Liu Wenli, Chin-Chance Catherine, Lee Eun-Jig, Lowe William L
Department of Medicine, Veterans Affairs Chicago Healthcare System, Lakeside Division, Chicago, Illinois 60611, USA.
Endocrinology. 2002 Oct;143(10):3802-12. doi: 10.1210/en.2002-220058.
To begin to determine whether IGF-I treatment represents a potential means of enhancing the survival of islet cell grafts after transplantation, the present studies established a model of beta-cell death secondary to loss of trophic support and examined the ability of IGF-I to prevent cell death. The studies were performed using the rat pancreatic beta-cell line, INS-1. Incubating INS-1 cells in RPMI 1640 and 0.25% BSA for 48 h increased cell death, as determined by lactate dehydrogenase release, compared with that of cells maintained in RPMI and 10% fetal calf serum. Addition of 100 ng/ml IGF-I to the serum-free medium decreased lactate dehydrogenase release to a level comparable to that found in cells maintained in fetal calf serum. Similar results were seen using a mouse beta-cell line, MIN6, infected with an adenovirus expressing IGF-I. Examination of IGF-I-stimulated signaling demonstrated that IGF-I increased the phosphorylation of protein kinase B in both cell lines, whereas IGF-I-induced phosphorylation of the MAPKs, ERK1 and -2, was observed only in INS-1 cells. The effect of IGF-I on phosphorylation of substrates of phosphatidylinositol 3-kinase (PI 3-kinase) or protein kinase B was also examined in INS-1 cells. IGF-I increased the phosphorylation of glycogen synthase kinase 3beta, BAD, FKHR, and p70(S6) kinase. Another pathway that has been shown to mediate the protective of IGF-I in some cell types is activation of cAMP response element-binding protein (CREB). IGF-I increased CREB phosphorylation at a concentration as low as 10 ng/ml, and this effect was inhibited by H89, a PKA inhibitor, and PD98059, a MAPK kinase inhibitor. Consistent with the effect of IGF-I on CREB phosphorylation, IGF-I increased the transcriptional activity of CREB, although it had no effect on CREB binding to DNA. Use of inhibitors of the PI 3-kinase (LY 294002) or ERK (PD98059) pathways or CREB phosphorylation (H89) in the cell death assay demonstrated partial abrogation of the protective effect of IGF-I with LY 294002. These data demonstrate that IGF-I protects pancreatic beta-cells from cell death secondary to loss of trophic support and that, although IGF-I activates several signaling pathways that contribute to its protective effect in other cell types, only activation of PI 3-kinase contributes to this effect in beta-cells.
为了开始确定胰岛素样生长因子-I(IGF-I)治疗是否代表一种增强移植后胰岛细胞移植存活率的潜在方法,本研究建立了一种因营养支持丧失导致的β细胞死亡模型,并研究了IGF-I预防细胞死亡的能力。研究使用大鼠胰腺β细胞系INS-1进行。与在含有10%胎牛血清的RPMI培养基中培养的细胞相比,将INS-1细胞在含有0.25%牛血清白蛋白(BSA)的RPMI 1640培养基中培养48小时会增加细胞死亡,这通过乳酸脱氢酶释放来确定。向无血清培养基中添加100 ng/ml的IGF-I可将乳酸脱氢酶释放降低至与在胎牛血清中培养的细胞相当的水平。使用感染了表达IGF-I的腺病毒的小鼠β细胞系MIN6也得到了类似结果。对IGF-I刺激的信号传导的检测表明,IGF-I在两种细胞系中均增加了蛋白激酶B的磷酸化,而仅在INS-1细胞中观察到IGF-I诱导的丝裂原活化蛋白激酶(MAPK)ERK1和ERK2的磷酸化。还在INS-1细胞中检测了IGF-I对磷脂酰肌醇-3激酶(PI 3-激酶)或蛋白激酶B底物磷酸化的影响。IGF-I增加了糖原合酶激酶3β、BAD、FKHR和p70(S6)激酶的磷酸化。在某些细胞类型中已显示介导IGF-I保护作用的另一条途径是激活环磷酸腺苷反应元件结合蛋白(CREB)。IGF-I在低至10 ng/ml的浓度下即可增加CREB的磷酸化,并且这种作用被蛋白激酶A(PKA)抑制剂H89和MAPK激酶抑制剂PD98059所抑制。与IGF-I对CREB磷酸化的作用一致,IGF-I增加了CREB的转录活性,尽管它对CREB与DNA的结合没有影响。在细胞死亡试验中使用PI 3-激酶(LY 294002)或ERK(PD98059)途径抑制剂或CREB磷酸化抑制剂(H89)表明,LY 294002可部分消除IGF-I的保护作用。这些数据表明,IGF-I可保护胰腺β细胞免受因营养支持丧失导致的细胞死亡,并且尽管IGF-I激活了几种在其他细胞类型中有助于其保护作用的信号传导途径,但在β细胞中仅PI 3-激酶的激活对这种作用有贡献。
Zotero 插件