Collagen integrity of the annulus fibrosus in degenerative disc disease individuals quantified with collagen hybridizing peptide

Author:

Dhiman Manmeet S.12ORCID,Bader Taylor J.23,Ponjevic Dragana24,Salo Paul T.25,Hart David A.256,Swamy Ganesh25ORCID,Matyas John R.24,Duncan Neil A.27

Affiliation:

1. Department of Biomedical Engineering University of Calgary Calgary Alberta Canada

2. McCaig Institute for Bone and Joint Health University of Calgary Calgary Alberta Canada

3. Department of Medical Sciences University of Calgary Calgary Alberta Canada

4. Faculty of Veterinary Medicine University of Calgary Calgary Alberta Canada

5. Department of Surgery, Cumming School of Medicine University of Calgary Calgary Alberta Canada

6. Faculty of Kinesiology University of Calgary Calgary Alberta Canada

7. Department of Civil Engineering University of Calgary Calgary Alberta Canada

Abstract

AbstractIntroductionDegenerative disc disease (DDD) is accompanied by structural changes in the intervertebral discs (IVD). Extra‐cellular matrix degradation of the annulus fibrosus (AF) has been linked with degeneration of the IVD. Collagen is a vital component of the IVD. Collagen hybridizing peptide (CHP) is an engineered protein that binds to degraded collagen, which we used to quantify collagen damage in AF. This method was used to compare AF samples obtained from donors with no DDD to AF samples from patients undergoing surgery for symptomatic DDD.MethodsFresh AF tissue was embedded in an optimal cutting temperature compound and cryosectioned at a thickness of 8 μm. Hematoxylin and Eosin staining was performed on sections for general histomorphological assessment. Serial sections were stained with Cy3‐conjugated CHP and the mean fluorescence intensity and areal fraction of Cy3‐positive staining were averaged for three regions of interest (ROI) on each CHP‐stained section.ResultsIncreases in mean fluorescence intensity (p = 0.0004) and percentage of positively stained area (p = 0.00008) with CHP were detected in DDD samples compared to the non‐DDD samples. Significant correlations were observed between mean fluorescence intensity and percentage of positively stained area for both non‐DDD (R = 0.98, p = 5E‐8) and DDD (R = 0.79, p = 0.0012) samples. No significant differences were detected between sex and the lumbar disc level subgroups of the non‐DDD and DDD groups. Only tissue pathology (non‐DDD versus DDD) influenced the measured parameters. No three‐way interactions between tissue pathology, sex, and lumbar disc level were observed.Discussion and ConclusionsThese findings suggest that AF collagen degradation is greater in DDD samples compared to non‐DDD samples, as evidenced by the increased CHP staining. Strong positive correlations between the two measured parameters suggest that when collagen degradation occurs, it is detected by this technique and is widespread throughout the tissue. This study provides new insights into the structural alterations associated with collagen degradation in the AF that occur during DDD.

Funder

Natural Sciences and Engineering Research Council of Canada

Publisher

Wiley

Reference57 articles.

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