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Direct observation of protein unfolded state compaction in the presence of macromolecular crowding

机译:在大分子拥挤的情况下直接观察蛋白质的未折叠状态压缩

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Proteins fold and function in cellular environments that are crowded with other macromolecules. As a consequence of excluded volume effects, compact folded states of proteins should be indirectly stabilized due to destabilization of extended unfolded conformations. Here, we assess the role of excluded volume in terms of protein stability, structural dimensions and folding dynamics using a sugar-based crowding agent, dextran 20, and the small ribosomal protein S16 as a model system. To specifically address dimensions, we labeled the protein with BODIPY at two positions and measured Trp-BODIPY distances under different conditions. As expected, we found that dextran 20 (200 mg/ml) stabilized the variants against urea-induced unfolding. At conditions where the protein is unfolded, F?rster resonance energy transfer measurements reveal that in the presence of dextran, the unfolded ensemble is more compact and there is residual structure left as probed by far-ultraviolet circular dichroism. In the presence of a crowding agent, folding rates are faster in the two-state regime, and at low denaturant concentrations, a kinetic intermediate is favored. Our study provides direct evidence for protein unfolded-state compaction in the presence of macromolecular crowding along with its energetic and kinetic consequences.
机译:蛋白质在与其他大分子拥挤的细胞环境中折叠并起作用。由于排除了体积效应,由于扩展的未折叠构象的不稳定,蛋白质的紧密折叠状态应间接稳定。在这里,我们使用糖基拥挤剂,葡聚糖20和小核糖体蛋白S16作为模型系统,评估了排除体积在蛋白质稳定性,结构尺寸和折叠动力学方面的作用。为了具体解决尺寸问题,我们在两个位置用BODIPY标记了蛋白质,并在不同条件下测量了Trp-BODIPY距离。正如预期的那样,我们发现右旋糖酐20(200 mg / ml)稳定了变体以抵抗尿素诱导的解折叠。在蛋白质解折叠的条件下,F ster共振能量转移测量表明,在葡聚糖的存在下,未折叠的集合更致密,并且残留的结构被远紫外圆二色性探测到。在拥挤剂的存在下,在两种状态下的折叠速率更快,并且在低变性剂浓度下,有利于动力学中间体。我们的研究为存在大分子拥挤以及其能量和动力学后果的蛋白质未折叠状态的压缩提供了直接证据。

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