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螺旋帽在蛋白质折叠中的动力学作用取决于具体环境。

Kinetic role of helix caps in protein folding is context-dependent.

作者信息

Kapp Gregory T, Richardson Jane S, Oas Terrence G

机构信息

Department of Biochemistry, Box 3711, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

Biochemistry. 2004 Apr 6;43(13):3814-23. doi: 10.1021/bi035683k.

DOI:10.1021/bi035683k
PMID:15049688
Abstract

Secondary structure punctuation through specific backbone and side chain interactions at the beginning and end of alpha-helices has been proposed to play a key role in hierarchical protein folding mechanisms [Baldwin, R. L., and Rose, G. D. (1999) Trends Biochem. Sci. 24, 26-33; Presta, L. G., and Rose, G. D. (1988) Science 240, 1632-1641]. We have made site-specific substitutions in the N- and C-cap motifs of the 5-helix protein monomeric lambda repressor (lambda(6-85)) and have measured the rate constants for folding and unfolding of each variant. The consequences of C-cap changes are strongly context-dependent. When the C-cap was located at the chain terminus, changes had little energetic and no kinetic effect. However, substitutions in a C-cap at the boundary between helix 4 and the subsequent interhelical loop resulted in large changes to the stability and rate constants of the variant, showing a substantial kinetic role for this interior C-cap and suggesting a general kinetic role for interior helix C-caps. Statistical preferences tabulated separately for internal and terminal C-caps also show only weak residue preferences in terminal C-caps. This kinetic distinction between interior and terminal C-caps can explain the discrepancy between the near-absence of stability and kinetic effects seen for C-caps of isolated peptides versus the very strong C-cap effects seen for proteins in statistical sequence preferences and mutational energetics. Introduction of consensus, in-register N-capping motifs resulted in increased stability, accelerated folding, and slower unfolding. The kinetic measurements indicate that some of the new native-state capping interactions remain unformed in the transition state. The accelerated folding rates could result from helix stabilization without invoking a specific role for N-caps in the folding reaction.

摘要

通过α-螺旋起始和末端特定的主链和侧链相互作用进行二级结构标点,被认为在蛋白质分级折叠机制中起关键作用[鲍德温,R. L.,和罗斯,G. D.(1999年)《生物化学趋势》24卷,26 - 33页;普雷斯塔,L. G.,和罗斯,G. D.(1988年)《科学》240卷,1632 - 1641页]。我们在5 - 螺旋蛋白单体λ阻遏物(λ(6 - 85))的N - 帽和C - 帽基序中进行了位点特异性取代,并测量了每个变体折叠和去折叠的速率常数。C - 帽变化的结果强烈依赖于上下文。当C - 帽位于链末端时,变化几乎没有能量效应,也没有动力学效应。然而,在螺旋4与随后的螺旋间环之间的边界处的C - 帽进行取代,导致变体的稳定性和速率常数发生很大变化,表明这个内部C - 帽具有重要的动力学作用,并暗示内部螺旋C - 帽具有普遍的动力学作用。分别列出的内部和末端C - 帽的统计偏好也表明末端C - 帽中只有较弱的残基偏好。内部和末端C - 帽之间的这种动力学差异可以解释在分离肽的C - 帽几乎没有稳定性和动力学效应与在统计序列偏好和突变能量学中蛋白质中非常强的C - 帽效应之间的差异。引入共有、对齐的N - 帽基序导致稳定性增加、折叠加速和去折叠减慢。动力学测量表明,一些新的天然态封端相互作用在过渡态中仍未形成。折叠速率的加速可能是由于螺旋稳定,而无需调用N - 帽在折叠反应中的特定作用。

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