4.6 Article

Lysine acetylation can generate highly charged enzymes with increased resistance toward irreversible inactivation

期刊

PROTEIN SCIENCE
卷 17, 期 8, 页码 1446-1455

出版社

COLD SPRING HARBOR LAB PRESS, PUBLICATIONS DEPT
DOI: 10.1110/ps.035154.108

关键词

amylase; charge ladders; industrial biotechnology; protein aggregation; protein engineering; sodium dodecyl sulfate; thermostability

资金

  1. NIGMS NIH HHS [GM051559, R01 GM051559, F32 GM081055, GM081055] Funding Source: Medline

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This paper reports that the acetylation of lysine e-NH3+ groups of a- amylase - one of the most important hydrolytic enzymes used in industry - produces highly negatively charged variants that are enzymatically active, thermostable, and more resistant than the wild- type enzyme to irreversible inactivation on exposure to denaturing conditions ( e. g., 1 h at 90 C in solutions containing 100- mM sodium dodecyl sulfate). Acetylation also protected the enzyme against irreversible inactivation by the neutral surfactant TRITON X- 100 ( polyethylene glycol p-( 1,1,3,3- tetramethylbutyl) phenyl ether), but not by the cationic surfactant, dodecyltrimethylammonium bromide ( DTAB). The increased resistance of acetylated aamylase toward inactivation is attributed to the increased net negative charge of a- amylase that resulted from the acetylation of lysine ammonium groups ( lysine e- NH3 + ! e- NHCOCH3). Increases in the net negative charge of proteins can decrease the rate of unfolding by anionic surfactants, and can also decrease the rate of protein aggregation. The acetylation of lysine represents a simple, inexpensive method for stabilizing bacterial a- amylase against irreversible inactivation in the presence of the anionic and neutral surfactants that are commonly used in industrial applications.

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