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甲状旁腺腺苷酸环化酶的高亲和力钙抑制作用不依赖于钙调蛋白。

The high affinity calcium inhibition of parathyroid adenylate cyclase is not calmodulin dependent.

作者信息

Oldham S B, Lipson L G

出版信息

Calcif Tissue Int. 1986 May;38(5):275-81. doi: 10.1007/BF02556606.

Abstract

To investigate the possible role of calmodulin in the calcium sensitivity of parathyroid adenylate cyclase (AC), the effect of the calmodulin inhibitor trifluoperazine hydrochloride (TFP) on the calcium sensitivity of forskolin-stimulated AC activity was investigated in membranes prepared from normal porcine parathyroid glands. TFP inhibited AC in a concentration-dependent manner, the IC50 being approximately 100 microM. The inhibition of the enzyme occurred at roughly the same concentration of TFP in the presence and absence of calcium. Another calmodulin inhibitor, N-(6-aminohexyl)-chloro-1-naphthalenesulfonamide (W-7), also inhibited AC in a calcium-independent manner with a IC50 of approximately 200 microM. The pattern of calcium inhibition of AC was compared in membranes prewashed with either EGTA or 2 microM ionic calcium plus 100 microM TFP in an attempt to remove endogenous calmodulin. Neither treatment significantly altered the apparent affinities of the two previously reported calcium inhibition sites, nor did they alter the relative contribution of the individual calcium inhibition sites to the overall calcium inhibition. Inclusion of 100 microM TFP in the incubation mixture resulted in no change in the apparent affinities of the calcium inhibition site although it did result in a significant decrease in the relative contribution of the high affinity site (P less than 0.05). Addition of exogenous calmodulin (5-50 micrograms/ml) had no significant effect on AC. We conclude from these studies that the inhibition of parathyroid AC by calcium is independent of calmodulin and that this enzyme has intrinsic high sensitivity to calcium.

摘要

为了研究钙调蛋白在甲状旁腺腺苷酸环化酶(AC)钙敏感性中可能发挥的作用,我们在从正常猪甲状旁腺制备的膜中,研究了钙调蛋白抑制剂盐酸三氟拉嗪(TFP)对福斯高林刺激的AC活性钙敏感性的影响。TFP以浓度依赖性方式抑制AC,IC50约为100μM。在有钙和无钙的情况下,该酶在大致相同的TFP浓度下受到抑制。另一种钙调蛋白抑制剂N-(6-氨基己基)-氯-1-萘磺酰胺(W-7)也以钙非依赖性方式抑制AC,IC50约为200μM。为了去除内源性钙调蛋白,我们比较了用EGTA或2μM离子钙加100μM TFP预洗涤的膜中AC的钙抑制模式。两种处理均未显著改变先前报道的两个钙抑制位点的表观亲和力,也未改变各个钙抑制位点对总体钙抑制的相对贡献。在孵育混合物中加入100μM TFP,钙抑制位点的表观亲和力没有变化,尽管它确实导致高亲和力位点的相对贡献显著降低(P<0.05)。添加外源性钙调蛋白(5-50μg/ml)对AC没有显著影响。我们从这些研究中得出结论,钙对甲状旁腺AC的抑制作用与钙调蛋白无关,并且该酶对钙具有内在的高敏感性。

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