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大鼠腮腺基底外侧质膜中依赖三磷酸腺苷(ATP)的钙离子(Ca2+)转运受钙调蛋白调节。

ATP-dependent Ca2+ transport in the rat parotid basolateral plasma membrane is regulated by calmodulin.

作者信息

Ambudkar I S, Horn V J, Baum B J

机构信息

Clinical Investigations and Patient Care Branch, National Institute of Dental Research, Bethesda, Maryland 20892.

出版信息

Arch Biochem Biophys. 1989 Feb 1;268(2):576-84. doi: 10.1016/0003-9861(89)90325-1.

Abstract

Calmodulin regulation of ATP-dependent Ca2+ transport activity was assessed in inverted basolateral plasma membrane vesicles (BLMV) isolated from rat parotid glands. The initial rate of Ca2+ transport in media containing 100 nM Ca2+ was stimulated by approximately 60% at maximal concentrations (300 nM) of exogenously added calmodulin (CAM). Half-maximal activation was obtained at 50 and 175 nM CAM in KCl and mannitol containing assay media, respectively. In the KCl medium, addition of 300 nM CAM increased the affinity of the BLMV Ca2+ transport activity for Ca2+ from approximately 70 nM, in the absence of added CAM, to approximately 50 nM. Vmax was consistently increased by approximately 20% under these conditions. When BLMV were treated with ethylene glycol bis(beta-aminoethylether) N,N'-tetraacetic acid (EGTA) (200 microM), the affinity of the transporter for Ca2+ decreased by 50% to approximately 150 nM, with no change in Vmax. When CAM was added to the EGTA-treated membranes, Ca2+ transport activity was comparable to that obtained when CAM was added directly to control, untreated BLMV. The CAM antagonists, trifluoperazine (TFP), W-7, and calmidazolium, inhibited Ca2+ transport in the presence of CAM. Half-maximal inhibition of transport was achieved by 12 microM TFP and 20 microM W-7. Calmidazolium (1 microM) inhibited Ca2+ transport by 75%. The inhibitory effects on ATP-dependent Ca2+ transport exerted by these agents were not due to an increase in the passive permeability of the membranes to Ca2+. Furthermore, in the absence of added CAM, the inhibitory effects of these agents on initial Ca2+ transport rate was decreased. The data presented suggest that the Ca2+-dependent interaction of CAM with the ATP-dependent Ca2+ transporter in rat parotid BLMV modifies the kinetic properties of this Ca2+ transporting mechanism.

摘要

在从大鼠腮腺分离出的基底外侧质膜翻转囊泡(BLMV)中评估了钙调蛋白对ATP依赖性Ca2+转运活性的调节作用。在含有100 nM Ca2+的培养基中,外源性添加的钙调蛋白(CAM)最大浓度(300 nM)时,Ca2+转运的初始速率被刺激了约60%。在含KCl和甘露醇的测定培养基中,分别在50 nM和175 nM CAM时获得半数最大激活。在KCl培养基中,添加300 nM CAM使BLMV Ca2+转运活性对Ca2+的亲和力从无添加CAM时的约70 nM增加到约50 nM。在这些条件下,Vmax持续增加约20%。当用乙二醇双(β-氨基乙基醚)N,N'-四乙酸(EGTA)(200 μM)处理BLMV时,转运体对Ca2+的亲和力降低50%至约150 nM,Vmax无变化。当将CAM添加到经EGTA处理的膜中时,Ca2+转运活性与直接将CAM添加到对照未处理的BLMV中时相当。CAM拮抗剂三氟拉嗪(TFP)、W-7和氯咪唑鎓在有CAM存在时抑制Ca2+转运。12 μM TFP和20 μM W-7实现了对转运的半数最大抑制。氯咪唑鎓(1 μM)抑制Ca2+转运75%。这些试剂对ATP依赖性Ca2+转运的抑制作用不是由于膜对Ca2+的被动通透性增加。此外,在无添加CAM时,这些试剂对初始Ca2+转运速率的抑制作用降低。所呈现的数据表明,CAM与大鼠腮腺BLMV中ATP依赖性Ca2+转运体的Ca2+依赖性相互作用改变了这种Ca2+转运机制的动力学特性。

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