A regenerative approach for temporomandibular joint repair: An in vitro and ex vivo study

Author:

Guastaldi Fernando P. S.1ORCID,Matheus Henrique R.12,Hadad Henrique13,Randolph Mark A.4,Redmond Robert W.5

Affiliation:

1. Department of Oral and Maxillofacial Surgery Massachusetts General Hospital, Harvard School of Dental Medicine Boston Massachusetts USA

2. Department of Diagnosis and Surgery, Division of Periodontics São Paulo State University (UNESP), School of Dentistry Araçatuba SP Brazil

3. Department of Diagnosis and Surgery, Oral & Maxillofacial Surgery Division São Paulo State University (UNESP), School of Dentistry Araçatuba SP Brazil

4. Division of Plastic and Reconstructive Surgery Massachusetts General Hospital, Harvard Medical School Boston Massachusetts USA

5. Wellman Center for Photomedicine Massachusetts General Hospital, Harvard Medical School Boston Massachusetts USA

Abstract

AbstractBackgroundCurrent clinical approaches to regenerate temporomandibular joint (TMJ) articulating cartilage defects only treat the symptoms (i.e. pain and dysfunction) and do not seek to restore joint integrity for long‐term relief. Therefore, we investigated a novel self‐assembling tissue‐engineered cartilage to overcome this significant clinical issue for TMJ regenerative purposes.ObjectivesExamine the maturation of dynamic self‐regenerating cartilage (dSRC) using auricular chondrocytes and evaluate a novel combinatorial approach with fractional laser treatment and dSRC implantation for TMJ cartilage repair.Materials and MethodsA suspension of 107 freshly harvested rabbit ear chondrocytes was cultured under a continuous reciprocating motion to form the dSRC. After 2, 4 and 8 weeks of culture, dSRC samples were stained with H&E, Safranin‐O and Toluidine Blue. Immunohistochemistry (IHC) was performed for collagens type I and II. Channels (300–500 μm diameter and 1.2–1.5 mm depth) were created in six freshly harvested condyles using a fractional Erbium laser. Two groups were tested: dSRC in a laser‐ablated lesion (experimental) and an empty laser‐ablated channel (control). TMJ condyles were cultured for up to 8 weeks and analysed as described above.ResultsH&E staining showed a high cell density in dSRC compared to native cartilage. All dSRC groups demonstrated intense Safranin‐O staining, indicating high glycosaminoglycan (GAG) production and intense Toluidine Blue staining showed high proteoglycan content. IHC confirmed that dSRC consisted predominantly of collagen type II. The experimental group showed improved cartilage repair at both time points compared to the empty channels.ConclusiondSRC viability and successful matrix formation were demonstrated in vitro. The combination of fractional laser ablation and dSRC implantation enhanced cartilage repair.

Funder

Massachusetts General Hospital

Publisher

Wiley

Reference27 articles.

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