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胰岛素基因在永生化大鼠海马和嗜铬细胞瘤 - 12细胞系中的表达。

Insulin gene expression in immortalized rat hippocampal and pheochromocytoma-12 cell lines.

作者信息

Singh B S, Rajakumar P A, Eves E M, Rosner M R, Wainer B H, Devaskar S U

机构信息

Department of Pediatrics, St. Louis University School of Medicine, Cardinal Glennon Children's Hospital, MO 63110, USA.

出版信息

Regul Pept. 1997 Mar 12;69(1):7-14. doi: 10.1016/s0167-0115(96)02120-9.

DOI:10.1016/s0167-0115(96)02120-9
PMID:9163577
Abstract

Employing reverse transcription-polymerase chain reaction and clonal cell lines derived by retroviral transduction of the temperature sensitive simian virus 40 large T-antigen into dispersed rat embryonic hippocampal cells, we detected the ancestral gene-insulin II mRNA in three progenitor subcloned cell lines. These cell lines upon differentiation are known to express markers indicative of commitment to either neuronal (H19-7; NF + , GFAP -), glial (H19-5; GFAP +, NF -), or bipotential (H583-5, NF +, GFAP + ) lineages. No duplicated, i.e., insulin I gene expression, was observed in any of the three cell lines. Induction of differentiation was associated with the persistence of insulin II mRNA and in the cells expressing a neuronal phenotype (H19-7; NF +, GFAP -) a relative doubling in insulin II mRNA level was present (P < 0.05). Minimal cellular insulin immunoreactivity was detected only in a subpopulation of cells with a differentiated neuronal phenotype. Radioimmunoassayable insulin peptide in the H19-7 cellular conditioned medium revealed a 5-fold increase in the differentiated state. In contrast, peripheral sympathetic PC-12 neuronal cells both in the undifferentiated and nerve growth factor-driven differentiated states, failed to express both insulin I and insulin II genes. We conclude that insulin II is expressed by cultured rat hippocampal clonal cell lines, and not by the peripheral sympathetic PC-12 neuronal cell line.

摘要

通过逆转录-聚合酶链反应以及将温度敏感型猿猴病毒40大T抗原经逆转录病毒转导至分散的大鼠胚胎海马细胞中衍生出的克隆细胞系,我们在三个祖细胞亚克隆细胞系中检测到了原始基因——胰岛素II mRNA。已知这些细胞系在分化时会表达一些标志物,表明它们分别向神经元(H19-7;神经丝蛋白阳性,胶质纤维酸性蛋白阴性)、神经胶质(H19-5;胶质纤维酸性蛋白阳性,神经丝蛋白阴性)或双潜能(H583-5,神经丝蛋白阳性,胶质纤维酸性蛋白阳性)谱系分化。在这三个细胞系中均未观察到胰岛素I基因的重复表达,即胰岛素I基因表达。分化诱导与胰岛素II mRNA的持续存在相关,并且在表达神经元表型的细胞(H19-7;神经丝蛋白阳性,胶质纤维酸性蛋白阴性)中,胰岛素II mRNA水平相对增加了一倍(P<0.05)。仅在具有分化神经元表型的细胞亚群中检测到了最低限度的细胞胰岛素免疫反应性。H19-7细胞条件培养基中的可通过放射免疫测定的胰岛素肽在分化状态下增加了5倍。相比之下,外周交感神经PC-12神经元细胞在未分化状态以及神经生长因子驱动的分化状态下均未能表达胰岛素I和胰岛素II基因。我们得出结论,胰岛素II由培养的大鼠海马克隆细胞系表达,而不由外周交感神经PC-12神经元细胞系表达。

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