A study of the relaxation parameters of a 13C-enriched methylene carbon and a 13C-enriched perdeuteromethylene carbon attached to chymotrypsin

J P G Malthouse; M D Finucane

摘要

pL-1-Chloro-4-phenyl-3-tosylamido[1-13C]butan-2-one (Tos-[1-13C]Phe-CH2Cl) and Tos-[1-13C,2H2]Phe-CH2Cl were prepared and used to alkylate delta-chymotrypsin. The relaxation parameters of the 13C-n.m.r. signal resulting from the alkylation of histidine-57 in both enzyme-inhibitor complexes were determined at 1.88 T and 6.34 T as well as the spin-lattice relaxation times of the backbone alpha-carbon atoms of the unenriched Tos-Phe-CH2-delta-chymotrypsin complex. It is concluded that the species examined do not have significant internal librational motions and that the rotational correlation time of the monomeric enzyme-inhibitor complex is 16.0 +/- 3.2 ns. The signal from the 13C-enriched atom of Tos-[1-13C,2H2]Phe-CH2Cl is split into a quintet (JCD = 23 Hz) whereas in the Tos-[1-13C,2H2]Phe-CH2-delta-chymotrypsin complex the signal from the 13C-enriched inhibitor carbon atom is decoupled. This decoupled signal had linewidths of 16 +/- 3 Hz and 52 +/- 2 Hz at 1.88 T and 6.34 T respectively, whereas linewidths at 40 +/- 2 Hz and 53 +/- 4 Hz were obtained for the same signal in the Tos-[1-13C]Phe-CH2-delta-chymotrypsin complex at 1.88 T and 6.34 T respectively. Therefore whereas deuteration produces a 2.5-fold reduction in linewidth at 1.88 T there is no significant decrease in the linewidth at 6.34 T. This result is explained by using the rigid rotor model, which predicts that the quadrupolar spin-lattice relaxation rate will be faster at low field strengths, resulting in more efficient deuterium decoupling by scalar relaxation of the second kind at lower field strengths. It is also predicted that deuterium decoupling by scalar relaxation will become less efficient as rotational correlation times increase. The consequences of these predictions for the detection of 13C-enriched atomic probes of proteins are discussed. It is also shown that a spin-echo pulse sequence can be used to remove signals due to protonated carbon atoms without attenuating the signal due to deuterated carbon atoms./p

机译：> L-1-氯-4-苯基-3-甲苯磺酰基[1-13C]丁-2-（Tos- [1-13C] Phe-CH2Cl）和Tos- [1-13C，2H2] Phe-制备CH 2 Cl并用于烷基化δ-胰凝乳蛋白酶。 13C-n.m.r。的弛豫参数确定两种酶-抑制剂复合物中组氨酸-57的烷基化产生的信号在1.88 T和6.34 T以及未富集的Tos-Phe-CH2-δ-的骨架α-碳原子的自旋晶格弛豫时间胰凝乳蛋白酶复合物。结论是，所检查的物种没有明显的内部自由运动，单体酶-抑制剂复合物的旋转相关时间为16.0 +/- 3.2 ns。来自Tos- [1-13C，2H2] Phe-CH2Cl的富含13C原子的信号分成五重音（JCD = 23 Hz），而在Tos- [1-13C，2H2] Phe-CH2-delta-胰凝乳蛋白酶复合物，来自13C富集的抑制剂碳原子的信号解耦。该去耦信号在1.88 T和6.34 T时分别具有16 +/- 3 Hz和52 +/- 2 Hz的线宽，而对于相同的信号，在40 +/- 2 Hz和53 +/- 4 Hz时获得的线宽。 Tos- [1-13C]Phe-CH2-δ-胰凝乳蛋白酶复合物分别在1.88 T和6.34 T时发生。因此，尽管氘代在1.88 T时线宽减少了2.5倍，但在6.34 T时线宽没有明显减少。使用刚性转子模型可以解释此结果，该模型预测四极自旋晶格的弛豫速率会更快在较低的场强下，通过第二种标量弛豫在较低的场强下导致更有效的氘去耦。还可以预测，随着旋转相关时间的增加，通过标量弛豫的氘去耦将变得效率较低。讨论了这些预测对检测富含13C的蛋白质原子探针的影响。研究还表明，自旋回波脉冲序列可用于去除质子化碳原子引起的信号，而不会衰减由于氘化碳原子引起的信号。

A study of the relaxation parameters of a 13C-enriched methylene carbon and a 13C-enriched perdeuteromethylene carbon attached to chymotrypsin

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