Probing amino acid side chains of the integral membrane protein PagP by solution NMR: Side chain immobilization facilitates association of secondary structures

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS ACS Applied Bio Materials Pub Date : 2024-01-12 DOI:10.1016/j.bbamem.2024.184281
Shaista Goel , M. Rafid Feisal , Gaddafi I. Danmaliki , Shaohui Yu , Philip B. Liu , Russell E. Bishop , Frederick G. West , Peter M. Hwang
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Abstract

Solution NMR spectroscopy of large protein systems is hampered by rapid signal decay, so most multidimensional studies focus on long-lived 1H-13C magnetization in methyl groups and/or backbone amide 1H-15N magnetization in an otherwise perdeuterated environment. Herein we demonstrate that it is possible to biosynthetically incorporate additional 1H-12C groups that possess long-lived magnetization using cost-effective partially deuterated or unlabeled amino acid precursors added to Escherichia coli growth media. This approach is applied to the outer membrane enzyme PagP in membrane-mimetic dodecylphosphocholine micelles.

We were able to obtain chemical shift assignments for a majority of side chain 1H positions in PagP using nuclear Overhauser enhancements (NOEs) to connect them to previously assigned backbone 1H-15N groups and newly assigned 1H-13C methyl groups. Side chain methyl-to-aromatic NOEs were particularly important for confirming that the amphipathic α-helix of PagP packs against its eight-stranded β-barrel, as indicated by previous X-ray crystal structures.

Interestingly, aromatic NOEs suggest that some aromatic residues in PagP that are buried in the membrane bilayer are highly mobile in the micellar environment, like Phe138 and Phe159. In contrast, Tyr87 in the middle of the bilayer is quite rigid, held in place by a hydrogen bonded network extending to the surface that resembles a classic catalytic triad: Tyr87-His67-Asp61. This hydrogen bonded arrangement of residues is not known to have any catalytic activity, but we postulate that its role is to immobilize Tyr87 to facilitate packing of the amphipathic α-helix against the β-barrel.

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通过溶液 NMR 探测整体膜蛋白 PagP 的氨基酸侧链:侧链固定化有助于二级结构的关联
大型蛋白质系统的溶液 NMR 光谱分析受到信号快速衰减的阻碍,因此大多数多维研究都侧重于甲基基团中的长效 1H-13C 磁化和/或骨架酰胺在其他氚化环境中的 1H-15N 磁化。在这里,我们证明了利用添加到大肠杆菌生长介质中的具有成本效益的部分氚化或未标记的氨基酸前体,可以生物合成地加入具有长效磁化的额外 1H-12C 基团。我们利用核欧豪瑟增强(NOE)技术获得了 PagP 中大多数侧链 1H 位置的化学位移分配,并将它们与之前分配的骨架 1H-15N 基团和新分配的 1H-13C 甲基基团连接起来。侧链甲基-芳香族 NOE 对于证实 PagP 的两性 α 螺旋与八股 β 管相匹配尤为重要,这一点在之前的 X 射线晶体结构中已经得到了证实。与此相反,位于双分子层中间的 Tyr87 却非常坚硬,它被一个延伸到表面的氢键网络固定在原位,该网络类似于一个典型的催化三元组:Tyr87-His67-Asp61。目前还不知道这种氢键残基排列具有任何催化活性,但我们推测其作用是固定 Tyr87,以促进两亲性 α 螺旋与 β 管的结合。
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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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