Proteomic characterization of mouse cartilage degradation in vitro

Wilson, Richard; Belluoccio, Daniele; Little, Christopher B.; Fosang, Amanda J.; Bateman, John F.

doi:10.1002/art.23789

Cited by 57 publications

(58 citation statements)

References 52 publications

(67 reference statements)

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“…In contrast, extraction with GuHCl results in greater representation of matrix components ( Fig. 4; Belluoccio et al, 2006;Wilson et al, 2008b). Sequential NaCl and GuHCl extraction can enrich sub-proteomes of interest and facilitate deeper mining of the cartilage proteome (Wilson and Bateman, 2008).…”

Section: Two-dimensional Electrophoresis: Sample Preparation Methodsmentioning

confidence: 92%

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Proteomics makes progress in cartilage and arthritis research

2009

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Section: Two-dimensional Electrophoresis: Sample Preparation Methodsmentioning

confidence: 92%

“…3). Proteolysis of CTGF is increased in IL-1 treated femoral heads, together with candidate proteases MMP-3 and MMP-13 (Wilson et al, 2008b). The CTGF expressed in OA cartilage and synovium may therefore be subject to post-translational regulation by MMPs (Smith et al, 2008).…”

Section: Proteomics Using Primary Chondrocytes and Cartilage Explantsmentioning

confidence: 93%

Proteomics makes progress in cartilage and arthritis research

2009

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“…Although proteomic changes conceivably underlie various skeletal malformation yet studying skeletal cell proteomics with respect to toxic substances has been limited. The preponderance of extracellular matrix (ECM) molecules such as collagens and highly anionic and nonhomogeneous proteoglycans which interfere with analytical procedures involving isoelectric focusing and 2D gel electrophoresis (Belluoccio et al, 2006;Wilson et al, 2008;Ruiz-Romero and Blanco, 2009;Gharbi et al, 2011). The cell culture system circumvents some of these problems by taking advantage of the fact that the ECM proteins are secreted into the culture media and those retained in the cell layer are much lower in concentration compared with in vivo obtained tissue proteins to interfere with 2D gel electrophoresis.…”

Section: Discussionmentioning

confidence: 99%

Effect of thiram on avian growth plate chondrocytes in culture

Rasaputra

Liyanage²,

Lay³

et al. 2013

J. Toxicol. Sci.

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-Thiram is a dithiocarbamate pesticide that causes tibial dyschondroplasia (TD), a growth plate defect, in poultry. Deaths of transitional zone chondrocytes appear to interrupt endochondral bone development leading to the broadening of growth plate. The mechanism of action of thiram on chondrocytes is not well understood. Since proteins play major roles in different aspects of cell's metabolism, growth, and survival, the objective of this study was to find whether thiram produces proteomic changes that could impair the development of chondrocytes. The chondrocytes, isolated from proximal tibial growth plates, were cultured with or without a sub-lethal concentration of thiram for 48 hr, and the cell proteins were extracted, and subjected to 2-D gel electrophoresis. The gel images were compared and statistically evaluated using Melanie software to identify differentially expressed protein spots. Of a total of 72 identifiable spots 3 were down-regulated and 2 up-regulated in thiram treated chondrocytes. In-gel trypsin digestion of the protein spots followed by their characterization by matrix-assisted laser desorption ionization-time-of-flight (MALDI-TOF) mass spectrometry identified 25 spots comprising of 23 proteins. Two of 3 down-regulated proteins were identified as a heat shock protein 70 (HSP 70) and a GALE (UDP-galactose-4 epimerase) protein isoform I. The up-regulated proteins were Serpin H1, a protein involved in collagen metabolism and a redox sensor NmrA-like (NMRAL) family domain protein-1. Both GALE and NMRAL proteins are implicated in energy metabolism and redox regulation whereas the HSP 70 protects cells against stress, and implicated in chondrocyte hypertrophy, an important event in endochondral bone formation. The failure of chondrocyte protective mechanisms such as associated with protection against cellular stress and energy metabolism appear to be the likely cause for chondrocyte death induced by thiram.

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“…41 THBS1 fragments were found in degenerated mouse cartilage and THBS2 functions as an endogenous regulator of inflammation in RA. 42,43 Taken together, expression of several genes coding for molecules involved in focal ahesions, ECM composition and ECM-receptor interaction was repressed in HSE stimulated alginate bead cultures.…”

Section: Human Alginate Bead Cultures As Part Of the Pannus Modelmentioning

confidence: 91%

Tissue‐engineered cartilage of porcine and human origin as in vitro test system in arthritis research

Göhring

Lübke

Andreas

et al. 2010

Biotechnology Progress

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The increasing prevalence of cartilage destruction during arthritis has entailed an intensified amount for in vitro cartilage models to analyze pathophysiological processes and to screen for antirheumatic drugs. Tissue engineering offers the opportunity to establish highly organized 3D cell cultures facilitating the formation of in vitro models that reflect the human situation. We report the comparison of porcine chondrocyte pellet and alginate bead cultures as model systems for human cartilage and the further development into a human system that was applied in an arthritis model. In porcine pellet and alginate cultures, formation of cartilage matrix similar to human matrix was verified by histology and PCR. As alginate beads could be cultivated batch-wise in one well of a multiwell plate, we further developed this setting into a human system. In contrast, each pellet had to be cultivated individually in one well of a multiwell plate, which is time consuming. Following stimulation of human chondrocyte alginate cultures with conditioned media from human synovial fibroblasts derived from arthritis patients, microarray analysis verified the induction of genes related to cartilage destruction (like MMP10, -12) and inflammation (like IL6, -8 and chemokines). Several genes are coding for proteins that are members of inflammatory and catabolic pathways. Belonging to the most affected pathways, we identified the focal adhesion, cytokine-cytokine receptor interaction, ECM-receptor signalling, Jak-STAT signalling, and toll-like receptor signalling pathways, all relevant in arthritis. Therefore, we demonstrate that engineered cartilage of porcine and human origin represents a powerful in vitro model for cartilage in vivo.

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Proteomic characterization of mouse cartilage degradation in vitro

Cited by 57 publications

References 52 publications

Proteomics makes progress in cartilage and arthritis research

Proteomics makes progress in cartilage and arthritis research

Effect of thiram on avian growth plate chondrocytes in culture

Tissue‐engineered cartilage of porcine and human origin as in vitro test system in arthritis research

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