Abstract

As part of a general study into the impact of quaternary structure on enzyme function, a library of 31 point mutations were engineered at the dimer–dimer interface of the homotetrameric (β/α) 8-barrel protein, N-acetylneuraminate lyase (NAL, EC 4.1.3.3). Disruption of the interface generated either soluble tetramers or putative dimers that were absolutely insoluble and inactive. Intriguingly, the soluble tetramers were found to have widely varying k cat values, hinting at a role for the interface in catalysis. Leucine 171 was identified as essential to interface integrity. We conclude that the dimer–dimer interface of NAL is intolerant to mutation and essential for functional expression.

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