首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Coexpression of the platelet-derived growth factor (PDGF) B chain and the PDGF beta receptor in isolated pancreatic islet cells stimulates DNA synthesis.
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Coexpression of the platelet-derived growth factor (PDGF) B chain and the PDGF beta receptor in isolated pancreatic islet cells stimulates DNA synthesis.

机译:血小板源生长因子(PDGF)B链和PDGFβ受体在分离的胰岛细胞中的共表达刺激了DNA的合成。

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摘要

Suspensions rich in pancreatic beta cells were transfected by means of electroporation or by using the liposome technique with DNA constructs coding for the B chain of platelet-derived growth factor (PDGF) and the PDGF alpha and beta receptors to induce a mitotic response in this slowly replicating cell type. Transfection with the B-chain construct induced synthesis of the PDGF B-chain homodimer (PDGF-BB) as assessed by the presence of 125I-labeled PDGF-BB competing activity in the conditioned medium of the transfected islet cells. Moreover, islet cells transfected with the PDGF beta-receptor construct exhibited increased immunofluorescence staining with a PDGF beta-receptor antibody. These cells also displayed increased 125I-labeled PDGF-BB binding compared with control transfected cells. Cotransfection with the B-chain construct or the addition of 10% fetal bovine serum or purified PDGF all induced DNA synthesis in islet cells transfected with the PDGF beta-receptor construct. Islet cells transfected with the PDGF alpha-receptor construct did not respond with stimulation of [3H]thymidine incorporation to any of the PDGF isoforms (PDGF-AA, -AB, or -BB). Cotransfection of the PDGF alpha- and beta-receptor constructs resulted in a loss of the DNA synthesis response to PDGF. The beta cells exhibited elevated levels of [3H]inositol trisphosphate after transfection with the B-chain and beta-receptor constructs, indicating activation of phospholipase C. Islet cells transfected with the different receptor constructs exhibited different patterns of tyrosine phosphorylation upon ligand activation. The results demonstrate that pancreatic islet cells can be stimulated to increase DNA synthesis by transfection with the PDGF beta-receptor gene, whereas cotransfection with the alpha-receptor gene may attenuate the growth response.
机译:通过电穿孔或使用脂质体技术将富含胰腺β细胞的悬浮液转染,该DNA构建体编码血小板衍生的生长因子(PDGF)B链以及PDGFα和β受体的B链,从而在此过程中缓慢诱导有丝分裂反应复制单元格类型。通过在转染的胰岛细胞的条件培养基中125 I标记的PDGF-BB竞争活性的存在评估,用B链构建体进行的转染诱导了PDGF B链同源二聚体(PDGF-BB)的合成。而且,用PDGFβ-受体构建体转染的胰岛细胞显示出用PDGFβ-受体抗体增加的免疫荧光染色。与对照转染的细胞相比,这些细胞还显示出125I标记的PDGF-BB结合增加。与B链构建体的共转染或添加10%胎牛血清或纯化的PDGF均可在用PDGFβ受体构建体转染的胰岛细胞中诱导DNA合成。用PDGFα受体构建体转染的胰岛细胞不响应[3H]胸苷掺入任何PDGF亚型(PDGF-AA,-AB或-BB)的刺激。 PDGFα和β受体构建体的共转染导致DNA合成对PDGF的反应丧失。在用B链和β受体构建体转染后,β细胞显示出升高的[3H]肌醇三磷酸水平,表明磷脂酶C的活化。用不同受体构建体转染的胰岛细胞在配体活化后显示出不同的酪氨酸磷酸化模式。结果表明,可以通过用PDGFβ受体基因转染来刺激胰岛细胞,以增加DNA合成,而与α受体基因共转染则可以减弱生长反应。

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