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培养的内皮细胞不会以自分泌方式对血小板衍生生长因子样蛋白产生反应。

Cultured endothelial cells do not respond to a platelet-derived growth-factor-like protein in an autocrine manner.

作者信息

Kazlauskas A, DiCorleto P E

出版信息

Biochim Biophys Acta. 1985 Sep 30;846(3):405-12. doi: 10.1016/0167-4889(85)90013-8.

Abstract

Cultured endothelial cells produce a growth factor similar or identical to platelet-derived growth factor (PDGF). Endothelial cells are able to proliferate in plasma-supplemented medium, while most nontransformed cells require serum-supplemented medium. Since PDGF is a major serum mitogen, we have tested the possibility that endothelial cells interact with and respond to the autologously produced PDGF-like (PDGF-c) protein. We have found that bovine aortic and rat heart endothelial cells express little or no cell surface PDGF receptors as determined by binding of pure 125I-PDGF. Treating these cells under acidic conditions, which release receptor-bound PDGF in control cells without affecting receptor function, did not reveal a population of cryptic receptors. In addition, when rat heart endothelial cells were grown in the presence of an antibody to PDGF, proliferation was unimpaired, though no detectable free PDGF was present in the medium. An equivalent amount of antibody completely blocked the mitogenic response of human fibroblasts that had been preincubated for 1 h at 37 degrees C with an equivalent dose of PDGF. Thus, endothelial cells do not respond mitogenically in a manner that would be expected from the interaction of autologously produced PDGF with its cell surface receptor. Endothelial cells were detergent-solubilized and immobilized on nitrocellulose in an attempt to detect the presence of intracellular PDGF receptors. Specific binding of 125I-PDGF to adsorbed, solubilized bovine aortic or rat heart endothelial cells was undetectable, though significant binding to adsorbed, solubilized fibroblasts, used as a positive control, was observed. We conclude that endothelial cells do not have detectable intracellular PDGF receptors.

摘要

培养的内皮细胞可产生一种与血小板衍生生长因子(PDGF)相似或相同的生长因子。内皮细胞能够在添加血浆的培养基中增殖,而大多数未转化细胞则需要添加血清的培养基。由于PDGF是一种主要的血清促有丝分裂原,我们测试了内皮细胞与自身产生的PDGF样(PDGF-c)蛋白相互作用并对其作出反应的可能性。我们发现,通过纯125I-PDGF的结合测定,牛主动脉和大鼠心脏内皮细胞几乎不表达或不表达细胞表面PDGF受体。在酸性条件下处理这些细胞,可在不影响受体功能的情况下释放对照细胞中与受体结合的PDGF,但未发现存在隐匿受体群体。此外,当大鼠心脏内皮细胞在存在抗PDGF抗体的情况下生长时,增殖不受影响,尽管培养基中未检测到游离的PDGF。等量的抗体完全阻断了人成纤维细胞的促有丝分裂反应,这些成纤维细胞在37℃下用等量剂量的PDGF预孵育1小时。因此,内皮细胞不会以自身产生的PDGF与其细胞表面受体相互作用所预期的方式对有丝分裂原作出反应。用去污剂溶解内皮细胞并固定在硝酸纤维素上,试图检测细胞内PDGF受体的存在。未检测到125I-PDGF与吸附的、溶解的牛主动脉或大鼠心脏内皮细胞的特异性结合,尽管观察到与用作阳性对照的吸附的、溶解的成纤维细胞有显著结合。我们得出结论,内皮细胞没有可检测到的细胞内PDGF受体。

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