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v-sis基因产物的生物合成:信号序列切割、糖基化和蛋白水解加工。

Biosynthesis of the v-sis gene product: signal sequence cleavage, glycosylation, and proteolytic processing.

作者信息

Hannink M, Donoghue D J

出版信息

Mol Cell Biol. 1986 Apr;6(4):1343-8. doi: 10.1128/mcb.6.4.1343-1348.1986.

Abstract

The v-sis oncogene and its cellular homolog c-sis encode chain B of platelet-derived growth factor. Cells transformed by v-sis produce a platelet-derived growth factor-related molecule which is able to stimulate the platelet-derived growth factor receptor in an autocrine fashion. Site-directed mutagenesis was used to construct several mutations which substitute charged residues for hydrophobic residues in the proposed signal sequence of the v-sis gene product. Two of these mutations resulted in the synthesis of altered v-sis gene products with an unexpected nuclear location and a loss of biological activity. We also report here the intracellular localization of the v-sis gene product to the endoplasmic reticulum-Golgi compartment, where signal sequence cleavage and N-linked glycosylation occur. The v-sis gene product contains no transmembrane regions, as it is completely protected within isolated microsomes from trypsin proteolysis. Site-directed mutagenesis was also used to alter a proposed proteolytic processing site in the v-sis gene product. This mutant v-sis gene, which encodes Asn-Ser in place of Lys-Arg at residues 110 to 111, was found to retain full biological activity.

摘要

v-sis癌基因及其细胞同源物c-sis编码血小板衍生生长因子的B链。被v-sis转化的细胞产生一种血小板衍生生长因子相关分子,该分子能够以自分泌方式刺激血小板衍生生长因子受体。利用定点诱变构建了几个突变体,这些突变体将v-sis基因产物的假定信号序列中的疏水残基替换为带电荷残基。其中两个突变导致合成了具有意外核定位和生物活性丧失的改变的v-sis基因产物。我们在此还报告了v-sis基因产物在内质网-高尔基体区室的细胞内定位,信号序列切割和N-连接糖基化在此发生。v-sis基因产物不包含跨膜区域,因为它在分离的微粒体中完全受到胰蛋白酶消化的保护。定点诱变还用于改变v-sis基因产物中一个假定的蛋白水解加工位点。发现这个突变的v-sis基因在第110至111位残基处编码天冬酰胺-丝氨酸而非赖氨酸-精氨酸,它保留了完整的生物活性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1477/367650/5cd838e8af3b/molcellb00088-0386-a.jpg

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