Subunits CHS exists as a homodimeric protein with each monomer approximately 42-45 kDa in size. Each monomer possesses a
β-keto synthase (KS) activity that catalyzes the sequential head to tail incorporation of two-carbon
acetate units into a growing polyketide chain. CHS contains a five layer αβαβα core, a location of the
active site and
dimerization interface that is highly similar to
thiolase-fold containing enzymes. The dimerization interface contains both hydrophobic and hydrophilic residues and is generally flat except for a pair of
N-terminal helices that lay entwined across the top. Although the helices are not involved in reaction, they may contain intracellular localization signals as in yeast thiolase. They may also undergo a conformational change to participate in the formation of transient multi-protein complexes with other enzymes in the various pathways diverging from the general
phenylpropanoid biosynthetic pathway.
Localization The enzyme is localized in the
cytosol, associating with the
endoplasmic reticulum membrane. In another study, it was shown that CHS and CHI co-localize at the nucleus as well.
Active site There are two distinct bi-lobed
active site cavities located at the bottom edge of each monomer’s αβαβα core. Identical six-residue loops, which meet at the
dimer interface, separate the two active sites from each other. The loops being with Thr132 in the active site and ends with a
cis-peptide bond to Pro138. A Met137 residue plugs a hole in the other monomer’s active site. Therefore, the active site is buried except for a 16 Å CoA-binding tunnel that connects the catalytic surface to the outer surrounding
milieu. The width of the tunnel is too narrow for the
aromatic substrates and products that must pass through it, implying that there must be some dynamic mobility within and around the tunnel when placed in solution. The active site contains a conserved
catalytic triad of Cys164, His303 and Asn336. These residues aid in multiple decarboxylation and condensation reactions, with Cys164 acting as the active site
nucleophile. Phe215 and Phe265 are two other important
amino acids that act as “gatekeepers” to block the lower protein of the opening between the CoA-binding tunnel and the active site cavity. This limits the access of water to the active site while accommodating substrates and intermediates of varying shapes and sizes. Phe215 also orients the substrates at the active site during elongation of the
polyketide intermediate. == Mechanism ==