Mechanisms of cellular retention of melanin bound drugs: Experiments and computational modeling

Sina Bahrpeyma; Mika Reinisalo; Laura Hellinen; Seppo Auriola; Eva M Del Amo; Arto Urtti

doi:10.1016/j.jconrel.2022.05.059

Mechanisms of cellular retention of melanin bound drugs: Experiments and computational modeling

J Control Release. 2022 Aug:348:760-770. doi: 10.1016/j.jconrel.2022.05.059. Epub 2022 Jun 25.

Authors

Sina Bahrpeyma¹, Mika Reinisalo², Laura Hellinen², Seppo Auriola², Eva M Del Amo², Arto Urtti³

Affiliations

¹ School of Pharmacy, Faculty of Health Sciences, University of Eastern Finland, 70210 Kuopio, Finland; Faculty of Pharmacy, University of Helsinki, 00014, University of Helsinki, Finland. Electronic address: sina.bahrpeyma@uef.fi.
² School of Pharmacy, Faculty of Health Sciences, University of Eastern Finland, 70210 Kuopio, Finland.
³ School of Pharmacy, Faculty of Health Sciences, University of Eastern Finland, 70210 Kuopio, Finland; Faculty of Pharmacy, University of Helsinki, 00014, University of Helsinki, Finland; Institute of Chemistry, St. Petersburg State University, Petergoff, Russian Federation. Electronic address: arto.urtti@uef.fi.

PMID: 35738465
DOI: 10.1016/j.jconrel.2022.05.059

Abstract

Melanin binding of drugs is known to increase drug concentrations and retention in pigmented eye tissues. Even though the correlation between melanin binding in vitro and exposure to pigmented eye in vivo has been shown, there is a discrepancy between rapid drug release from melanin particles in vitro and the long in vivo retention in the pigmented tissues. We investigated mechanisms and kinetics of pigment-related drug retention experimentally using isolated melanin particles from porcine retinal pigment epithelium and choroid, isolated porcine eye melanosomes, and re-pigmented ARPE-19 cells in a dynamic flow system. The experimental studies were supplemented with kinetic simulations. Affinity and capacity of levofloxacin, terazosin, papaverine, and timolol binding to melanin revealed K_d values of ≈ 50-150 μM and B_max ≈ 40-112 nmol.mg^-1. The drugs were released from melanin in <1 h (timolol) or in 6-12 h (other drugs). The drugs were released slower from the melanosomes than from melanin; the experimental differences ranged from 1.2-fold (papaverine) to 7.4-fold (timolol). Kinetic simulations supported the role of the melanosomal membrane in slowing down the release of melanin binders. In release studies from the pigmented ARPE-19 cells, drugs were released from the cellular melanin to the extracellular space in ≈ 1 day (timolol) and ≈ 11 days (levofloxacin), i.e., much slower than the release from melanin or melanosomes. Simulations of drug release from pigmented cells in the flow system matched the experimental data and enabled further sensitivity analyses. The simulations demonstrated a significant prolongation of drug retention in the cells as a function of decreasing drug permeability in the melanosomal membranes and increasing melanin content in the cells. Overall, we report the impact of cellular factors in prolonging drug retention and release from melanin-containing cells. These data and simulations will facilitate the design of melanin binding drugs with prolonged ocular actions.

Keywords: Melanin binding; Melanosome; Modeling; Ocular pharmacokinetics; Pigment; Retinal pigment epithelium.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Computer Simulation
Levofloxacin
Melanins* / chemistry
Papaverine / metabolism
Retinal Pigment Epithelium
Swine
Timolol*

Substances

Melanins
Levofloxacin
Timolol
Papaverine