Human Enteroid Monolayers: A Novel, Functionally-Stable Model for Investigating Oral Drug Disposition

Christopher Arian; Eimear O Mahony; James W MacDonald; Theo K Bammler; Mark Donowitz; Edward J Kelly; Kenneth E Thummel

doi:10.1124/dmd.124.001551

Human Enteroid Monolayers: A Novel, Functionally-Stable Model for Investigating Oral Drug Disposition

Drug Metab Dispos. 2024 May 14:DMD-AR-2023-001551. doi: 10.1124/dmd.124.001551. Online ahead of print.

Authors

Christopher Arian¹, Eimear O Mahony², James W MacDonald³, Theo K Bammler³, Mark Donowitz⁴, Edward J Kelly⁵, Kenneth E Thummel⁶

Affiliations

¹ Department of Pharmaceutics, University of Washington, United States.
² Pharmaceutics, University of Washington, United States.
³ University of Washington, United States.
⁴ Medicine, Johns Hopkins, United States.
⁵ Pharmaceutics, University of Washington, United States thummel@uw.edu.
⁶ Department of Pharmaceutics, University of Washington, United States thummel@uw.edu.

PMID: 38744527
DOI: 10.1124/dmd.124.001551

Abstract

To further the development of an in vitro model which faithfully recapitulates drug disposition of orally administered drugs, we investigated the utility of human enteroid monolayers to simultaneously assess intestinal drug absorption and first-pass metabolism processes. We cultured human enteroid monolayers from three donors, derived via biopsies containing duodenal stem cells that were propagated and then differentiated atop permeable Transwell® inserts, and confirmed transformation into a largely enterocyte population via RNA-seq analysis and immunocytochemical (ICC) assays. Proper cell morphology was assessed and confirmed via bright field microscopy and ICC imaging of tight junction proteins and other apically and basolaterally localized proteins. Enteroid monolayer barrier integrity was demonstrated by elevated transepithelial electrical resistance (TEER) that stabilized after 10 days in culture and persisted for 42 days. These results were corroborated by low paracellular transport probe permeability at 7 and 21 days in culture. The activity of a prominent drug metabolizing enzyme, CYP3A, was confirmed at 7, 21, and 42 days culture under basal, 1α,25(OH)2 vitamin D3-induced, and 6',7'-dihydroxybergamottin-inhibited conditions. The duration of these experiments is particularly noteworthy, as this is the first study assessing drug metabolizing enzymes and transporters (DMET) expression/function for enteroids cultured for greater than 12 days. The sum of these results suggests enteroid monolayers are a promising ex vivo model to investigate and quantitatively predict an orally administered drug's intestinal absorption and/or metabolism. Significance Statement This study presents a novel ex vivo model of the human intestine, human intestinal organoid (enteroid) monolayers, that maintain barrier function and metabolic functionality for up to 42-days in culture. The incorporation of both barrier integrity and metabolic function over an extended period within the same model is an advancement over historically used in vitro systems, which either lack one or both of these attributes or have limited viability.

Keywords: intestinal bioavailability; organotypic models.