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溶菌酶和α-乳白蛋白中瞬时折叠中间体的比较。

Comparison of the transient folding intermediates in lysozyme and alpha-lactalbumin.

作者信息

Kuwajima K, Hiraoka Y, Ikeguchi M, Sugai S

出版信息

Biochemistry. 1985 Feb 12;24(4):874-81. doi: 10.1021/bi00325a010.

DOI:10.1021/bi00325a010
PMID:3994996
Abstract

Refolding kinetics of two homologous proteins, lysozyme and alpha-lactalbumin, were studied by following the time-dependent changes in the circular dichroism spectra in the aromatic and the peptide regions. The refolding was initiated by 20-fold dilution of the protein solutions originally unfolded at 6 M guanidine hydrochloride, at pH 1.5 for lysozyme and pH 7.0 for alpha-lactalbumin at 4.5 degrees C. In the aromatic region, almost full changes in ellipticity that were expected from the equilibrium differences in the spectra between the native and unfolded proteins were observed kinetically. The major fast phase of lysozyme folding has a decay time of 15 s. The decay time of alpha-lactalbumin depends on the presence or absence of bound Ca2+: 10 s for the holoprotein and 100 s for the apoprotein. In the peptide region, however, most of the ellipticity changes of the two proteins occur within the dead time (less than 3 s) of the present measurements. This demonstrates existence of an early folding intermediate which is still unfolded when measured by the aromatic bands but has folded secondary structure as measured by the peptide bands. Extrapolation of the ellipticity changes to zero time at various wavelengths gives a spectrum of the folding intermediate. Curve fitting of the peptide spectra to estimate the secondary structure fractions has shown that the two proteins assume a similar structure at an early stage of folding and that the intermediate has a structure similar to that of partially unfolded species produced by heat and, for alpha-lactalbumin, also by acid and a moderate concentration of guanidine hydrochloride.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过跟踪芳香族区域和肽区域圆二色光谱随时间的变化,研究了两种同源蛋白质——溶菌酶和α-乳白蛋白的重折叠动力学。重折叠通过将最初在6M盐酸胍中展开的蛋白质溶液进行20倍稀释来启动,溶菌酶在pH 1.5、4.5℃条件下展开,α-乳白蛋白在pH 7.0、4.5℃条件下展开。在芳香族区域,动力学上观察到了从天然态和未折叠态蛋白质光谱的平衡差异预期的椭圆率几乎完全变化。溶菌酶折叠的主要快速阶段的衰减时间为15秒。α-乳白蛋白的衰减时间取决于是否存在结合的Ca2+:全蛋白为10秒,脱辅基蛋白为100秒。然而,在肽区域,两种蛋白质的大部分椭圆率变化发生在本测量的死时间(小于3秒)内。这表明存在一种早期折叠中间体,用芳香族谱带测量时它仍未折叠,但用肽谱带测量时具有折叠的二级结构。将不同波长下的椭圆率变化外推到零时间得到折叠中间体的光谱。对肽谱进行曲线拟合以估计二级结构分数表明,两种蛋白质在折叠早期呈现相似结构,并且该中间体具有与热产生的部分未折叠物种相似的结构,对于α-乳白蛋白,酸和中等浓度盐酸胍产生的部分未折叠物种也具有相似结构。(摘要截断于250字)

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