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Human venous blood derivatives as fetal bovine serum substitute for fibroblast culture cells in a fibrin construct
Chisini, Luiz Alexandre; Conde, Marcus Cristian Muniz; Karam, Sarah Arangurem; Carvalho, Rodrigo Varella de; Tarquinio, Sandra Beatriz Chaves; Demarco, Flávio Fernando.
  • Chisini, Luiz Alexandre; Federal University of Pelotas. School of Dentistry. Department of Restorative Dentistry. Pelotas. BR
  • Conde, Marcus Cristian Muniz; Federal University of Pelotas. School of Dentistry. Department of Restorative Dentistry. Pelotas. BR
  • Karam, Sarah Arangurem; Catholic University of Pelotas. Pelotas. BR
  • Carvalho, Rodrigo Varella de; Federal University of Pelotas. School of Dentistry. Department of Restorative Dentistry. Pelotas. BR
  • Tarquinio, Sandra Beatriz Chaves; Federal University of Pelotas. School of Dentistry. Diagnostic Center for Oral Diseases. Pelotas. BR
  • Demarco, Flávio Fernando; Catholic University of Pelotas. Pelotas. BR
Braz. j. oral sci ; 23: e240327, 2024. ilus
Artículo en Inglés | LILACS, BBO | ID: biblio-1553444
ABSTRACT
Aim: Venous blood derivatives (VBDs) have been suggested as substitutes for Fetal Bovine Serum (FBS) to improve the clinical transition of cell-based therapies. The literature is not clear about which is the best VBDs substitute. The present study aimed to evaluate the influence of VBDs on cell viability and describe a new method to seed these cells in a 3D Platelet-Rich Fibrin (PRF). Methods: Blood was processed to obtain Platelet-Poor Plasma from PRF (P-PRF), Human Serum (HS), Platelet-Poor Plasma from PRP (P-PRP), activated-PRP (a-PRP), and Platelet lysate (PL). Cells were supplemented with each VBD at 10% and FBS at 10% was the control. Cell viability (fibroblast 3T3/NIH) test was evaluated with MTT assay in two ways: i) cell-seeded and expanded with VBD; ii) cell-seed with FBS and expanded with VBD. To seed the Fibrin construct, cells were suspended in PBS and dropped into the blood sample before performing Choukroun's protocol for PRF. Constructs were cultured for 7 days in VBD supplements and FBS. Histological and Immunohistochemical analysis with vimentin was performed. Cell viability was analyzed by one-way ANOVA. Results: VBD's production time was very heterogeneous. Cells expanded in HS and a-PRP has grown faster. VBD-supplemented culture media provided cell culture highly sensible to trypsin/EDTA 0.25%. Cells seeded and expanded with VBD presented viability comparable to FBS in HS, a-PRP, and P-PRP (p>0.05) and lower in P-PRF and PL groups (p<0.05). The viability of cell seed with FBS and expanded with VBD was similar between P-PRF, a-PRP, PL, and FBS (p>0.05) and lower in HS and P-PRP (p<0.005). PRF-seeded cells showed a positive expression of vimentin and were able to maintain all cells supplemented with VBD. Conclusion: VBD supplements were able to maintain fibroblast cells in 2D and 3D cultures. The new method of the fibrin-cell construct was efficient to insert the cells into the fibrin network

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Texto completo: Disponible Índice: LILACS (Américas) Asunto principal: Sangre / Plaquetas / Albúmina Sérica Bovina / Fibrina / Células / Fibroblastos / Fibrina Rica en Plaquetas Idioma: Inglés Revista: Braz. j. oral sci Asunto de la revista: Odontología Año: 2024 Tipo del documento: Artículo País de afiliación: Brasil Institución/País de afiliación: Catholic University of Pelotas/BR / Federal University of Pelotas/BR

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Texto completo: Disponible Índice: LILACS (Américas) Asunto principal: Sangre / Plaquetas / Albúmina Sérica Bovina / Fibrina / Células / Fibroblastos / Fibrina Rica en Plaquetas Idioma: Inglés Revista: Braz. j. oral sci Asunto de la revista: Odontología Año: 2024 Tipo del documento: Artículo País de afiliación: Brasil Institución/País de afiliación: Catholic University of Pelotas/BR / Federal University of Pelotas/BR