首页> 美国卫生研究院文献>The EMBO Journal >Isolation and characterization of S. cerevisiae mutants defective in somatostatin expression: cloning and functional role of a yeast gene encoding an aspartyl protease in precursor processing at monobasic cleavage sites.
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Isolation and characterization of S. cerevisiae mutants defective in somatostatin expression: cloning and functional role of a yeast gene encoding an aspartyl protease in precursor processing at monobasic cleavage sites.

机译:生长抑素表达有缺陷的酿酒酵母突变体的分离和鉴定:单价切割位点前体加工中编码天冬氨酰蛋白酶的酵母基因的克隆和功能作用。

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摘要

The peptide somatostatin exists as two different molecular species. In addition to the most common form, somatostatin-14, there is also a fourteen amino acid N-terminally extended form of the tetradecapeptide, somatostatin-28. Both peptides are synthesized as larger precursors containing paired basic and monobasic amino acids at their processing sites, which upon cleavage generate either somatostatin-14 or -28, respectively. In some species of fish two distinct, but homologous, precursors (prosomatostatin-I and -II) give rise to somatostatin-14 and -28, respectively. Whereas anglerfish prosomatostatin-II was previously shown to release exclusively somatostatin-28, the yeast Saccharomyces cerevisiae proteolytically matures the homologous prosomatostatin-I precursor to somatostatin-28 and -14 as well as to a lysine-extended form of somatostatin-14. The Kex2 endoprotease appears to be essential for the formation of lysine somatostatin-14 and is involved either directly or indirectly in the release of mature somatostatin-14. The isolation of yeast mutants defective in somatostatin-28 expression (sex mutant) allowed the cloning of a non-essential gene, which encodes an aspartyl protease, whose disruption severely affects the cleavage of mature somatostatin-28 from both somatostatin precursors. We conclude that two distinct endoproteases, which demonstrate some cross specificity in vivo, are involved in the proteolytic maturation of prosomatostatin at mono- and dibasic processing sites in yeast.
机译:肽生长抑素以两种不同的分子形式存在。除了最常见的生长抑素-14形式外,四十肽生长抑素-28还具有十四个氨基酸的N末端延伸形式。两种肽均被合成为较大的前体,在其加工位点含有成对的碱性氨基酸和一元氨基酸,它们在切割时分别生成生长抑素14或-28。在某些鱼类中,两种截然不同但同源的前体(前列腺抑素-I和-II)分别导致生长抑素-14和-28。先前已证明angle鱼的前列腺抑素-II仅释放生长抑素-28,而酿酒酵母酵母则使同源的前列腺抑素-I前体成为生长抑素-28和-14以及生长抑素-14的赖氨酸延伸形式。 Kex2内切蛋白酶似乎对赖氨酸生长抑素14的形成至关重要,并且直接或间接参与成熟生长抑素14的释放。分离生长抑素28表达有缺陷的酵母突变体(性突变)可以克隆一个非必需基因,该基因编码天冬氨酰蛋白酶,其破坏严重影响成熟生长抑素28从两种生长抑素前体的裂解。我们得出的结论是,两种不同的内切蛋白酶在体内表现出一些交叉特异性,它们参与了原抑素在酵母中一元和二元加工位点的蛋白水解成熟。

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