Here, we show a site-specific branched fusion protein of P450 with its electron transfer proteins constructed using enzymatic cross-linking with a transglutaminase from Streptomyces mobaraensis (TGase). A branched fusion protein of P450 system, which was composed of one molecule each of P450 from Pseudomonas putida (P450cam) which catalyzes stereo-selective hydroxylation of d-camphor, putidaredoxin (Pdx) and putidaredoxin reductase (Pdr), showed higher catalytic activity (306 min-1) and coupling efficiency (99 %) than the reconstitution system due to the intramolecular electron transfer. Many substrates for P450s are highly hydrophobic and P450-catalyzed reactions are preferable to be conducted in nonaqueous media. The regeneration of NADH is also required due to its cost. We finally examined the hydroxylation of d-camphor by the fusion protein using NADH-regeneration driven by a hyper thermostable alcohol dehydrogenase in a reversed micella system. The hydroxylation of d-camphor and the regeneration of NADH were observed even in a reversed micellar system, while those were not observed using the reconstitution system.
This unique site-specific branched structure simply increased local concentration of proteins without serious loss of freedoms and activities of each protein. Therefore, enzymatic posttranslational protein manipulation can be a powerful alternative to conventional strategies for the creation of multi-component enzyme systems with novel proteinaceous architecture.