Deferoxamine Suppresses Collagen Cleavage and Protease, Cytokine, and COL10A1 Expression and Upregulates AMPK and Krebs Cycle Genes in Human Osteoarthritic Cartilage

IF 2.3 Q2 RHEUMATOLOGY
E. Tchetina, G. Markova, A. Poole, D. Zukor, J. Antoniou, S. Makarov, A. N. Kuzin
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引用次数: 20

Abstract

This study reports the effects of the iron chelator deferoxamine (DFO) on collagen cleavage, inflammation, and chondrocyte hypertrophy in relation to energy metabolism-related gene expression in osteoarthritic (OA) articular cartilage. Full-depth explants of human OA knee articular cartilage from arthroplasty were cultured with exogenous DFO (1–50 μM). Type II collagen cleavage and phospho-adenosine monophosphate-activated protein kinase (pAMPK) concentrations were measured using ELISAs. Gene expression studies employed real-time PCR and included AMPK analyses in PBMCs. In OA explants collagen cleavage was frequently downregulated by 10–50 μM DFO. PCR analysis of 7 OA patient cartilages revealed that 10 μM DFO suppressed expression of MMP-1, MMP-13, IL-1β, and TNFα and a marker of chondrocyte hypertrophy, COL10A1. No changes were observed in the expression of glycolysis-related genes. In contrast, expressions of genes associated with the mitochondrial Krebs cycle (TCA), AMPK, HIF1α, and COL2A1 were upregulated. AMPK gene expression was reduced in OA cartilage and increased in PBMCs from the same patients compared to healthy controls. Our studies demonstrate that DFO is capable of suppressing excessive collagenase-mediated type II collagen cleavage in OA cartilage and reversing phenotypic changes. The concomitant upregulation of proanabolic TCA-related gene expressions points to a potential for availability of energy generating substrates required for matrix repair by end-stage OA chondrocytes. This might normally be prevented by high whole-body energy requirements indicated by elevated AMPK expression in PBMCs of OA patients.
去铁胺抑制人骨关节炎软骨中胶原裂解和蛋白酶、细胞因子和COL10A1的表达,上调AMPK和Krebs循环基因
本研究报道了铁螯合剂去铁胺(DFO)对骨性关节炎(OA)关节软骨中与能量代谢相关的基因表达有关的胶原裂解、炎症和软骨细胞肥大的影响。采用外源性DFO (1-50 μM)培养人工OA膝关节软骨。采用elisa法检测II型胶原裂解率和单磷酸磷酸腺苷活化蛋白激酶(pAMPK)浓度。基因表达研究采用实时荧光定量PCR,包括AMPK分析。在OA外植体中,10-50 μM的DFO经常下调胶原的裂解。对7例OA患者软骨的PCR分析显示,10 μM DFO抑制了MMP-1、MMP-13、IL-1β、tnf - α和软骨细胞肥大标志物COL10A1的表达。糖酵解相关基因的表达未见变化。相反,与线粒体克雷布斯循环(TCA)、AMPK、HIF1α和COL2A1相关的基因表达上调。与健康对照组相比,OA软骨中AMPK基因表达减少,而同一患者的pbmc中AMPK基因表达增加。我们的研究表明,DFO能够抑制OA软骨中过多的胶原酶介导的II型胶原裂解,并逆转表型变化。伴随的原合成代谢tca相关基因表达的上调表明,终末期OA软骨细胞有可能获得基质修复所需的能量生成底物。这通常可以通过OA患者pbmc中AMPK表达升高所指示的高全身能量需求来预防。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
CiteScore
4.40
自引率
0.00%
发文量
9
审稿时长
24 weeks
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