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Studies on proinsulin and proglucagon biosynthesis and conversion at the subcellular level: II. Distribution of radioactive peptide hormones and hormone precursors in subcellular fractions after pulse and pulse- chase incubation of islet tissue

机译:亚细胞水平的胰岛素原和胰高血糖素原生物合成和转化的研究:II。胰岛组织脉冲和脉冲追逐孵育后,亚细胞级分中放射性肽激素和激素前体的分布

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摘要

Anglerfish proinsulin and insulin were selectively labeled with [(14)C]isoleucine, while proglucagon, conversion intermediate(s), and glucagon were selectively labeled with[(3)H]tryptophan. After various periods of continuous or pulse-chase incubation, islet tissue was subjected to subcellular fractionation. Fraction extracts were analyzed by gel filtration for their content of precursor, conversion intermediate(s), and product peptides. Of the seven subcellular fractions prepared after each incubation, only the microsome and secretory granule fractions yielded significant amounts of labeled insulin-related and glucagon-related peptides. After short-pulse incubations, levels of both [(14)C]proinsulin and [(3)H]proglucagon (mol wt approximately 12,000) were highest in the microsome fraction. This fraction is therefore identified as the site of synthesis. With increasing duration of continuous incubation or during chase incubation in the absence of isotopes, proinsulin, proglucagon, and conversion intermediate(s) are transported to secretory granules. Conversion of proinsulin to insulin and proglucagon to a approximately 4,900 mol wt conversion intermediate and 3,500 mol wt glucagon occurs in the secretory granules. Converting activity also was observed in the microsome fraction. The recovery of most of the incorporated radioactivity in microsome and secretory granule fractions indicates that the newly synthesized islet peptides are relegated to a membrane-bound state soon after synthesis at the RER is completed. This finding supports the concept of intracisternal sequestration and intragranular maintenance of peptides synthesized for export from the cell of origin.
机译:r鱼的胰岛素原和胰岛素用[(14)C]异亮氨酸选择性标记,而胰高血糖素,转化中间体和胰高血糖素则用[(3H] H]色氨酸选择性标记。在连续或脉冲追踪培养的各个时期后,将胰岛组织进行亚细胞分级分离。通过凝胶过滤分析馏分提取物的前体,转化中间体和产物肽的含量。每次温育后制备的七个亚细胞级分中,只有微粒体和分泌颗粒级分产生大量的标记胰岛素相关和胰高血糖素相关肽。短脉冲温育后,微粒体级分中[(14)C]胰岛素原和[(3)H]胰高血糖素的水平(摩尔重量约为12,000)最高。因此该部分被鉴定为合成位点。在不存在同位素的情况下,随着连续孵育持续时间的增加或在追踪孵育过程中,胰岛素原,胰高血糖素原和转化中间体会被运输到分泌颗粒中。在分泌颗粒中发生胰岛素原向胰岛素的转化,胰岛素原和胰高血糖素的转化为大约4,900mol wt的转化中间体和3,500mol wt的胰高血糖素。在微粒体级分中也观察到了转化活性。在微粒体和分泌颗粒部分中大部分掺入的放射性的恢复表明,新合成的胰岛肽在RER合成完成后不久就降级为膜结合状态。这一发现支持了脑池内隔离和合成后从原代细胞输出的肽的颗粒内维持的概念。

著录项

  • 作者

    Noe, BD; Baste, CA; Bauer, GE;

  • 作者单位
  • 年度 1977
  • 总页数
  • 原文格式 PDF
  • 正文语种 {"code":"en","name":"English","id":9}
  • 中图分类

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