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百日咳毒素导致的核苷酸交换和cGMP磷酸二酯酶激活使转导素失活。

Nucleotide exchange and cGMP phosphodiesterase activation by pertussis toxin inactivated transducin.

作者信息

Ramdas L, Disher R M, Wensel T G

机构信息

Department of Biochemistry, Baylor College of Medicine, Houston, Texas 77030.

出版信息

Biochemistry. 1991 Dec 17;30(50):11637-45. doi: 10.1021/bi00114a005.

Abstract

Transducin, the signal coupling protein of retinal rod photoreceptor cells, is one of a family of G proteins that can be inactivated by pertussis toxin. We have investigated the nature of this inactivation in order to determine (1) whether it requires the toxin-catalyzed transfer of ADP-ribose from NAD+ to cysteine-347 of the alpha subunit and (2) whether it involves locking the alpha subunit in the inactive conformation characteristic of its GDP-bound state, or is limited to disruption of binding to photoexcited rhodopsin (R*). Our results indicate that all observed effects of pertussis toxin treatment, including a shift in the electrophoretic mobility of transducin's alpha subunit and functional inactivation, require NAD+ and that the appearance of the shift parallels incorporation of ADP-ribose. We have also found that, apart from interactions with photoexcited rhodopsin, the functional properties of ADP-ribosylated transducin are essentially the same as those of unmodified transducin. Normal spontaneous nucleotide exchange kinetics and the ability to activate cGMP phosphodiesterase are preserved following quantitative ADP-ribosylation, as are the abilities to hydrolyze GTP, to bind to a dye affinity column, and to display enhanced fluorescence upon addition of Al3+ and F-. Thus, ADP-ribosylation merely blocks catalysis of transducin nucleotide exchange by R* and does not lock transducin in an inactive state.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

转导蛋白是视网膜视杆光感受器细胞的信号偶联蛋白,是一类可被百日咳毒素灭活的G蛋白家族成员之一。我们研究了这种灭活的本质,以确定:(1)它是否需要毒素催化将ADP - 核糖从NAD⁺转移至α亚基的半胱氨酸 - 347;(2)它是否涉及将α亚基锁定在其结合GDP状态的无活性构象中,或者仅限于破坏与光激发视紫红质(R*)的结合。我们的结果表明,百日咳毒素处理所观察到的所有效应,包括转导蛋白α亚基电泳迁移率的改变和功能失活,都需要NAD⁺,并且迁移率改变的出现与ADP - 核糖的掺入平行。我们还发现,除了与光激发视紫红质的相互作用外,ADP - 核糖基化的转导蛋白的功能特性与未修饰的转导蛋白基本相同。定量ADP - 核糖基化后,正常的自发核苷酸交换动力学以及激活cGMP磷酸二酯酶的能力得以保留,水解GTP、结合染料亲和柱以及在添加Al³⁺和F⁻时显示增强荧光的能力也得以保留。因此,ADP - 核糖基化仅阻断R*对转导蛋白核苷酸交换的催化作用,而不会将转导蛋白锁定在无活性状态。(摘要截短于250字)

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