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膜免疫球蛋白(membrane Ig)和CD40与细胞外调节激酶信号通路的差异偶联。

Differential coupling of membrane Ig and CD40 to the extracellularly regulated kinase signaling pathway.

作者信息

Purkerson J M, Parker D C

机构信息

Department of Molecular Microbiology and Immunology, Oregon Health Sciences University, Portland 97201, USA.

出版信息

J Immunol. 1998 Mar 1;160(5):2121-9.

PMID:9498749
Abstract

Coupling of membrane Ig (mIg) and CD40 to the extracellularly regulated kinase (ERK) signal transduction pathway was examined in the WEHI-231 B lymphoma and normal mouse B cells. Cross-linking mIg induces ERK activation in both WEHI-231 and normal B cells. In contrast, CD40 cross-linking failed to induce ERK activation in WEHI-231, but signals through CD40 were more effective than mIg as a stimulus for ERK activation in normal B cells. However, several lines of evidence suggest that CD40 and the B cell Ag regulate ERK through distinct pathways that converge at the level of MEK-1, mitogen-activated protein kinase kinase. Abs to mIg or CD40 induced MEK-1 activation with different kinetics. Cross-linking of mIg, but not CD40, induced tyrosine phosphorylation of the SHC adapter molecule that couples receptors to Ras-dependent signaling pathways. Finally, agents that elevate cAMP, causing protein kinase A-mediated inhibition of Raf-1, inhibited activation of ERK in response to mIg cross-linking, but had no affect on ERK activation in response to anti-CD40 or Jun N-terminal kinase activation by signals through either receptor. Thus, CD40 uses an unidentified protein kinase A-insensitive MEK kinase, rather than Raf-1, to regulate ERK activity.

摘要

在WEHI-231 B淋巴瘤细胞和正常小鼠B细胞中检测了膜免疫球蛋白(mIg)和CD40与细胞外调节激酶(ERK)信号转导通路的偶联情况。mIg交联可诱导WEHI-231细胞和正常B细胞中的ERK激活。相比之下,CD40交联未能在WEHI-231细胞中诱导ERK激活,但在正常B细胞中,通过CD40的信号作为ERK激活的刺激物比mIg更有效。然而,几条证据表明,CD40和B细胞抗原通过在丝裂原活化蛋白激酶激酶MEK-1水平汇聚的不同途径调节ERK。针对mIg或CD40的抗体以不同的动力学诱导MEK-1激活。mIg交联而非CD40交联诱导了将受体与Ras依赖性信号通路偶联的SHC衔接分子的酪氨酸磷酸化。最后,提高cAMP水平从而导致蛋白激酶A介导的Raf-1抑制的试剂,抑制了mIg交联引起的ERK激活,但对通过任一受体的信号引起的抗CD40或Jun N末端激酶激活所导致的ERK激活没有影响。因此,CD40使用一种未确定的对蛋白激酶A不敏感的MEK激酶,而非Raf-1,来调节ERK活性。

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