In vitro observation of macrophage polarization and gingival fibroblast behavior on three‐dimensional xenogeneic collagen matrixes

Collagen biomaterials are widely used for soft tissue augmentation. Cross‐linking techniques for collagen matrix (CM) achieve mechanical and volumetric stability; nevertheless, cross‐linking may compromise biocompatibility. The aim of the present study was to investigate two different three‐dimensio...

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Veröffentlicht in:Journal of biomedical materials research. Part A 2020-06, Vol.108 (6), p.1408-1418
Hauptverfasser: Fujioka‐Kobayashi, Masako, Ülgür, Ismail I., Katagiri, Hiroki, Vuignier, Sandra, Schaller, Benoit
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container_end_page 1418
container_issue 6
container_start_page 1408
container_title Journal of biomedical materials research. Part A
container_volume 108
creator Fujioka‐Kobayashi, Masako
Ülgür, Ismail I.
Katagiri, Hiroki
Vuignier, Sandra
Schaller, Benoit
description Collagen biomaterials are widely used for soft tissue augmentation. Cross‐linking techniques for collagen matrix (CM) achieve mechanical and volumetric stability; nevertheless, cross‐linking may compromise biocompatibility. The aim of the present study was to investigate two different three‐dimensional (3D) porcine‐derived CMs, noncross‐linked (ncl)_CM and cross‐linked (cl)_CM, for their effects on macrophages (Mφ) and gingival fibroblasts. The effects of the CMs on the cell viability, proliferation, and polarization of Mφ derived from human monocyte THP‐1 cells were assessed. The effects of paracrine factors from Mφ cultured on the CMs were further studied in human gingival fibroblasts (HGF‐1 cells). The spongy layer of ncl_CM was partially resorbed after 1 day of culture. cl_CM maintained increased numbers of viable cells when compared with ncl_CM on day 3 for both THP‐1 and HGF‐1 cells. Higher mRNA levels of M1 markers, including IL‐1 and IL‐6, were found in Mφ cultured on cl_CM, while no significant differences were observed in M2 marker expression levels, including Arg1 and CD206, for cells cultured on both CMs when compared with those of the control. Furthermore, the conditioned medium collected from Mφ cultured on both CMs decreased cell viability. Nevertheless, neither of the CM‐conditioned media influenced the mRNA levels of TGF‐β, COL1a2, and PDGF‐A in HGF‐1 cells when compared with the control media. A comparison showed that cl_CM tended to result in more viable cells than ncl_CM, while cl_CM polarized Mφ toward an M1 phenotype, which was confirmed by the observation of increased mRNA levels of pro‐inflammatory cytokines.
doi_str_mv 10.1002/jbm.a.36911
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Higher mRNA levels of M1 markers, including IL‐1 and IL‐6, were found in Mφ cultured on cl_CM, while no significant differences were observed in M2 marker expression levels, including Arg1 and CD206, for cells cultured on both CMs when compared with those of the control. Furthermore, the conditioned medium collected from Mφ cultured on both CMs decreased cell viability. Nevertheless, neither of the CM‐conditioned media influenced the mRNA levels of TGF‐β, COL1a2, and PDGF‐A in HGF‐1 cells when compared with the control media. 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subjects Biocompatibility
Biomaterials
Biomedical materials
Cell culture
Cell proliferation
Cell viability
Collagen
collagen matrix
cross‐linked collagen
Cytokines
Fibroblasts
Gingiva
human gingival fibroblast
Inflammation
macrophage polarization
Macrophages
Markers
Monocytes
mRNA
noncross‐linked collagen
Paracrine signalling
Phenotypes
Platelet-derived growth factor
Polarization
soft tissue regeneration
Soft tissues
title In vitro observation of macrophage polarization and gingival fibroblast behavior on three‐dimensional xenogeneic collagen matrixes
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