Maeda Kenji, Hägglund Per, Finnie Christine, Svensson Birte, Henriksen Anette
Enzyme and Protein Chemistry, Department of Systems Biology, Technical University of Denmark, DK-2800 Kongens Lyngby, Denmark.
Protein Sci. 2008 Jun;17(6):1015-24. doi: 10.1110/ps.083460308. Epub 2008 Apr 18.
H-type thioredoxins (Trxs) constitute a particularly large Trx sub-group in higher plants. Here, the crystal structures are determined for the two barley Trx h isoforms, HvTrxh1 and HvTrxh2, in the partially radiation-reduced state to resolutions of 1.7 A, and for HvTrxh2 in the oxidized state to 2.0 A. The two Trxs have a sequence identity of 51% and highly similar fold and active-site architecture. Interestingly, the four independent molecules in the crystals of HvTrxh1 form two relatively large and essentially identical protein-protein interfaces. In each interface, a loop segment of one HvTrxh1 molecule is positioned along a shallow hydrophobic groove at the primary nucleophile Cys40 of another HvTrxh1 molecule. The association mode can serve as a model for the target protein recognition by Trx, as it brings the Met82 Cgamma atom (gamma position as a disulfide sulfur) of the bound loop segment in the proximity of the Cys40 thiol. The interaction involves three characteristic backbone-backbone hydrogen bonds in an antiparallel beta-sheet-like arrangement, similar to the arrangement observed in the structure of an engineered, covalently bound complex between Trx and a substrate protein, as reported by Maeda et al. in an earlier paper. The occurrence of an intermolecular salt bridge between Glu80 of the bound loop segment and Arg101 near the hydrophobic groove suggests that charge complementarity plays a role in the specificity of Trx. In HvTrxh2, isoleucine corresponds to this arginine, which emphasizes the potential for specificity differences between the coexisting barley Trx isoforms.
H型硫氧还蛋白(Trxs)在高等植物中构成了一个特别大的Trx亚组。在这里,测定了两种大麦Trx h亚型HvTrxh1和HvTrxh2在部分辐射还原状态下的晶体结构,分辨率为1.7 Å,以及HvTrxh2在氧化状态下的晶体结构,分辨率为2.0 Å。这两种Trxs的序列同一性为51%,具有高度相似的折叠和活性位点结构。有趣的是,HvTrxh1晶体中的四个独立分子形成了两个相对较大且基本相同的蛋白质-蛋白质界面。在每个界面中,一个HvTrxh1分子的环段沿着另一个HvTrxh1分子的初级亲核半胱氨酸Cys40处的浅疏水凹槽定位。这种结合模式可以作为Trx识别靶蛋白的模型,因为它使结合环段的Met82 Cγ原子(作为二硫键硫的γ位置)靠近Cys40硫醇。这种相互作用涉及反平行β-折叠样排列中的三个特征性主链-主链氢键,类似于Maeda等人在早期论文中报道的Trx与底物蛋白之间工程化共价结合复合物结构中观察到的排列。结合环段的Glu80与疏水凹槽附近的Arg101之间存在分子间盐桥,这表明电荷互补性在Trx的特异性中起作用。在HvTrxh2中,异亮氨酸对应于这个精氨酸,这强调了共存的大麦Trx亚型之间存在特异性差异的可能性。