PEER-REVIEWED PUBLICATION

2026

Nutrient deprivation of tendon-derived cells and its effect on collagen matrix integrity – mimicking graft remodelling after ACL reconstruction in vitro

Mansoor A K, Dekker S, et al.

Connective Tissue Research

Eindhoven University of Technology

RESEARCH SUMMARY
This study investigated whether the nutrient-poor environment experienced by tendon grafts after ACL reconstruction (and the presence of dead/dying cells in auto-/allografts) directly compromises collagen matrix integrity via a cell-driven catabolic response. Rat tendon-derived cells were embedded in reconstituted collagen type I to create in vitro “tendon-mimics” using a constrained culture system, then exposed for 7 days to media conditions designed to mimic post-surgical nutrient restriction: complete medium (5 mM glucose, 2.5% serum), mild deprivation (0.5 mM glucose, no serum), extreme deprivation (0 mM glucose, no serum), and a frozen control (freeze–thaw cycles plus 0 mM glucose, no serum). Cell viability (PI/DAPI, LDH), mimic compaction, collagen fiber alignment (collagen probe + confocal; orientation analysis), mechanics, and secreted/activated MMP activity (collagen/gelatin zymography) were quantified. While extreme deprivation and freezing significantly reduced viability, tendon-mimic mechanical properties did not deteriorate under nutrient deprivation or freezing; instead, only the complete medium group showed increased stiffness and failure stress over time, consistent with cell-driven compaction/remodeling when nutrients are available. Zymography showed no nutrient-deprivation–induced increase in catabolic enzymes; rather, higher active MMP2 and MMP8 signals were most evident in the complete medium condition, supporting the interpretation that nutrient-deprived viable cells lack the energy to generate contractile forces or produce/activate MMPs at levels that alter bulk mechanics. Overall, the work suggests that nutrient deprivation alone does not cause tendon-derived cells to compromise collagen matrix integrity in this simplified in vitro model, and that early graft weakening in vivo likely involves additional factors beyond direct resident-cell catabolism under starvation.

CELLSCALE INSTRUMENT USED

BioTester

Mechanical testing of the collagenous tendon-mimics was performed using a CellScale BioTester 5000 tensile tester equipped with a 0.5 N load cell to evaluate whether nutrient deprivation (or freeze–thaw) alters tissue-mimic mechanical integrity. After 7 days in the assigned culture conditions, mimic width was measured at three central locations, then mimics were cut from the Velcro anchors and tested immediately in uniaxial tension to failure. The test was run at a constant strain rate of 100% of the initial gauge length per minute (gauge length ≈4050 µm, visually corrected for tautness). Force–displacement data and images were recorded throughout. Cross-sectional area was estimated by assuming the measured width represented the diameter and calculating CSA = π(0.5D)^2, enabling conversion to stress–strain. Because the curves did not show a clear nonlinear toe region, apparent modulus was computed as the slope from the origin to the failure point. BioTester-derived modulus and failure stress demonstrated that nutrient deprivation and freezing did not reduce mechanical properties relative to baseline; only the complete-medium group showed improved stiffness/strength, supporting the conclusion that nutrient-deprived cells do not actively degrade or weaken the collagenous matrix under these conditions.
AUTHORS

Amal K. Mansoor, Sylvia Dekker, Keita Ito, Jasper Foolen.

PUBLICATION DETAILS
JOURNAL

Connective Tissue Research

YEAR

2026

INSTITUTIONS

Eindhoven University of Technology

COUNTRIES

Netherlands

INSTRUMENT USED

BioTester

TESTING METHODS

Tensile Testing

RESEARCH APPLICATIONS

Musculoskeletal Tissue Engineering & MechanicsTendon Tissue Engineering & Ligament Mechanics

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