1b and c). The noncovalent inhibitors including benzamidine, leupeptin and
nafamostat mesylate also showed weak inhibition of HsaD (Fig. 1b) compared to PMSF and DCI. MGL like HsaD catalyses the turnover of highly hydrophobic substrates: as such the inhibitors STI571 order that have been identified tend to be insoluble (e.g. pristimerin and NAM). Although pristimerin is the most active noncovalent inhibitor tested (35% inhibition at 50 μM – Fig. 2a), further investigation was hampered by its poor aqueous solubility under conditions that are required for HsaD to remain active. NAM and JZL184 are covalent inhibitors: JZL184 like DCI and PMSF modifies the catalytic serine of MGL (Long et al., 2009), while NAM modifies a cysteine in the active site of MGL (Saario et al., 2005). Consistent Fulvestrant nmr with the lack of a cysteine residue in the active site of HsaD, NAM does not significantly inhibit HsaD (Fig. 2a). JZL 184 proved a better inhibitor (Fig. 2a) but was difficult to work with due to its hydrophobic nature and hence poor solubility. A series of specific acetylcholinesterase inhibitors were tested for inhibition of HsaD (Fig. 2b). These included eserine, edrophonium, tacrine, neostigmine, pyridostigmine and trichlorfon. After incubation with HsaD, trichlorfon inhibited poorly. Eserine and neostigmine show better inhibition, but still not as strong as was observed with DCI (c. 30% inhibition at 1 mM). The other
acetylcholinesterase inhibitors did not significantly inhibit HsaD. Two mechanisms have been proposed for the hydrolysis of substrates by MCP hydrolases. The first is based on the mechanism known to occur in serine proteases and proceeds via an acyl enzyme and tetrahedral intermediate (Ruzzini et al., 2012). The second requires a keto-enol tautomerization resulting in a gem-diol intermediate (Horsman et al., 2007). Recent mutagenesis experiments combined with structural studies resulted in trapping of the acyl enzyme intermediate of HOPDA hydrolysis, by another member of the C-C bond hydrolase family, BphD (Ruzzini et al., 2012) strongly supporting the first mechanism. Inhibition by PMSF and
DCI is also consistent with this mechanism as PMSF and DCI act as tetrahedral and acyl enzyme intermediate analogues, respectively, when they modify the active Vitamin B12 site serine. The most successful inhibitors were those that covalently modify HsaD (e.g. DCI). The primary issue with DCI and other covalent inhibitors tends to be their broad specificity profile making them poor starting points for inhibitor design. To help understand the specificity observed among the covalent inhibitors, the structure of HsaD modified with PMSF was solved (Fig. 3). Although density was observed for the sulphonate group covalently linked to Ser114, there was insufficient density to accommodate the phenylmethyl group of PMSF. A lack of electron density for PMSF in the structure with HsaD might suggest that PMSF acts reversibly.