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甘氨酸延伸胃泌素调节人胚肾细胞生长。

Glycine-extended gastrin regulates HEK cell growth.

作者信息

Stepan V M, Krametter D F, Matsushima M, Todisco A, Delvalle J, Dickinson C J

机构信息

Department of Pediatrics, University of Michigan, Medical Center, Ann Arbor, Michigan 48109, USA.

出版信息

Am J Physiol. 1999 Aug;277(2):R572-81. doi: 10.1152/ajpregu.1999.277.2.R572.

Abstract

Posttranslational processing of progastrin to a carboxy terminally amidated form (G-NH(2)) is essential for its effect on gastric acid secretion and other biological effects mediated by gastrin/CCK-B receptors. The immediate biosynthetic precursor of G-NH(2), glycine-extended gastrin (G-Gly), does not stimulate gastric acid secretion at physiological concentrations but is found in high concentrations during development. G-NH(2) and G-Gly have potent growth stimulatory effects on gastrointestinal tissues, and G-NH(2) can stimulate proliferation of human kidney cells. Thus we sought to explore the actions of G-NH(2) and G-Gly on the human embryonic kidney cell line HEK 293. HEK 293 cells showed specific binding sites for (125)I-labeled Leu(15)-G17-NH(2) and (125)I-Leu(15)-G(2-17)-Gly. Both G-NH(2) and G-Gly induced a dose-dependent increase in [(3)H]thymidine incorporation, and both peptides together significantly increased [(3)H]thymidine incorporation above the level of either peptide alone. G-NH(2) and G-Gly were detected by radioimmunoassay in serum-free conditioned media. Antibodies directed against G-NH(2) and G-Gly lead to a significant reduction in [(3)H]thymidine incorporation. G-NH(2) but not G-Gly increased intracellular Ca(2+) concentration. We conclude that G-NH(2) and G-Gly act cooperatively via distinct receptors to stimulate the growth of a nongastrointestinal cell line (HEK 293) in an autocrine fashion.

摘要

胃泌素原向羧基末端酰胺化形式(G-NH₂)的翻译后加工对于其对胃酸分泌的影响以及由胃泌素/CCK-B受体介导的其他生物学效应至关重要。G-NH₂的直接生物合成前体,甘氨酸延伸型胃泌素(G-Gly),在生理浓度下不刺激胃酸分泌,但在发育过程中浓度较高。G-NH₂和G-Gly对胃肠道组织具有强大的生长刺激作用,并且G-NH₂可以刺激人肾细胞的增殖。因此,我们试图探究G-NH₂和G-Gly对人胚肾细胞系HEK 293的作用。HEK 293细胞显示出对¹²⁵I标记的Leu¹⁵-G17-NH₂和¹²⁵I-Leu¹⁵-G₂₋₁₇-Gly的特异性结合位点。G-NH₂和G-Gly均诱导了[³H]胸苷掺入的剂量依赖性增加,并且两种肽共同作用时显著增加了[³H]胸苷掺入量,高于单独任何一种肽的水平。通过放射免疫测定法在无血清条件培养基中检测到了G-NH₂和G-Gly。针对G-NH₂和G-Gly的抗体导致[³H]胸苷掺入量显著降低。G-NH₂而非G-Gly增加了细胞内Ca²⁺浓度。我们得出结论,G-NH₂和G-Gly通过不同的受体以自分泌方式协同作用,刺激非胃肠道细胞系(HEK 293)的生长。

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