A simple, cost-effective method for generating murine colonic 3D enteroids and 2D monolayers for studies of primary epithelial cell function

Elizabeth H Fernando; Michael Dicay; Martin Stahl; Marilyn H Gordon; Andrew Vegso; Cristiane Baggio; Laurie Alston; Fernando Lopes; Kristi Baker; Simon Hirota; Derek M McKay; Bruce Vallance; Wallace K MacNaughton

doi:10.1152/ajpgi.00152.2017

A simple, cost-effective method for generating murine colonic 3D enteroids and 2D monolayers for studies of primary epithelial cell function

Am J Physiol Gastrointest Liver Physiol. 2017 Nov 1;313(5):G467-G475. doi: 10.1152/ajpgi.00152.2017. Epub 2017 Jul 27.

Affiliations

¹ Department of Physiology and Pharmacology and Gastrointestinal Research Group, University of Calgary, Calgary, Alberta, Canada.
² Department of Pediatrics, British Columbia Children's Hospital, University of British Columbia, Vancouver, British Columbia, Canada; and.
³ Department of Oncology, University of Alberta, Edmonton, Alberta, Canada.
⁴ Department of Physiology and Pharmacology and Gastrointestinal Research Group, University of Calgary, Calgary, Alberta, Canada; wmacnaug@ucalgary.ca.

PMID: 28751424
DOI: 10.1152/ajpgi.00152.2017

Abstract

Cancer cell lines have been the mainstay of intestinal epithelial experimentation for decades, due primarily to their immortality and ease of culture. However, because of the inherent biological abnormalities of cancer cell lines, many cellular biologists are currently transitioning away from these models and toward more representative primary cells. This has been particularly challenging, but recent advances in the generation of intestinal organoids have brought the routine use of primary cells within reach of most epithelial biologists. Nevertheless, even with the proliferation of publications that use primary intestinal epithelial cells, there is still a considerable amount of trial and error required for laboratories to establish a consistent and reliable method to culture three-dimensional (3D) intestinal organoids and primary epithelial monolayers. We aim to minimize the time other laboratories spend troubleshooting the technique and present a standard method for culturing primary epithelial cells. Therefore, we have described our optimized, high-yield, cost-effective protocol to grow 3D murine colonoids for more than 20 passages and our detailed methods to culture these cells as confluent monolayers for at least 14 days, enabling a wide variety of potential future experiments. By supporting and expanding on the current literature of primary epithelial culture optimization and detailed use in experiments, we hope to help enable the widespread adoption of these innovative methods and allow consistency of results obtained across laboratories and institutions.NEW & NOTEWORTHY Primary intestinal epithelial monolayers are notoriously difficult to maintain culture, even with the recent advances in the field. We describe, in detail, the protocols required to maintain three-dimensional cultures of murine colonoids and passage these primary epithelial cells to confluent monolayers in a standardized, high-yield and cost-effective manner.

Keywords: epithelial monolayers; intestine; mouse; primary cell culture.

MeSH terms

Animals
Cells, Cultured
Colon* / pathology
Colon* / physiology
Epithelial Cells* / pathology
Epithelial Cells* / physiology
Intestinal Mucosa* / pathology
Intestinal Mucosa* / physiology
Mice
Organoids* / pathology
Organoids* / physiology
Primary Cell Culture / methods*