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首页> 外文期刊>Biochimica et biophysica acta: BBA: International journal of biochemistry, biophysics and molecular biololgy. Proteins and Proteomics >Unfolding and refolding of porcine odorant binding protein in guanidinium hydrochloride: equilibrium studies at neutral pH
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Unfolding and refolding of porcine odorant binding protein in guanidinium hydrochloride: equilibrium studies at neutral pH

机译:盐酸胍中猪气味结合蛋白的折叠和重折叠:中性pH下的平衡研究

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摘要

Unfolding and refolding studies on porcine odorant binding protein (pOBP) have been performed at pH 7 in the presence of guanidinium hydrochloride (GdnHCl). Unfolding, monitored by following changes of protein fluorescence and circular dichroism (CD), was found to be a reversible process, in terms of recovered structure and function. The equilibrium transition data were fitted by a simple two-state sigmoidal function of denaturant concentration and the thermodynamic folding parameters, derived from the two techniques, were very similar (average values: C_(1/2) ≈ 2.4 M, m ≈ 2 kcal mol~(-1)M~(-1), ΔG_(unf, w)~0 ≈ 4.7 kcal mol~(-1)). The transition was independent of protein concentration, indicating that only monomeric species are involved. Only a minor protective effect by the fluorescent ligand 1-amino-anthracene (AMA) against protein unfolding was detected, whereas dihydromyrcenol (DHM) stabilised the protein to a larger extent (ΔC_(1/2) ≈ 0.5 M). Refolding was complete, when the protein, denatured with GdnHCl, was diluted with buffer. On the other hand, refolding by dialysis was largely prevented by concomitant aggregation. The present results on pOBP are compared with those on bovine OBP (bOBP)[Biochim. Biophys. Acta 1599 (2002)90], where subunit folding is accompanied by domain swapping. We finally suggest that the generally observed two-state folding of many lipocalins is probably favoured by their β-barrel topology.
机译:在盐酸胍(GdnHCl)存在下,在pH 7下进行了猪气味结合蛋白(pOBP)的展开和重折叠研究。通过恢复蛋白质的结构和功能,通过跟踪蛋白质荧光和圆二色性(CD)的变化来监测其展开是可逆的过程。平衡转变数据通过变性剂浓度的简单二态S形函数拟合,并且从这两种技术得出的热力学折叠参数非常相似(平均值:C_(1/2)≈2.4 M,m≈2 kcal mol〜(-1)M〜(-1),ΔG_(unf,w)〜0≈4.7 kcal mol〜(-1))。过渡与蛋白质浓度无关,表明仅涉及单体种类。仅检测到荧光配体1-氨基蒽(AMA)对蛋白质展开的较小保护作用,而二氢月桂烯醇(DHM)则在更大程度上稳定了蛋白质(ΔC_(1/2)≈0.5 M)。当用GdnHCl变性的蛋白质用缓冲液稀释时,重折叠完成。另一方面,伴随的聚集在很大程度上阻止了透析的复性。将目前在pOBP上的结果与在牛OBP(bOBP)上的结果进行比较[Biochim。生物物理学。 Acta 1599(2002)90],其中亚单位折叠伴随着域交换。我们最后建议,通常观察到的许多脂环蛋白的两态折叠可能受到其β桶形拓扑结构的支持。

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