Bibbins K B, Boeuf H, Varmus H E
Department of Microbiology and Immunology, University of California at San Francisco 94143.
Mol Cell Biol. 1993 Dec;13(12):7278-87. doi: 10.1128/mcb.13.12.7278-7287.1993.
Src homology 2 (SH2) domains are found in a variety of signaling proteins and bind phosphotyrosine-containing peptide sequences. To explore the binding properties of the SH2 domain of the Src protein kinase, we used immobilized phosphopeptides to bind purified glutathione S-transferase-Src SH2 fusion proteins. With this assay, as well as a free-peptide competition assay, we have estimated the affinities of the Src SH2 domain for various phosphopeptides relative to a Src SH2-phosphopeptide interaction whose Kd has been determined previously (YEEI-P; Kd = 4 nM). Two Src-derived phosphopeptides, one containing the regulatory C-terminal Tyr-527 and another containing the autophosphorylation site Tyr-416, bind the Src SH2 domain in a specific though low-affinity manner (with about 10(4)-lower affinity than the YEEI-P peptide). A platelet-derived growth factor receptor (PDGF-R) phosphopeptide containing Tyr-857 does not bind appreciably to the Src SH2 domain, suggesting it is not the PDGF-R binding site for Src as previously reported. However, another PDGF-R-derived phosphopeptide containing Tyr-751 does bind the Src SH2 domain (with an affinity approximately 2 orders of magnitude lower than that of YEEI-P). All of the phosphopeptides which bind to the Src SH2 domain contain a glutamic acid at position -3 or -4 with respect to phosphotyrosine; changing this residue to alanine greatly diminishes binding. We have also tested Src SH2 mutants for their binding properties and have interpreted our results in light of the recent crystal structure solution for the Src SH2 domain. Mutations in various conserved and nonconserved residues (R155A, R155K, N198E, H201R, and H201L) cause slight reductions in binding, while two mutations cause severe reductions. The W148E mutant domain, which alters the invariant tryptophan that marks the N-terminal border of the SH2 domain, binds poorly to phosphopeptides. Inclusion of the SH3 domain in the fusion protein partially restores the binding by the W148E mutant. A change in the invariant arginine that coordinates twice with phosphotyrosine in the peptide (R175L) results in a nearly complete loss of binding. The R175L mutant does display high affinity for the PDGF-R peptide containing Tyr-751, via an interaction that is at least partly phosphotyrosine independent. We have used this interaction to show that the R175L mutation also disrupts the intramolecular interaction between the Src SH2 domain and the phosphorylated C terminus within the context of the entire Src protein; thus, the binding properties observed for mutant domains in an in vitro assay appear to mimic those that occur in vivo.
Src同源2(SH2)结构域存在于多种信号蛋白中,可结合含磷酸酪氨酸的肽序列。为了探究Src蛋白激酶SH2结构域的结合特性,我们使用固定化的磷酸肽来结合纯化的谷胱甘肽S-转移酶-Src SH2融合蛋白。通过该检测方法以及游离肽竞争检测法,我们估算了Src SH2结构域与各种磷酸肽的亲和力,相对于先前已确定Kd值(YEEI-P;Kd = 4 nM)的Src SH2-磷酸肽相互作用。两种源自Src的磷酸肽,一种包含调节性C末端酪氨酸-527,另一种包含自磷酸化位点酪氨酸-416,以特定但低亲和力的方式结合Src SH2结构域(亲和力比YEEI-P肽低约10^4倍)。含酪氨酸-857的血小板衍生生长因子受体(PDGF-R)磷酸肽与Src SH2结构域的结合不明显,这表明它并非如先前报道的那样是Src与PDGF-R的结合位点。然而,另一种含酪氨酸-751的源自PDGF-R的磷酸肽确实能结合Src SH2结构域(亲和力比YEEI-P低约2个数量级)。所有与Src SH2结构域结合的磷酸肽在磷酸酪氨酸的-3或-4位均含有谷氨酸;将该残基变为丙氨酸会大大降低结合力。我们还测试了Src SH2突变体的结合特性,并根据最近解析的Src SH2结构域晶体结构来解释我们的结果。各种保守和非保守残基(R155A、R155K、N198E、H201R和H201L)的突变导致结合力略有降低,而有两个突变则导致结合力严重降低。W148E突变结构域改变了标志着SH2结构域N末端边界的不变色氨酸,与磷酸肽的结合很差。融合蛋白中包含SH3结构域可部分恢复W148E突变体的结合力。肽中与磷酸酪氨酸有两次配位的不变精氨酸发生改变(R175L)会导致结合几乎完全丧失。R175L突变体确实对含酪氨酸-751的PDGF-R肽表现出高亲和力,其相互作用至少部分不依赖于磷酸酪氨酸。我们利用这种相互作用表明,在完整Src蛋白的背景下,R175L突变也破坏了Src SH2结构域与磷酸化C末端之间的分子内相互作用;因此,在体外检测中观察到的突变结构域的结合特性似乎与体内发生的情况相似。
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