Single-molecule optical tweezers reveals folding steps of the domain swapping mechanism of a protein

被引:2
|
作者
Bustamante, Andres [1 ]
Rivera, Rodrigo [1 ]
Floor, Martin [2 ,3 ]
Babul, Jorge [4 ]
Baez, Mauricio [1 ]
机构
[1] Univ Chile, Fac Ciencias Quim & Farmaceut, Dept Bioquim & Biol Mol, Santiago, Chile
[2] Univ Vic, Fac Sci & Technol, Bioinformat & Med Stat Grp, Univ Cent Catalunya, Vic, Spain
[3] Univ Int Catalunya, Fac Med & Hlth Sci, Dept Basic Sci, Sant Cugat Del Valles, Spain
[4] Univ Chile, Fac Ciencias, Dept Biol, Santiago, Chile
关键词
FORKHEAD-DOMAIN; DNA-BINDING; DYNAMICS; P13SUC1; TRAJECTORIES; PATHWAY; MODELS;
D O I
10.1016/j.bpj.2021.09.026
中图分类号
Q6 [生物物理学];
学科分类号
071011 ;
摘要
Domain swapping is a mechanism of protein oligomerization by which two or more subunits exchange structural elements to generate an intertwined complex. Numerous studies support a diversity of swapping mechanisms in which structural elements can be exchanged at different stages of the folding pathway of a subunit. Here, we used single-molecule optical twee-zers technique to analyze the swapping mechanism of the forkhead DNA-binding domain of human transcription factor FoxP1. FoxP1 populates folded monomers in equilibrium with a swapped dimer. We generated a fusion protein linking two FoxP1 do-mains in tandem to obtain repetitive mechanical folding and unfolding trajectories. Thus, by stretching the same molecule several times, we detected either the independent folding of each domain or the elusive swapping step between domains. We found that a swapped dimer can be formed directly from fully or mostly folded monomer. In this situation, the interaction be-tween the monomers in route to the domain-swapped dimer is the rate-limiting step. This approach is a useful strategy to test the different proposed domain swapping mechanisms for proteins with relevant physiological functions.
引用
收藏
页码:4809 / 4818
页数:10
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