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Introduction of tenomodulin by gene transfection vectors for rat bone tissue regeneration

INTRODUCTION: Periodontal ligament is regenerated in association with hard tissue regeneration. Tenomodulin (Tnmd) expression has been confirmed in periodontal ligament and it reportedly inhibits angiogenesis or is involved in collagen fibril maturation. The introduction of Tnmd by gene transfection...

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Autores principales: Wang, Han, Tenkumo, Taichi, Nemoto, Eiji, Kanda, Yoshiaki, Ogawa, Toru, Sasaki, Keiichi
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Japanese Society for Regenerative Medicine 2023
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Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9842804/
https://www.ncbi.nlm.nih.gov/pubmed/36712960
http://dx.doi.org/10.1016/j.reth.2022.12.008
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author Wang, Han
Tenkumo, Taichi
Nemoto, Eiji
Kanda, Yoshiaki
Ogawa, Toru
Sasaki, Keiichi
author_facet Wang, Han
Tenkumo, Taichi
Nemoto, Eiji
Kanda, Yoshiaki
Ogawa, Toru
Sasaki, Keiichi
author_sort Wang, Han
collection PubMed
description INTRODUCTION: Periodontal ligament is regenerated in association with hard tissue regeneration. Tenomodulin (Tnmd) expression has been confirmed in periodontal ligament and it reportedly inhibits angiogenesis or is involved in collagen fibril maturation. The introduction of Tnmd by gene transfection in bone tissue regeneration therapy might inhibit topical hard tissue formation and induce the formation of dense fibrous tissue. Therefore, the effect of Tnmd introduction by gene transfection technique in vitro and in vivo was investigated in this study. METHODS: Osteogenesis- and chondrogenesis-related gene expression levels in osteoblastic cells (MC3T3E1) and rat bone marrow derived cells were detected using qPCR three days after gene transfection with plasmid DNA (Tnmd) using non-viral gene transfection vectors: a calcium phosphate-based gene transfection vector (CaP(Tnmd)) or a cationic polymer-based reagent (JetPEI (Tnmd)). Next, an atelocollagen scaffold with or without CaP (Tnmd) or JetPEI (Tnmd) was implanted into a rat calvaria bone defect, and the remaining bone defect volume and the tissue reaction at 28 days after surgery were evaluated. RESULTS: Runx 2 and SP7 mRNA was reduced by JetPEI (Tnmd) in both cells, but not in CaP(Tnmd). The volume of expressed Tnmd was at 9 ng/mL in both gene transfection vector. The remaining bone defect volume of JetPEI (Tnmd) was significantly bigger than that of the other groups and CaP (EGFP), and that of CaP (Tnmd) was significantly bigger than that of CaP (EGFP). CONCLUSIONS: Tnmd introduction treatment inhibits bone formation in artificial bone defect, however, the effect of that was dependent on non-viral gene transfection vector.
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spelling pubmed-98428042023-01-26 Introduction of tenomodulin by gene transfection vectors for rat bone tissue regeneration Wang, Han Tenkumo, Taichi Nemoto, Eiji Kanda, Yoshiaki Ogawa, Toru Sasaki, Keiichi Regen Ther Original Article INTRODUCTION: Periodontal ligament is regenerated in association with hard tissue regeneration. Tenomodulin (Tnmd) expression has been confirmed in periodontal ligament and it reportedly inhibits angiogenesis or is involved in collagen fibril maturation. The introduction of Tnmd by gene transfection in bone tissue regeneration therapy might inhibit topical hard tissue formation and induce the formation of dense fibrous tissue. Therefore, the effect of Tnmd introduction by gene transfection technique in vitro and in vivo was investigated in this study. METHODS: Osteogenesis- and chondrogenesis-related gene expression levels in osteoblastic cells (MC3T3E1) and rat bone marrow derived cells were detected using qPCR three days after gene transfection with plasmid DNA (Tnmd) using non-viral gene transfection vectors: a calcium phosphate-based gene transfection vector (CaP(Tnmd)) or a cationic polymer-based reagent (JetPEI (Tnmd)). Next, an atelocollagen scaffold with or without CaP (Tnmd) or JetPEI (Tnmd) was implanted into a rat calvaria bone defect, and the remaining bone defect volume and the tissue reaction at 28 days after surgery were evaluated. RESULTS: Runx 2 and SP7 mRNA was reduced by JetPEI (Tnmd) in both cells, but not in CaP(Tnmd). The volume of expressed Tnmd was at 9 ng/mL in both gene transfection vector. The remaining bone defect volume of JetPEI (Tnmd) was significantly bigger than that of the other groups and CaP (EGFP), and that of CaP (Tnmd) was significantly bigger than that of CaP (EGFP). CONCLUSIONS: Tnmd introduction treatment inhibits bone formation in artificial bone defect, however, the effect of that was dependent on non-viral gene transfection vector. Japanese Society for Regenerative Medicine 2023-01-12 /pmc/articles/PMC9842804/ /pubmed/36712960 http://dx.doi.org/10.1016/j.reth.2022.12.008 Text en © 2022 The Japanese Society for Regenerative Medicine. Production and hosting by Elsevier B.V. https://creativecommons.org/licenses/by-nc-nd/4.0/This is an open access article under the CC BY-NC-ND license (http://creativecommons.org/licenses/by-nc-nd/4.0/).
spellingShingle Original Article
Wang, Han
Tenkumo, Taichi
Nemoto, Eiji
Kanda, Yoshiaki
Ogawa, Toru
Sasaki, Keiichi
Introduction of tenomodulin by gene transfection vectors for rat bone tissue regeneration
title Introduction of tenomodulin by gene transfection vectors for rat bone tissue regeneration
title_full Introduction of tenomodulin by gene transfection vectors for rat bone tissue regeneration
title_fullStr Introduction of tenomodulin by gene transfection vectors for rat bone tissue regeneration
title_full_unstemmed Introduction of tenomodulin by gene transfection vectors for rat bone tissue regeneration
title_short Introduction of tenomodulin by gene transfection vectors for rat bone tissue regeneration
title_sort introduction of tenomodulin by gene transfection vectors for rat bone tissue regeneration
topic Original Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9842804/
https://www.ncbi.nlm.nih.gov/pubmed/36712960
http://dx.doi.org/10.1016/j.reth.2022.12.008
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