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T2* weighted Deconvolution of NMR Spectra: Application to 2D Homonuclear MAS Solid-State NMR of Membrane Proteins

机译:NMR谱的T2 *加权解卷积:在膜蛋白的二维同质MAS固态NMR中的应用

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摘要

2D homonuclear NMR spectroscopy is an essential technique to characterize small and large molecules, such as organic compounds, metabolites, and biomacromolecules at atomic resolution. However, for complex samples 2D homonuclear spectra display poor resolution, making spectral assignment very cumbersome. Here, we propose a new method that exploits the differential T2* relaxation times of individual resonances and resolves the 2D NMR peaks into pseudo-3D spectra, where time is the 3rd dimension. T2* weIghted DEconvolution or TIDE analyzes individual free induction decays (FIDs) and dissects them into sub-FIDs that are transformed into pseudo-3D spectra combining Fourier transformation and covariance NMR. TIDE achieves higher resolution and sensitivity for NMR spectra than classical covariance NMR reducing offset-dependent artifacts. We demonstrate the performance of TIDE for magic angle spinning (MAS) [13C,13C]-DARR NMR spectra of single- and multi-span membrane proteins embedded in lipid bilayers. Since TIDE is applicable to all type of homonuclear correlation experiments for liquid and solid samples, we anticipate that it will be a general method for processing NMR data of biomacromolecules, complex mixtures of metabolites as well as material samples.
机译:2D同核NMR光谱学是一种以原子分辨率表征有机分子,有机化合物,代谢物和大分子的小分子的必不可少的技术。但是,对于复杂的样品,二维同核光谱显示出较差的分辨率,从而使光谱分配非常麻烦。在这里,我们提出了一种新的方法,该方法利用各个共振的差分T2 *弛豫时间并将2D NMR峰解析为伪3D谱,其中时间为3 rd 维。 T2 *加权解卷积或TIDE分析单个的自由感应衰变(FID),并将其分解为子FID,然后将其结合傅里叶变换和协方差NMR转换为伪3D光谱。与经典协方差NMR相比,TIDE对NMR光谱具有更高的分辨率和灵敏度,从而减少了偏移相关的伪影。我们证明了TIDE对嵌入脂质中的单跨膜和多跨膜蛋白的幻角旋转(MAS)[ 13 C, 13 C] -DARR NMR光谱的性能双层。由于TIDE适用于液体和固体样品的所有类型的同核相关实验,因此我们预计它将成为处理生物大分子,代谢物的复杂混合物以及材料样品的NMR数据的通用方法。

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