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热稳定膜蛋白在磷脂/去污剂混合胶束中的可逆去折叠。

Reversible unfolding of a thermophilic membrane protein in phospholipid/detergent mixed micelles.

机构信息

Laboratorio de Biofísica Molecular, Instituto de Química y Fisicoquímica Biológicas, Universidad de Buenos Aires-CONICET, Buenos Aires, Argentina.

出版信息

J Mol Biol. 2010 Mar 26;397(2):550-9. doi: 10.1016/j.jmb.2010.01.045. Epub 2010 Jan 28.

DOI:10.1016/j.jmb.2010.01.045
PMID:20114054
Abstract

Folding mechanisms and stability of membrane proteins are poorly understood because of the known difficulties in finding experimental conditions under which reversible denaturation could be possible. In this work, we describe the equilibrium unfolding of Archaeoglobus fulgidus CopA, an 804-residue alpha-helical membrane protein that is involved in transporting Cu(+) throughout biological membranes. The incubation of CopA reconstituted in phospholipid/detergent mixed micelles with high concentrations of guanidinium hydrochloride induced a reversible decrease in fluorescence quantum yield, far-UV ellipticity, and loss of ATPase and phosphatase activities. Refolding of CopA from this unfolded state led to recovery of full biological activity and all the structural features of the native enzyme. CopA unfolding showed typical characteristics of a two-state process, with DeltaG(w) degrees =12.9 kJ mol(-)(1), m=4.1 kJ mol(-1) M(-1), C(m)=3 M, and DeltaCp(w) degrees =0.93 kJ mol(-1) K(-1). These results point out to a fine-tuning mechanism for improving protein stability. Circular dichroism spectroscopic analysis of the unfolded state shows that most of the secondary and tertiary structures were disrupted. The fraction of Trp fluorescence accessible to soluble quenchers shifted from 0.52 in the native state to 0.96 in the unfolded state, with a significant spectral redshift. Also, hydrophobic patches in CopA, mainly located in the transmembrane region, were disrupted as indicated by 1-anilino-naphtalene-8-sulfonate fluorescence. Nevertheless, the unfolded state had a small but detectable amount of residual structure, which might play a key role in both CopA folding and adaptation for working at high temperatures.

摘要

膜蛋白的折叠机制和稳定性理解甚少,因为已知在寻找可能的条件下,膜蛋白的可逆变性是很困难的。在这项工作中,我们描述了产甲烷八叠球菌 CopA 的平衡变性,CopA 是一种 804 个残基的α螺旋膜蛋白,参与通过生物膜转运 Cu(+)。在磷脂/去污剂混合胶束中再组装的 CopA 用高浓度盐酸胍孵育,可诱导荧光量子产率、远紫外椭圆度以及 ATPase 和磷酸酶活性的可逆下降。从这种变性状态中重新折叠 CopA 导致恢复了完全的生物学活性和天然酶的所有结构特征。CopA 的变性显示出典型的两态过程特征,DeltaG(w) degrees =12.9 kJ mol(-)(1),m=4.1 kJ mol(-1) M(-1),C(m)=3 M,DeltaCp(w) degrees =0.93 kJ mol(-1) K(-1)。这些结果表明存在一种微调机制来提高蛋白质稳定性。变性状态的圆二色性光谱分析表明,大部分二级和三级结构被破坏。可与可溶性猝灭剂接触的色氨酸荧光的分数从天然状态的 0.52 转移到变性状态的 0.96,并且光谱明显红移。此外,CopA 中的疏水区,主要位于跨膜区,如 1-苯胺基-8-萘磺酸荧光所示,被破坏。然而,变性状态具有少量但可检测到的残留结构,这可能在 CopA 折叠和适应高温工作中都发挥关键作用。

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