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一种24千道尔顿蛋白与NHE1(钠氢交换体的普遍存在的同工型)的共免疫沉淀。

Coimmunoprecipitation of a 24-kDa protein with NHE1, the ubiquitous isoform of the Na+/H+ exchanger.

作者信息

Goss G, Orlowski J, Grinstein S

机构信息

Division of Cell Biology, Hospital for Sick Children, Toronto, Ontario, Canada.

出版信息

Am J Physiol. 1996 May;270(5 Pt 1):C1493-502. doi: 10.1152/ajpcell.1996.270.5.C1493.

DOI:10.1152/ajpcell.1996.270.5.C1493
PMID:8967452
Abstract

Ancillary proteins have been proposed to account for phosphorylation-independent regulation of the Na+/H+ exchanger (NHE), but such putative proteins have not been identified. Here we describe the specific association of NHE1 with a protein of approximately 24 kDa (p24). Immunoprecipitation of NHE1 from lysates of [35S] cysteine- and/or methionine-labeled cells with the use of an anti-NHE1 antibody demonstrated specific coimmunoprecipitation of p24 with NHE1. The stoichiometry of p24 relative to NHE1, assessed by their radiolabel content, was consistent between experiments and among cell types. Immunoblotting demonstrated that p24 is not a proteolytic product of NHE1. Internal deletion mutants and chimeras of NHE1/NHE3 suggest that p24 binds to residues 515-566 or 695-815 of NHE1 or to the transmembrane region of both NHE1 and NHE3. Protein p24 is not constitutively phosphorylated nor could phosphorylation be induced by serum or phorbol ester treatment. Binding of p24 to NHE1 is Ca2+ independent. Protein p24 failed to bind [gamma-32P]GTP in a blot-overlay assay, suggesting that it is not a low-molecular-weight GTP-binding protein. Identification of the p24:NHE1 interaction may contribute to our understanding of antiporter regulation.

摘要

辅助蛋白被认为可解释钠氢交换体(NHE)的磷酸化非依赖性调节,但尚未鉴定出此类假定蛋白。在此,我们描述了NHE1与一种约24 kDa的蛋白(p24)的特异性结合。使用抗NHE1抗体从[35S]半胱氨酸和/或甲硫氨酸标记的细胞裂解物中免疫沉淀NHE1,结果显示p24与NHE1特异性共免疫沉淀。通过其放射性标记含量评估,p24相对于NHE1的化学计量在实验之间以及不同细胞类型之间是一致的。免疫印迹表明p24不是NHE1的蛋白水解产物。NHE1/NHE3的内部缺失突变体和嵌合体表明,p24与NHE1的515 - 566或695 - 815残基结合,或者与NHE1和NHE3的跨膜区域结合。蛋白p24不是组成性磷酸化的,血清或佛波酯处理也不能诱导其磷酸化。p24与NHE1的结合不依赖于Ca2+。在印迹覆盖分析中,蛋白p24未能结合[γ-32P]GTP,这表明它不是一种低分子量GTP结合蛋白。鉴定p24与NHE1的相互作用可能有助于我们理解反向转运体的调节。

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