1 Department of Bio-Medical Engineering, Virginia Tech and Virginia College of Osteopathic Medicine , RheuMatrix, Inc., Blacksburg, Virginia.
DNA Cell Biol. 2014 Aug;33(8):550-65. doi: 10.1089/dna.2013.2198. Epub 2014 Jun 6.
We applied global gene expression arrays, quantitative real-time PCR, immunostaining, and functional assays to untangle the role of High Mobility Groups proteins (HMGs) in human osteoarthritis (OA)-affected cartilage. Bioinformatics analysis showed increased mRNA expression of Damage-Associated Molecular Patterns (DAMPs): HMGA, HMGB, HMGN, SRY, LEF1, HMGB1, MMPs, and HMG/RAGE-interacting molecules (spondins and S100A4, S100A10, and S100A11) in human OA-affected cartilage as compared with normal cartilage. HMGB2 was down-regulated in human OA-affected cartilage. Immunohistological staining identified HMGB1 in chondrocytes in the superficial cartilage. Cells of the deep cartilage and subchondral bone showed increased expression of HMGB1 in OA-affected cartilage. HMGB1 was expressed in the nucleus, cytosol, and extracellular milieu of chondrocytes in cartilage. Furthermore, HMGB1 was spontaneously released from human OA-affected cartilage in ex vivo conditions. The effects of recombinant HMGB1 was tested on human cartilage and chondrocytes in vitro. HMGB1 stimulated mRNA of 2 NFκB gene enhancers (NFκB1 and NFκB2), 16 CC and CXC chemokines (IL-8, CCL2, CCL20, CCL3, CCL3L1, CCL3L3, CCL4, CCL4L1, CCL4L2, CCL5, CCL8, CXCL1, CXCL10, CXCL2, CXCL3, and CXCL6) by ≥10-fold. Furthermore, HMGB1 and IL-1β and/or tumor necrosis factor α (but not HMGI/Y) also significantly induced inducible nitric oxide synthase, NO, and interleukin (IL)-8 production in human cartilage and chondrocytes. The recombinant HMGB1 utilized in this study shows properties that are similar to disulfide-HMGB1. The differential, stage and/or tissue-specific expression of HMGB1, HMGB2, and S100A in cartilage was associated with regions of pathology and/or cartilage homeostasis in human OA-affected cartilage. Noteworthy similarities in the expression of mouse and human HMGB1 and HMGB2 were conserved in normal and arthritis-affected cartilage. The multifunctional forms of HMGB1 and S100A could perpetuate damage-induced cartilage inflammation in late-stage OA-affected joints similar to sterile inflammation. The paracrine effects of HMGB1 can induce chemokines and NO that are perceived to change cartilage homeostasis in human OA-affected cartilage.
我们应用全基因表达谱芯片、实时定量 PCR、免疫组化和功能分析来理清高迁移率族蛋白(HMGBs)在人类骨关节炎(OA)软骨中的作用。生物信息学分析显示,在人类 OA 软骨中,损伤相关分子模式(DAMPs)的 mRNA 表达增加:HMGA、HMGB、HMGN、SRY、LEF1、HMGB1、基质金属蛋白酶(MMPs)和 HMGB/RAGE 相互作用分子(spondins 和 S100A4、S100A10 和 S100A11)。HMGB2 在人类 OA 软骨中下调。免疫组织化学染色显示,在浅层软骨的软骨细胞中存在 HMGB1。深层软骨和软骨下骨的细胞在 OA 软骨中 HMGB1 的表达增加。HMGB1 存在于软骨细胞的核、细胞质和细胞外基质中。此外,HMGB1 在离体条件下从人类 OA 软骨中自发释放。在体外,用重组 HMGB1 测试对人软骨和软骨细胞的影响。HMGB1 刺激 2 个 NFκB 基因增强子(NFκB1 和 NFκB2)、16 个 CC 和 CXC 趋化因子(IL-8、CCL2、CCL20、CCL3、CCL3L1、CCL3L3、CCL4、CCL4L1、CCL4L2、CCL5、CCL8、CXCL1、CXCL10、CXCL2、CXCL3 和 CXCL6)的 mRNA 表达增加了 10 倍以上。此外,HMGB1 和白细胞介素-1β(IL-1β)和/或肿瘤坏死因子-α(TNF-α)(但不是 HMGI/Y)也显著诱导人软骨和软骨细胞中诱导型一氧化氮合酶(iNOS)、NO 和白细胞介素(IL)-8 的产生。本研究中使用的重组 HMGB1 具有类似于二硫键-HMGB1 的特性。HMGB1、HMGB2 和 S100A 在软骨中的差异、阶段和/或组织特异性表达与人类 OA 软骨中病理和/或软骨稳态的区域相关。在正常和关节炎性软骨中,HMGB1 和 HMGB2 的小鼠和人类表达的相似性保持不变。HMGB1 和 S100A 的多功能形式可能会在晚期 OA 关节中引发类似于无菌炎症的损伤诱导性软骨炎症。HMGB1 的旁分泌作用可以诱导趋化因子和 NO,这些物质被认为会改变人类 OA 软骨中的软骨稳态。
