Michalangeli V P, Hunt N H, Martin T J
J Endocrinol. 1977 Jan;72(1):69-79. doi: 10.1677/joe.0.0720069.
Several aspects of the activation of adenylate cyclase by guanosine 5'-triphosphate (GTP), 5'-guanylylimidodiphosphate (Gpp(NH)p) and bovine parathyroid hormone (bPTH) have been studied in chick kidney plasma membrane preparations. GTP (10(-4) mol/l), Gpp(NH)p (10(-4) mol/l) and bPTH (10 i.u./ml) activated adenylate cyclase without any significant time lag. However a 2 min delay was observed before the activity of the enzyme increased after the addition of bPTH (-6 leads to +34) to incubations. The early (0-3 min) effects of GTP and Gpp(NH)p upon chick kidney adenylate cyclase activity were antagonized by the addition of the alternative guanyl nucleotide. After 5 min of incubation with kidney plasma membranes, Gpp(NH)p induced a stable state of activation of adenylate cyclase which was not reversible by subsequent addition of GTP. GTP did not induce an irreversible state of enzyme activation. In pre-incubation studies, GTP did not produce a persistent enzyme activation and did not modify the effect of Gpp(NH)p added subsequently at the incubation stage. Gpp(NH)p produced a stable state of activation of adenylate cyclase which was not inhibited by addition of GTP at the incubation stage. Bovine PTH (2-34) inhibited the effect of bPTH upon adenylate cyclase activity when the native hormone (10 i.u./ml) had been incubated with plasma membranes for up to 8 min before addition of the analogue (5 mug/ml). Incubation of plasma membranes with bPTH (2-34) for as little as 10 s prevented activation of adenylate cyclase by subsequent addition of bPTH. This pattern was confirmed in pre-incubation studies. After pre-incubation of kidney membranes with bPTH and bPTH (2-34), followed by washing, an acid extract of the membranes contained immunoreactive bPTH. Gpp(NH)p produced a greater increase in adenylate cyclase activity in membranes pre-incubated with bPTH or bPTH (2-34) than in membranes pre-incubated with buffer alone, suggesting that the hormone and analogue facilitated the interaction of Gpp(NH)p with adenylate cyclase.
在鸡肾质膜制剂中,对鸟苷5'-三磷酸(GTP)、5'-鸟苷酰亚胺二磷酸(Gpp(NH)p)和牛甲状旁腺激素(bPTH)激活腺苷酸环化酶的几个方面进行了研究。GTP(10⁻⁴mol/l)、Gpp(NH)p(10⁻⁴mol/l)和bPTH(10国际单位/毫升)激活腺苷酸环化酶时没有明显的时间延迟。然而,在向孵育体系中添加bPTH(-6至+34)后,观察到酶活性增加前有2分钟的延迟。添加另一种鸟苷酸会拮抗GTP和Gpp(NH)p对鸡肾腺苷酸环化酶活性的早期(0 - 3分钟)影响。与肾质膜孵育5分钟后,Gpp(NH)p诱导腺苷酸环化酶达到稳定的激活状态,随后添加GTP不能使其逆转。GTP不会诱导酶的不可逆激活状态。在预孵育研究中,GTP不会产生持续的酶激活,也不会改变随后在孵育阶段添加Gpp(NH)p所产生的效果。Gpp(NH)p产生腺苷酸环化酶的稳定激活状态,在孵育阶段添加GTP不会抑制该状态。当天然激素(10国际单位/毫升)与质膜孵育长达8分钟后再添加类似物(5微克/毫升)时,牛PTH(2 - 34)会抑制bPTH对腺苷酸环化酶活性的影响。用bPTH(2 - 34)孵育质膜仅10秒就能阻止随后添加bPTH对腺苷酸环化酶的激活。这种模式在预孵育研究中得到了证实。用bPTH和bPTH(2 - 34)对肾膜进行预孵育然后洗涤后,膜的酸提取物中含有免疫反应性bPTH。与仅用缓冲液预孵育的膜相比,Gpp(NH)p在用bPTH或bPTH(2 - 34)预孵育的膜中使腺苷酸环化酶活性增加得更多,这表明激素和类似物促进了Gpp(NH)p与腺苷酸环化酶之间的相互作用。
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