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A practical guide to genetic engineering of pancreatic β-cellsin vivo: Getting a grip on RIP and MIP

机译:胰腺β细胞基因工程实用指南体内:掌握RIP和MIP

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摘要

In vivo gene manipulation is a cornerstone approach in modern physiology. Cre-Lox technology has been extensively used to delete genes and activate reporters in pancreatic β-cells, bringing new insight into the pathophysiology of diabetes. In all cases, it is important to understand the expression domain of the specific reporter-Cre combination in order to correctly interpret the data. In the case of targeted genes with significant expression and function in the brain, the use of Ins2 promoter driven Cre, commonly known as RIP-Cre, has been shown to confound data interpretation when appropriate controls are not present. The recent article from the Philipson group in Islets provides an important characterization of a new Cre-deleter model, referred to as MIP1-CreER, which employs the mouse Ins1 promoter. This Ins1 promoter, recapitulating the expression pattern of the endogenous Ins1 gene, does not drive significant transgene expression in the brain and therefore is highly specific for deleting genes or turning on reporters in the pancreatic β-cell. This model promises to be widely used in the field of islet biology. Here, I review recent developments in the area of in vivo gene modification and predict areas where such tools will be refined further.
机译:体内基因操纵是现代生理学的基础方法。 Cre-Lox技术已被广泛用于删除基因并激活胰腺β细胞中的报告基因,为糖尿病的病理生理学带来了新的见解。在所有情况下,重要的是要了解特定报告基因-Cre组合的表达域,以便正确解释数据。对于在大脑中具有明显表达和功能的靶向基因而言,当不存在适当的对照物时,已证明使用Ins2启动子驱动的Cre(通常称为RIP-Cre)会混淆数据解释。来自胰岛的Philipson组的最新文章提供了一个新的Cre-deleter模型的重要特征,该模型称为MIP1-CreER,它使用小鼠Ins1启动子。该Ins1启动子概括了内源Ins1基因的表达模式,不会驱动大脑中明显的转基因表达,因此对于删除胰腺β细胞中的基因或开启报告基因具有高度特异性。该模型有望在胰岛生物学领域广泛使用。在这里,我回顾了体内基因修饰领域的最新进展,并预测了将进一步完善此类工具的领域。

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