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How Aggregation and Conformational Scrambling of Unfolded States Govern Fluorescence Emission Spectra

机译:展开状态的聚集和构象加扰如何控制荧光发射光谱。

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摘要

In a case study on five homologous α-amylases we analyzed the properties of unfolded states as obtained from treatments with GndHCl and with elevated temperatures. In particular the wavelength of the tryptophan fluorescence emission peak (λmax) is a valuable parameter to characterize properties of the unfolded state. In all cases with a typical red shift of the emission spectrum occurring during structural unfolding we observed a larger magnitude of this shift for GndHCl-induced unfolding as compared to thermal unfolding. Although a quantitative relation between aggregation and reduction of the unfolding induced red shifts cannot be given, our data indicate that protein aggregation contributes significantly to smaller magnitudes of red shifts as observed during thermal unfolding. In addition, other properties of the unfolded states, most probable structural compactness or simply differences in the conformational scrambling, also affect the magnitude of red shifts. For the irreversible unfolding α-amylases studied here, transition temperatures and magnitudes of red shifts are strongly depending on heating rates. Lower protein concentrations and smaller heating rates lead to larger red shifts upon thermal unfolding, indicating that under these conditions the protein aggregation is less pronounced.
机译:在对五种同源α-淀粉酶的案例研究中,我们分析了用GndHCl和高温处理获得的未折叠状态的特性。特别地,色氨酸荧光发射峰的波长(λmax)是表征未折叠状态的特性的有价值的参数。在所有情况下,在结构展开期间发生发射光谱的典型红移,与热展开相比,我们观察到GndHCl诱导的展开具有较大的这种移位幅度。尽管无法给出聚集与未折叠引起的红移减少之间的定量关系,但我们的数据表明,蛋白质聚集显着有助于较小程度的红移,如在热展开过程中观察到的。此外,展开状态的其他属性,最可能的结构紧凑性或构象加扰中的简单差异也影响红移的大小。对于此处研究的不可逆的α-淀粉酶,转变温度和红移的幅度强烈取决于加热速率。较低的蛋白质浓度和较小的加热速率会导致热解折叠时出现较大的红移,表明在这些条件下蛋白质的聚集不太明显。

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