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An in vitro system for studying insulin release: effects of glucose and glucose-6-phosphate

机译:研究胰岛素释放的体外系统:葡萄糖和6-磷酸葡萄糖的作用

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1. Investigation of the ionic requirements of the in vitro insulin release system, which consists of cod islet plasma membrane and rabbit islet granules incubated at pH 6.5, showed that the presence of Ca2+ was obligatory for the system to operate.2. Glucose-initiated insulin release was as effective in the presence of β-γ-methylene ATP, as it was in the presence of ATP. This analogue of ATP is a substrate neither for adenylate cyclase nor for any known animal membrane proteases. The effect of ATP on glucose mediated release is allosteric.3. Glucose (16 mM)-initiated insulin release was slower than that induced by glucose-6-phosphate (4 mM); 150 and 120 sec, respectively.4. The lag found with glucose-mediated insulin release was dependent upon glucose concentration. The lower the glucose concentration, the longer the lag. With 1 mM glucose the lag extended to 30 min.5. Once insulin release was initiated, the rate and amount of insulin release was independent of the glucose concentration.6. Pre-incubation of membranes with Ca2+, glucose and ATP prior to the addition of granules, abolished the extended lag that had been obtained with 1 mM glucose. Events in the plasma membrane are the major contributor to the generation of the extended lag.7. The glucose analogue 5′thio-D-glucose, although not able to release insulin, was shown to compete with glucose for the glucoreceptor. By increasing the ratio of analogue to glucose the lag time increased. Thus, the lag time is dependent upon the `effective' external glucose concentration.8. The max. amount of insulin released by 4 ng of membrane in the presence of glucose (16 mM) was 300 ng. The fact that membranes became refractory to glucose after this max. amount of insulin was released showed that recycling of release sites was not taking place in vitro and that granule: granule interactions were not occurring.9. The 120 sec lag before glucose-6-phosphate-initiated release was independent of glucose-6-phosphate concentration. The rate of insulin release with glucose-6-phosphate was concentration dependent.10. Glucose-6-phosphate did not cause further insulin release from a membrane that had released the max. amount of insulin it was capable of in the presence of glucose. The addition of tolbutamide (10 mM) to such a membrane did cause insulin release. This suggests that glucose and glucose-6-phosphate share a final common pathway.11. Adrenaline and somatostatin did not inhibit glucose-mediated insulin release.
机译:1.对体外胰岛素释放系统(由鳕鱼胰岛质膜和在pH 6.5下孵育的兔胰岛颗粒组成)的离子需求的研究表明,Ca 2 + 的存在是必需的。系统运行2。在β-γ-亚甲基ATP存在下,葡萄糖引发的胰岛素释放与在ATP存在下一样有效。 ATP的这种类似物既不是腺苷酸环化酶的底物,也不是任何已知动物膜蛋白酶的底物。 ATP对葡萄糖介导的释放的影响是变构的。3。葡萄糖(16 mM)引发的胰岛素释放比6-磷酸葡萄糖(4 mM)诱导的释放慢。分别为150秒和120秒4。发现葡萄糖介导的胰岛素释放的滞后取决于葡萄糖浓度。葡萄糖浓度越低,滞后时间越长。葡萄糖浓度为1 mM时,延迟延长至30分钟5。一旦开始释放胰岛素,胰岛素释放的速率和量就与葡萄糖浓度无关。6。在添加颗粒之前,先用Ca 2 + ,葡萄糖和ATP对膜进行预温育,从而消除了用1 mM葡萄糖获得的延长的滞后。质膜中的事件是产生延长的滞后的主要因素。7。葡萄糖类似物5'硫代-D-葡萄糖虽然不能释放胰岛素,但显示出与葡萄糖竞争葡萄糖受体。通过增加类似物与葡萄糖的比例,滞后时间增加了。因此,滞后时间取决于“有效”外部葡萄糖浓度8。最高在葡萄糖(16 mM)存在下,4 ng膜释放的胰岛素量为300 ng。在此最大值之后,膜对葡萄糖变得难治。胰岛素的释放量表明,释放部位没有在体外循环,并且颗粒与颗粒之间没有相互作用。9。葡萄糖-6-磷酸引发的释放之前的120秒延迟与葡萄糖6-磷酸浓度无关。用6-磷酸葡萄糖释放胰岛素的速率与浓度有关。10。 6-磷酸葡萄糖不会导致胰岛素从最大释放量的膜上进一步释放。在葡萄糖存在下能够吸收的胰岛素量。向该膜中添加甲苯磺丁酰胺(10 mM)确实会导致胰岛素释放。这表明葡萄糖和6-磷酸葡萄糖共有一个最终的共同途径。11。肾上腺素和生长抑素不抑制葡萄糖介导的胰岛素释放。

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