Identification of glutamate β54 as the covalent‐catalytic residue in the active site of glutaconate CoA‐transferase from Acidaminococcus fermentans

In the course of glutamate fermentation by Acidaminococcus fermentans glutaconate coenzyme A‐transferase catalyzes the transfer of CoAS − from acetyl‐CoA to ( R )‐2‐hydroxyg;utarate, forming ( R )‐2‐hydroxyglutaryl‐CoA. Glutamate (E) 54 of the β‐subunit was postulated to be directly involved in catalysis by formation of a CoASH ester intermediate [(1994) Eur. J. Biochem., in press]. In order to prove this preliminary result, the following mutations, βE54A, βE64A, βE54Q and βE54D, were introduced by mismatch oligonucleotide priming. As expected, βE54A was inactive (0.02% of the wild‐type), whereas βE64A and βE54D were active, 30% and >7%, respectively. However, no CoASH intermediate was detected in the latter mutant, indicating a change in the catalytic mechanism. The activity of the βE54Q mutant increased from 1% to almost 100% upon incubation with acetyl‐CoA and glutaconate at 37°C within 40 h. Hence, the substrates induced the conversion of the mutant glutamine residue into the glutamate residue of the wild‐type enzyme.