4.7 Article

Aging-Related Phenotypic Conversion of Medullary Microglia Enhances Intraoral Incisional Pain Sensitivity

期刊

出版社

MDPI
DOI: 10.3390/ijms21217871

关键词

microglia; M1; M2; senescence-accelerated mice; SAMP8; SAMR1; TNF-α IL-10; intraoral incision; orofacial mechanical allodynia

资金

  1. Sato Fund
  2. Uemura Fund
  3. KAKENHI [18K17157, 18K09732, 19K10049, 20K18619]
  4. Nihon University Multidisciplinary Research Grant [18-014]
  5. Nihon University Chairman of the Board of Trustees Grant (2019-2020)
  6. Dental Research Center in Nihon University School of Dentistry
  7. Grants-in-Aid for Scientific Research [18K17157, 20K18619, 18K09732] Funding Source: KAKEN

向作者/读者索取更多资源

Activated microglia involved in the development of orofacial pain hypersensitivity have two major polarization states. The aim of this study was to assess the involvement of the aging-related phenotypic conversion of medullary microglia in the enhancement of intraoral pain sensitivity using senescence-accelerated mice (SAM)-prone/8 (SAMP8) and SAM-resistant/1 (SAMR1) mice. Mechanical head-withdrawal threshold (MHWT) was measured for 21 days post palatal mucosal incision. The number of CD11c-immunoreactive (IR) cells [affective microglia (M1)] and CD163-IR cells [protective microglia (M2)], and tumor-necrosis-factor-alpha (TNF-alpha)-IR M1 and interleukin (IL)-10-IR M2 were analyzed via immunohistochemistry on days 3 and 11 following incision. The decrease in MHWT observed following incision was enhanced in SAMP8 mice. M1 levels and the number of TNF-alpha-IR M1 were increased on day 3 in SAMP8 mice compared with those in SAMR1 mice. On day 11, M1 and M2 activation was observed in both groups, whereas IL-10-IR M2 levels were attenuated in SAMP8 mice, and the number of TNF-alpha-IR M1 cells increased, compared to those in SAMR1 mice. These results suggest that the mechanical allodynia observed following intraoral injury is potentiated and sustained in SAMP8 mice due to enhancement of TNF-alpha signaling, M1 activation, and an attenuation of M2 activation accompanying IL-10 release.

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