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通过内源性GTP水解实现转导素的亚秒级失活。

Subsecond deactivation of transducin by endogenous GTP hydrolysis.

作者信息

Vuong T M, Chabre M

机构信息

Laboratoire de Biophysique Moléculaire et Cellulaire, (Unité Associée 520 du CNRS) Centre d'études Nucléaires de Grenoble, France.

出版信息

Nature. 1990 Jul 5;346(6279):71-4. doi: 10.1038/346071a0.

Abstract

The response of a retinal rod cell to a weak flash of light is mediated by a receptor/GTP-binding protein (rhodopsin/transducin) signal transduction system and terminates within a second. The T alpha subunit of transducin (composed of subunits T alpha, T beta and T gamma) is triggered by photoexcited rhodopsin (R*) to release GDP and bind GTP. The binding of GTP causes release of the T alpha unit from T beta gamma and allows it to modulate the activity of an enzyme that generates a second messenger. Termination of the response requires the hydrolysis of the GTP by intrinsic GTPase. As with other G proteins, the GTPase activity of transducin seems to be slow. Reported in vitro turnover rates of a few molecules of GTP hydrolysed per molecule of transducin per minute imply a T alpha-GTP deactivation time of many seconds. But this time might be only a small fraction of that of the GTPase cycle. We have now used time-resolved microcalorimetry in bovine rod outer segments (ROS) to monitor the heat release due to the hydrolysis of GTP by a transducin population that had been quickly activated by flash illumination of rhodopsin. The enthalpy of GTP hydrolysis is released within 1 s at 23 degrees C. This deactivation time seems to be independent of any diffusible factor in the preparation and concurs with the termination kinetics of the rod's response. Thereafter, transducin seems unable to reload GTP for many seconds. This refractory 'resetting' time may account for the low steady-state GTPase rates in vitro.

摘要

视网膜视杆细胞对微弱闪光的反应是由受体/鸟苷三磷酸(GTP)结合蛋白(视紫红质/转导素)信号转导系统介导的,且在一秒内终止。转导素的Tα亚基(由Tα、Tβ和Tγ亚基组成)由光激发的视紫红质(R*)触发,释放GDP并结合GTP。GTP的结合导致Tα亚基从Tβγ释放,并使其能够调节产生第二信使的酶的活性。反应的终止需要内在的GTP酶水解GTP。与其他G蛋白一样,转导素的GTP酶活性似乎较慢。报道的体外周转率是每分钟每分子转导素水解几分子GTP,这意味着Tα-GTP失活时间为许多秒。但这个时间可能只是GTP酶循环时间的一小部分。我们现在已经在牛视杆外段(ROS)中使用时间分辨微量热法来监测由于视紫红质闪光照射快速激活的转导素群体水解GTP而产生的热释放。在23摄氏度下,GTP水解的焓在1秒内释放。这个失活时间似乎与制剂中的任何可扩散因子无关,并且与视杆细胞反应的终止动力学一致。此后,转导素似乎在许多秒内无法重新加载GTP。这个难治性的“重置”时间可能解释了体外低稳态GTP酶速率的原因。

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