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荧光蛋白 rsCherryRev1.4 中一种不寻常的二硫键连接的二聚化。

An unusual disulfide-linked dimerization in the fluorescent protein rsCherryRev1.4.

机构信息

Biochemistry, Molecular and Structural Biology, Department of Chemistry, KU Leuven, 3001 Leuven, Belgium.

出版信息

Acta Crystallogr F Struct Biol Commun. 2023 Feb 1;79(Pt 2):38-44. doi: 10.1107/S2053230X23000572. Epub 2023 Feb 2.

Abstract

rsCherryRev1.4 has been reported as one of the reversibly photoswitchable variants of mCherry, and is an improved version with a faster off-switching speed and lower switching fatigue at high light intensities than its precursor rsCherryRev. However, rsCherryRev1.4 still has some limitations such as a tendency to dimerize as well as complex photophysical properties. Here, the crystal structure of rsCherryRev1.4 was determined at a resolution of 2 Å and it was discovered that it forms a dimer that shows disulfide bonding between the protomers. Mutagenesis, gel electrophoresis and size-exclusion chromatography strongly implicate Cys24 in this process. Replacing Cys24 in rsCherryRev1.4 resulted in a much lower tendency towards dimerization, while introducing Cys24 into mCherry correspondingly increased its dimerization. In principle, this finding opens the possibility of developing redox sensors based on controlled dimerization via disulfide cross-linking in fluorescent proteins, even though the actual application of engineering such sensors still requires additional research.

摘要

rsCherryRev1.4 被报道为 mCherry 的一种可光开关变体,是一种改良版本,与前体 rsCherryRev 相比,它具有更快的关闭速度和在高强度光下更低的开关疲劳。然而,rsCherryRev1.4 仍然存在一些限制,例如倾向于二聚化以及复杂的光物理性质。在这里,rsCherryRev1.4 的晶体结构在 2Å 的分辨率下被确定,发现它形成一个二聚体,在原聚体之间显示二硫键结合。突变、凝胶电泳和尺寸排阻色谱强烈暗示 Cys24 在这个过程中起作用。在 rsCherryRev1.4 中替换 Cys24 导致二聚化的趋势大大降低,而将 Cys24 引入 mCherry 则相应增加了其二聚化。原则上,这一发现为基于荧光蛋白中二硫键交联的可控二聚化开发氧化还原传感器开辟了可能性,尽管工程化此类传感器的实际应用仍需要进一步研究。

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