A subscription to JoVE is required to view this content. Sign in or start your free trial.
Isolation of Salivary Epithelial Cells from Human Salivary Glands for In Vitro Growth as Salispheres or Monolayers
In This Article
Summary
We present a method for isolating and cultivating primary human salivary gland-derived epithelial cells. These cells exhibit gene expression patterns consistent with them being of salivary epithelial origin and can be grown as salispheres on basement membrane matrices derived from Engelbreth-Holm-Swarm tumor cells or as monolayers on treated culture dishes.
Abstract
The salivary glands are a site of significant interest for researchers interested in multiple aspects of human disease. One goal of researchers is to restore function of glands damaged by radiation therapies or due to pathologies associated with Sjögren's syndrome. A second goal of researchers is to define the mechanisms by which viruses replicate within glandular tissue where they can then gain access to salivary fluids important for horizontal transmission. These goals highlight the need for a robust and accessible in vitro salivary gland model that can be utilized by researchers interested in the above mentioned as well as related research areas. Here we discuss a simple protocol to isolate epithelial cells from human salivary glands and propagate them in vitro. Our protocol can be further optimized to meet the needs of individual studies. Briefly, salivary tissue is mechanically and enzymatically separated to isolate single cells or small clusters of cells. Selection for epithelial cells occurs by plating onto a basement membrane matrix in the presence of media optimized to promote epithelial cell growth. These resulting cultures can be maintained as three-dimensional clusters, termed "salispheres", or grown as a monolayer on treated plastic tissue culture dishes. This protocol results in the outgrowth of a heterogenous population of mainly epithelial cells that can be propagated for 5-8 passages (15-20 population doublings) before undergoing cellular senescence.
Introduction
In mammals the salivary glands are organized into 3 pairs of major salivary glands: the parotid, submandibular, and sublingual glands. There also exists a series of minor glands located on the tongue and scattered throughout the oral cavity1. The major glands are responsible for the bulk volume of saliva produced2. In addition to providing antimicrobial protection through secreted factors, the saliva is important in the process of chewing and lubricating food as it passes through the esophagus2. As such, salivary gland dysfunction represents a medical issue where sufferers who are unable to produc....
Protocol
These protocols and studies have been reviewed and approved by the Institutional Review Board at the University of Cincinnati (Federal-wide Assurance #00003152, IRB protocol 2016-4183). Salivary tissue is commonly resected in many head and neck surgical procedures and is usually uninvolved by the malignant process. Typically, freshly resected salivary gland tissue is used within 2-4 h after removal from the patient (Figure 1A).
1. Reagent Preparation
- <.......
Representative Results
Two-three days after plating cells from digested tissue onto BMM, cells will readily form small clusters that will continue to expand in size up to 15-20 cells per cluster (Figure 2A). Cellular debris and detached dead cells are typically seen and should be removed by aspirating and replenishing with fresh media. Cells will continue to proliferate as salispheres for about 3-10 days, or as long as the BMM layer remains intact. Occasionally, due to partial brea.......
Discussion
Salivary dysfunction represents a concern for the quality of life for those suffering from Sjögren's syndrome as well as those undergoing radiation therapy for cancers adjacent to the salivary glands3,4,5,16. One proposed therapy to treat these patients is to grow functional salivary stem cells or organoids in vitro, which can then be inserted into damaged salivary gland to replace aff.......
Acknowledgements
We would like to thank James P. Bridges for providing significant guidance on the methodologies involved for culturing primary cells. Matthew J. Beucler was supported by National Institutes of Health Training Grant T32-ES007250. This work was also supported by National Institutes of Health grants R01-AI121028 and R21-DE026267 awarded to William E. Miller.
....Materials
| Name | Company | Catalog Number | Comments |
| 100 mm culture dishes | Thermo Scientific | 172931 | |
| 15 mL conical tubes | Thermo Scientific | 339651 | |
| 50 mL conical tubes | Thermo Scientific | 339653 | |
| Bronchial Epithelial Cell Growth Media | Lonza | CC-3171 | Add bullet kit as per manufacturer's instructions. Supplement with 20 mL of charcoal stripped serum. |
| Cell strainer 70 µm nylon mesh | Fisher | 22-363-548 | |
| Charcoal stripped fetal bovine serum | Gibco | 12676-029 | |
| Collagenase type III | Worthington | LS004182 | Store at 4 °C. |
| Cryogenic Tube | Fisher | 5000-0020 | |
| Dispase | Cell Applications | 07923 | Dissolve collagenase to make a 0.15% (w/v) stock. Filter sterilize then store at -20 °C. |
| Dissecting scissors | Fisher | 08-940 | |
| Dulbecco phosphate buffered saline | Corning | 55-031-PC | |
| General Chemicals | Sigma | ||
| PathClear Basement membrane extract | Cultrex | 3432-005-01 | Thaw at 4 °C at least 24 hr prior to use. Always handle on ice. |
| Six-well culture dishes | Falcon | 353046 | |
| Surgical forceps | Fisher | 22-079-742 | |
| Trypsin-EDTA solution | Corning | 25-052-CI |
References
- Kessler, A. T., Bhatt, A. A. Review of the Major and Minor Salivary Glands, Part 1: Anatomy, Infectious, and Inflammatory Processes. Journal of Clinical Imaging Science. 8, 47 (2018).
- Holmberg, K. V., Hoffman, M. P., Ligtenberg, A. J. M., Veerman, E. C. I.
This article has been published
Video Coming Soon
ABOUT JoVE
Copyright © 2024 MyJoVE Corporation. All rights reserved