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使用θ玻璃发射器在快速混合后研究电喷雾纳米液滴中的蛋白质折叠与去折叠。

Investigating protein folding and unfolding in electrospray nanodrops upon rapid mixing using theta-glass emitters.

作者信息

Mortensen Daniel N, Williams Evan R

机构信息

Department of Chemistry, University of California , Berkeley, California 94720-1460, United States.

出版信息

Anal Chem. 2015 Jan 20;87(2):1281-7. doi: 10.1021/ac503981c. Epub 2014 Dec 31.

Abstract

Theta-glass emitters are used to rapidly mix two solutions to induce either protein folding or unfolding during nanoelectrospray (nanoESI). Mixing acid-denatured myoglobin with an aqueous ammonium acetate solution to increase solution pH results in protein folding during nanoESI. A reaction time and upper limit to the droplet lifetime of 9 ± 2 μs is obtained from the relative abundance of the folded conformer in these rapid mixing experiments compared to that obtained from solutions at equilibrium and a folding time constant of 7 μs. Heme reincorporation does not occur, consistent with the short droplet lifetime and the much longer time constant for this process. Similar mixing experiments with acid-denatured cytochrome c and the resulting folding during nanoESI indicate a reaction time of between 7 and 25 μs depending on the solution composition. The extent of unfolding of holo-myoglobin upon rapid mixing with theta-glass emitters is less than that reported previously ( Fisher et al. Anal. Chem. 2014 , 86 , 4581 - 4588 ), a result that is attributed to the much smaller, ∼1.5 μm, average o.d. tips used here. These results indicate that the time frame during which protein folding or unfolding can occur during nanoESI depends both on the initial droplet size, which can be varied by changing the emitter tip diameter, and on the solution composition. This study demonstrates that protein folding or unfolding processes that occur on the ∼10 μs time scale can be readily investigated using rapid mixing with theta-glass emitters combined with mass spectrometry.

摘要

θ型玻璃发射器用于在纳米电喷雾(nanoESI)过程中快速混合两种溶液,以诱导蛋白质折叠或展开。将酸变性的肌红蛋白与醋酸铵水溶液混合以提高溶液pH值,会导致在纳米电喷雾过程中蛋白质折叠。通过这些快速混合实验中折叠构象异构体的相对丰度与平衡溶液中获得的相对丰度相比,得到反应时间和液滴寿命上限为9±2μs,折叠时间常数为7μs。血红素重新掺入未发生,这与短的液滴寿命和该过程长得多的时间常数一致。用酸变性的细胞色素c进行类似的混合实验以及在纳米电喷雾过程中产生的折叠表明,根据溶液组成,反应时间在7到25μs之间。与θ型玻璃发射器快速混合时,全肌红蛋白的展开程度小于先前报道的程度(Fisher等人,《分析化学》,2014年,86卷,4581 - 4588页),这一结果归因于此处使用的平均外径小得多,约为1.5μm的尖端。这些结果表明,在纳米电喷雾过程中蛋白质折叠或展开能够发生的时间框架既取决于初始液滴大小(可通过改变发射器尖端直径来改变),也取决于溶液组成。这项研究表明,使用与θ型玻璃发射器快速混合并结合质谱法,可以很容易地研究在约10μs时间尺度上发生的蛋白质折叠或展开过程。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/502a/4303338/dea722e713cd/ac-2014-03981c_0006.jpg

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