Capture and 3D culture of colonic crypts and colonoids in a microarray platform

Asad A. Ahmad; Ballard; Barker; Christopher E. Sims; Dufour; Formeister; Fuchs; Gracz; Grosberg; Huh; Huh; Huh; Jang; Jung; Kim; Kovarik; Lee; Miura; Nancy L. Allbritton; Ninov; Okamoto; Ootani; Ornoff; Pai; Pavak K. Shah; Ramadan; Sato; Sato; Sato; Sato; Schepers; Schuijers; Scott T. Magness; Stelzner; Sung; Sung; VanDussen; Wang; Wilson; Wong; Yui; Yuli Wang; Zheng

Capture and 3D culture of colonic crypts and colonoids in a microarray platform

Authors: Asad A. Ahmad
Ballard
Barker
Christopher E. Sims
Dufour
Formeister
Fuchs
Gracz
Grosberg
Huh
Huh
Huh
Jang
Jung
Kim
Kovarik
Lee
Miura
Nancy L. Allbritton
Ninov
Okamoto
Ootani
Ornoff
Pai
Pavak K. Shah
Ramadan
Sato
Sato
Sato
Sato
Schepers
Schuijers
Scott T. Magness
Stelzner
Sung
Sung
VanDussen
Wang
Wilson
Wong
Yui
Yuli Wang
Zheng
Publication date: 1 January 2013
Publisher: 'Royal Society of Chemistry (RSC)'
Doi

Abstract

Crypts are the basic structural and functional units of colonic epithelium and can be isolated from the colon and cultured in vitro into multi-cell spheroids termed “colonoids”. Both crypts and colonoids are ideal building blocks for construction of an in vitro tissue model of the colon. Here we proposed and tested a microengineered platform for capture and in vitro 3D culture of colonic crypts and colonoids. An integrated platform was fabricated from polydimethylsiloxane which contained two fluidic layers separated by an array of cylindrical microwells (150-μm diameter, 150-μm depth) with perforated bottoms (30-μm opening, 10-μm depth) termed “microstrainers”. As fluid moved through the array, crypts or colonoids were retained in the microstrainers with a >90% array-filling efficiency. Matrigel as an extracellular matrix was then applied to the microstrainers to generate isolated Matrigel pockets encapsulating the crypts or colonoids. After supplying the essential growth factors, epidermal growth factor, Wnt-3A, R-spondin 2 and noggin, 63±13% of the crypts and 77±8% of the colonoids cultured in the microstrainers over a 48–72 h period formed viable 3D colonoids. Thus colonoid growth on the array was similar to that under standard culture conditions (78±5%). Additionally the colonoids displayed the same morphology and similar numbers of stem and progenitor cells as those under standard culture conditions. Immunofluorescence staining confirmed that the differentiated cell-types of the colon, goblet cells, enteroendocrine cells and absorptive enterocytes, formed on the array. To demonstrating the utility of the array in tracking the colonoid fate, quantitative fluorescence analysis was performed on the arrayed colonoids exposed to reagents such as Wnt-3A and the γ-secretase inhibitor LY-411575. The successful formation of viable, multi-cell type colonic tissue on the microengineered platform represents a first step in the building of a “colon-on-a-chip” with the goal of producing the physiologic structure and organ-level function of the colon for controlled experiments

Similar works

Full text

Available Versions

Crossref

info:doi/10.1039%2Fc3lc50813g

Last time updated on 03/12/2019

Carolina Digital Repository

cdr.lib.unc.edu:1r66j791n

Last time updated on 24/11/2020