Wang, Yulan; Zhang, Yufeng; Jing, Dai; Shuang, Yang; Miron, Richard John (2016). Enamel matrix derivative improves gingival fibroblast cell behavior cultured on titanium surfaces. Clinical oral investigations, 20(4), pp. 685-695. Springer 10.1007/s00784-015-1558-5
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Enamel matrix derivative improves gingival fibroblast cell behavior cultured on titanium surfaces.pdf - Published Version Available under License Publisher holds Copyright. Download (773kB) | Preview |
OBJECTIVE
Although an extensive amount of research has demonstrated the positive effects of an enamel matrix derivative (EMD) on soft tissue wound healing around intrabony defects, little information is available describing its effect on peri-implant soft tissues, an area that has recently gained tremendous awareness due to the increasing prevalence of peri-implantitis. The aim of the present study was to assess the role of EMD when gingival fibroblasts were cultured on titanium surface with different surface topographies.
METHODS
Human primary gingival fibroblasts were cultured on pickled (PT) and sand-blasted with large grit followed by acid etching (SLA) surfaces and assessed for cell adhesion at 2, 4, and 8 h, cell morphology at 2, 4, 8, and 24 h as well as cell proliferation at 1, 3, and 5 days post-seeding. Furthermore, genes encoding collagen 1a1, vascular endothelial growth factor-A (VEGF-A), and fibronectin were assessed by real-time PCR. Human gingival fibroblasts were also quantified for their ability to synthesize a collagen matrix on the various titanium surfaces with and without EMD by immunofluorescence staining.
RESULTS
The results from the present study demonstrate that EMD significantly increased cell spreading at 2, 4, 8, and 24 h on PT surfaces and 4, 8, and 24 h on SLA surfaces. Furthermore, proliferation at 5 days on PT surfaces and 3 and 5 days on SLA surfaces was also increased for groups containing EMD. Real-time PCR results demonstrated that the culture of gingival fibroblasts with EMD significantly increased extracellular matrix synthesis of collagen 1 as well as improved mRNA levels of VEGF-A and fibronectin. Collagen1 immuno-fluorescent staining revealed a significantly higher area of staining for cells seeded on PT + EMD at 7 and 14 days and 14 days for SLA + EMD when compared to control samples.
CONCLUSION
The results from the present study favor the use of EMD for colonization of gingival fibroblasts on titanium surfaces by increasing cell growth, spreading, and synthesis of an extracellular matrix. The improvements were primarily irrespective of surface topography. Future animal and human studies are necessary to fully characterize the beneficial effects of incorporating EMD during soft tissue regeneration of implant protocols.
CLINICAL RELEVANCE
The use of EMD may speed up the quality of soft tissue integration around dental implants by facilitating gingival cell attachment, proliferation, and matrix synthesis of collagen 1.
Item Type: |
Journal Article (Original Article) |
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Division/Institute: |
04 Faculty of Medicine > School of Dental Medicine > Department of Periodontology 04 Faculty of Medicine > School of Dental Medicine 04 Faculty of Medicine > School of Dental Medicine > Periodontics Research 04 Faculty of Medicine > School of Dental Medicine > Oral Surgery Research |
UniBE Contributor: |
Zhang, Yufeng, Miron, Richard John |
Subjects: |
600 Technology > 610 Medicine & health |
ISSN: |
1432-6981 |
Publisher: |
Springer |
Language: |
English |
Submitter: |
Eveline Carmen Schuler |
Date Deposited: |
08 Mar 2017 11:14 |
Last Modified: |
05 Dec 2022 15:00 |
Publisher DOI: |
10.1007/s00784-015-1558-5 |
PubMed ID: |
26269319 |
Uncontrolled Keywords: |
Emdogain; Enamel matrix derivative; Gingival fibroblasts; Soft tissue healing; Titanium implants |
BORIS DOI: |
10.7892/boris.92186 |
URI: |
https://boris.unibe.ch/id/eprint/92186 |
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