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β-淀粉样前体蛋白在两个不同细胞位置的胞外域磷酸化。

Ectodomain phosphorylation of beta-amyloid precursor protein at two distinct cellular locations.

作者信息

Walter J, Capell A, Hung A Y, Langen H, Schnölzer M, Thinakaran G, Sisodia S S, Selkoe D J, Haass C

机构信息

Central Institute of Mental Health, Department of Molecular Biology, J5, 68159 Mannheim, Germany.

出版信息

J Biol Chem. 1997 Jan 17;272(3):1896-903. doi: 10.1074/jbc.272.3.1896.

DOI:10.1074/jbc.272.3.1896
PMID:8999878
Abstract

The beta-amyloid precursor protein (betaAPP) is a transmembrane protein that is exclusively phosphorylated on serine residues within its ectodomain. To identify the cellular site of betaAPP phosphorylation, we took advantage of an antibody that specifically detects the free C terminus of beta-secretase-cleaved betaAPP containing the Swedish missense mutation (APPssw-beta). This antibody previously established the cellular location of the beta-secretase cleavage of Swedish betaAPP as a post-Golgi secretory compartment (Haass, C., Lemere, C., Capell, A., Citron, M., Seubert, P., Schenk, D., Lannfelt, L., and Selkoe, D. J. (1995) Nature Med. 1, 1291-1296). We have now localized the selective ectodomain phosphorylation of betaAPP to the same compartment. Moreover, the phosphorylation sites of betaAPP were identified at Ser198 and Ser206 of betaAPP695 by tryptic peptide mapping, mass spectrometry, and site-directed mutagenesis. Intracellular phosphorylation of betaAPP was inhibited by Brefeldin A and by incubating cells at 20 degrees C, thus excluding phosphorylation in the endoplasmic reticulum or trans-Golgi network. Ectodomain phosphorylation within a post-Golgi compartment occurred not only with mutant Swedish betaAPP, but also with wild type betaAPP. In addition to phosphorylation within a post-Golgi compartment, betaAPP was also found to undergo phosphorylation at the cell surface by an ectoprotein kinase. Therefore, this study revealed two distinct cellular locations for betaAPP phosphorylation.

摘要

β-淀粉样前体蛋白(βAPP)是一种跨膜蛋白,其胞外结构域内仅在丝氨酸残基上发生磷酸化。为了确定βAPP磷酸化的细胞位点,我们利用了一种抗体,该抗体可特异性检测含有瑞典错义突变(APPssw-β)的β-分泌酶切割的βAPP的游离C末端。该抗体先前已确定瑞典βAPP的β-分泌酶切割的细胞位置为高尔基体后分泌区室(哈斯,C.,勒梅尔,C.,卡佩尔,A.,西特龙,M.,舒伯特,P.,申克,D.,兰费尔特,L.,和塞尔科,D.J.(1995年)《自然医学》1,1291 - 1296)。我们现在已将βAPP的选择性胞外结构域磷酸化定位到同一区室。此外,通过胰蛋白酶肽图谱分析、质谱分析和定点诱变,在βAPP695的Ser198和Ser206处鉴定出了βAPP的磷酸化位点。βAPP的细胞内磷酸化受到布雷菲德菌素A的抑制,并且通过在20℃下培养细胞来抑制,从而排除了在内质网或反式高尔基体网络中的磷酸化。高尔基体后区室内的胞外结构域磷酸化不仅发生在突变的瑞典βAPP中,也发生在野生型βAPP中。除了在高尔基体后区室内的磷酸化外,还发现βAPP在细胞表面被一种胞外蛋白激酶磷酸化。因此,这项研究揭示了βAPP磷酸化的两个不同细胞位置。

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