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利用被困离子淌度质谱-质谱技术探索 HMGA2·DNA 复合物的构象和结合动力学。

Exploring the Conformational and Binding Dynamics of HMGA2·DNA Complexes Using Trapped Ion Mobility Spectrometry-Mass Spectrometry.

机构信息

Department of Chemistry and Biochemistry, Florida International University, Miami, Florida 33199, United States.

Department of Chemistry, University of Texas, Austin, Texas 78712 United States.

出版信息

J Am Soc Mass Spectrom. 2022 Jul 6;33(7):1103-1112. doi: 10.1021/jasms.2c00101. Epub 2022 Jun 10.

Abstract

The mammalian high mobility group protein AT-hook 2 (HMGA2) is an intrinsically disordered DNA-binding protein expressed during embryogenesis. In the present work, the conformational and binding dynamics of HMGA2 and HMGA2 in complex with a 22-nt (DNA) and a 50-nt (DNA) AT-rich DNA hairpin were investigated using trapped ion mobility spectrometry-mass spectrometry (TIMS-MS) under native starting solvent conditions (e.g., 100 mM aqueous NHAc) and collision-induced unfolding/dissociation (CIU/CID) as well as solution fluorescence anisotropy to assess the role of the DNA ligand when binding to the HMGA2 protein. CIU-TIMS-CID-MS/MS experiments showed a significant reduction of the conformational space and charge-state distribution accompanied by an energy stability increase of the native HMGA2 upon DNA binding. Fluorescence anisotropy experiments and CIU-TIMS-CID-MS/MS demonstrated for the first time that HMGA2 binds with high affinity to the minor groove of AT-rich DNA oligomers and with lower affinity to the major groove of AT-rich DNA oligomers (minor groove occupied by a minor groove binder Hoechst 33258). The HMGA2·DNA22 complex (18.2 kDa) 1:1 and 1:2 stoichiometry suggests that two of the AT-hook sites are accessible for DNA binding, while the other AT-hook site is probably coordinated by the C-terminal motif peptide (CTMP). The HMGA2 transition from disordered to ordered upon DNA binding is driven by the interaction of the three basic AT-hook residues with the minor and/or major grooves of AT-rich DNA oligomers.

摘要

哺乳动物的高迁移率族蛋白 ATH 盒 2(HMGA2)是一种固有无序的 DNA 结合蛋白,在胚胎发生过程中表达。在本工作中,使用离子阱迁移谱-质谱联用技术(TIMS-MS)在天然起始溶剂条件(例如,100 mM 水溶液)下以及在碰撞诱导展开/解离(CIU/CID)下,研究了 HMGA2 和 HMGA2 与富含 AT 的 22-nt(DNA)和 50-nt(DNA)发夹 DNA 复合物的构象和结合动力学,以及溶液荧光各向异性,以评估当与 HMGA2 蛋白结合时 DNA 配体的作用。CIU-TIMS-CID-MS/MS 实验表明,在 DNA 结合后,HMGA2 的构象空间和电荷态分布显著减少,同时能量稳定性增加。荧光各向异性实验和 CIU-TIMS-CID-MS/MS 首次表明,HMGA2 以高亲和力结合富含 AT 的 DNA 寡聚物的小沟,以较低亲和力结合富含 AT 的 DNA 寡聚物的大沟(由小沟结合物 Hoechst 33258 占据的小沟)。HMGA2·DNA22 复合物(18.2 kDa)1:1 和 1:2 化学计量表明,两个 AT 钩位点可用于 DNA 结合,而另一个 AT 钩位点可能由 C 端基序肽(CTMP)协调。HMGA2 在 DNA 结合时从无序到有序的转变是由三个碱性 AT 钩残基与富含 AT 的 DNA 寡聚物的小沟和/或大沟的相互作用驱动的。

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