Murphy M E, Moult J, Bleackley R C, Gershenfeld H, Weissman I L, James M N
Department of Biochemistry, University of Alberta, Edmonton, Canada.
Proteins. 1988;4(3):190-204. doi: 10.1002/prot.340040306.
Two genes that are expressed when precursor cytotoxic T lymphocytes are transformed to T killer cells have been cloned and sequenced. The derived amino acid sequences, coding for cytotoxic cell protease 1 (CCP1) and Hannuka factor (HF) are highly homologous to members of the serine proteinase family. Comparative molecular model building using the known three-dimensional structures and the derived amino acid sequences of the lymphocyte enzymes has provided useful structural information, especially in predicting the conformations of the substrate binding sites. In applying this modelling procedure, we used the X-ray structures of four serine proteinases to provide a structurally based sequence alignment: alpha-chymotrypsin (CHT), bovine trypsin (BT), Streptomyces griseus trypsin (SGT), and rat mast cell protease 2 (RMCP2). The root mean square differences in alpha-carbon atom positions among these four structures when compared in a pairwise fashion range from 0.79 to 0.97 A for structurally equivalent residues. The sequences of the two lymphocyte enzymes were then aligned to these proteinases using chemical criteria and the superimposed X-ray structures as guides. The alignment showed that the sequence of CCP1 was most similar to RMCP2, whereas HF has regions of homology with both RMCP2 and BT. With RMCP2 as a template for CCP1 and the two enzymes RMCP2 and BT as templates for HF, the molecular models were constructed. Intramolecular steric clashes that resulted from the replacement of amino acid side chains of the templates by the aligned residues of CCP1 and HF were relieved by adjustment of the side chain conformational angles in an interactive computer graphics device. This process was followed by energy minimization of the enzyme model to optimize the stereochemical geometry and to relieve any remaining unacceptably close nonbonded contacts. The resulting model of CCP1 has an arginine residue at position 226 in the specificity pocket, thereby predicting a substrate preference for P1 aspartate or glutamate residues. The model also predicts favorable binding for a small hydrophobic residue at the P2 position of the substrate. The primary specificity pocket of HF resembles that of BT and therefore predicts a lysine or arginine preference for the P1 residue. The arginine at position 99 in the model of HF suggests a preference for aspartate or glutamate side chains in the P2 position of the substrate. Both CCP1 and HF have a free cysteine in the segment of polypeptide 88 to 93.(ABSTRACT TRUNCATED AT 400 WORDS)
当前体细胞毒性T淋巴细胞转化为T杀伤细胞时表达的两个基因已被克隆和测序。编码细胞毒性细胞蛋白酶1(CCP1)和哈努卡因子(HF)的推导氨基酸序列与丝氨酸蛋白酶家族成员高度同源。利用已知的三维结构和淋巴细胞酶的推导氨基酸序列进行比较分子模型构建,提供了有用的结构信息,特别是在预测底物结合位点的构象方面。在应用此建模程序时,我们使用了四种丝氨酸蛋白酶的X射线结构来提供基于结构的序列比对:α-胰凝乳蛋白酶(CHT)、牛胰蛋白酶(BT)、灰色链霉菌胰蛋白酶(SGT)和大鼠肥大细胞蛋白酶2(RMCP2)。当以成对方式比较时,这四种结构中α-碳原子位置的均方根差异对于结构等效残基范围为0.79至0.97埃。然后,使用化学标准并以叠加的X射线结构为指导,将这两种淋巴细胞酶的序列与这些蛋白酶进行比对。比对表明,CCP1的序列与RMCP2最相似,而HF在与RMCP2和BT两者中都有同源区域。以RMCP2为CCP1的模板,以RMCP2和BT这两种酶为HF的模板,构建了分子模型。通过在交互式计算机图形设备中调整侧链构象角,缓解了由CCP1和HF的比对残基取代模板氨基酸侧链导致的分子内空间冲突。此过程之后是对酶模型进行能量最小化,以优化立体化学几何结构并缓解任何剩余的不可接受的紧密非键接触。所得的CCP1模型在特异性口袋的第226位有一个精氨酸残基,从而预测对P1天冬氨酸或谷氨酸残基的底物偏好。该模型还预测底物P2位置的小疏水残基有良好的结合。HF的主要特异性口袋类似于BT的口袋,因此预测对P1残基有赖氨酸或精氨酸偏好。HF模型中第99位的精氨酸表明对底物P2位置的天冬氨酸或谷氨酸侧链有偏好。CCP1和HF在多肽88至93段都有一个游离的半胱氨酸。(摘要截短于400字)
