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睾酮通过磷脂酶C-磷脂酰肌醇-4,5-二磷酸(PLC-PIP2)途径调节支持细胞膜上的ATP敏感性钾(K(+)ATP)通道。

Testosterone modulates K(+)ATP channels in Sertoli cell membrane via the PLC-PIP2 pathway.

作者信息

Loss E S, Jacobsen M, Costa Z S, Jacobus A P, Borelli F, Wassermann G F

机构信息

Departamento de Fisiologia ICBS, UFRGS, Porto Alegre, Brazil.

出版信息

Horm Metab Res. 2004 Aug;36(8):519-25. doi: 10.1055/s-2004-825753.

DOI:10.1055/s-2004-825753
PMID:15326560
Abstract

Testosterone at physiological intratesticular concentrations induces a dose-dependent depolarisation and an increase in input resistance together with an increment of 45Ca2+ uptake in the Sertoli cells from seminiferous tubules of immature rat. Previous studies have implicated K(+)ATP channels in these testosterone actions. This study demonstrates that testosterone and sulphonylureas (glibenclamide and tolbutamide) depolarise the membrane potential, augment resistance and 45Ca2+ uptake in the Sertoli cells of seminiferous tubules from 10-15 day-old rats. These actions were nullified by the presence of the K(+)ATP channel opener diazoxide. The depolarisation was also observed with the impermeant bovine serum albumin-bound testosterone. Testosterone actions were blocked by both pertussis toxin and the phospholipase C (PLC) inhibitor U73122 implying the involvement of PLC - phosphatidylinositol 4-5 bisphosphate (PIP2) hydrolysis via G protein in testosterone actions. Polycations, including spermine and LaCl3, depolarised the membrane potential and increased the resistance. Hyperpolarisation caused by EGTA was reversed by LaCl3 and by the presence of testosterone. This last effect was nullified by the presence of U73122. All of the above results indicate that the action of testosterone on the Sertoli cell membrane is exercised on the K(+)ATP channels through PLC-PIP2 hydrolysis that closes the channel, depolarises the membrane, and stimulates 45Ca2+ uptake.

摘要

生理浓度的睾丸内睾酮可诱导未成熟大鼠生精小管支持细胞出现剂量依赖性去极化,并增加输入电阻,同时增加45Ca2+摄取。以往研究表明K(+)ATP通道参与了这些睾酮作用。本研究表明,睾酮和磺酰脲类药物(格列本脲和甲苯磺丁脲)可使10 - 15日龄大鼠生精小管支持细胞的膜电位去极化,增加电阻和45Ca2+摄取。K(+)ATP通道开放剂二氮嗪可消除这些作用。与不可渗透的牛血清白蛋白结合的睾酮也可观察到去极化现象。百日咳毒素和磷脂酶C(PLC)抑制剂U73122均可阻断睾酮的作用,这意味着PLC - 磷脂酰肌醇4,5 - 二磷酸(PIP2)经G蛋白水解参与了睾酮作用。包括精胺和LaCl3在内的多阳离子可使膜电位去极化并增加电阻。EGTA引起的超极化可被LaCl3和睾酮逆转。U73122可消除这一最终效应。上述所有结果表明,睾酮对支持细胞膜的作用是通过PLC - PIP2水解作用于K(+)ATP通道实现的,该水解作用会关闭通道,使膜去极化,并刺激45Ca2+摄取。

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