Noel Amanda F, Bilsel Osman, Kundu Agnita, Wu Ying, Zitzewitz Jill A, Matthews C Robert
Department of Biochemistry and Molecular Pharmacology, University of Massachusetts Medical School, Worcester, MA 01605, USA.
J Mol Biol. 2009 Apr 10;387(4):1002-16. doi: 10.1016/j.jmb.2008.12.061. Epub 2009 Jan 6.
Spontaneous mutations at numerous sites distant from the active site of human immunodeficiency virus type 1 protease enable resistance to inhibitors while retaining enzymatic activity. As a benchmark for probing the effects of these mutations on the conformational adaptability of this dimeric beta-barrel protein, the folding free-energy surface of a pseudo-wild-type variant, HIV-PR(*), was determined by a combination of equilibrium and kinetic experiments on the urea-induced unfolding/refolding reactions. The equilibrium unfolding reaction was well described by a two-state model involving only the native dimeric form and the unfolded monomer. The global analysis of the kinetic folding mechanism reveals the presence of a fully folded monomeric intermediate that associates to form the native dimeric structure. Independent analysis of a stable monomeric version of the protease demonstrated that a small-amplitude fluorescence phase in refolding and unfolding, not included in the global analysis of the dimeric protein, reflects the presence of a transient intermediate in the monomer folding reaction. The partially folded and fully folded monomers are only marginally stable with respect to the unfolded state, and the dimerization reaction provides a modest driving force at micromolar concentrations of protein. The thermodynamic properties of this system are such that mutations can readily shift the equilibrium from the dimeric native state towards weakly folded states that have a lower affinity for inhibitors but that could be induced to bind to their target proteolytic sites. Presumably, subsequent secondary mutations increase the stability of the native dimeric state in these variants and, thereby, optimize the catalytic properties of the resistant human immunodeficiency virus type 1 protease.
人类免疫缺陷病毒1型蛋白酶活性位点以外众多位点的自发突变可使其在保留酶活性的同时对抑制剂产生抗性。作为探究这些突变对这种二聚体β桶状蛋白构象适应性影响的基准,通过对尿素诱导的去折叠/再折叠反应进行平衡和动力学实验相结合的方法,确定了伪野生型变体HIV-PR(*)的折叠自由能表面。平衡去折叠反应可用仅涉及天然二聚体形式和去折叠单体的两态模型很好地描述。对动力学折叠机制的全局分析揭示了存在一个完全折叠的单体中间体,该中间体缔合形成天然二聚体结构。对蛋白酶稳定单体形式的独立分析表明,在二聚体蛋白的全局分析中未包括的再折叠和去折叠过程中的一个小幅度荧光相,反映了单体折叠反应中存在一个瞬时中间体。部分折叠和完全折叠的单体相对于去折叠状态仅略微稳定,并且在微摩尔浓度的蛋白质下,二聚化反应提供适度的驱动力。该系统的热力学性质使得突变能够轻易地将平衡从二聚体天然状态转移到对抑制剂亲和力较低但可被诱导结合其靶蛋白水解位点的弱折叠状态。据推测,随后的二级突变增加了这些变体中天然二聚体状态的稳定性,从而优化了抗性人类免疫缺陷病毒1型蛋白酶的催化特性。