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NMR spectra of PB2 627 the RNA-binding domain in influenza A virus RNA polymerase that contains the pathogenicity factor lysine 627 and improvement of the spectra by small osmolytes

机译:PB2 627的NMR光谱甲型流感病毒RNA聚合酶中的RNA结合域其中含有致病因子赖氨酸627并且通过小渗透压改善了光谱

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摘要

The influenza A virus, which has an RNA genome, requires RNA-dependent RNA polymerase for transcription and replication. The polymerase is comprised of the subunits PA, PB1, and PB2. The C-terminal RNA-binding domain in PB2 contains lysine 627 (PB2 627), which is associated with pathogenicity and host range. However, the structure and molecular mechanism of PB2 627 in solution remain obscure. Here, we investigated PB2 627 in solution by nuclear magnetic resonance (NMR) and detected inhomogeneity in the intensities of backbone amide proton signals due to local fluctuations in structure. To characterize the effects of chemical chaperones on spectral data and improve the data quality, we tested 20 different additives, including L-arginine L-glutamate salt, (L-arginine)2SO4, glycerol, β-octylglucoside, 3-[(3-cholamidopropyl) dimethylammonio]-1-propanesulfonate, Na2SO4, 1,5-diaminopentane, 1,4-diaminobutane, trehalose, sucrose, glycine, trimethylamine N-oxide, β-alanine, L-α-alanine, hydroxyectoine, betaine, L-proline, and non-detergent sulfobetaine 195, 201, and 256. We evaluated the quality of the resulting spectra by calculating the standard deviation and average of the ratio of signal intensities to noise level of amide peaks, as well as the ratio of the standard deviation to the average. NMR-profile analysis revealed diverse effects of additives on the dynamic properties of PB2 627. Based on such criteria, we found that small osmolytes such as glycine and L-α-alanine reduced structural fluctuations and improved the quality of spectral data, which is likely to facilitate a detailed NMR-based structural analysis. The methodology developed here may also be more generally useful for evaluating the effects of chemical chaperones on the structural integrity of proteins.
机译:具有RNA基因组的甲型流感病毒需要依赖于RNA的RNA聚合酶进行转录和复制。聚合酶由亚基PA,PB1和PB2组成。 PB2中的C端RNA结合结构域包含赖氨酸627(PB2 627),这与致病性和宿主范围有关。但是,溶液中PB2 627的结构和分子机理仍然不清楚。在这里,我们通过核磁共振(NMR)研究了溶液中的PB2 627,并检测到由于结构的局部波动而导致的主链酰胺质子信号强度的不均匀性。为了表征化学分子伴侣对光谱数据的影响并改善数据质量,我们测试了20种不同的添加剂,包括L-精氨酸L-谷氨酸盐,(L-精氨酸)2SO4,甘油,β-辛基葡萄糖苷,3-[(3-碳酰氨基丙基)二甲基铵] -1-丙磺酸盐,Na2SO4、1,5-二氨基戊烷,1,4-二氨基丁烷,海藻糖,蔗糖,甘氨酸,三甲胺N-氧化物,β-丙氨酸,L-α-丙氨酸,羟基ectoine,甜菜碱,L-脯氨酸和非去污剂磺基甜菜碱195、201和256。我们通过计算标准偏差和信号强度与酰胺峰噪声水平之比的平均值以及标准品的比率,来评估所得光谱的质量偏离平均值。 NMR谱分析揭示了添加剂对PB2 627动力学特性的不同影响。基于这样的标准,我们发现甘氨酸和L-α-丙氨酸等小渗透物减少了结构波动并改善了光谱数据的质量,这很可能以便进行详细的基于NMR的结构分析。此处开发的方法学也可能更普遍地用于评估化学分子伴侣对蛋白质结构完整性的影响。

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