Pericellular heparan sulfate proteoglycans: Role in regulating the biosynthetic response of nucleus pulposus cells to osmotic loading

Carly M Krull; Jordan Rife; Brett Klamer; Devina Purmessur; Benjamin A Walter

doi:10.1002/jsp2.1209

Pericellular heparan sulfate proteoglycans: Role in regulating the biosynthetic response of nucleus pulposus cells to osmotic loading

JOR Spine. 2022 Jun 3;5(2):e1209. doi: 10.1002/jsp2.1209. eCollection 2022 Jun.

Authors

Carly M Krull¹, Jordan Rife¹, Brett Klamer², Devina Purmessur^{1

3

4}, Benjamin A Walter^{1

3

4}

Affiliations

¹ Department of Biomedical Engineering The Ohio State University Columbus Ohio USA.
² Department of Biomedical Informatics, Center for Biostatistics The Ohio State University Columbus Ohio USA.
³ Department of Orthopedics The Ohio State University Wexner Medical Center Columbus Ohio USA.
⁴ Spine Research Institute The Ohio State University Columbus Ohio USA.

Abstract

Background: Daily physiologic loading causes fluctuations in hydration of the intervertebral disc (IVD); thus, the embedded cells experience cyclic alterations to their osmotic environment. These osmotic fluctuations have been described as a mechanism linking mechanics and biology, and have previously been shown to promote biosynthesis in chondrocytes. However, this phenomenon has yet to be fully interrogated in the IVD. Additionally, the specialized extracellular matrix surrounding the cells, the pericellular matrix (PCM), transduces the biophysical signals that cells ultimately experience. While it is known that the PCM is altered in disc degeneration, whether it disrupts normal osmotic mechanotransduction has yet to be determined. Thus, our objectives were to assess: (1) whether dynamic osmotic conditions stimulate biosynthesis in nucleus pulposus cells, and (2) whether pericellular heparan sulfate proteoglycans (HSPGs) modulate the biosynthetic response to osmotic loading.

Methods: Bovine nucleus pulposus cells isolated with retained PCM were encapsulated in 1.5% alginate beads and treated with or without heparinase III, an enzyme that degrades the pericellular HSPGs. Beads were subjected to 1 h of daily iso-osmotic, hyper-osmotic, or hypo-osmotic loading for 1, 2, or 4 weeks. At each timepoint the total amount of extracellular and pericellular sGAG/DNA were quantified. Additionally, whether osmotic loading triggered alterations to HSPG sulfation was assessed via immunohistochemistry for the heparan sulfate 6-O-sulfertransferase 1 (HS6ST1) enzyme.

Results: Osmotic loading significantly influenced sGAG/DNA accumulation with a hyper-osmotic change promoting the greatest sGAG/DNA accumulation in the pericellular region compared with iso-osmotic conditions. Heparanase-III treatment significantly reduced extracellular sGAG/DNA but pericellular sGAG was not affected. HS6ST1 expression was not affected by osmotic loading.

Conclusion: Results suggest that hyper-osmotic loading promotes matrix synthesis and that modifications to HSPGs directly influence the metabolic responses of cells to osmotic fluctuations. Collectively, results suggest degeneration-associated modifications to pericellular HSPGs may contribute to the altered mechanobiology observed in disease.

Keywords: heparan sulfate proteoglycan; intervertebral disc; mechanotransduction; nucleus pulposus; osmotic; pericellular matrix.

Grants and funding

R21 AR076611/AR/NIAMS NIH HHS/United States