2, a chloride channel widely expressed in mammalian tissues, is activated by hyperpolarisation and extracellular acidification. Deletion of amino acids 16-61 in rat ClC-2 abolishes voltage and pH dependence in two-electrode voltage-clamp experiments in amphibian oocytes. These results have been interpreted in terms of a ball-and-chain type of mechanism in which the N-terminus would behave as a ball that is removed from an inactivating site upon hyperpolarisation. We now report whole-cell patch-clamp measurements in mammalian cells showing hyperpolarization-activation of rClC-2Delta16-61 differing only in presenting faster opening and closing kinetics than rClC-2. The lack of time and voltage dependence observed previously was reproduced, however, in nystatin-perforated patch experiments. The behaviour of wild-type rClC-2 did not differ between conventional and nystatin-perforated patches. Similar results were obtained with ClC-2 from guinea-pig. One possible explanation of the results is that some diffusible component is able to lock the channel in an open state but does so only to the mutated channel. Alternative explanations involving the osmotic state of the cell and cytoskeleton structure are also considered. Low extracellular pH activates the wild-type channel but not rClC-2Delta16-61 when expressed in oocytes, a result that had been interpreted to suggest that protons affect the ball-and-chain mechanism. In our experiments no difference was seen in the effect of extracellular pH upon rClC-2 and rClC-2Delta16-61 in either recording configuration, suggesting that protons act independently from possible effects of the N-terminus on gating. Our observations of voltage-dependent gating of the N-terminal deleted ClC-2 are an argument against a ball-and-chain mechanism for this channel.
氯离子通道蛋白2(ClC-2)是一种在哺乳动物组织中广泛表达的氯离子通道,可被超极化和细胞外酸化激活。在两栖类卵母细胞的双电极电压钳实验中,大鼠ClC-2中16 - 61位氨基酸的缺失消除了电压和pH依赖性。这些结果被解释为一种球链型机制,其中N端表现为一个球,在超极化时从失活位点移除。我们现在报告在哺乳动物细胞中进行的全细胞膜片钳测量结果,显示rClC-2Delta16 - 61的超极化激活,其与rClC-2的不同之处仅在于具有更快的开闭动力学。然而,在制霉菌素穿孔膜片实验中重现了先前观察到的缺乏时间和电压依赖性的现象。野生型rClC-2在传统膜片和制霉菌素穿孔膜片之间的行为没有差异。用豚鼠的ClC-2也得到了类似的结果。对这些结果的一种可能解释是,某些可扩散成分能够将通道锁定在开放状态,但仅对突变通道起作用。还考虑了涉及细胞渗透状态和细胞骨架结构的其他解释。低细胞外pH激活野生型通道,但在卵母细胞中表达时不激活rClC-2Delta16 - 61,这一结果曾被解释为表明质子影响球链机制。在我们的实验中,在任何一种记录配置下,细胞外pH对rClC-2和rClC-2Delta16 - 61的影响都没有差异,这表明质子的作用独立于N端对门控的可能影响。我们对N端缺失的ClC-2的电压依赖性门控的观察结果反对该通道的球链机制。