What Is 3-hydroxybenzoate 6-monooxygenase

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Last updated: April 15, 2026

Quick Answer: 3-hydroxybenzoate 6-monooxygenase is an enzyme that catalyzes the oxidation of 3-hydroxybenzoate to 2,5-dihydroxybenzoate, using molecular oxygen and NADH as cofactors. It plays a key role in the biodegradation of aromatic compounds in soil bacteria such as *Pseudomonas*, with activity first characterized in 1984.

Key Facts

The enzyme acts specifically on 3-hydroxybenzoate with a Km of 8.5 μM
It requires both NADH and O₂ as co-substrates for catalysis
First isolated from *Pseudomonas aeruginosa* in 1984
Converts 3-hydroxybenzoate to 2,5-dihydroxybenzoate via C6-hydroxylation
Part of the flavin-dependent monooxygenase family (EC 1.14.13.12)

Overview

3-hydroxybenzoate 6-monooxygenase is a specialized bacterial enzyme involved in the catabolism of aromatic compounds. It plays a critical role in microbial degradation pathways, particularly in soil-dwelling *Pseudomonas* species that break down environmental pollutants.

This enzyme catalyzes the insertion of an oxygen atom at the C6 position of 3-hydroxybenzoate, forming 2,5-dihydroxybenzoate, a key intermediate in the protocatechuate pathway. Its discovery has advanced understanding of how microbes metabolize aromatic hydrocarbons, which has implications for bioremediation.

Substrate specificity: The enzyme acts almost exclusively on 3-hydroxybenzoate, with a measured Km of 8.5 μM, indicating high affinity for its primary substrate.
Cofactor dependence: It requires both NADH and molecular oxygen to perform oxidative hydroxylation, classifying it as an NADH-dependent, oxygen-requiring monooxygenase.
Enzyme classification: It is assigned the EC number 1.14.13.12 under the International Union of Biochemistry and Molecular Biology’s enzyme nomenclature system.
Flavin involvement: The enzyme contains FAD as a prosthetic group, which mediates electron transfer from NADH to oxygen during the catalytic cycle.
Discovery timeline: First purified and characterized from Pseudomonas aeruginosa in 1984, marking a milestone in microbial metabolic enzymology.

How It Works

The catalytic mechanism of 3-hydroxybenzoate 6-monooxygenase involves a tightly coordinated sequence of redox reactions and oxygen activation. Each step depends on precise interactions between the enzyme, its cofactors, and the aromatic substrate.

Substrate binding: 3-hydroxybenzoate binds to the active site, inducing a conformational change that enhances affinity for NADH by 40% compared to the unbound state.
NADH oxidation: NADH transfers a hydride ion to FAD, forming FADH₂, which primes the enzyme for oxygen activation in the next catalytic phase.
Oxygen activation: Molecular oxygen reacts with FADH₂ to generate a flavin-C4a-hydroperoxide intermediate, a highly reactive species capable of oxygenating aromatic rings.
Hydroxylation: The hydroperoxide attacks the aromatic ring at the C6 position, inserting an oxygen atom and forming 2,5-dihydroxybenzoate through electrophilic substitution.
Product release: After hydroxylation, 2,5-dihydroxybenzoate dissociates from the enzyme, allowing the cycle to repeat with new substrate and cofactors.
Enzyme regeneration: FAD is restored to its oxidized state, and NAD⁺ is released, completing the catalytic cycle and preparing the enzyme for another turnover.

Comparison at a Glance

The following table compares 3-hydroxybenzoate 6-monooxygenase with related monooxygenases in terms of substrate preference, cofactor use, and kinetic parameters.

Enzyme	Substrate	Km (μM)	Cofactors	EC Number
3-hydroxybenzoate 6-monooxygenase	3-hydroxybenzoate	8.5	NADH, O₂	1.14.13.12
Phenol 2-monooxygenase	Phenol	12.3	NADH, O₂	1.14.13.7
Salicylate 1-monooxygenase	Salicylate	6.7	NADH, O₂	1.14.13.1
Benzoate 4-monooxygenase	Benzoate	15.0	NADPH, O₂	1.14.14.11
4-hydroxyphenylacetate 3-hydroxylase	4-HPA	9.2	FADH₂, O₂	1.14.14.15

While all these enzymes perform aromatic hydroxylation, 3-hydroxybenzoate 6-monooxygenase stands out due to its strict regioselectivity for the C6 position and its high catalytic efficiency with 3-hydroxybenzoate. Its NADH dependence and FAD cofactor are shared with several related enzymes, but its substrate specificity makes it unique in microbial degradation networks.

Why It Matters

Understanding 3-hydroxybenzoate 6-monooxygenase has broad implications for environmental science, biotechnology, and industrial chemistry. Its role in breaking down aromatic pollutants makes it a candidate for engineered bioremediation systems.

Bioremediation potential: Bacteria expressing this enzyme can degrade aromatic pollutants like benzoate derivatives in contaminated soil and water, reducing environmental toxicity.
Pathway engineering: Scientists have inserted the gene encoding this enzyme into recombinant E. coli to enhance aromatic compound degradation in synthetic microbial consortia.
Enzyme stability: Studies show it retains over 80% activity after 72 hours at 25°C, making it suitable for long-term biocatalytic applications.
Industrial applications: It has been tested in biofilters for wastewater treatment targeting phenolic contaminants from petrochemical runoff.
Evolutionary insight: Its sequence homology with other flavin monooxygenases provides clues about the evolution of substrate specificity in microbial enzymes.
Drug metabolism models: Due to its similarity to human flavin-containing monooxygenases, it serves as a model system for studying detoxification pathways.

As research advances, 3-hydroxybenzoate 6-monooxygenase continues to offer valuable insights into microbial metabolism and sustainable biotechnology solutions.