Eddy Matthew T, Su Yongchao, Silvers Robert, Andreas Loren, Clark Lindsay, Wagner Gerhard, Pintacuda Guido, Emsley Lyndon, Griffin Robert G
Department of Chemistry, Massachusetts Institute of Technology, Cambridge, MA, 02139, USA.
J Biomol NMR. 2015 Apr;61(3-4):299-310. doi: 10.1007/s10858-015-9903-1. Epub 2015 Jan 30.
The human voltage dependent anion channel 1 (VDAC) is a 32 kDa β-barrel integral membrane protein that controls the transport of ions across the outer mitochondrial membrane. Despite the determination of VDAC solution and diffraction structures, a structural basis for the mechanism of its function is not yet fully understood. Biophysical studies suggest VDAC requires a lipid bilayer to achieve full function, motivating the need for atomic resolution structural information of VDAC in a membrane environment. Here we report an essential step toward that goal: extensive assignments of backbone and side chain resonances for VDAC in DMPC lipid bilayers via magic angle spinning nuclear magnetic resonance (MAS NMR). VDAC reconstituted into DMPC lipid bilayers spontaneously forms two-dimensional lipid crystals, showing remarkable spectral resolution (0.5-0.3 ppm for (13)C line widths and <0.5 ppm (15)N line widths at 750 MHz). In addition to the benefits of working in a lipid bilayer, several distinct advantages are observed with the lipid crystalline preparation. First, the strong signals and sharp line widths facilitated extensive NMR resonance assignments for an integral membrane β-barrel protein in lipid bilayers by MAS NMR. Second, a large number of residues in loop regions were readily observed and assigned, which can be challenging in detergent-solubilized membrane proteins where loop regions are often not detected due to line broadening from conformational exchange. Third, complete backbone and side chain chemical shift assignments could be obtained for the first 25 residues, which comprise the functionally important N-terminus. The reported assignments allow us to compare predicted torsion angles for VDAC prepared in DMPC 2D lipid crystals, DMPC liposomes, and LDAO-solubilized samples to address the possible effects of the membrane mimetic environment on the conformation of the protein. Concluding, we discuss the strengths and weaknesses of the reported assignment approach and the great potential for even more complete assignment studies and de novo structure determination via (1)H detected MAS NMR.
人类电压依赖性阴离子通道1(VDAC)是一种32 kDa的β-桶状整合膜蛋白,它控制离子穿过线粒体外膜的运输。尽管已确定了VDAC的溶液结构和衍射结构,但其功能机制的结构基础尚未完全明了。生物物理研究表明,VDAC需要脂质双层才能实现完整功能,这促使人们需要了解其在膜环境中的原子分辨率结构信息。在此,我们报告了朝着这一目标迈出的重要一步:通过魔角旋转核磁共振(MAS NMR)对DMPC脂质双层中的VDAC主链和侧链共振进行了广泛的归属。重组到DMPC脂质双层中的VDAC自发形成二维脂质晶体,显示出卓越的光谱分辨率(在750 MHz下,(13)C线宽为0.5 - 0.3 ppm,(15)N线宽<0.5 ppm)。除了在脂质双层中工作的优势外,脂质晶体样品还具有几个明显的优点。首先,强信号和尖锐的线宽有助于通过MAS NMR对脂质双层中的整合膜β-桶状蛋白进行广泛的NMR共振归属。其次,环区的大量残基很容易被观察到并进行了归属,这在去污剂溶解的膜蛋白中可能具有挑战性,因为环区常常由于构象交换导致的线宽展宽而无法被检测到。第三,对于构成功能重要的N端的前25个残基,可以获得完整的主链和侧链化学位移归属。所报告的归属使我们能够比较在DMPC二维脂质晶体、DMPC脂质体和LDAO溶解样品中制备的VDAC的预测扭转角,以探讨膜模拟环境对蛋白质构象的可能影响。最后,我们讨论了所报告的归属方法的优缺点,以及通过(1)H检测的MAS NMR进行更完整的归属研究和从头结构测定的巨大潜力。
