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T细胞生长因子的人类受体。翻译后可变加工、磷酸化、硫酸化的证据以及受体前体形式结合T细胞生长因子的能力。

The human receptor for T-cell growth factor. Evidence for variable post-translational processing, phosphorylation, sulfation, and the ability of precursor forms of the receptor to bind T-cell growth factor.

作者信息

Leonard W J, Depper J M, Krönke M, Robb R J, Waldmann T A, Greene W C

出版信息

J Biol Chem. 1985 Feb 10;260(3):1872-80.

PMID:2981876
Abstract

The T-cell growth factor (TCGF) receptor on phytohemagglutinin-activated normal peripheral blood T-cells is characterized as a glycoprotein with an apparent Mr = 55,000 that contains N-linked and O-linked carbohydrate with only approximately 33,000 daltons of peptide structure (p33) as evaluated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. There are two N-linked glycosylated intermediate precursor forms (apparent Mr = 35,000 (p35) and 37,000 (p37]. This receptor differs from the TCGF receptor on HUT-102B2 cells (apparent Mr = 50,000) because of differences in post-translational processing. Experiments with the carboxylic ionophore monensin demonstrate blockade of the transition of the p35 and p37 receptor precursor forms to the mature receptor, presumably secondary to inhibition of Golgi-associated receptor processing. We identify the primary translation product of TCGF receptor mRNA as intermediate in size between the p33 and the p35/p37 forms. We further demonstrate that the p33, p35, and p37 precursor forms, but not the primary translation product, are all capable of binding TCGF. Thus, the removal of the signal peptide and/or conformational changes of the primary translation product are necessary for ligand binding; however, the extensive post-translational modifications are not. Lastly, we demonstrate that at least some TCGF receptors are phosphorylated and sulfated, and that TCGF receptors on phytohemagglutinin-activated normal T-cells are more heavily sulfated than those on HUT-102B2 cells.

摘要

植物血凝素激活的正常外周血T细胞上的T细胞生长因子(TCGF)受体被表征为一种糖蛋白,其表观分子量为55,000,含有N-连接和O-连接的碳水化合物,通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳评估,其肽结构(p33)仅约33,000道尔顿。有两种N-连接的糖基化中间前体形式(表观分子量为35,000(p35)和37,000(p37))。由于翻译后加工的差异,该受体与HUT-102B2细胞上的TCGF受体(表观分子量为50,000)不同。用羧酸离子载体莫能菌素进行的实验表明,p35和p37受体前体形式向成熟受体的转变被阻断,推测这是由于高尔基体相关受体加工受到抑制所致。我们将TCGF受体mRNA的主要翻译产物鉴定为大小介于p33和p35/p37形式之间的中间体。我们进一步证明,p33、p35和p37前体形式,但不是主要翻译产物,都能够结合TCGF。因此,信号肽的去除和/或主要翻译产物的构象变化是配体结合所必需的;然而,广泛的翻译后修饰并非必需。最后,我们证明至少一些TCGF受体被磷酸化和硫酸化,并且植物血凝素激活的正常T细胞上的TCGF受体比HUT-102B2细胞上的受体硫酸化程度更高。

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