Corrales F J, Fersht A R
Medical Research Council Unit for Protein Function and Design, University of Cambridge, United Kingdom.
Proc Natl Acad Sci U S A. 1995 Jun 6;92(12):5326-30. doi: 10.1073/pnas.92.12.5326.
We have analyzed the pathway of folding of barnase bound to GroEL to resolve the controversy of whether proteins can fold while bound to chaperonins (GroEL or Cpn60) or fold only after their release into solution. Four phases in the folding were detected by rapid-reaction kinetic measurements of the intrinsic fluorescence of both wild type and barnase mutants. The phases were assigned from their rate laws, sensitivity to mutations, and correspondence to regain of catalytic activity. At high ratios of denatured barnase to GroEL, 4 mol of barnase rapidly bind per 14-mer of GroEL. At high ratios of GroEL to barnase, 1 mol of barnase binds with a rate constant of 3.5 x 10(7) s-1.M-1. This molecule then refolds with a low rate constant that changes on mutation in parallel with the rate constant for the folding in solution. This rate constant corresponds to the regain of the overall catalytic activity of barnase and increases 15-fold on the addition of ATP to a physiologically relevant value of approximately 0.4 s-1. The multiply bound molecules of barnase that are present at high ratios of GroEL to barnase fold with a rate constant that is also sensitive to mutation but is 10 times higher. If the 110-residue barnase can fold when bound to GroEL and many moles can bind simultaneously, then smaller parts of large proteins should be able to fold while bound.
我们分析了与GroEL结合的巴纳酶的折叠途径,以解决蛋白质在与伴侣蛋白(GroEL或Cpn60)结合时是否能折叠,还是仅在释放到溶液中后才能折叠这一争议。通过对野生型和巴纳酶突变体的内在荧光进行快速反应动力学测量,检测到折叠过程中的四个阶段。这些阶段根据其速率定律、对突变的敏感性以及与催化活性恢复的对应关系来确定。在变性巴纳酶与GroEL的比例较高时,每14聚体的GroEL能快速结合4摩尔的巴纳酶。在GroEL与巴纳酶的比例较高时,1摩尔的巴纳酶以3.5×10⁷ s⁻¹·M⁻¹的速率常数结合。然后该分子以较低的速率常数重新折叠,该常数在突变时会发生变化,且与在溶液中折叠的速率常数平行变化。这个速率常数对应于巴纳酶整体催化活性的恢复,在添加ATP至生理相关值约0.4 s⁻¹时增加15倍。在GroEL与巴纳酶比例较高时存在的多个结合的巴纳酶分子以一个对突变也敏感但高10倍的速率常数折叠。如果110个残基的巴纳酶在与GroEL结合时能折叠且许多摩尔能同时结合,那么大蛋白质的较小部分在结合时应该也能折叠。
