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      Role of IL‐6 and STAT3 signaling in dihydropyridine‐induced gingival overgrowth fibroblasts

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      https://www.riss.kr/link?id=O111700952

      • 저자
      • 발행기관
      • 학술지명
      • 권호사항
      • 발행연도

        2021년

      • 작성언어

        -

      • Print ISSN

        1354-523X

      • Online ISSN

        1601-0825

      • 등재정보

        SCI;SCIE;SCOPUS

      • 자료형태

        학술저널

      • 수록면

        1796-1805   [※수록면이 p5 이하이면, Review, Columns, Editor's Note, Abstract 등일 경우가 있습니다.]

      • 구독기관
        • 전북대학교 중앙도서관  
        • 성균관대학교 중앙학술정보관  
        • 부산대학교 중앙도서관  
        • 전남대학교 중앙도서관  
        • 제주대학교 중앙도서관  
        • 중앙대학교 서울캠퍼스 중앙도서관  
        • 인천대학교 학산도서관  
        • 숙명여자대학교 중앙도서관  
        • 서강대학교 로욜라중앙도서관  
        • 충남대학교 중앙도서관  
        • 한양대학교 백남학술정보관  
        • 이화여자대학교 중앙도서관  
        • 고려대학교 도서관  
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      다국어 초록 (Multilingual Abstract)

      This study analyzed the role of the interleukin (IL)‐6/signal transducer and activator of transcription 3 (STAT3) pathway in dihydropyridine‐induced gingival overgrowth (DIGO) fibroblasts.
      Tissue samples were obtained through surgical dissection from five DIGO patients and five healthy individuals. Cell cultures were conditioned with nifedipine (Nif) (0.34 µM) and stimulated with IL‐1β (10 ng/ml) to clarify whether IL‐6 upregulates extracellular matrix overproduction or has an impact on the cell proliferation rate of DIGO fibroblasts. STAT3 was knocked down using short hairpin (sh)RNA to determine its role in collagen (Col) type I alpha 1 (Colα1(I)) synthesis.
      Results showed that phosphorylated (p)STAT3 nuclear translocation was activated by a simulated autocrine concentration (50 ng/ml) of IL‐6, and application of an anti‐IL‐6 antibody significantly decreased the pSTAT3/STAT3 ratio in DIGO fibroblasts. STAT3 knockdown significantly decreased STAT3 and Colα1(I) expressions in DIGO cells. DIGO tissues presented stronger proliferating cell nuclear antigen (PCNA) expression than did healthy individuals under the effect of IL‐1β/Nif treatment.
      Gingival inflammation (e.g., IL‐1β) and taking dihydropyridine (e.g., Nif) may additively stimulate Col overproduction through the IL‐6−STAT3−Colα1(I) cascade in DIGO cells. IL‐6–STAT3 signaling may be considered a target for the control of DIGO.
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      This study analyzed the role of the interleukin (IL)‐6/signal transducer and activator of transcription 3 (STAT3) pathway in dihydropyridine‐induced gingival overgrowth (DIGO) fibroblasts. Tissue samples were obtained through surgical dissection f...

      This study analyzed the role of the interleukin (IL)‐6/signal transducer and activator of transcription 3 (STAT3) pathway in dihydropyridine‐induced gingival overgrowth (DIGO) fibroblasts.
      Tissue samples were obtained through surgical dissection from five DIGO patients and five healthy individuals. Cell cultures were conditioned with nifedipine (Nif) (0.34 µM) and stimulated with IL‐1β (10 ng/ml) to clarify whether IL‐6 upregulates extracellular matrix overproduction or has an impact on the cell proliferation rate of DIGO fibroblasts. STAT3 was knocked down using short hairpin (sh)RNA to determine its role in collagen (Col) type I alpha 1 (Colα1(I)) synthesis.
      Results showed that phosphorylated (p)STAT3 nuclear translocation was activated by a simulated autocrine concentration (50 ng/ml) of IL‐6, and application of an anti‐IL‐6 antibody significantly decreased the pSTAT3/STAT3 ratio in DIGO fibroblasts. STAT3 knockdown significantly decreased STAT3 and Colα1(I) expressions in DIGO cells. DIGO tissues presented stronger proliferating cell nuclear antigen (PCNA) expression than did healthy individuals under the effect of IL‐1β/Nif treatment.
      Gingival inflammation (e.g., IL‐1β) and taking dihydropyridine (e.g., Nif) may additively stimulate Col overproduction through the IL‐6−STAT3−Colα1(I) cascade in DIGO cells. IL‐6–STAT3 signaling may be considered a target for the control of DIGO.

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