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首页> 外文期刊>Molecular and Cellular Biochemistry: An International Journal for Chemical Biology >Induction of cytokine production in cholesteatoma keratinocytes by extracellular high-mobility group box chromosomal protein 1 combined with DNA released by apoptotic cholesteatoma keratinocytes
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Induction of cytokine production in cholesteatoma keratinocytes by extracellular high-mobility group box chromosomal protein 1 combined with DNA released by apoptotic cholesteatoma keratinocytes

机译:细胞外高迁移率组蛋白酶蛋白1结合凋亡胆管瘤角质细胞释放的DNA诱导细胞因子产生胆囊瘤角质细胞的细胞因子产生

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High-mobility group box chromosomal protein 1 (HMGB-1), a nuclear DNA binding protein, was recently rediscovered as a new proinflammatory cytokine. The purpose of this study was to determine HMGB-1 expression in vivo and to identify the effect of extracellular HMGB-1 in inflammatory process associated with bone destruction in cholesteatoma. We investigated the expression and location of HMGB-1 in the cholesteatoma and healthy skin using an immunofluorescence assay. We also detected apoptosis and DNA fragments in the cholesteatoma by TUNEL staining. HMGB-1 concentration in apoptotic supernatants from UV light-treated cells, culture supernatants and its translocation in cholesteatoma keratinocytes stimulated by supernatants from UV light-treated cells were measured by immunoblot analysis and immunofluorescence assay. Cultures of human cholesteatoma keratinocytes were exposed to CpG-DNA, HMGB-1, or CpG-DNA complexed to HMGB-1 for 24 h. Cytokines in the culture supernatant were measured by ELISA. In addition, levels of proinflammatory cytokines released by cholesteatoma keratinocytes stimulated by supernatants from UV light-treated cells with or without anti-HMGB-1 antibodies and supernatants from UV light-treated cells with DNase 1 were measured by enzyme-linked immunosorbent assay. The expression of HMGB-1 in cholesteatoma increased and it translocated both to the cytoplasm and extracellular space. Furthermore, the HMGB-1 concentration in supernatants increased significantly after addition of supernatants from UV light-treated cells. TNF-alpha and IL-1 beta can be induced by purified HMGB-1 combined with CpG-DNA in the cholesteatoma keratinocytes. In addition, supernatants of apoptotic cells containing HMGB-1-DNA were effective in inducing TNF-alpha and IL-1 beta secretion. This study suggested that persistent expression of extracellular HMGB-1 and DNA fragments in cholesteatoma leads to TNF-alpha and IL-1 beta production, causing bone resorption and destruction. Thus, we have implicated that HMGB-1-DNA complexes might act as a key molecule involved in bone resorption associated with cholesteatoma.
机译:最近将高迁移率组框染色体1(HMGB-1),核DNA结合蛋白,作为新的促炎细胞因子重新发现。本研究的目的是测定体内HMGB-1表达,并鉴定细胞外HMGB-1在胆脂瘤骨破坏相关的炎症过程中的作用。我们研究了使用免疫荧光测定法在胆脂瘤和健康皮肤中的HMGB-1的表达和位置。我们还通过TUNEL染色检测胆囊炎中的细胞凋亡和DNA片段。通过免疫印迹分析和免疫荧光测定法测定来自UV轻微处理细胞,培养上清液,培养上清液,培养上清液中培养物的角质形成细胞中的胆能瘤的角质形成细胞中的血液抑制剂中的HMGB-1浓度。将人胆囊瘤角质细胞的培养物暴露于CpG-DNA,HMGB-1或CPG-DNA络合至HMGB-1的24小时。通过ELISA测量培养上清液中的细胞因子。此外,通过酶联免疫吸附测定法测量来自用抗HMGB-1抗体的上清液和来自UV轻微处理细胞的上清液刺激的胆囊炎角蛋白酶释放的促炎细胞因子的水平。 HMGB-1在胆甾瘤中的表达增加,并且易于细胞质和细胞外空间的易用。此外,在从UV轻微处理细胞中加入上清液后,上清液中的HMGB-1浓度显着增加。可以通过纯化的HMGB-1与CPG-DNA联合胆怯瘤角质形成细胞来诱导TNF-α和IL-1β。此外,含有HMGB-1-DNA的凋亡细胞的上清液可有效诱导TNF-α和IL-1β分泌。该研究表明,胆甾瘤细胞外HMGB-1和DNA片段的持续表达导致TNF-α和IL-1β产生,导致骨吸收和破坏。因此,我们涉及HMGB-1-DNA复合物可以作为涉及与胆脂瘤相关的骨吸收中的关键分子。

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