Grams F, Reinemer P, Powers J C, Kleine T, Pieper M, Tschesche H, Huber R, Bode W
Max-Planck-Institut für Biochemie, Martinsried, Germany.
Eur J Biochem. 1995 Mar 15;228(3):830-41. doi: 10.1111/j.1432-1033.1995.tb20329.x.
Matrix metalloproteinases (MMPs) are a family of zinc endopeptidases involved in tissue remodeling. They have also been implicated in various disease processes including tumour invasion and joint destruction and are therefore attractive targets for inhibitor design. For rational drug design, information of inhibitor binding at the atomic level is essential. Recently, we have published the refined high-resolution crystal structure of the catalytic domain of human neutrophil collagenase (HNC) complexed with the inhibitor Pro-Leu-Gly-NHOH, which is a mimic for the unprimed (P3-P1) residues of a bound peptide substrate. We have now determined two additional HNC complexes formed with the thiol inhibitor HSCH2CH(CH2Ph)CO-L-Ala-Gly-NH2 and another hydroxamate inhibitor, HONHCOCH(iBu)CO-L-Ala-Gly-NH2, which were both refined to R-values of 0.183/0.198 at 0.240/0.225-nm resolution. The inhibitor thiol and hydroxamate groups ligand the catalytic zinc, giving rise to a slightly distorted tetrahedral and trigonal-bipyramidal coordination sphere, respectively. The thiol inhibitor diastereomer with S-configuration at the P1' residue (corresponding to an L-amino acid analog) binds to HNC. Its peptidyl moiety mimics binding of primed (P1'-P3') residues of the substrate. In combination with our first structure a continuous hexapeptide corresponding to a peptide substrate productively bound to HNC was constructed and energy-minimized. Proteolytic cleavage of this Michaelis complex is probably general base-catalyzed as proposed for thermolysin, i.e. a glutamate assists nucleophilic attack of a water molecule. Although there are many structural and mechanistic similarities to thermolysin, substrate binding to MMPs differs due to the interactions beyond S1'-P1'. While thermolysin binds substrates with a kink at P1', substrates are bound in an extended conformation in the collagenases. This property explains the tolerance of thermolysin for D-amino acid residues at the P1' position, in contrast to the collagenases. The third inhibitor, HONHCOCH(iBu)CO-L-Ala-Gly-NH2, unexpectedly binds in a different manner than anticipated from its design and binding mode in thermolysin. Its hydroxamate group obviously interacts with the catalytic zinc in a favourable bidentate manner, but in contrast its isobutyl (iBu) side chain remains outside of the S1' pocket, presumably due to severe constraints imposed by the adjacent planar hydroxamate group. Instead, the C-terminal Ala-Gly-NH2 tail adopts a bent conformation and inserts into this S1' pocket, presumably in a non-optimized manner. Both the isobutyl side chain and the C-terminal peptide tail could be replaced by other, better fitting groups.(ABSTRACT TRUNCATED AT 250 WORDS)
基质金属蛋白酶(MMPs)是一族参与组织重塑的锌内肽酶。它们也与包括肿瘤侵袭和关节破坏在内的各种疾病过程有关,因此是抑制剂设计的有吸引力的靶点。对于合理的药物设计,抑制剂在原子水平上的结合信息至关重要。最近,我们发表了人中性粒细胞胶原酶(HNC)催化结构域与抑制剂Pro-Leu-Gly-NHOH复合的精制高分辨率晶体结构,该抑制剂是结合肽底物未引发(P3-P1)残基的模拟物。我们现在确定了另外两种与硫醇抑制剂HSCH2CH(CH2Ph)CO-L-Ala-Gly-NH2和另一种异羟肟酸酯抑制剂HONHCOCH(iBu)CO-L-Ala-Gly-NH2形成的HNC复合物,它们在0.240/0.225纳米分辨率下均精制到R值为0.183/0.198。抑制剂硫醇和异羟肟酸酯基团分别与催化锌配位,产生略微扭曲的四面体和三角双锥配位球。在P1'残基处具有S构型(对应于L-氨基酸类似物)的硫醇抑制剂非对映异构体与HNC结合。其肽基部分模拟底物引发(P1'-P3')残基的结合。结合我们的第一个结构,构建并能量最小化了与HNC有效结合的对应于肽底物的连续六肽。这种米氏复合物的蛋白水解裂解可能如嗜热菌蛋白酶那样是一般碱催化的,即谷氨酸协助水分子的亲核攻击。尽管与嗜热菌蛋白酶有许多结构和机制上的相似性,但由于S1'-P1'以外的相互作用,底物与MMPs的结合有所不同。嗜热菌蛋白酶在P1'处结合有扭结的底物,而底物在胶原酶中以伸展构象结合。这一特性解释了嗜热菌蛋白酶对P1'位置D-氨基酸残基的耐受性,这与胶原酶不同。第三种抑制剂HONHCOCH(iBu)CO-L-Ala-Gly-NH2出乎意料地以与其在嗜热菌蛋白酶中的设计和结合模式预期不同的方式结合。其异羟肟酸酯基团显然以有利的双齿方式与催化锌相互作用,但相反,其异丁基(iBu)侧链留在S1'口袋之外,可能是由于相邻平面异羟肟酸酯基团施加的严重限制。相反,C末端的Ala-Gly-NH2尾巴采取弯曲构象并插入这个S1'口袋,可能是以非优化的方式。异丁基侧链和C末端肽尾巴都可以被其他更合适的基团取代。(摘要截断于250字)
