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胰岛素、胰岛素样生长因子及表皮生长因子对大鼠(IEC-6)和人(FHs 74 Int)肠细胞有丝分裂及双糖酶活性的影响

Effects of insulin, insulin-like growth factors and epidermal growth factor on mitogenesis and disaccharidase activity in rat (IEC-6) and human (FHs 74 Int) intestinal cells.

作者信息

Chao J C, Donovan S

机构信息

School of Nutrition and Health Sciences, Taipei, Taiwan, ROC.

出版信息

Chin J Physiol. 1996;39(4):253-63.

PMID:9058010
Abstract

Proliferation and differentiation of rat (IEC-6) and human (FHs) small intestinal cells in the presence of epidermal growth factor (EGF), insulin, insulin-like growth factor (IGF)-I, -II, and des[1-3]tripeptide-IGF-I(des-IGF-I) were examined. Thymidine incorporation into IEC-6 cells was significantly increased by insulin, IGF-I, des-IGF-I, IGF-II, and IGF-I+EGF, but not by EGF alone. In contrast, thymidine incorporation into FHs cells was increased only by insulin, IGF-I, and the combination of IGF-I and EGF. Mitogenic activities of IGF-I at 5 nM and insulin at 700 nM (IEC-6) or 1400 nM (FHs) were equivalent, suggesting that both acted through the type I IGF receptor in both cells. IEC-6 cells secreted consistently one predominant IGF binding protein (IGFBP) with M(r) of 28.5 kDa, while FHs cells secreted several IGFBPs with M(r) from 43 to 24 kDa. Mitogenic activity of IGF-I at 5 nM was equal to des-IGF-I at 0.005 nM, indicating that endogenously produced IGFBPs likely inhibit IGF-I action. In IEC-6 cells, IGFBP-2 secretion, but not mRNA expression, was decreased by EGF and IGF-I+EGF treatments, suggesting post-transcriptional regulation. IGF-II and EGF were more potent than IGF-I at increasing maltase and sucrase activities, suggesting that these growth factors may stimulate differentiation to a greater degree than mitogenesis.

摘要

研究了在表皮生长因子(EGF)、胰岛素、胰岛素样生长因子(IGF)-I、-II和去[1-3]三肽-IGF-I(des-IGF-I)存在的情况下大鼠(IEC-6)和人(FHs)小肠细胞的增殖和分化。胰岛素、IGF-I、des-IGF-I、IGF-II和IGF-I + EGF可显著增加IEC-6细胞中的胸苷掺入,但单独的EGF则无此作用。相比之下,FHs细胞中的胸苷掺入仅在胰岛素、IGF-I以及IGF-I和EGF联合作用下增加。5 nM的IGF-I和700 nM(IEC-6)或1400 nM(FHs)的胰岛素的促有丝分裂活性相当,表明二者均通过两种细胞中的I型IGF受体发挥作用。IEC-6细胞持续分泌一种主要的IGF结合蛋白(IGFBP),其分子量为28.5 kDa,而FHs细胞分泌几种分子量从43至24 kDa的IGFBP。5 nM的IGF-I的促有丝分裂活性与0.005 nM的des-IGF-I相当,表明内源性产生的IGFBP可能抑制IGF-I的作用。在IEC-6细胞中,EGF和IGF-I + EGF处理可降低IGFBP-2的分泌,但不影响其mRNA表达,提示存在转录后调控。IGF-II和EGF在增加麦芽糖酶和蔗糖酶活性方面比IGF-I更有效,表明这些生长因子可能在更大程度上刺激分化而非有丝分裂。

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