BLBS102-c04 BLBS102-Simpson March 21, 2012 11:59 Trim: 276mm X 219mm Printer Name: Yet to Come
58 Part 1: Principles/Food AnalysisOH OHOHOORPolymerR R
Monohydroxyphenol o-DihydroxyphenolCresolase reactionsProtein-Cu 2 + + O 2Protein-Cu 2 – O 2 + monophenol + 2H+Protein-Cu 2 +2 + 2 e–Protein-(Cu 2 +2)n Protein-(Cu+)n + O 2 Protein-(Cu+)n – O 2Protein-(Cu+)nO + OH–+ 2e–+ ne–o-Diphenolo-DiphenolMonophenoln = 2 in high cresolase preparations
n = 1 in high catecholase preparationso-Quinoneo-Diphenolo-Quinone+ 2eProtein-Cu 2 +Overall oxidation reactionsactivationProtein-Cu 2 +2 + o-diphenol + H 2 OProtein-Cu 2 – O 2o-QuinoneMonophenolase
(cresolase)Diphenoloxidase
(catecholase)Figure 4.2.Simplified mechanism for the hydroxylation and oxidation of diphenol by phenoloxidase.Catechol oxidase and laccase are distinguishable both on the
basis of their phenolic substrates (Figure 4.1), and their inhibitor
specificities (Marshall et al. 2000).
Catecholase activity is more important than cresolase action
in food because most of the phenolic substrates in food are
dihydroxyphenols (Mathew and Parpia 1971).
This bifunctional enzyme, PPO, containing copper in its
structure, has been described as an oxygen and four electron-
transferring phenol oxidase (Jolley et al. 1974). Figure 4.2 shows
a simplified mechanism for the hydroxylation and oxidation of
phenols by PPO. Both mechanisms involve the two copper moi-
eties on the PPO.
PPO, active between pH 5 and 7, does not have a very sharp pH
optimum. At lower pH values of approximately 3, the enzyme
is irreversibly inactivated. Reagents that complex or remove
copper from the prosthetic group of the enzyme inactivate the
enzyme (Fennema 1976).SubstratesAlthough tyrosine is the major substrate for certain phenolases,
other phenolic compounds such as caffeic acid and chlorogenic
acid also serve as substrate (Fennema 1976). Structurally, they
contain an aromatic ring bearing one or more hydroxyl groups,
together with a number of other substituents (Marshall et al.
2000). Structures of common phenolic compounds present in
foods are shown in Figure 4.3. Phenolic subtrates of PPO in
fruits, vegetables, and seafood are listed in Table 4.1. The sub-
strate specificity of PPO varies in accordance with the source of
the enzyme. Phenolic compounds and PPO are, in general, di-
rectly responsible for enzymatic browning reactions in damaged
fruits during postharvest handling and processing. The relation-
ship of the rate of browning to phenolic content and PPO activity
has been reported for various fruits. In addition to serving as
PPO substrates, phenolic compounds act as inhibitors of PPOs
(Marshall et al. 2000).