Polverini Eugenia, Rangaraj Godha, Libich David S, Boggs Joan M, Harauz George
Dipartimento di Fisica and CNISM, Università di Parma, V. le Usberti, 7/A, 43100 Parma, Italy.
Biochemistry. 2008 Jan 8;47(1):267-82. doi: 10.1021/bi701336n. Epub 2007 Dec 8.
Myelin basic protein (MBP) is a multifunctional protein involved in maintaining the stability and integrity of the myelin sheath by a variety of interactions with membranes and with cytoskeletal and other proteins. A central segment of MBP is highly conserved in mammals and consists of a membrane surface-associated amphipathic alpha-helix, immediately followed by a proline-rich segment that we hypothesize is an SH3 ligand. We show by circular dichroic spectroscopy that this proline-rich segment forms a polyproline type II helix in vitro under physiological conditions and that phosphorylation at a constituent threonyl residue has a stabilizing effect on its conformation. Using SH3 domain microarrays, we observe that the unmodified recombinant murine 18.5 kDa MBP isoform (rmC1 component) binds the following SH3 domains: Yes1 > PSD95 > cortactin = PexD = Abl = Fyn = c-Src = Itk in order of decreasing affinity. A quasi-deiminated form of the protein (rmC8) binds the SH3 domains Yes1 > Fyn > cortactin = c-Src > PexD = Abl. Phosphorylation of rmC1 at 1-2 threonines within the proline-rich segment by mitogen-activated protein kinase in vitro has no effect on the binding specificity to the SH3 domains on the array. An SH3 domain of chicken Fyn is also demonstrated to bind to lipid membrane-associated C1, phosphorylated C1, and rmC8. Molecular docking simulations of the interaction of the putative SH3 ligand of classic MBP with the human Fyn SH3 domain indicate that the strength of the interaction is of the same order of magnitude as with calmodulin and that the molecular recognition and association is mediated by some weak CH...pi interactions between the ligand prolyl residues and the aromatic ones of the SH3 binding site. One such interaction is well-conserved and involves the stacking of an MBP-peptide prolyl and an SH3 domain tryptophanyl residue, as in most other SH3-ligand complexes. Lysyl and arginyl residues in the peptide canonically interact via salt bridges and cation-pi interactions with negatively charged and aromatic residues in the SH3 domain binding site. Posttranslational modifications (phosphorylation or methylation) of the ligand cause noticeable shifts in the conformation of the flexible peptide and its side chains but do not predict any major inhibition of the binding beyond somewhat less favorable interactions for peptides with phosphorylated seryl or threonyl residues.
髓鞘碱性蛋白(MBP)是一种多功能蛋白,通过与膜、细胞骨架及其他蛋白的多种相互作用,参与维持髓鞘的稳定性和完整性。MBP的一个中央片段在哺乳动物中高度保守,由一个与膜表面相关的两亲性α-螺旋组成,紧接着是一个富含脯氨酸的片段,我们推测它是一个SH3配体。我们通过圆二色光谱表明,这个富含脯氨酸的片段在生理条件下于体外形成多聚脯氨酸II型螺旋,并且在一个组成性苏氨酰残基处的磷酸化对其构象有稳定作用。使用SH3结构域微阵列,我们观察到未修饰的重组小鼠18.5 kDa MBP异构体(rmC1组分)按亲和力递减顺序结合以下SH3结构域:Yes1 > PSD95 > 皮层肌动蛋白 = PexD = Abl = Fyn = c-Src = Itk。该蛋白的一种准脱亚氨基形式(rmC8)结合SH3结构域的顺序为Yes1 > Fyn > 皮层肌动蛋白 = c-Src > PexD = Abl。体外丝裂原活化蛋白激酶使富含脯氨酸片段内的1 - 2个苏氨酸磷酸化对rmC1与阵列上SH3结构域的结合特异性没有影响。鸡Fyn的一个SH3结构域也被证明可结合脂质膜相关的C1、磷酸化的C1和rmC8。经典MBP假定的SH3配体与人类Fyn SH3结构域相互作用的分子对接模拟表明,相互作用的强度与钙调蛋白的相互作用强度处于同一数量级,并且分子识别和缔合是由配体脯氨酰残基与SH3结合位点的芳香族残基之间的一些弱CH...π相互作用介导的。其中一种这样的相互作用高度保守,涉及MBP肽的脯氨酰残基与SH3结构域的色氨酰残基的堆积,这与大多数其他SH3 - 配体复合物的情况相同。肽中的赖氨酰和精氨酰残基通常通过盐桥和阳离子 - π相互作用与SH3结构域结合位点中的带负电荷和芳香族残基相互作用。配体的翻译后修饰(磷酸化或甲基化)会导致柔性肽及其侧链的构象发生明显变化,但除了对含磷酸化丝氨酰或苏氨酰残基的肽的相互作用稍不利外,并未预测到对结合有任何重大抑制作用。
