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胰高血糖素生物合成过程中前胰高血糖素依次代谢裂解为胰高血糖素的证据。

Evidence of sequential metabolic cleavage of proglucagon to glucagon in glucagon biosynthesis.

作者信息

Noe B D, Bauer G E

出版信息

Endocrinology. 1975 Oct;97(4):868-77. doi: 10.1210/endo-97-4-868.

Abstract

Following a 30 min preincubation in medium containing no isotopes, anglerfish islet tissue was incubated in the presence of [3H]tryptophan and [14C]isoleucine for 20 min. A portion of the tissue was removed for immediate extraction. The remainder was washed thoroughly with unlabeled medium and post-incubated in medium containing an excess of unlabeled tryptophan and isoleucine for varying periods of time. The distribution of radioactive proteins in alcoholic tissue extracts was analyzed by gel filtration and polyacrylamide gel electrophoresis. The distribution of immunoreactive glucagon was determined by radioimmunoassay. Following the 20 min pulse incubation, only proinsulin was labeled with [14C]isoleucine. Two glucagon immunoreactive molecules, one larger than proinsulin (mol wt near 11,400) and the other slightly smaller than proinsulin (mol wt near 9,000), were the primary proteins labeled with [3H]tryptophan following the 20 min. pulse. During chase incubations of increasing duration, 3H-radioactivity appeared in a glucagon immunoreactive molecule with the approximate molecular size of glucagon and increased with chase time while radioactivity in the 11,400 mol wt tryptophan-labeled molecule decreased. With increasing chase time, the 3H-radioactivity attributable to the 9,000 mol wt tryptophan-labeled molecule initially increased and subsequently decreased which is consistent with the pattern that would be expected for a conversion intermediate. The presence of glucagon immunoreactivity in [3H]tryptophan-labeled molecules having molecular weights near that of proinsulin was established by radioimmunoassay of alternate gel slices following electrophoresis of labeled proteins recovered from the proinsulin containing portions of gel filtration eluates. That [14C]isoleucine became incorporated into insulin and [3H]tryptophan became incorporated into glucagon was established by determination of the distribution of radioactivity in polyacrylamide gels following electrophoresis of labeled proteins recovered from the insulin and glucagon containing portions of gel filtration eluates. These results provide preliminary evidence for sequential metabolic cleavage of proglucagon in glucagon biosynthesis.

摘要

在不含同位素的培养基中预孵育30分钟后,将安康鱼胰岛组织在[3H]色氨酸和[14C]异亮氨酸存在的情况下孵育20分钟。取出一部分组织立即进行提取。其余组织用未标记的培养基彻底洗涤,并在含有过量未标记色氨酸和异亮氨酸的培养基中进行不同时间的后孵育。通过凝胶过滤和聚丙烯酰胺凝胶电泳分析酒精性组织提取物中放射性蛋白质的分布。通过放射免疫测定法测定免疫反应性胰高血糖素的分布。在20分钟的脉冲孵育后,只有胰岛素原被[14C]异亮氨酸标记。两种胰高血糖素免疫反应性分子,一种比胰岛素原大(分子量接近11,400),另一种比胰岛素原略小(分子量接近9,000),是20分钟脉冲后被[3H]色氨酸标记的主要蛋白质。在延长的追踪孵育期间,3H放射性出现在分子量与胰高血糖素近似的胰高血糖素免疫反应性分子中,并随追踪时间增加,而分子量为11,400的色氨酸标记分子中的放射性降低。随着追踪时间的增加,归因于分子量为9,000的色氨酸标记分子的3H放射性最初增加,随后降低,这与转化中间体预期的模式一致。通过对从凝胶过滤洗脱液中含胰岛素原部分回收的标记蛋白质进行电泳后,对交替凝胶切片进行放射免疫测定,确定了分子量接近胰岛素原的[3H]色氨酸标记分子中存在胰高血糖素免疫反应性。通过对从凝胶过滤洗脱液中含胰岛素和胰高血糖素部分回收的标记蛋白质进行电泳后,测定聚丙烯酰胺凝胶中放射性分布,确定了[14C]异亮氨酸掺入胰岛素中,[3H]色氨酸掺入胰高血糖素中。这些结果为胰高血糖素生物合成过程中胰高血糖素原的顺序代谢裂解提供了初步证据。

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