Abstract
Histamine levels in the human brain are controlled by rather peculiar metabolic pathways. In the first step, histamine is enzymatically methylated at its imidazole Nτ atom, and the produced N-methylhistamine undergoes an oxidative deamination catalyzed by monoamine oxidase B (MAO-B), as is common with other monoaminergic neurotransmitters and neuromodulators of the central nervous system. The fact that histamine requires such a conversion prior to oxidative deamination is intriguing since MAO-B is known to be relatively promiscuous towards monoaminergic substrates; its in-vitro oxidation of N-methylhistamine is about 10 times faster than that for histamine, yet this rather subtle difference appears to be governing the decomposition pathway. This work clarifies the MAO-B selectivity toward histamine and N-methylhistamine by multiscale simulations of the rate-limiting hydride abstraction step for both compounds in the gas phase, in aqueous solution, and in the enzyme, using the established empirical valence bond methodology, assisted by gas-phase density functional theory (DFT) calculations. The computed barriers are in very good agreement with experimental kinetic data, especially for relative trends among systems, thereby reproducing the observed MAO-B selectivity. Simulations clearly demonstrate that solvation effects govern the reactivity, both in aqueous solution as well as in the enzyme although with an opposing effect on the free energy barrier. In the aqueous solution, the transition-state structure involving histamine is better solvated than its methylated analog, leading to a lower barrier for histamine oxidation. In the enzyme, the higher hydrophobicity of N-methylhistamine results in a decreased number of water molecules at the active side, leading to decreased dielectric shielding of the preorganized catalytic electrostatic environment provided by the enzyme. This renders the catalytic environment more efficient for N-methylhistamine, giving rise to a lower barrier relative to histamine. In addition, the transition state involving N-methylhistamine appears to be stabilized by the surrounding nonpolar residues to a larger extent than with unsubstituted histamine, contributing to a lower barrier with the former.
Highlights
Histamine is a biologically important amine that exerts its effect through interaction with histamine receptors (H1 R, H2 R, H3 R, and H4 R) [1,2,3]
The factors affecting MAO selectivity are still poorly understood. We have addressed this issue by using a combination of classical molecular dynamics simulations, evaluations of binding free energy using the molecular mechanics Poisson–Boltzmann surface area (MM–PBSA) methodology, and quantum mechanical calculations within a cluster model of an enzyme [19]
In our previous empirical valence bond (EVB) studies of MAO enzymes, we have successfully demonstrated that monoamine oxidase B (MAO-B) lowers the barrier for the oxidative deamination of dopamine by more than nine orders of magnitude compared to the reaction in aqueous solution [36]
Summary
Histamine is a biologically important amine that exerts its effect through interaction with histamine receptors (H1 R, H2 R, H3 R, and H4 R) [1,2,3]. Histamine is a mediator of many different physiological processes, such as the contraction of smooth muscle tissues, dilatation of blood vessels, and gastric acid secretion It plays important roles in neurotransmission and immunomodulation. In the other pathway prevalent in the brain, histamine N-methyltransferase (HNMT) catalyzes the transfer of a methyl group to the secondary imidazole amine forming N-methylhistamine, rendering it inactive at histamine receptor sites [9]. This compound is metabolized by monoamine oxidase B (MAO-B) forming N-methylimidazole acetaldehyde [10]. The fact that MAO-B prefers N-methylhistamine over histamine pinpoints its considerable selectivity towards two compounds differing only in a single methyl group distant from the reactive ethylamino center
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