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重组突触体ATP酶介导的钙离子转运与氢离子逆向转运及净电荷转移有关。

Ca2+ transport by reconstituted synaptosomal ATPase is associated with H+ countertransport and net charge displacement.

作者信息

Salvador J M, Inesi G, Rigaud J L, Mata A M

机构信息

Departamento de Bioquímica y Biología Molecular y Genética, Facultad de Ciencias, Universidad de Extremadura, 06071 Badajoz, Spain.

出版信息

J Biol Chem. 1998 Jul 17;273(29):18230-4. doi: 10.1074/jbc.273.29.18230.

Abstract

The synaptosomal plasma membrane Ca2+-ATPase (PMCA) purified from pig brain was reconstituted with liposomes prepared by reverse phase evaporation at a lipid to protein ratio of 150/1 (w/w). ATP-dependent Ca2+ uptake and H+ ejection by the reconstituted proteoliposomes were demonstrated by following light absorption and fluorescence changes undergone by arsenazo III and 8-hydroxy-1,3, 6-pyrene trisulfonate, respectively. Ca2+ uptake was increased up to 2-3-fold by the H+ ionophore carbonyl cyanide p-trifluoromethoxyphenylhydrazone, consistent with relief of an inhibitory transmembrane pH gradient (i.e. lumenal alkalinization) generated by H+ countertransport. The stoichiometric ratio of Ca2+/H+ countertransport was 1.0/0.6, and the ATP/Ca2+ coupling stoichiometry was 1/1 at 25 degrees C. The electrogenic character of the Ca2+/H+ countertransport was demonstrated by measuring light absorption changes undergone by oxonol VI. It was shown that a 20 mV steady state potential (positive on the lumenal side) was formed as a consequence of net charge transfer associated with the 1/1 Ca2+/H+ countertransport. Calmodulin stimulated ATPase activity, Ca2+ uptake, and H+ ejection, demonstrating that these parameters are linked by the same mechanism of PMCA regulation.

摘要

从猪脑中纯化得到的突触体质膜Ca2+ -ATP酶(PMCA),与通过反相蒸发法制备的脂质体以脂质与蛋白质150/1(w/w)的比例重组。通过分别跟踪偶氮胂III和8-羟基-1,3,6-芘三磺酸盐的吸光变化和荧光变化,证明了重组蛋白脂质体的ATP依赖性Ca2+摄取和H+排出。H+离子载体羰基氰对三氟甲氧基苯腙使Ca2+摄取增加了2 - 3倍,这与由H+反向转运产生的抑制性跨膜pH梯度(即内腔碱化)的缓解一致。在25℃下,Ca2+/H+反向转运的化学计量比为1.0/0.6,ATP/Ca2+偶联化学计量比为1/1。通过测量氧杂萘邻酮VI的吸光变化,证明了Ca2+/H+反向转运的生电特性。结果表明,由于与1/1 Ca2+/H+反向转运相关的净电荷转移,形成了20 mV的稳态电位(内腔侧为正)。钙调蛋白刺激ATP酶活性、Ca2+摄取和H+排出,表明这些参数通过PMCA调节的相同机制相互关联。

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