PEER-REVIEWED PUBLICATION

2024

Development of Muscle Tendon Junction in vitro Using Aligned Electrospun PCL Fibres

Iwasaki N, Roldo M, et al.

Engineered Regeneration

University of Portsmouth, Maastricht University (MERLN Institute for Technology-Inspired Regenerative Medicine)

RESEARCH SUMMARY
This study developed an in vitro muscle–tendon junction (MTJ) model using aligned electrospun polycaprolactone (PCL) fiber scaffolds to assess how cyclic tensile strain and muscle–tendon co-culture regulate MTJ-associated markers. Aligned PCL fibers were produced using a gap-collector electrospinning setup and collagen-coated to enhance cell adhesion. Human myoblasts and tenocytes were seeded on opposite sides of the same aligned fiber strip to create an interface model and cultured for 7 or 14 days with or without cyclic strain. Cyclic strain (10%,1 Hz) increased fiber alignment and significantly increased cell alignment relative to unstrained controls, and prolonged cyclic strain increased cell elongation (aspect ratio) at day 14. MTJ marker gene expression (COL22,PAX,TAL) was upregulated most strongly under combined co-culture plus cyclic strain, with COL22 and PAX significantly increased by day 7 and TAL increased by day 14. Immunofluorescence and quantitative mean fluorescence intensity analysis showed markedly higher collagen 22 and paxillin protein production under strained co-culture conditions (largest effects at day 14), and co-culture under strain produced higher MTJ-marker protein levels than strained mono-cultures. Overall, the data indicate that cyclic strain and muscle–tendon co-culture synergize to promote MTJ-like molecular signatures on aligned electrospun scaffolds.

CELLSCALE INSTRUMENT USED

MechanoCulture B1

A commercial CellScale MechanoCulture B1 (MCB1) tensile bioreactor was used to apply cyclic uniaxial strain to collagen-coated aligned electrospun PCL fiber constructs seeded with human myoblasts and tenocytes. After 24 h post-seeding, fiber strips were fixed into the bioreactor using a 24-pin mounting ring and cultured submerged in complete medium while receiving cyclic strain of approximately 10% at 1 Hz for 1 h/day for 7 or 14 days. This CellScale-enabled mechanical stimulation was the key experimental input used to quantify strain-driven changes in cell orientation and elongation, and to evaluate mechanoregulation of MTJ marker gene expression (COL22,PAX,TAL) and protein production (collagen 22 and paxillin) in mono-culture versus co-culture conditions.
AUTHORS

Nodoka Iwasaki, Marta Roldo, Aikaterina Karali, Alberto Sensini, Gordon Blunn.

PUBLICATION DETAILS
JOURNAL

Engineered Regeneration

YEAR

2024

INSTITUTIONS

University of Portsmouth, Maastricht University (MERLN Institute for Technology-Inspired Regenerative Medicine)

COUNTRIES

Netherlands, United Kingdom

INSTRUMENT USED

MechanoCulture B1

TESTING METHODS

Hydrated and Temperature Controlled TestingTensile Testing

RESEARCH APPLICATIONS

MechanotransductionSkeletal Muscle & Volumetric Muscle LossTendon Tissue Engineering & Ligament Mechanics

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