Targeting cathepsin L (CL) by specific ribozymes decreases CL protein synthesis and cartilage destruction in rheumatoid arthritis

J Schedel; C A Seemayer; T Pap; M Neidhart; S Kuchen; B A Michel; R E Gay; U Müller-Ladner; S Gay; W Zacharias

doi:10.1038/sj.gt.3302265

Targeting cathepsin L (CL) by specific ribozymes decreases CL protein synthesis and cartilage destruction in rheumatoid arthritis

Gene Ther. 2004 Jul;11(13):1040-7. doi: 10.1038/sj.gt.3302265.

Authors

J Schedel¹, C A Seemayer, T Pap, M Neidhart, S Kuchen, B A Michel, R E Gay, U Müller-Ladner, S Gay, W Zacharias

Affiliation

¹ Center of Experimental Rheumatology and WHO Collaborating Center for Molecular Biology and Novel Therapeutic Strategies for Rheumatic Diseases, Department of Rheumatology, University Hospital of Zurich, Zurich, Switzerland.

PMID: 15164093
DOI: 10.1038/sj.gt.3302265

Abstract

The present study was undertaken to examine whether ribozymes cleaving specifically cathepsin L (CL) mRNA are able to decrease the synthesis of CL protease in rheumatoid arthritis synovial fibroblasts (RA-SF) and thereby reduce the invasiveness into cartilage both in vitro and in the SCID mouse coimplantation model of RA. Two different ribozymes that cleave CL mRNA specifically at positions 533 (RzCL533) and 790 (RzCL790) were generated. Using retroviral gene transfer, RA-SF were transduced with the ribozyme constructs or the empty vector. To examine the effect of the ribozymes on the mRNA level, quantitative analysis for CL mRNA was performed using real-time PCR. For evaluation on the protein level, ELISA using specific anti-CL antibodies was performed. In addition, transduced RA-SF were examined in vitro in a three-dimensional destruction assay evaluating their ability to degrade extracellular matrix produced by human chondrocytes. Matrix destruction was monitored by the release of soluble glycosaminoglycans (sGAG). Using the in vivo SCID mouse coimplantation model of RA, RzCL533-transduced RA-SF and control cells were coimplanted with human cartilage for 60 days. After being killed, invasion of RA-SF into the cartilage was evaluated by using a semiquantitative score. Transduction of RA-SF with RzCL533 and RzCL790 ribozymes decreased significantly the expression of CL mRNA to 44% (range 25-62%) and 20% (range 1-43%), respectively, when compared to mock-transduced cells. The protein concentration of CL in the cell culture supernatants of transduced RA-SF was decreased from 16.0 ng/ml in the mock constructs to 4.1 and 8.2 ng/ml (mean), respectively. Using the in vitro cartilage destruction assay, the release of sGAG decreased to 46 and 60%, respectively, after 14 days when compared to mock-transduced cells. In the SCID mouse coimplantation model of RA, RzCL533-transduced RA-SF revealed a significant lower cartilage invasion when compared to mock and untransduced cells. Using retroviral gene transfer, ribozymes cleaving CL mRNA inhibit specifically the synthesis of this matrix-degrading enzyme and reduce cartilage destruction in in vitro and in vivo models. Our study therefore suggests that ribozymes targeting CL could be a novel and efficient tool to inhibit joint destruction in RA.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Arthritis, Rheumatoid / metabolism
Arthritis, Rheumatoid / pathology
Arthritis, Rheumatoid / therapy*
Cartilage, Articular / pathology
Cathepsin L
Cathepsins / biosynthesis
Cathepsins / genetics*
Cells, Cultured
Cysteine Endopeptidases
Fibroblasts / metabolism
Genetic Therapy / methods*
Humans
Mice
Mice, SCID
RNA, Catalytic / administration & dosage*
Synovial Membrane / metabolism
Transduction, Genetic / methods

Substances

RNA, Catalytic
Cathepsins
Cysteine Endopeptidases
CTSL protein, human
Cathepsin L
Ctsl protein, mouse