肌浆网腔Ca2+可接触到骨骼肌Ca2+释放通道的胞质激活和失活位点。
Sarcoplasmic reticulum lumenal Ca2+ has access to cytosolic activation and inactivation sites of skeletal muscle Ca2+ release channel.
作者信息
Tripathy A, Meissner G
机构信息
Department of Biochemistry and Biophysics, University of North Carolina, Chapel Hill 27599-7260, USA.
出版信息
Biophys J. 1996 Jun;70(6):2600-15. doi: 10.1016/S0006-3495(96)79831-4.
The effects of sarcoplasmic reticulum lumenal (trans) Ca2+ on cytosolic (cis) ATP-activated rabbit skeletal muscle Ca2+ release channels (ryanodine receptors) were examined using the planar lipid bilayer method. Single channels were recorded in symmetric 0.25 M KCl media with K+ as the major current carrier. With nanomolar [Ca2+] in both bilayer chambers, the addition of 2 mM cytosolic ATP greatly increased the number of short channel openings. As lumenal [Ca2+] was increased from < 0.1 microM to approximately 250 microM, increasing channel activities and events with long open time constants were seen at negative holding potentials. Channel activity remained low at positive holding potentials. Further increase in lumenal [Ca2+] to 1, 5, and 10 mM resulted in a decrease in channel activities at negative holding potentials and increased activities at positive holding potentials. A voltage-dependent activation by 50 microM lumenal Ca2+ was also observed when the channel was minimally activated by < 1 microM cytosolic Ca2+ in the absence of ATP. With microM cytosolic Ca2+ in the presence or absence of 2 mM ATP, single-channel activities showed no or only a weak voltage dependence. Other divalent cations (Mg2+, Ba2+) could not replace lumenal Ca2+. On the contrary, cytosolic ATP-activated channel activities were decreased as lumenal Ca2+ fluxes were reduced by the addition of 1-5 mM BaCl2 or MgCl2 to the lumenal side, which contained 50 microM Ca2+. An increase in [KCl] from 0.25 M to 1 M also reduced single-channel activities. Addition of the "fast" Ca2+ buffer 1,2-bis(2-aminophenoxy)ethanetetraacetic acid (BAPTA) to the cls chamber increased cytosolic ATP-, lumenal Ca(2+)-activated channel activities to a nearly maximum level. These results suggested that lumenal Ca2+ flowing through the skeletal muscle Ca2+ release channel may regulate channel activity by having access to cytosolic Ca2+ activation and Ca2+ inactivation sites that are located in "BAPTA-inaccessible" and "BAPTA-accessible" spaces, respectively.
利用平面脂质双层法研究了肌浆网腔(反式)Ca2+ 对胞质(顺式)ATP激活的兔骨骼肌Ca2+ 释放通道(雷诺丁受体)的影响。在以K+ 作为主要电流载体的对称0.25 M KCl介质中记录单通道电流。在双层腔室中均含有纳摩尔浓度的[Ca2+]时,加入2 mM胞质ATP可显著增加短通道开放的次数。当腔室侧[Ca2+]从<0.1 μM增加到约250 μM时,在负保持电位下可观察到通道活性增加以及具有长开放时间常数的事件增多。在正保持电位下,通道活性仍然较低。当腔室侧[Ca2+]进一步增加到1、5和10 mM时,负保持电位下的通道活性降低,而正保持电位下的活性增加。当通道在无ATP的情况下被<1 μM胞质Ca2+ 最小程度激活时,还观察到50 μM腔室Ca2+ 引起的电压依赖性激活。在有或无2 mM ATP的情况下,当胞质Ca2+ 浓度为微摩尔时,单通道活性无电压依赖性或仅表现出较弱的电压依赖性。其他二价阳离子(Mg2+、Ba2+)不能替代腔室Ca2+。相反,当向含有50 μM Ca2+ 的腔室侧加入1 - 5 mM BaCl2 或MgCl2 以减少腔室Ca2+ 通量时,胞质ATP激活的通道活性降低。[KCl]从0.25 M增加到1 M也会降低单通道活性。向顺式腔室中加入“快速”Ca2+ 缓冲剂1,2 - 双(2 - 氨基苯氧基)乙烷四乙酸(BAPTA)可使胞质ATP、腔室Ca2+ 激活的通道活性增加到接近最大水平。这些结果表明,流经骨骼肌Ca2+ 释放通道的腔室Ca2+ 可能通过分别作用于位于“BAPTA不可及”和“BAPTA可及”空间的胞质Ca2+ 激活位点和Ca2+ 失活位点来调节通道活性。
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