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钙调蛋白和一种内源性抑制因子对蛙视杆细胞中环鸟苷酸门控离子通道的调节作用。

Modulation of the cGMP-gated ion channel in frog rods by calmodulin and an endogenous inhibitory factor.

作者信息

Gordon S E, Downing-Park J, Zimmerman A L

机构信息

Section of Physiology, Brown University, Providence, RI 02912, USA.

出版信息

J Physiol. 1995 Aug 1;486 ( Pt 3)(Pt 3):533-46. doi: 10.1113/jphysiol.1995.sp020832.

DOI:10.1113/jphysiol.1995.sp020832
PMID:7473217
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1156544/
Abstract
  1. Outer segment patches excised in the light were used to investigate the effects of exogenous calmodulin and an endogenous inhibitory factor on the cGMP-gated channel of frog rods. 2. Calmodulin shifted to the right the dose-response relation for activation of the channels by 8-Br-cGMP, but did not change the maximum current or the form of the relation. Reversal of this effect by removal of calmodulin was accelerated by brief exposure to saturating [8-Br-cGMP]. Inhibition by calmodulin required calcium and gave as much as a 5-fold decrease in current for an [8-Br-cGMP] functionally comparable to the presumed physiological [cGMP]. 3. Exposure to low [Ca2+]i (tens of nanomolar) appeared to irreversibly remove or inactivate an endogenous channel inhibitory factor from the patches, increasing the current at low [8-Br-cGMP]. Like calmodulin, this factor slowed the voltage-dependent channel-gating kinetics and did not change the maximum current. However, unlike calmodulin, the endogenous factor remained stably associated with the patches at high [Ca2+]i (1 microM), even with exposure to saturating [8-Br-cGMP]. 4. After the low-Ca2+ treatment increased the current, calmodulin reduced the current to about the same level as it had before the low-Ca2+ treatment, giving a larger fractional suppression. Furthermore, patches with high initial sensitivity to 8-Br-cGMP had small low-Ca2+ effects and large calmodulin effects, while the reverse was true for patches with low initial agonist sensitivity. 5. Application of trypsin to the intracellular surface of the patch prevented the responses to calmodulin and to low [Ca2+]i, suggesting involvement of a cytoplasmic portion of the channel. However, trypsin also reduced the total agonist-induced patch current. 6. Our results are consistent with a model in which calmodulin and an endogenous calcium-binding protein compete for the same site, inhibiting channel opening or cGMP binding. The tight association of the endogenous factor with the channel even at relatively low [Ca2+]i suggests that in the transducing rod it may inhibit the channels most of the time in darkness and in dim light, preventing any potential inhibitory effects of calmodulin. The endogenous factor would be expected to leave the channel only in bright or prolonged light, when the [Ca2+]i is thought to be very low.
摘要
  1. 在光照下切除的外段膜片用于研究外源性钙调蛋白和内源性抑制因子对蛙视杆细胞环鸟苷酸门控通道的影响。2. 钙调蛋白使8-溴环鸟苷酸激活通道的剂量-反应关系向右移动,但不改变最大电流或关系的形式。通过短暂暴露于饱和[8-溴环鸟苷酸]可加速去除钙调蛋白后这种效应的逆转。钙调蛋白的抑制作用需要钙,对于与假定生理[环鸟苷酸]功能相当的[8-溴环鸟苷酸],电流可降低多达5倍。3. 暴露于低[钙离子]i(几十纳摩尔)似乎不可逆地从膜片中去除或使内源性通道抑制因子失活,增加了低[8-溴环鸟苷酸]时的电流。与钙调蛋白一样,该因子减慢了电压依赖性通道门控动力学,且不改变最大电流。然而,与钙调蛋白不同的是,即使在高[钙离子]i(1微摩尔)下暴露于饱和[8-溴环鸟苷酸],内源性因子仍稳定地与膜片结合。4. 低钙处理增加电流后,钙调蛋白将电流降低至与低钙处理前大致相同的水平,产生更大的分数抑制。此外,对8-溴环鸟苷酸初始敏感性高的膜片低钙效应小而钙调蛋白效应大,而对初始激动剂敏感性低的膜片则相反。5. 将胰蛋白酶应用于膜片的细胞内表面可阻止对钙调蛋白和低[钙离子]i的反应,表明通道的细胞质部分参与其中。然而,胰蛋白酶也降低了总的激动剂诱导的膜片电流。6. 我们的结果与一个模型一致,即钙调蛋白和一种内源性钙结合蛋白竞争同一位点,抑制通道开放或环鸟苷酸结合。即使在相对低的[钙离子]i下,内源性因子与通道紧密结合,这表明在转导视杆细胞中,它可能在黑暗和弱光下大部分时间抑制通道,防止钙调蛋白的任何潜在抑制作用。预计内源性因子仅在强光或长时间光照下离开通道,此时[钙离子]i被认为非常低。
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f8c9/1156544/334f320bbc6e/jphysiol00317-0017-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f8c9/1156544/334f320bbc6e/jphysiol00317-0017-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f8c9/1156544/334f320bbc6e/jphysiol00317-0017-a.jpg

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