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影响胰腺β细胞胰岛素分泌的细胞外蛋白质相互作用的共培养分析。

Coculture analysis of extracellular protein interactions affecting insulin secretion by pancreatic beta cells.

作者信息

Zhang Charles, Suckow Arthur T, Chessler Steven D

机构信息

Pediatric Diabetes Research Center, University of California, San Diego.

出版信息

J Vis Exp. 2013 Jun 15(76):e50365. doi: 10.3791/50365.

Abstract

Interactions between cell-surface proteins help coordinate the function of neighboring cells. Pancreatic beta cells are clustered together within pancreatic islets and act in a coordinated fashion to maintain glucose homeostasis. It is becoming increasingly clear that interactions between transmembrane proteins on the surfaces of adjacent beta cells are important determinants of beta-cell function. Elucidation of the roles of particular transcellular interactions by knockdown, knockout or overexpression studies in cultured beta cells or in vivo necessitates direct perturbation of mRNA and protein expression, potentially affecting beta-cell health and/or function in ways that could confound analyses of the effects of specific interactions. These approaches also alter levels of the intracellular domains of the targeted proteins and may prevent effects due to interactions between proteins within the same cell membrane to be distinguished from the effects of transcellular interactions. Here a method for determining the effect of specific transcellular interactions on the insulin secreting capacity and responsiveness of beta cells is presented. This method is applicable to beta-cell lines, such as INS-1 cells, and to dissociated primary beta cells. It is based on coculture models developed by neurobiologists, who found that exposure of cultured neurons to specific neuronal proteins expressed on HEK293 (or COS) cell layers identified proteins important for driving synapse formation. Given the parallels between the secretory machinery of neuronal synapses and of beta cells, we reasoned that beta-cell functional maturation might be driven by similar transcellular interactions. We developed a system where beta cells are cultured on a layer of HEK293 cells expressing a protein of interest. In this model, the beta-cell cytoplasm is untouched while extracellular protein-protein interactions are manipulated. Although we focus here primarily on studies of glucose-stimulated insulin secretion, other processes can be analyzed; for example, changes in gene expression as determined by immunoblotting or qPCR.

摘要

细胞表面蛋白之间的相互作用有助于协调相邻细胞的功能。胰腺β细胞聚集在胰岛内,并以协调的方式发挥作用以维持葡萄糖稳态。越来越清楚的是,相邻β细胞表面跨膜蛋白之间的相互作用是β细胞功能的重要决定因素。通过在培养的β细胞或体内进行敲低、敲除或过表达研究来阐明特定跨细胞相互作用的作用,需要直接干扰mRNA和蛋白质表达,这可能会以混淆特定相互作用影响分析的方式影响β细胞的健康和/或功能。这些方法还会改变靶向蛋白细胞内结构域的水平,并可能阻止区分同一细胞膜内蛋白质之间相互作用的影响与跨细胞相互作用的影响。本文介绍了一种确定特定跨细胞相互作用对β细胞胰岛素分泌能力和反应性影响的方法。该方法适用于β细胞系,如INS-1细胞,以及解离的原代β细胞。它基于神经生物学家开发的共培养模型,他们发现将培养的神经元暴露于HEK293(或COS)细胞层上表达的特定神经元蛋白可鉴定出对驱动突触形成很重要的蛋白。鉴于神经元突触和β细胞分泌机制之间的相似性,我们推测β细胞功能成熟可能由类似的跨细胞相互作用驱动。我们开发了一个系统,其中β细胞在表达感兴趣蛋白的HEK293细胞层上培养。在这个模型中,β细胞的细胞质未受影响,而细胞外蛋白质-蛋白质相互作用则受到操控。尽管我们在此主要关注葡萄糖刺激的胰岛素分泌研究,但也可以分析其他过程;例如,通过免疫印迹或qPCR确定的基因表达变化。

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引用本文的文献

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本文引用的文献

1
Transcellular neuroligin-2 interactions enhance insulin secretion and are integral to pancreatic β cell function.
J Biol Chem. 2012 Jun 8;287(24):19816-26. doi: 10.1074/jbc.M111.280537. Epub 2012 Apr 23.
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J Vis Exp. 2011 Apr 13(50):2096. doi: 10.3791/2096.
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