Detecting cathepsin activity in human osteoarthritis via activity-based probes

被引:50
作者
Ben-Aderet, Louisa [1 ]
Merquiol, Emmanuelle [2 ]
Fahham, Duha [2 ]
Kumar, Ashok [1 ]
Reich, Eli [1 ]
Ben-Nun, Yael [2 ]
Kandel, Leonid [3 ]
Haze, Amir [3 ]
Liebergall, Meir [3 ]
Kosinska, Marta K. [4 ]
Steinmeyer, Juergen [4 ]
Turk, Boris [5 ]
Blum, Galia [2 ]
Dvir-Ginzberg, Mona [1 ]
机构
[1] Hebrew Univ Jerusalem, Inst Dent Sci, Lab Cartilage Biol, IL-9112001 Jerusalem, Israel
[2] Hebrew Univ Jerusalem, Inst Drug Res, Sch Pharm, IL-9112001 Jerusalem, Israel
[3] Hadassah Mt Scopus Hosp, Joint Replacement & Reconstruct Surg Unit, Jerusalem, Israel
[4] Univ Giessen, Dept Orthopaed, Lab Expt Orthopaed, D-35390 Giessen, Germany
[5] Jozef Stefan Inst, Dept Biochem & Mol & Struct Biol, Ljubljana, Slovenia
基金
欧盟第七框架计划;
关键词
CYSTEINE PROTEASE ACTIVITY; FEMORAL-HEAD CARTILAGE; RHEUMATOID-ARTHRITIS; MATRIX METALLOPROTEINASES; ARTICULAR-CARTILAGE; HUMAN CHONDROCYTES; EXPRESSION; SIRT1; PATHOPHYSIOLOGY; INHIBITION;
D O I
10.1186/s13075-015-0586-5
中图分类号
R5 [内科学];
学科分类号
100201 [内科学];
摘要
Introduction: Lysosomal cathepsins have been reported to contribute to Osteoarthritis (OA) pathophysiology due to their increase in pro-inflammatory conditions. Given the causal role of cathepsins in OA, monitoring their specific activity could provide means for assessing OA severity. To this end, we herein sought to assess a cathepsin activity-based probe (ABP), GB123, in vitro and in vivo. Methods: Protein levels and activity of cathepsins B and S were monitored by immunoblot analysis and GB123 labeling in cultured primary chondrocytes and conditioned media, following stimuli with tumor necrosis factor alpha (TNF alpha) and/or Interleukin 1 beta (IL-1 beta). Similarly, cathepsin activity was examined in sections of intact cartilage (IC) and degraded cartilage (DC) regions of OA. Finally, synovial fluid (SF) and serum from donors with no signs of diseases, early OA, late OA and rheumatoid arthritis (RA) patients were analyzed with GB123 to detect distinct activity levels of cathepsin B and S. Results: Cathepsin activity in cell lysates, conditioned media explants and DC sections showed enhanced enzymatic activity of cathepsins B and S. Further histological analysis revealed that cathepsin activity was found higher in superficial zones of DC than in IC. Examining serum and SF revealed that cathepsin B is significantly elevated with OA severity in serum and SF, yet levels of cathepsin S are more correlated with synovitis and RA. Conclusions: Based on our data, cathepsin activity monitored by ABPs correlated well with OA severity and joint inflammation, directing towards a novel etiological target for OA, which possesses significant translational potential in developing means for non-invasive detection of early signs of OA.
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页数:13
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