Metabolism of serine/glycine lipids by human gingival cells in culture

Tyler M Guido; Samuel D Ratcliffe; Amanda Rahmlow; Matthew A Zambrello; Anthony A Provates; Robert B Clark; Michael B Smith; Frank C Nichols

doi:10.1111/omi.12439

Metabolism of serine/glycine lipids by human gingival cells in culture

Mol Oral Microbiol. 2024 Jun;39(3):103-112. doi: 10.1111/omi.12439. Epub 2023 Oct 18.

Authors

Tyler M Guido¹, Samuel D Ratcliffe¹, Amanda Rahmlow¹, Matthew A Zambrello¹, Anthony A Provates², Robert B Clark³, Michael B Smith⁴, Frank C Nichols¹

Affiliations

¹ Division of Periodontology, University of Connecticut School of Dental Medicine, Farmington, Connecticut, USA.
² Center for Environmental Science and Engineering, Storrs, Connecticut, USA.
³ Department of Immunology, University of Connecticut School of Medicine, Farmington, Connecticut, USA.
⁴ Department of Chemistry, University of Connecticut, Storrs, Connecticut, USA.

PMID: 37850509
PMCID: PMC11024056 (available on 2025-06-01)
DOI: 10.1111/omi.12439

Abstract

Porphyromonas gingivalis produces five classes of serine/glycine lipids that are recovered in lipid extracts from periodontitis-afflicted teeth and diseased gingival tissues, particularly at sites of periodontitis. Because these lipids are recovered in diseased gingival tissues, the purpose of the present study was to evaluate the capacity of cultured human gingival fibroblasts (HGF), keratinocytes, and macrophages to hydrolyze these lipids. We hypothesize that one or more of these cell types will hydrolyze the serine/glycine lipids. The primary aim was to treat these cell types for increasing time in culture with individual highly enriched serine/glycine lipid preparations. At specified times, cells and culture media samples were harvested and extracted for hydrolysis products. The serine/glycine lipids and hydrolysis products were quantified using liquid chromatography-mass spectrometry (LC-MS) and free fatty acids were quantified using gas chromatograph-mass spectrometer. LC-MS analysis used two different mass spectrometric methods. This study revealed that treatment of HGF or macrophage (THP1) cells with lipid (L) 654 resulted in breakdown to L342 and subsequent release into culture medium. However, L654 was converted only to L567 in gingival keratinocytes. By contrast, L1256 was converted to L654 by fibroblasts and macrophages but no further hydrolysis or release into medium was observed. Gingival keratinocytes showed no hydrolysis of L1256 to smaller lipid products but because L1256 was not recovered in these cells, it is not clear what hydrolysis products are produced from L1256. Although primary cultures of gingival fibroblasts and macrophages are capable of hydrolyzing specific serine/glycine lipids, prior analysis of lipid extracts from diseased gingival tissues revealed significantly elevated levels of L1256 in diseased tissues. These results suggest that the hydrolysis of bacterial lipids in gingival tissues may reduce the levels of specific lipids, but the hydrolysis of L1256 is not sufficiently rapid to prevent significant accumulation at periodontal disease sites.

Keywords: Porphyromonas gingivalis; fibroblasts; keratinocytes; lipids; macrophages; metabolism.

MeSH terms

Cells, Cultured
Chromatography, Liquid
Culture Media
Fibroblasts* / metabolism
Gas Chromatography-Mass Spectrometry
Gingiva* / cytology
Gingiva* / metabolism
Glycine* / metabolism
Humans
Hydrolysis
Keratinocytes* / metabolism
Lipid Metabolism
Lipids / analysis
Macrophages* / metabolism
Mass Spectrometry
Periodontitis / metabolism
Periodontitis / microbiology
Porphyromonas gingivalis / metabolism
Serine* / metabolism

Grants and funding

R01 DE027642/DE/NIDCR NIH HHS/United States