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Characterisation of BHK-21 cells engineered to secrete human insulin

机译:工程化分泌人胰岛素的BHK-21细胞的表征

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Autoimmune destruction of β cells in the pancreas leads to type I, or insulin dependent diabetes mellitus (IDDM), through the loss of endogenous insulin production capacity. This paper describes an attempt to generate ‘artificial’β cells using the fibroblast cell line BHK21. Stable transfectants expressing the human preproinsulin (PPI) gene were isolated and characterised. The resulting clone selected for further analysis (BHK-PPI-C16) was capable of secreting 0.12 pmol proinsulin/hr/105 cells and maintained a steady cellular proinsulin content of 0.36 ± 0.04 pmol l?1. There was no processing of the proinsulin to mature insulin. The cells were unresponsive to glucose but there was increased proinsulin secretion in the presence of agents that stimulated formation of intracellular cAMP. Transfection of cDNAs for the key elements of the glucose sensing apparatus (GLUT2 and glucokinase) led to a subphysiological stimulation of secretion when glucokinase was transfected alone while there was a complete loss of insulin secretion when both components were overexpressed. The deleterious effect on proinsulin secretion observed upon co-expression of the glucose sensing genes may have implications for applications requiring multigene expression in BHK21 cells.
机译:胰腺中β细胞的自身免疫破坏会导致内源性胰岛素生产能力丧失,从而导致I型或胰岛素依赖型糖尿病(IDDM)。本文介绍了使用成纤维细胞系BHK21生成“人工”β细胞的尝试。分离并表征了表达人胰岛素原(PPI)基因的稳定转染子。选择用于进一步分析的所得克隆(BHK-PPI-C16)能够分泌0.12pmol胰岛素原/ hr / 105细胞,并维持稳定的细胞胰岛素原含量为0.36±0.04pmol l-1。没有将胰岛素原加工为成熟胰岛素。细胞对葡萄糖无反应,但是在刺激细胞内cAMP形成的药物存在下,胰岛素原分泌增加。当单独转染葡萄糖激酶时,转染葡萄糖传感装置关键元件(GLUT2和葡萄糖激酶)的cDNA会导致分泌的亚生理刺激,而当两种成分都过表达时,胰岛素分泌会完全丧失。共表达葡萄糖感测基因时观察到的对胰岛素原分泌的有害作用可能对需要在BHK21细胞中多基因表达的应用有影响。

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