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肿瘤坏死因子信号转导。一种26 kDa细胞溶质蛋白的组织特异性丝氨酸磷酸化。

Tumor necrosis factor signal transduction. Tissue-specific serine phosphorylation of a 26-kDa cytosolic protein.

作者信息

Schütze S, Scheurich P, Pfizenmaier K, Krönke M

机构信息

Clinical Research Group of the Max-Planck-Society, University of Göttingen, Federal Republic of Germany.

出版信息

J Biol Chem. 1989 Feb 25;264(6):3562-7.

PMID:2536751
Abstract

Binding of tumor necrosis factor-alpha (TNF-alpha) to its receptor on U937 cells results in rapid and TNF dose-dependent phosphorylation of a cytosolic protein with an apparent molecular mass of 26,000 kDa (p26) and an isoelectric point of 5.6. Half-maximal phosphorylation of p26 was achieved at concentrations of 1.8 ng/ml and was detectable within 20 s of TNF-alpha treatment. p26 is phosphorylated exclusively at serine residues. p26 phosphorylation occurs at 37 degrees C as well as at 14 degrees C, indicating that internalization of the TNF receptor is not required for serine kinase activation. Dephosphorylation of p26 starts 10 min after TNF-induced phosphorylation, suggesting a possible regulatory function of this cytosolic protein within the post-TNF receptor signaling system. p26 is also phosphorylated upon treatment with lymphotoxin. In contrast, both interferon-gamma and lipopolysaccharide fail to induce p26 phosphorylation. Whereas phosphorylated p26 was detected in the TNF-sensitive breast cancer cell line CRL1500, other TNF-responsive tumor cell lines investigated lacked enhanced phosphorylation of p26 in response to TNF, indicating that the 26-kDa phosphoprotein (pp26) may be a cell type-specific second messenger molecule involved in TNF signal transduction in some, but not all, target cells. p26 is also phosphorylated in a subclone of U937 (U937.C27) that responds to TNF-alpha with differentiation, yet is resistant to TNF-alpha-mediated growth inhibition. In contrast, p26 is not phosphorylated in another U937 derivative (U937.G3) that is resistant to both TNF-alpha-induced growth arrest and differentiation, suggesting that pp26 may play a role in the TNF signaling pathway linked to differentiation processes rather than to growth control.

摘要

肿瘤坏死因子-α(TNF-α)与其在U937细胞上的受体结合,导致一种表观分子量为26,000 kDa(p26)、等电点为5.6的胞质蛋白发生快速且依赖TNF剂量的磷酸化。在1.8 ng/ml的浓度下可实现p26的半最大磷酸化,且在TNF-α处理20秒内即可检测到。p26仅在丝氨酸残基处被磷酸化。p26的磷酸化在37℃以及14℃时均可发生,这表明丝氨酸激酶的激活不需要TNF受体的内化。p26的去磷酸化在TNF诱导的磷酸化开始10分钟后启动,提示这种胞质蛋白可能在TNF受体后信号系统中具有潜在的调节功能。用淋巴毒素处理后p26也会发生磷酸化。相比之下,干扰素-γ和脂多糖均不能诱导p26磷酸化。虽然在TNF敏感的乳腺癌细胞系CRL1500中检测到了磷酸化的p26,但所研究的其他TNF反应性肿瘤细胞系在TNF刺激下缺乏p26磷酸化增强的情况,这表明26 kDa的磷蛋白(pp26)可能是一种细胞类型特异性的第二信使分子,在部分而非所有靶细胞的TNF信号转导中发挥作用。p26在U937的一个亚克隆(U937.C27)中也会被磷酸化,该亚克隆对TNF-α有分化反应,但对TNF-α介导的生长抑制具有抗性。相反,在另一个对TNF-α诱导的生长停滞和分化均有抗性的U937衍生物(U937.G3)中,p26未被磷酸化,这表明pp26可能在与分化过程而非生长控制相关的TNF信号通路中发挥作用。

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