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胰蛋白酶对胰腺β细胞中钾离子ATP通道的修饰作用。

Modification of K-ATP channels in pancreatic beta-cells by trypsin.

作者信息

Proks P, Ashcroft F M

机构信息

University Laboratory of Physiology, Oxford, UK.

出版信息

Pflugers Arch. 1993 Jun;424(1):63-72. doi: 10.1007/BF00375103.

Abstract

The inside-out configuration of the patch-clamp method was used to study the effects of trypsin on the activity of ATP-sensitive potassium (K-ATP) channels from isolated mouse pancreatic beta-cells. Trypsin (20 micrograms/ml) irreversibly enhanced channel activity around twofold by reducing the interburst intervals without altering the burst kinetics. No effect on the single channel conductance or the inward rectification produced by internal Mg2+ was observed: however, the protease did reduce the inhibitory effect of Mg2+ on channel activity. Trypsin both prevented rundown of K-ATP channel activity and reactivated the channels after complete rundown. These effects of trypsin were absent in the presence of trypsin inhibitor. The protease also reduced the inhibitory effect of ATP on channel activity, increasing the dissociation constant from 7 to 49 microM. Trypsin removed the activating effect of ADP (0.1 mmol/l) on channel activity and reduced the inhibitory effect of tolbutamide (0.5 mmol/l). Carboxypeptidase A did not activate K-ATP channels in excised patches, although it was able to slightly reactivate channels after complete rundown, whereas chymotrypsin increased K-ATP channel activity but it did not produce reactivation. The effects of papain were similar to those of trypsin.

摘要

采用膜片钳技术的外向膜片配置来研究胰蛋白酶对分离的小鼠胰腺β细胞中ATP敏感性钾通道(K-ATP通道)活性的影响。胰蛋白酶(20微克/毫升)通过缩短爆发间期不可逆地使通道活性增强约两倍,而不改变爆发动力学。未观察到对单通道电导或内部Mg2+产生的内向整流的影响:然而,该蛋白酶确实降低了Mg2+对通道活性的抑制作用。胰蛋白酶既能防止K-ATP通道活性的衰减,又能在完全衰减后使通道重新激活。在存在胰蛋白酶抑制剂的情况下,胰蛋白酶的这些作用消失。该蛋白酶还降低了ATP对通道活性的抑制作用,使解离常数从7微摩尔增加到49微摩尔。胰蛋白酶消除了ADP(0.1毫摩尔/升)对通道活性的激活作用,并降低了甲苯磺丁脲(0.5毫摩尔/升)的抑制作用。羧肽酶A在切除的膜片中不能激活K-ATP通道,尽管它能够在完全衰减后使通道稍有重新激活,而胰凝乳蛋白酶增加了K-ATP通道活性,但未产生重新激活作用。木瓜蛋白酶的作用与胰蛋白酶相似。

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