IL-2-induced signal transduction: involvement of tyrosine kinase and IL-2 receptor gamma chain.

Lymphokine research Pub Date : 1990-01-01
K Sugamura, T Takeshita, H Asao, S Kumaki, K Ohbo, K Ohtani, M Nakamura
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Abstract

We previously established a monoclonal antibody, TU11 mAb, which is specific for human IL-2 receptor (IL-2R) beta chain (p75) and does not inhibit IL-2-binding to IL-2R beta. Using TU11 mAb, we first demonstrated the existence of a third component, p64, of IL-2R, tentatively named the gamma chain of IL-2R. TU11 mAb precipitated not only the beta chain but also the alpha and gamma chains in the lysates of cells bearing the high-affinity IL-2R in the presence of IL-2 without any chemical crosslinker. The gamma chain was also detected in lymphoid MOLT alpha beta and MOLT beta cells, which were stably transfected with both alpha and beta cDNA, and with beta cDNA alone, respectively, but not in fibroblastoid COS alpha beta and COS beta cells, which were stably transfected with both alpha and beta cDNA, and with beta cDNA alone, respectively. Furthermore, IL-2-mediated growth signals were transduced in the lymphoid transfectant cells but not in the fibroblastoid transfectant cells, suggesting the possibility that the gamma chain along with the beta chain has an essential role in the transduction of IL-2-mediated growth signals. Using TU11 mAb, we secondly demonstrated that IL-2 rapidly induces tyrosine phosphorylation of both the beta and gamma chains in an IL-2-dose-dependent manner. The tyrosine phosphorylation of beta and gamma chains were also detected in the lymphoid transfectant cells but not in the fibroblastoid transfectant cells, indicating the correlation between tyrosine kinase activation and IL-2-mediated growth signaling. The beta chain was phosphorylated in in vitro on serine, threonine and tyrosine residues, but the gamma chain was phosphorylated in in vitro predominantly on tyrosine residues, suggesting the possibility that the gamma chain itself is a tyrosine kinase molecule.

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IL-2诱导的信号转导:酪氨酸激酶和IL-2受体γ链的参与。
我们之前建立了一种单克隆抗体TU11 mAb,它对人IL-2受体(IL-2R) β链(p75)具有特异性,并且不抑制IL-2与IL-2R β的结合。使用TU11 mAb,我们首先证明了IL-2R的第三个成分p64的存在,暂定名为IL-2R的γ链。在没有任何化学交联剂的IL-2存在的情况下,TU11 mAb在携带高亲和力IL-2R的细胞的裂解物中不仅沉淀β链,还沉淀α链和γ链。在分别稳定转染α和β cDNA和单独转染β cDNA的淋巴样MOLT α β和MOLT β细胞中也检测到γ链,但在分别稳定转染α和β cDNA和单独转染β cDNA的成纤维样COS α β和COS β细胞中未检测到γ链。此外,il -2介导的生长信号在淋巴样转染细胞中被转导,而在成纤维细胞样转染细胞中不被转导,这表明γ链和β链可能在il -2介导的生长信号转导中起重要作用。利用TU11 mAb,我们证明了IL-2以剂量依赖的方式快速诱导β链和γ链的酪氨酸磷酸化。在淋巴样转染细胞中也检测到β链和γ链的酪氨酸磷酸化,但在成纤维细胞样转染细胞中未检测到,这表明酪氨酸激酶激活与il -2介导的生长信号传导之间存在相关性。β链在体外被丝氨酸、苏氨酸和酪氨酸残基磷酸化,但γ链在体外主要被酪氨酸残基磷酸化,这表明γ链本身可能是酪氨酸激酶分子。
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