| Literature DB >> 3112942 |
S Sprang, T Standing, R J Fletterick, R M Stroud, J Finer-Moore, N H Xuong, R Hamlin, W J Rutter, C S Craik.
Abstract
The structure of the Asn102 mutant of trypsin was determined in order to distinguish whether the reduced activity of the mutant at neutral pH results from an altered active site conformation or from an inability to stabilize a positive charge on the active site histidine. The active site structure of the Asn102 mutant of trypsin is identical to the native enzyme with respect to the specificity pocket, the oxyanion hole, and the orientation of the nucleophilic serine. The observed decrease in rate results from the loss of nucleophilicity of the active site serine. This decreased nucleophilicity may result from stabilization of a His57 tautomer that is unable to accept the serine hydroxyl proton.Entities:
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Year: 1987 PMID: 3112942 DOI: 10.1126/science.3112942
Source DB: PubMed Journal: Science ISSN: 0036-8075 Impact factor: 47.728