Heterologous expression of human transketolase

Abstract

Transketolase belongs to the family of thiamin diphosphate dependent enzymes. The aim of this study was to establish a bacterial expression system for human transketolase in order to investigate the functional characteristics of mammalian transketolases. The level of recombinant human enzyme expressed in Escherichia coli was modest. Purification of recombinant transketolase and separation from the E. coli enzyme has been greatly simplified by means of a non-cleavable hexa-histidine tag. The highest specific activity was 13.5 U/mg and the K m values were 0.27±0.02 and 0.51±0.05 mM for the substrates d-xylulose 5-phosphate and d-ribose 5-phosphate, respectively. Binding of cofactors to the apoenzyme showed the expected hysteresis. Without preincubation, the K m values for thiamin diphosphate and for Mg 2+ were, respectively, 4.1±0.8 and 2.5±0.4 μM, but after 1 h of preincubation these values were 85±16 nM and 0.74±0.23 μM. The kinetic constants are similar to those of the native enzyme purified from human erythrocytes. Despite the modest expression level the reported system is well suited to a variety of functional studies.