MyD88 exacerbates inflammation‐induced bone loss by modulating dynamic equilibrium between Th17/Treg cells and subgingival microbiota dysbiosis

Author:

Hsiao Po‐Yan1,Huang Ren‐Yeong123ORCID,Huang Lin‐Wei4,Chu Ching‐Liang5,Dyke Thomas Van67,Mau Lian‐Ping8,Cheng Chia‐Dan23,Sung Cheng‐En23ORCID,Weng Pei‐Wei910,Wu Yu‐Chiao311,Shieh Yi‐Shing311,Cheng Wan‐Chien123

Affiliation:

1. Graduate Institute of Life Sciences National Defense Medical Center Taipei Taiwan

2. Department of Periodontology School of Dentistry Tri‐Service General Hospital and National Defense Medical Center Taipei Taiwan

3. Graduate Institute of Dental Sciences National Defense Medical Center Taipei Taiwan

4. Graduate Institute of Microbiology and Immunology National Defense Medical Center Taipei Taiwan

5. Graduate Institute of Immunology College of Medicine National Taiwan University Taipei Taiwan

6. Oral Medicine, Infection, and Immunity Harvard School of Dental Medicine Boston Massachusetts USA

7. Department of Applied Oral Sciences The Forsyth Institute Cambridge Massachusetts USA

8. Department of Periodontics Chi Mei Medical Center Tainan Taiwan

9. Department of Orthopaedics Shuang Ho Hospital Taipei Medical University New Taipei City Taiwan

10. Department of Orthopaedics, School of Medicine College of Medicine, Taipei Medical University Taipei Taiwan

11. Department of Operative Dentistry and Endodontics School of Dentistry Tri‐Service General Hospital and National Defense Medical Center Taipei Taiwan

Abstract

AbstractBackgroundThis study aimed to investigate the contribution of myeloid differentiation primary‐response gene 88 (MyD88) on the differentiation of T helper type 17 (Th17) and regulatory T (Treg) cells and the emerging subgingival microbiota dysbiosis in Porphyromonas gingivalis‐induced experimental periodontitis.MethodsAlveolar bone loss, infiltrated inflammatory cells, immunostained cells for tartrate‐resistant acid phosphatase (TRAP), the receptor activator of nuclear factor‐kB ligand (RANKL), and osteoprotegerin (OPG) were quantified by microcomputerized tomography and histological staining between age‐ and sex‐matched homozygous littermates (wild‐type [WT, Myd88+/+] and Myd88−/− on C57BL/6 background). The frequencies of Th17 and Treg cells in cervical lymph nodes (CLNs) and spleen were determined by flow cytometry. Cytokine expression in gingival tissues, CLNs, and spleens were studied by quantitative polymerase chain reaction (qPCR). Analysis of the composition of the subgingival microbiome and functional annotation of prokaryotic taxa (FAPROTAX) analysis were performed.ResultsP. gingivalis‐infected Myd88−/− mice showed alleviated bone loss, TRAP+ osteoclasts, and RANKL/OPG ratio compared to WT mice. A significantly higher percentage of Foxp3+CD4+ T cells in infected Myd88−/− CLNs and a higher frequency of RORγt+CD4+ T cells in infected WT mice was noted. Increased IL‐10 and IL‐17a expressions in gingival tissue at D14–D28 then declined in WT mice, whereas an opposite pattern was observed in Myd88−/− mice. The Myd88−/− mice exhibited characteristic increases in gram‐positive species and species having probiotic properties, while gram‐negative, anaerobic species were noted in WT mice. FAPROTAX analysis revealed increased aerobic chemoheterotrophy in Myd88−/− mice, whereas anaerobic chemoheterotrophy was noted in WT mice after P. gingivalis infection.ConclusionsMyD88 plays an important role in inflammation‐induced bone loss by modulating the dynamic equilibrium between Th17/Treg cells and dysbiosis in P. gingivalis‐induced experimental periodontitis.

Funder

Chi Mei Medical Center

National Science and Technology Council

Publisher

Wiley

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