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Single scan TROSY and E.COSY suite of experiments for the measurement of residual dipolar couplings in proteins

机译:单扫描TROSY和E.COSY实验套件,用于测量蛋白质中残留的偶极偶合

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Simple modifications of the gradient enhanced version of the TROSY experiment allow to obtain four different spectra containing each one of the components of the H–N doublet in15N labelled proteins. By measuring the difference in peak position among these four spectra, residual dipolar coupling values can be obtained for medium sized proteins. This experiment, which exploits the use of pulse field gradients to select the15N coherence pathway, produces excellent results in terms of water suppression. Moreover, tuning of a single delay in the sequence reduces notably the presence of artifacts. The performance of this suite of experiments, that we called TEC (Trosy–E.Cosy) experiment, is tested against aJ-modulation method, inherently more accurate but more time consuming, for the accuracy in the observed values of residual dipolar couplings. For larger proteins, the use of this strategy allows to select the most favourable combination of peaks giving the sharpest signals.
机译:TROSY实验的梯度增强版本的简单修改允许获得四个不同的光谱,其中包含15 N标记的蛋白质中H–N双峰的每个成分。通过测量这四个光谱中峰位置的差异,可以获得中等大小蛋白质的残留偶极耦合值。该实验利用脉冲场梯度来选择15 N相干路径,在抑制水方面产生了极好的结果。此外,序列中单个延迟的调整显着减少了伪像的出现。这套实验的性能,我们称为TEC(Trosy–E.Cosy)实验,相对于JJ调制方法进行了测试,这种方法本质上更准确但更耗时,以观察到残留偶极耦合值的准确性。对于较大的蛋白质,使用此策略可以选择给出最清晰信号的最有利的峰组合。

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