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利用紫外共振拉曼光谱研究蛋白质中的酪氨酸氢键和环境效应。

Tyrosine hydrogen-bonding and environmental effects in proteins probed by ultraviolet resonance Raman spectroscopy.

作者信息

Hildebrandt P G, Copeland R A, Spiro T G, Otlewski J, Laskowski M, Prendergast F G

机构信息

Department of Chemistry, Princeton University, New Jersey 08544.

出版信息

Biochemistry. 1988 Jul 26;27(15):5426-33. doi: 10.1021/bi00415a007.

DOI:10.1021/bi00415a007
PMID:3179264
Abstract

Ultraviolet resonance Raman spectra with 229-nm excitation are reported for aqueous tyrosine and for ovomucoid third domain proteins from chicken [OMCHI3(-)] and from chachalaca [OMCHA(-)], as well as alpha 1-, alpha 2-, and beta-purothionin. At this excitation wavelength interference from phenylalanine is minimized, and it is possible to determine the frequencies of the Tyr ring modes nu 8a and nu 8b. The nu 8b frequency decreases with the degree of Tyr H-bond donation, reaching a limiting value for deprotonated tyrosine. This spectroscopic indicator of H-bond strength was calibrated by using the model compound p-cresol in H-bond acceptor solutions for which the enthalpy of H-bond formation can be obtained from the literature. With this calibration it is possible to estimate Tyr H-bond enthalpies in proteins for which Tyr is a H-bond donor; values of 13.7, 9.6, and 11.2 kcal/mol were found for OMCHA3(-) and for alpha 1- (or alpha 2-) and beta-purothionin, respectively. The intensity of the 1176-cm-1 nu 9a band of Tyr excited at 229 nm and also the intensity ratio of the Tyr 830/850-cm-1 Fermi doublet excited at 200 nm both correlate strongly with the estimated H-bond enthalpies, but large deviations are seen for the purothionins, reflecting a special environment for the Tyr residue of these proteins, which is believed to be constrained in a hydrophobic pocket. The molar intensity of the strong approximately 1000-cm-1 nu 12 band of phenylalanine in aqueous solution is about half the value observed in most proteins.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

本文报道了在229nm激发波长下,酪氨酸水溶液、来自鸡的卵类粘蛋白第三结构域蛋白[OMCHI3(-)]和来自冠雉的该结构域蛋白[OMCHA(-)]以及α1-、α2-和β-硫堇蛋白的紫外共振拉曼光谱。在此激发波长下,苯丙氨酸的干扰最小化,从而能够确定酪氨酸环模式ν8a和ν8b的频率。ν8b频率随酪氨酸氢键供体程度降低,对于去质子化酪氨酸达到极限值。通过在氢键受体溶液中使用模型化合物对甲酚校准该氢键强度的光谱指标,其氢键形成焓可从文献中获取。通过此校准,可以估计酪氨酸作为氢键供体的蛋白质中的酪氨酸氢键焓;OMCHA3(-)以及α1-(或α2-)和β-硫堇蛋白的该值分别为13.7、9.6和11.2 kcal/mol。在229nm激发的酪氨酸1176cm-1的ν9a带强度以及在200nm激发的酪氨酸830/850cm-1费米双峰强度比均与估计的氢键焓密切相关,但硫堇蛋白存在较大偏差,反映出这些蛋白质中酪氨酸残基处于特殊环境,据信其被限制在疏水口袋中。水溶液中苯丙氨酸约1000cm-1的强ν12带的摩尔强度约为大多数蛋白质中观察值的一半。(摘要截短于250字)

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