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本文引用的文献

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Molecular dynamics of an alpha-helical polypeptide: Temperature dependence and deviation from harmonic behavior.α-螺旋多肽的分子动力学:温度依赖性和非简谐行为。
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10
Internal dynamics and overall motion of lysozyme studied by fluorescence depolarization of the eosin lysozyme complex.
J Biomol Struct Dyn. 1983 Oct;1(1):299-318. doi: 10.1080/07391102.1983.10507441.

抑制剂结合对溶菌酶内部运动的影响。

Influence of inhibitor binding on the internal motions of lysozyme.

作者信息

Cross A J, Fleming G R

出版信息

Biophys J. 1986 Sep;50(3):507-12. doi: 10.1016/S0006-3495(86)83488-9.

DOI:10.1016/S0006-3495(86)83488-9
PMID:3756301
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1329727/
Abstract

Time-resolved laser-induced fluorescence depolarization measurements of internal motions in lysozyme are presented. The fluorescent dye eosin binds in a one-to-one complex with the enzyme, and is used both to measure the overall tumbling time constants and to probe the motions of residues in the region of binding. The precision and accuracy of the present method for determining the overall tumbling time constants compare favorably with those from other methods used in the literature. The extent of the internal motions, as described by a model independent order parameter, S2, is temperature dependent, and changes when the inhibitor N,N',N"-triacetylchitotriose, (GlcNAc)3, is bound to the active site of the enzyme. The observed temperature dependence and changes in S2 upon binding of (GlcNAc)3 are interpreted in terms of a nonharmonic model of the effective potential that is consistent with the picture of concerted motions in the protein. The values of the parameters of the potential that reproduce the data with and without the bound inhibitor imply that (GlcNAc)3 binding causes an increase in the rigidity of the protein, which agree qualitatively with other results on the lysozyme-(GlcNAc)3 system.

摘要

本文介绍了溶菌酶内部运动的时间分辨激光诱导荧光去极化测量。荧光染料曙红与该酶以一对一的复合物形式结合,用于测量整体翻滚时间常数以及探测结合区域内残基的运动。本方法测定整体翻滚时间常数的精度和准确性与文献中使用的其他方法相比具有优势。由与模型无关的序参数S2描述的内部运动程度与温度有关,并且当抑制剂N,N',N"-三乙酰壳三糖(GlcNAc)3与酶的活性位点结合时会发生变化。根据与蛋白质中协同运动图景一致的有效势的非谐模型,解释了观察到的温度依赖性以及(GlcNAc)3结合后S2的变化。再现有无结合抑制剂数据的势参数值表明,(GlcNAc)3结合导致蛋白质刚性增加,这与溶菌酶-(GlcNAc)3系统的其他结果在定性上是一致的。