A novel in vivo model for evaluating functional restoration of a tissue-engineered salivary gland

Swati Pradhan-Bhatt; Daniel A Harrington; Randall L Duncan; Mary C Farach-Carson; Xinqiao Jia; Robert L Witt

doi:10.1002/lary.24297

A novel in vivo model for evaluating functional restoration of a tissue-engineered salivary gland

Laryngoscope. 2014 Feb;124(2):456-61. doi: 10.1002/lary.24297. Epub 2013 Aug 6.

Authors

Swati Pradhan-Bhatt¹, Daniel A Harrington, Randall L Duncan, Mary C Farach-Carson, Xinqiao Jia, Robert L Witt

Affiliation

¹ Department of Biological Sciences, Biomedical Engineering Program, University of Delaware, Newark, Delaware; Department of Materials Sciences and Engineering, Biomedical Engineering Program , University of Delaware, Newark, Delaware; Department of Otolaryngology-Head and Neck Surgery, Thomas Jefferson University, Philadelphia, Pennsylvania, U.S.A.

Abstract

Objectives/hypothesis: To create a novel model for development of a tissue-engineered salivary gland from human salivary gland cells that retains progenitor cell markers useful for treatment of radiation-induced xerostomia.

Study design: A three-dimensional (3D) hyaluronic acid (HA)-based hydrogel scaffold was used to encapsulate primary human salivary gland cells and to obtain organized acini-like spheroids. Hydrogels were implanted into rat models, and cell viability and receptor expression were evaluated.

Methods: A parotid gland surgical resection model for xenografting was developed. Salivary cells loaded in HA hydrogels formed spheroids and in vitro were implanted in the three-fourths resected parotid bed of athymic rats. Implants were removed after 1 week and analyzed for spheroid viability and phenotype retention.

Results: Spheroids in 3D stained positive for HA receptors CD168/RHAMM and CD44, which is also a progenitor cell marker. The parotid gland three-fourths resection model was well-tolerated by rodent hosts, and the salivary cell/hydrogel scaffolds were adherent to the remaining parotid gland, with no obvious signs of inflammation. A majority of human cells in the extracted hydrogels demonstrated robust expression of CD44.

Conclusions: A 3D HA-based hydrogel scaffold that supported long-term culture of salivary gland cells into organized spheroids was established. An in vivo salivary gland resection model was developed that allowed for integration of the 3D HA hydrogel scaffold with the existing glandular parenchyma. The expression of CD44 among salivary cultures may partially explain their regenerative potential, and the expression of CD168/RHAMM along with CD44 may aid the development of these 3D spheroids into regenerated salivary glands.

Level of evidence: NA.

Keywords: Bioartificial organ; hyaluronic acid receptors; hyaluronic acid-based hydrogels; progenitor cells; regeneration; salivary gland; three-dimensional cell culture; tissue engineering.

Publication types

Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't

MeSH terms

Adult
Animals
Humans
Hydrogels
Male
Middle Aged
Rats
Rats, Sprague-Dawley
Recovery of Function
Salivary Glands / physiology
Salivary Glands / surgery*
Tissue Engineering / methods

Substances

Hydrogels

Abstract

Publication types

MeSH terms

Substances

Grants and funding