L-选择素的细胞质尾部通过一个新的碱性结合基序与衔接蛋白复合物AP-1亚基μ1A相互作用。
The cytoplasmic tail of L-selectin interacts with the adaptor-protein complex AP-1 subunit μ1A via a novel basic binding motif.
作者信息
Dib Karim, Tikhonova Irina G, Ivetic Aleksandar, Schu Peter
机构信息
From the Max Planck Institute for Biochemistry, Department of Molecular Medicine, 82152 Martinsried, Germany,
the Center for Experimental Medicine, Queen's University Belfast, Belfast BT9 7BL, Northern Ireland, United Kingdom.
出版信息
J Biol Chem. 2017 Apr 21;292(16):6703-6714. doi: 10.1074/jbc.M116.768598. Epub 2017 Feb 24.
L-selectin regulates leukocyte adhesion and rolling along the endothelium. Proteins binding to the cytoplasmic tail of L-selectin regulate L-selectin functions. We used L-selectin cytoplasmic tail peptide pulldown assays combined with high sensitivity liquid chromatography/mass spectrometry to identify novel L-selectin tail-binding proteins. Incubation of the L-selectin tail with cell extracts from phorbol 12-myristate 13-acetate-stimulated Raw 264.7 macrophages resulted in the binding of μ1A of the clathrin-coated vesicle AP-1 complex. Furthermore, full-length GST-μ1A and the GST-μ1A C-terminal domain, but not the GST-μ1A N-terminal domain, bind to L-selectin tail peptide, and the intracellular pool of L-selectin colocalizes with AP-1 at the -Golgi network. We identified a novel basic protein motif consisting of a cluster of three dibasic residues (RR, KK, and KK) in the membrane-proximal domain of the L-selectin tail as well as a doublet of aspartic acid residues (DD) in the membrane-distal end of the L-selectin tail involved in μ1A binding. Stimulation of Raw 264.7 macrophages with PMA augmented the amount of μ1A associated with anti-L-selectin immunoprecipitates. However, full-length GST-μ1A did not bind to the phospho-L-selectin tail or phospho-mimetic S364D L-selectin tail. Accordingly, we propose that phosphorylation of μ1A is required for interaction with the L-selectin tail and that L-selectin tail phosphorylation may regulate this interaction Molecular docking of the L-selectin tail to μ1A was used to identify the μ1A surface domain binding the L-selectin tail and to explain how phosphorylation of the L-selectin tail abrogates μ1A interaction. Our findings indicate that L-selectin is transported constitutively by the AP-1 complex, leading to the formation of a -Golgi network reserve pool and that phosphorylation of the L-selectin tail blocks AP-1-dependent retrograde transport of L-selectin.
L-选择素调节白细胞在内皮上的黏附和滚动。与L-选择素细胞质尾结合的蛋白质调节L-选择素的功能。我们使用L-选择素细胞质尾肽下拉实验结合高灵敏度液相色谱/质谱来鉴定新的L-选择素尾结合蛋白。用佛波酯12-肉豆蔻酸酯13-乙酸酯刺激的Raw 264.7巨噬细胞的细胞提取物与L-选择素尾一起孵育,导致网格蛋白包被囊泡AP-1复合物的μ1A结合。此外,全长GST-μ1A和GST-μ1A C末端结构域,但不是GST-μ1A N末端结构域,与L-选择素尾肽结合,并且L-选择素的细胞内池与AP-1在反式高尔基体网络共定位。我们在L-选择素尾的膜近端结构域中鉴定出一个由三个双碱性残基(RR、KK和KK)簇组成的新的碱性蛋白基序,以及在L-选择素尾的膜远端参与μ1A结合的一对天冬氨酸残基(DD)。用佛波酯刺激Raw 264.7巨噬细胞增加了与抗L-选择素免疫沉淀相关的μ1A量。然而,全长GST-μ1A不与磷酸化的L-选择素尾或磷酸化模拟物S364D L-选择素尾结合。因此,我们提出μ1A的磷酸化是与L-选择素尾相互作用所必需的,并且L-选择素尾的磷酸化可能调节这种相互作用。L-选择素尾与μ1A的分子对接用于鉴定结合L-选择素尾的μ1A表面结构域,并解释L-选择素尾的磷酸化如何消除μ1A相互作用。我们的研究结果表明,L-选择素由AP-1复合物组成性转运,导致反式高尔基体网络储备池的形成,并且L-选择素尾的磷酸化阻断了L-选择素依赖于AP-1的逆行转运。
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