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通过紧密过渡态实现的微秒级蛋白质折叠。

Microsecond protein folding through a compact transition state.

作者信息

Burton R E, Huang G S, Daugherty M A, Fullbright P W, Oas T G

机构信息

Department of Biochemistry, Duke University Medical Center, Durham, NC 27710, USA.

出版信息

J Mol Biol. 1996 Oct 25;263(2):311-22. doi: 10.1006/jmbi.1996.0577.

Abstract

Dynamic NMR methods have been employed to measure the folding and unfolding rate constants of two extremely fast-folding proteins. lambda 6-85, a truncated, monomeric form of the N-terminal domain of lambda repressor, refolds with a lifetime of approximately 250 microseconds. These methods have also been applied to a thermostable lambda 6-85 variant with alanine substituted for glycine residues 46 and 48 in the third helix (G46A/G48A). Both proteins exhibit linear ln (kf,u) versus [urea] plots, consistent with two-state folding for both proteins. When extrapolated to 0M urea, the data indicate that G46A/G48A folds with a lifetime of less than 20 microseconds. The slopes of the ln (kf,u) versus [urea] curves (mu and mf) indicate that the modest Gly-->Ala double mutation dramatically changes the transition state solvent accessibility. The transition state for lambda 6-85 has a fractional accessibility (mu/(mu-mf)) of 0.61, whereas the transition state for G46A/G48A is much more native-like, with a fractional accessibility of 0.16. The extraordinary change in the folding pathway that these mutations induce suggests that the intrinsic stability of helix 3 is an important determinant of the folding mechanism.

摘要

动态核磁共振方法已被用于测量两种折叠速度极快的蛋白质的折叠和去折叠速率常数。λ6 - 85是λ阻遏蛋白N端结构域的截短单体形式,其重新折叠的寿命约为250微秒。这些方法也已应用于一种热稳定的λ6 - 85变体,该变体在第三螺旋中的甘氨酸残基46和48被丙氨酸取代(G46A/G48A)。两种蛋白质均呈现ln(kf,u)对[尿素]的线性图谱,这与两种蛋白质的两态折叠一致。外推至0M尿素时,数据表明G46A/G48A的折叠寿命小于20微秒。ln(kf,u)对[尿素]曲线的斜率(μ和mf)表明,适度的甘氨酸→丙氨酸双突变显著改变了过渡态的溶剂可及性。λ6 - 85的过渡态的分数可及性(μ/(μ - mf))为0.61,而G46A/G48A的过渡态更类似天然态,分数可及性为0.16。这些突变所诱导的折叠途径的显著变化表明,螺旋3的内在稳定性是折叠机制的一个重要决定因素。

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