Specific carbonyl enrichment with 17O of amino acid OMe esters by up to 10(3) times over natural abundance was affected by treating [17O]-alpha-COOH amino acids with SOCl2 in MeOH. Carbonyl-[17O]-Gly-NH2, Gly-NHCH3 and Gly-N(CH3)2 were obtained from [17O]-Gly-OMe by (methyl)aminolysis with NH3, CH3NH2 and (CH3)2NH gases respectively. Peptide [17O]-carboxamides were prepared by (methyl)aminolysis of Z-Pro-Leu-[17O]-Gly-OMe followed by catalytic hydrogenation to remove the Z group. 17O chemical shifts of amino acid and peptide carboxamides in H2O, MeOH, CH3CN and DMSO were 260-324 p.p.m. downfield relative to H2O, depending on alpha-NH2 ionization, substitution on both amino groups and solvent H bonding, primarily to amide oxygen. Introduction of an amide-N methyl group usually caused upfield shifts (approx. -10 p.p.m.), attributed to elimination of one NH bond, while a second N methylation had the opposite effect. Amino acid and peptide OMe ester carbonyl-[17O] resonances appeared 326-359 p.p.m. downfield relative to H2O reflecting on side chain interactions, state of alpha-NH2 ionization and H-bonding with the solvent. Effective rotational correlation times for glycine and peptide carboxamide-[17O], calculated from T2 relaxation data, were of similar magnitude to values derived from solution properties and depended on the molecular weight and solvent viscosity.

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http://dx.doi.org/10.1111/j.1399-3011.1984.tb03131.xDOI Listing

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