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在小鼠睾丸间质细胞瘤细胞中,肥大细胞脱颗粒肽和心房利钠因子对鸟苷酸环化酶偶联的心房利钠因子受体活性的调节:G蛋白的作用

Modulation of guanylate cyclase-coupled atrial natriuretic factor receptor activity by mastoparan and ANF in murine Leydig tumor cells: role of G-proteins.

作者信息

Khurana M L, Pandey K N

机构信息

Department of Biochemistry and Molecular Biology, Medical College of Georgia, School of Medicine, Augusta 30912-2100.

出版信息

Biochim Biophys Acta. 1994 Oct 20;1224(1):61-7. doi: 10.1016/0167-4889(94)90113-9.

Abstract

Mastoparan potently stimulated catalytic activity of guanylate cyclase-coupled atrial natriuretic factor receptor (GC-A/ANF-R), both in the plasma membranes and intact Leydig tumor (MA-10) cells. In plasma membrane preparations, a maximum of 5-fold GC catalytic activity was stimulated by 100 microM mastoparan and the half maximum stimulation (EC50) was achieved at 40 microM concentration. Mastoparan potentiated GC activity by more than 40%, above the level, stimulated by ANF. Mas 7, an active analog of mastoparan, stimulated the GC activity in a similar manner to mastoparan whereas Mas 17, an inactive analog, did not enhance GC activity. In membranes prepared from mastoparan-treated intact MA-10 cells, GC catalytic activity was enhanced by more than 4-fold as compared with untreated control cells. Pretreatment of membranes with either anti-Gs alpha or anti-Gi alpha antibodies had no effect on mastoparan-stimulated GC activity, however, anti-Go alpha antibodies inhibited the stimulatory effect of mastoparan by almost 50%. Agents known to modulate the effect of mastoparan such as EGTA (Ca2+ chelator), W7 (calmodulin inhibitor) and staurosporine (protein kinase C inhibitor) had no effect on the mastoparan-stimulated GC activity. Mastoparan enhanced the ANF-stimulated GC activity in detergent solubilized membrane preparations without a significant change in ANF-binding capacity. The data establish a role for mastoparan in the ANF-dependent stimulation of GC-A/ANF-R catalytic activity, both in the plasma membrane preparations and intact Leydig tumor (MA-10) cells. Furthermore, these findings provide new evidence that mastoparan (isolated from wasp venom) potently stimulates guanylate cyclase activity of GC-A/ANF-R by activating G-proteins.

摘要

马斯托帕兰能有效刺激与鸟苷酸环化酶偶联的心房利钠因子受体(GC-A/ANF-R)的催化活性,无论是在质膜还是完整的莱迪希肿瘤(MA-10)细胞中。在质膜制剂中,100μM的马斯托帕兰可使GC催化活性最大增强5倍,在40μM浓度时达到最大刺激的一半(EC50)。马斯托帕兰使GC活性增强超过40%,高于ANF刺激的水平。马斯托帕兰的活性类似物Mas 7以与马斯托帕兰相似的方式刺激GC活性,而无活性类似物Mas 17则不增强GC活性。在用马斯托帕兰处理的完整MA-10细胞制备的膜中,与未处理的对照细胞相比,GC催化活性增强了4倍以上。用抗Gsα或抗Giα抗体预处理膜对马斯托帕兰刺激的GC活性没有影响,然而,抗Goα抗体几乎抑制了马斯托帕兰的刺激作用50%。已知调节马斯托帕兰作用的试剂,如EGTA(Ca2+螯合剂)、W7(钙调蛋白抑制剂)和星形孢菌素(蛋白激酶C抑制剂)对马斯托帕兰刺激的GC活性没有影响。马斯托帕兰在去污剂溶解的膜制剂中增强了ANF刺激的GC活性,而ANF结合能力没有显著变化。这些数据确立了马斯托帕兰在质膜制剂和完整的莱迪希肿瘤(MA-10)细胞中对GC-A/ANF-R催化活性的ANF依赖性刺激中的作用。此外,这些发现提供了新的证据,表明马斯托帕兰(从黄蜂毒液中分离)通过激活G蛋白有效刺激GC-A/ANF-R的鸟苷酸环化酶活性。

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