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首页> 外文期刊>Journal of pharmaceutical sciences. >Steady-state tryptophan fluorescence spectroscopy study to probe tertiary structure of proteins in solid powders.
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Steady-state tryptophan fluorescence spectroscopy study to probe tertiary structure of proteins in solid powders.

机译:稳态色氨酸荧光光谱研究可探测固体粉末中蛋白质的三级结构。

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The purpose of this work was to obtain information about protein tertiary structure in solid state by using steady state tryptophan (Trp) fluorescence emission spectroscopy on protein powders. Beta-lactoglobulin (betaLg) and interferon alpha-2a (IFN) powder samples were studied by fluorescence spectroscopy using a front surface sample holder. Two different sets of dried betaLg samples were prepared by vacuum drying of solutions: one containing betaLg, and the other containing a mixture of betaLg and guanidine hydrochloride. Dried IFN samples were prepared by vacuum drying of IFN solutions and by vacuum drying of polyethylene glycol precipitated IFN. The results obtained from solid samples were compared with the emission scans of these proteins in solutions. The emission scans obtained from protein powders were slightly blue-shifted compared to the solution spectra due to the absence of water. The emission scans were red-shifted for betaLg samples dried from solutions containing GuHCl. The magnitude of the shifts in lambda(max) depended on the extent of drying of the samples, which was attributed to the crystallization of GuHCl during the drying process. The shifts in the lambda(max) of the Trp emission spectrum are associated with the changes in the tertiary structure of betaLg. In the case of IFN, the emission scans obtained from PEG-precipitated and dried sample were different compared to the emission scans obtained from IFN in solution and from vacuum dried IFN. The double peaks observed in this sample were attributed to the unfolding of the protein. In the presence of trehalose, the two peaks converged to form a single peak, which was similar to solution emission spectra, whereas no change was observed in the presence of mannitol. We conclude that Trp fluorescence spectroscopy provides a simple and reliable means to characterize Trp microenvironment in protein powders that is related to the tertiary conformation of proteins in the solid state. This study shows that the use of fluorescence spectroscopy of proteins can be extended from simple protein aqueous solutions to protein powders, precipitates, and semidried protein samples to gain understanding of protein tertiary structure in these physical states.
机译:这项工作的目的是通过对蛋白质粉末使用稳态色氨酸(Trp)荧光发射光谱法获得有关固态蛋白质三级结构的信息。使用前表面样品架通过荧光光谱法研究了β-乳球蛋白(betaLg)和干扰素α-2a(IFN)粉末样品。通过真空干燥溶液来制备两组不同的干燥betaLg样品:一组包含betaLg,另一组包含betaLg和盐酸胍的混合物。通过真空干燥IFN溶液和真空干燥聚乙二醇沉淀的IFN来制备干燥的IFN样品。从固体样品获得的结果与溶液中这些蛋白质的发射扫描进行了比较。由于没有水,与溶液光谱相比,从蛋白质粉末获得的发射扫描略微蓝移。对于从含有GuHCl的溶液中干燥的betaLg样品,发射扫描发生红移。 lambda(max)的变化幅度取决于样品的干燥程度,这归因于干燥过程中GuHCl的结晶。 Trp发射光谱的λ(max)的变化与betaLg的三级结构的变化相关。在IFN的情况下,从PEG沉淀和干燥的样品获得的发射扫描与从溶液中的IFN和真空干燥的IFN获得的发射扫描不同。在该样品中观察到的双峰归因于蛋白质的展开。在海藻糖存在下,两个峰会聚形成一个峰,与溶液发射光谱相似,而在甘露糖醇存在下未观察到变化。我们得出结论,Trp荧光光谱法提供了一种简单而可靠的方法来表征蛋白质粉末中的Trp微环境,该环境与固态蛋白质的第三级构象有关。这项研究表明,蛋白质荧光光谱的使用可以从简单的蛋白质水溶液扩展到蛋白质粉末,沉淀物和半干蛋白质样品,以了解这些物理状态下的蛋白质三级结构。

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