A customizable and defined medium supporting culturing of , , and human oral epithelial cells.

Appl Environ Microbiol

Department of Preventive Dentistry, Academic Centre for Dentistry Amsterdam (ACTA), University of Amsterdam and Free University Amsterdam, Amsterdam, the Netherlands.

Published: August 2024

AI Article Synopsis

  • A new culture medium, "mDMEM-DMP," was developed to effectively support the growth of fungi, bacteria, and human oral cell lines, addressing the limitations of traditional mediums like DMEM and mDMEM.
  • The addition of HEPES enhanced the medium's effectiveness by improving growth and stabilizing pH, although higher concentrations had diminishing returns on growth.
  • The versatility of mDMEM-DMP allows for comprehensive studies of microbial and human interactions, crucial for understanding both health and disease.

Article Abstract

Unlabelled: an opportunistic oral pathogen, synergizes with , allowing bacteria to co-invade and systemically disseminate within the host. Studying human-microbe interactions creates the need for a universal culture medium that supports fungal, bacterial, and human cell culturing, while allowing sensitive analytical approaches such as OMICs and chromatography techniques. In this study, we established a fully defined, customizable adaptation of Dulbecco's modified Eagle medium (DMEM), allowing multi-kingdom culturing of , , and human oral cell lines, whereas minimal version of DMEM (mDMEM) did not support growth of , and neither did supplementation with dextrose, MEM non-essential amino acids, pyruvate, and Glutamax. This new medium composition, designated as "mDMEM-DMP," promoted growth of all tested strains. Addition of 25 mM 4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid (HEPES) further improved growth, while higher concentrations did not improve growth any further. Higher concentrations of HEPES did result in prolonged stabilization of medium pH. mDMEM-DMP promoted (hyphal) monoculturing and co-culturing on both solid and semi-solid surfaces. In contrast to , addition of HEPES reduced maximum culture optical density (OD). Finally, only buffered mDMEM-DMP (100 mM HEPES) was successful in maintaining the metabolic activity of human oral Ca9-22 and HO1N1 cell lines for 24 hours. Altogether, our findings show that mDMEM-DMP is a versatile and potent culture medium for both microbial and human cell culturing, providing a customizable platform to study human as well as microbial molecular physiology and putative interactions.

Importance: Interaction between microbes and the host are in the center of interest both in disease and in health. In order to study the interactions between microbes of different kingdoms and the host, alternative media are required. Synthetic media are useful as they allow addition of specific components. In addition, well-defined media are required if high-resolution analyses such as metabolomics and proteomics are desired. We describe the development of a synthetic medium to study the interactions between and human oral epithelial cells. Our findings show that mDMEM-DMP is a versatile and potent culture medium for both microbial and human cell culturing, providing a customizable platform to study human as well as microbial molecular physiology and putative interactions.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11337806PMC
http://dx.doi.org/10.1128/aem.00360-24DOI Listing

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