Rajan Sindhu, Dickson Lorna M, Mathew Elizabeth, Orr Caitlin M O, Ellenbroek Johanne H, Philipson Louis H, Wicksteed Barton
Kovler Diabetes Center, The University of Chicago, USA ; Department of Medicine, Section of Adult and Pediatric Endocrinology, Diabetes and Metabolism, The University of Chicago, USA.
Kovler Diabetes Center, The University of Chicago, USA ; Department of Medicine, Section of Adult and Pediatric Endocrinology, Diabetes and Metabolism, The University of Chicago, USA ; Committee on Molecular Metabolism and Nutrition, The University of Chicago, USA.
Mol Metab. 2015 Feb 3;4(4):265-76. doi: 10.1016/j.molmet.2015.01.010. eCollection 2015 Apr.
Glucagon-like peptide 1 (GLP-1) enhances insulin secretion and protects β-cell mass. Diabetes therapies targeting the GLP-1 receptor (GLP-1R), expressed in numerous tissues, have diminished dose-response in patients with type 2 diabetes compared with healthy human controls. The aim of this study was to determine the mechanistic causes underlying the reduced efficacy of GLP-1R ligands.
Using primary mouse islets and the β-cell line MIN6, outcomes downstream of the GLP-1R were analyzed: Insulin secretion; phosphorylation of the cAMP-response element binding protein (CREB); cAMP responses. Signaling systems were studied by immunoblotting and qRT-PCR, and PKA activity was assayed. Cell surface localization of the GLP-1R was studied by confocal microscopy using a fluorescein-tagged exendin-4 and GFP-tagged GLP-1R.
Rodent β-cells chronically exposed to high glucose had diminished responses to GLP-1R agonists including: diminished insulin secretory response; reduced phosphorylation of (CREB); impaired cAMP response, attributable to chronically increased cAMP levels. GLP-1R signaling systems were affected by hyperglycemia with increased expression of mRNAs encoding the inducible cAMP early repressor (ICER) and adenylyl cyclase 8, reduced PKA activity due to increased expression of the PKA-RIα subunit, reduced GLP-1R mRNA expression and loss of GLP-1R from the cell surface. To specifically examine the loss of GLP-1R from the plasma membrane a GLP-1R-GFP fusion protein was employed to visualize subcellular localization. Under low glucose conditions or when PKA activity was inhibited, GLP-1R-GFP was found at the plasma membrane. Conversely high glucose, expression of a constitutively active PKA subunit, or exposure to exendin-4 or forskolin led to GLP-1R-GFP internalization. Mutation of serine residue 301 of the GLP-1R abolished the glucose-dependent loss of the receptor from the plasma membrane. This was associated with a loss of an interaction between the receptor and the small ubiquitin-related modifier (SUMO), an interaction that was found to be necessary for internalization of the receptor.
These data show that glucose acting, at least in part, via PKA leads to the loss of the GLP-1R from the cell surface and an impairment of GLP-1R signaling, which may underlie the reduced clinical efficacy of GLP-1R based therapies in individuals with poorly controlled hyperglycemia.
胰高血糖素样肽1(GLP-1)可增强胰岛素分泌并保护β细胞数量。靶向在多种组织中表达的GLP-1受体(GLP-1R)的糖尿病治疗药物,与健康人类对照相比,在2型糖尿病患者中的剂量反应有所降低。本研究的目的是确定GLP-1R配体疗效降低的机制原因。
使用原代小鼠胰岛和β细胞系MIN6,分析GLP-1R下游的结果:胰岛素分泌;环磷酸腺苷反应元件结合蛋白(CREB)的磷酸化;环磷酸腺苷反应。通过免疫印迹和qRT-PCR研究信号系统,并测定蛋白激酶A(PKA)活性。使用荧光素标记的艾塞那肽-4和绿色荧光蛋白标记的GLP-1R,通过共聚焦显微镜研究GLP-1R的细胞表面定位。
长期暴露于高葡萄糖的啮齿动物β细胞对GLP-1R激动剂的反应减弱,包括:胰岛素分泌反应减弱;CREB磷酸化减少;环磷酸腺苷反应受损,这归因于环磷酸腺苷水平的长期升高。GLP-1R信号系统受到高血糖的影响,编码诱导型环磷酸腺苷早期阻遏物(ICER)和腺苷酸环化酶8的mRNA表达增加,由于PKA-RIα亚基表达增加导致PKA活性降低,GLP-1R mRNA表达减少以及GLP-1R从细胞表面丢失。为了具体研究GLP-1R从质膜的丢失,采用GLP-1R-绿色荧光蛋白融合蛋白来观察亚细胞定位。在低葡萄糖条件下或当PKA活性被抑制时,在质膜上发现GLP-1R-绿色荧光蛋白。相反,高葡萄糖、组成型活性PKA亚基的表达,或暴露于艾塞那肽-4或福斯高林会导致GLP-1R-绿色荧光蛋白内化。GLP-1R丝氨酸残基301的突变消除了受体从质膜上的葡萄糖依赖性丢失。这与受体和小泛素相关修饰物(SUMO)之间相互作用的丧失有关,发现这种相互作用是受体内化所必需的。
这些数据表明,葡萄糖至少部分通过PKA起作用,导致GLP-1R从细胞表面丢失以及GLP-1R信号传导受损,这可能是GLP-1R基础疗法在血糖控制不佳的个体中临床疗效降低的原因。
Zotero 插件
