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Induced superficial chondrocyte death reduces catabolic cartilage damage in murine posttraumatic osteoarthritis
Minjie Zhang, … , Gregory D. Jay, Matthew L. Warman
Minjie Zhang, … , Gregory D. Jay, Matthew L. Warman
Published July 18, 2016
Citation Information: J Clin Invest. 2016;126(8):2893-2902. https://doi.org/10.1172/JCI83676.
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Research Article Bone biology

Induced superficial chondrocyte death reduces catabolic cartilage damage in murine posttraumatic osteoarthritis

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Abstract

Joints that have degenerated as a result of aging or injury contain dead chondrocytes and damaged cartilage. Some studies have suggested that chondrocyte death precedes cartilage damage, but how the loss of chondrocytes affects cartilage integrity is not clear. In this study, we examined whether chondrocyte death undermines cartilage integrity in aging and injury using a rapid 3D confocal cartilage imaging technique coupled with standard histology. We induced autonomous expression of diphtheria toxin to kill articular surface chondrocytes in mice and determined that chondrocyte death did not lead to cartilage damage. Moreover, cartilage damage after surgical destabilization of the medial meniscus of the knee was increased in mice with intact chondrocytes compared with animals whose chondrocytes had been killed, suggesting that chondrocyte death does not drive cartilage damage in response to injury. These data imply that chondrocyte catabolism, not death, contributes to articular cartilage damage following injury. Therefore, therapies targeted at reducing the catabolic phenotype may protect against degenerative joint disease.

Authors

Minjie Zhang, Sriniwasan B. Mani, Yao He, Amber M. Hall, Lin Xu, Yefu Li, David Zurakowski, Gregory D. Jay, Matthew L. Warman

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Figure 2

DTA-induced killing of surface chondrocytes.

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DTA-induced killing of surface chondrocytes.
(A) Schematic depicting the...
(A) Schematic depicting the experimental timeline for inducing DTA-mediated cell death by administering tamoxifen from 21 to 30 days of age and then monitoring chondrocyte division by administering EdU from 31 to 40 days of age. Animals were analyzed after the final EdU dose. (B) Confocal images showing EdU-positive chondrocyte nuclei in a plane 20 μm below the surface of DAPI-stained femoral heads of a control mouse (Prg4CreERt2+R26mTmG/+ mouse) (left) and a DTA-ablated mouse (Prg4CreERt2/+R26mTmG/DTA mouse) (right). Note the decreased numbers of total (blue) and dividing (pink) chondrocyte nuclei in the DTA-ablated mouse. (C and D) Confocal femoral head images taken at different planar depths (10, 20, 30, and 40 μm) in control mice (C) and DTA-ablated mice (D) identify DAPI-stained chondrocyte nuclei (blue), nonrecombined membrane–anchored dTomato-expressing chondrocytes (red), and Cre-recombined membrane-anchored eGFP-expressing chondrocytes (green). Identical thresholds were employed for all images. Insets indicate DAPI windows (pseudocolored white) from a 100 μm × 100 μm area in the center of the image. (E and F) Bar graphs depicting the mean (± SD) values for chondrocyte density and chondrocyte number for the femoral (E) and humeral (F) heads of control (blue bars) and DTA-ablated (red bars) mice (n = 5). *P < 0.05, between control and DTA-ablated mice using Student’s t test. Scale bar: 100 μm.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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