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第三种钙调节的视杆细胞外段膜鸟苷酸环化酶转导机制。

Third calcium-modulated rod outer segment membrane guanylate cyclase transduction mechanism.

作者信息

Krishnan A, Goraczniak R M, Duda T, Sharma R K

机构信息

Department of Cell Biology, University of Medicine and Dentistry of New Jersey, Stratford 08084, USA.

出版信息

Mol Cell Biochem. 1998 Jan;178(1-2):251-9. doi: 10.1023/a:1006860018300.

Abstract

Ca2+-modulated rod outer segment membrane guanylate cyclase (ROS-GC1) has been cloned and reconstituted to show that it is regulated by two processes: one inhibitory, the other stimulatory. The inhibitory process is consistent with its linkage to phototransduction; the physiology of the stimulatory process is probably linked to neuronal transmission. In both regulatory processes, calcium modulation of the cyclase takes place through the calcium binding proteins; guanylate cyclase activating proteins (GCAP1 and GCAP2) in the case of the phototransduction process and calcium-dependent GCAP (CD-GCAP) in the case of the stimulatory process. The cyclase domains involved in the two processes are located at two different sites on the ROS-GC1 intracellular region. The GCAP1-modulated domain resides within the aa 447-730 segment of ROS-GC1 and the CD-GCAP-modulated domain resides within the aa 731-1054 segment. In the present study the GCAP2-dependent Ca2+ modulation of the cyclase activity has been reconstituted using recombinant forms of GCAP2 and ROS-GC1, and its mutants. The results indicate that consistent to phototransduction, GCAP2 at low Ca2+ concentration (10 nM) maximally stimulates the cyclase activity of the wild-type and its mutants: ext (deleted aa 8-408), kin (deleted aa 447-730) and hybrid consisting of the ext, transmembrane and kin domains of ANF-RGC and the C-terminal domain, aa 731-1054, of ROS-GC1. In all cases, it inhibits the cyclase activity with an IC50 of about 140 nM. A previous study has shown that under identical conditions the kin and the hybrid mutant are at best only minimally stimulated. Thus, the GCAP1 and GCAP2 signal transduction mechanisms are different, occurring through different modules of ROS-GC1. These findings also demonstrate that the intracellular region of ROS-GC1 is composed of multiple modules, each designed to mediate a particular calcium-specific signalling pathway.

摘要

钙调节的视杆细胞外段膜鸟苷酸环化酶(ROS-GC1)已被克隆并重组,结果表明它受两个过程调节:一个是抑制过程,另一个是刺激过程。抑制过程与其与光转导的联系一致;刺激过程的生理学可能与神经元传递有关。在这两个调节过程中,环化酶的钙调节都是通过钙结合蛋白进行的:在光转导过程中是鸟苷酸环化酶激活蛋白(GCAP1和GCAP2),在刺激过程中是钙依赖性GCAP(CD-GCAP)。参与这两个过程的环化酶结构域位于ROS-GC1细胞内区域的两个不同位点。GCAP1调节的结构域位于ROS-GC1的447-730氨基酸片段内,而CD-GCAP调节的结构域位于731-1054氨基酸片段内。在本研究中,使用GCAP2和ROS-GC1的重组形式及其突变体,对环化酶活性的GCAP2依赖性钙调节进行了重组。结果表明,与光转导一致,低钙浓度(10 nM)下的GCAP2最大程度地刺激野生型及其突变体的环化酶活性:ext(缺失8-408氨基酸)、kin(缺失447-730氨基酸)以及由ANF-RGC的ext、跨膜和kin结构域与ROS-GC1的C末端结构域(731-1054氨基酸)组成的杂合体。在所有情况下,它以约140 nM的IC50抑制环化酶活性。先前的一项研究表明,在相同条件下,kin和杂合突变体充其量只能受到最小程度的刺激。因此,GCAP1和GCAP2的信号转导机制不同,是通过ROS-GC1的不同模块发生的。这些发现还表明,ROS-GC1的细胞内区域由多个模块组成,每个模块都旨在介导特定的钙特异性信号通路。

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