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三触角相互作用氨肽酶F1与不同配体的结构解释了其催化机制。

Structures of the tricorn-interacting aminopeptidase F1 with different ligands explain its catalytic mechanism.

作者信息

Goettig Peter, Groll Michael, Kim Jeong-Sun, Huber Robert, Brandstetter Hans

机构信息

Max-Planck-Institut für Biochemie, Abteilung Strukturforschung, Am Klopferspitz 18a, D-82152 Martinsried, Germany.

出版信息

EMBO J. 2002 Oct 15;21(20):5343-52. doi: 10.1093/emboj/cdf552.

Abstract

F1 is a 33.5 kDa serine peptidase of the alpha/beta-hydrolase family from the archaeon Thermoplasma acidophilum. Subsequent to proteasomal protein degradation, tricorn generates small peptides, which are cleaved by F1 to yield single amino acids. We have solved the crystal structure of F1 with multiwavelength anomalous dispersion (MAD) phasing at 1.8 A resolution. In addition to the conserved catalytic domain, the structure reveals a chiefly alpha-helical domain capping the catalytic triad. Thus, the active site is accessible only through a narrow opening from the protein surface. Two structures with molecules bound to the active serine, including the inhibitor phenylalanyl chloromethylketone, elucidate the N-terminal recognition of substrates and the catalytic activation switch mechanism of F1. The cap domain mainly confers the specificity for hydrophobic side chains by a novel cavity system, which, analogously to the tricorn protease, guides substrates to the buried active site and products away from it. Finally, the structure of F1 suggests a possible functional complex with tricorn that allows efficient processive degradation to free amino acids for cellular recycling.

摘要

F1是一种来自嗜酸性嗜热栖热菌的α/β-水解酶家族的33.5 kDa丝氨酸肽酶。在蛋白酶体蛋白质降解之后,三触角蛋白酶产生小肽,这些小肽被F1切割以产生单个氨基酸。我们利用多波长反常散射(MAD)相位法在1.8 Å分辨率下解析了F1的晶体结构。除了保守的催化结构域外,该结构还揭示了一个主要由α-螺旋组成的结构域覆盖催化三联体。因此,活性位点只能通过蛋白质表面的一个狭窄开口进入。两种含有与活性丝氨酸结合分子的结构,包括抑制剂苯丙氨酰氯甲基酮,阐明了F1对底物的N端识别和催化激活开关机制。帽状结构域主要通过一个新颖的腔系统赋予对疏水侧链的特异性,该系统类似于三触角蛋白酶,将底物引导至埋藏的活性位点并将产物带离该位点。最后,F1的结构表明它可能与三触角蛋白酶形成功能复合物,从而实现高效的连续降解以产生游离氨基酸用于细胞循环利用。

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