Abstract

Muscle wasting occurs during aging, HIV infection, cancer, and numerous other pathological conditions, resulting in a significant decrease in quality of life and a financial burden of $18.5 billion in 2000. While 3D in vitro models of skin and lung tissue have proven essential in elucidating mechanisms of homeostasis and disease progression, analogous models of skeletal muscle do not exist. We propose a 3D model of primary human skeletal muscle that utilizes an engineered extracellular matrix (eECM), gradients of chemotactic cues, and cellular patterning. This collaborative proposal combines complementary expertise in cell microenvironment engineering and human muscle progenitor cell (hMuPC) and myoblast biology.
Aim 1 is to develop and optimize a 3D eECM to enhance the proliferation of hMuPCs. Previous results show that hMuPCs are critically responsive to the biochemistry and biomechanics of the microenvironment and have diminished proliferation and regeneration following 2D culture. Customized eECM will be made from a protein-engineered biomaterial that enables independent tuning of biomechanics (elastic moduli = 1-100 kPa) and cell-ligand density (0-100,000 ligands/micron3). Viability, proliferation, and myogenic differentiation of hMuPCs will be directly compared between 2D and 3D cultures utilizing identical eECM.
Aim 2 is to develop a 3D in vitro model of hMuPC migration. Little is known about the soluble cues that regulate hMuPC migration to sites of regeneration in vivo. Time-lapse imaging of hMuPC migration speed, directional persistence, and filopodia extension will be performed in a microfluidic device that enables the formation of stable concentration profiles. Migration will be compared on 2D and in 3D eECM in response to gradients and uniform concentrations of putative chemotactic cues. Migration in response to cell lysates from young (18-25 years old), old (60-80 years old), and dystrophic human skeletal muscle biopsies will be quantified to identify potential novel regulators of chemotaxis.
Aim 3 is to develop a 3D patterned mimic of human skeletal muscle tissue. Human myoblasts will be cultured on patterned eECM to induce myotube fusion and alignment. Fiber fusion rate, maturity, nuclear index, and alignment will be compared on eECM of varying pattern geometry, biomechanics, and biochemistry. Multiple sheets of aligned myotubes will be layered together with hMuPCs to create a dynamic model of regenerating muscle tissue.
These aims will lead to new 3D technologies for tissue culture, fundamental new insights in skeletal muscle biology, and potential new clinical therapies to activate hMuPCs and stimulate regeneration of muscle damaged during wasting and aging.

Public Health Relevance

Proposal Title: 3D Bioengineering Strategies to Mimic Human Skeletal Muscle Progenitor Cell Niches Relevance to Public Health: This proposal describes an innovative approach to enable the three-dimensional culture of primary human muscle tissue, which is impossible to achieve using current technologies. Our approach involves the design of a novel, tunable scaffold material and the engineering of a microfluidic device for 3D cultures. The ability to reproducibly culture 3D tissues outside of the body will enable scientists to develop high-throughput screens of pharmaceutical targets and to test new hypotheses and models of physiology and disease.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Arthritis and Musculoskeletal and Skin Diseases (NIAMS)
Type
Exploratory/Developmental Grants (R21)
Project #
1R21AR062359-01
Application #
8136875
Study Section
Special Emphasis Panel (ZHL1-CSR-N (M2))
Program Officer
Boyce, Amanda T
Project Start
2011-09-01
Project End
2013-08-31
Budget Start
2011-09-01
Budget End
2012-08-31
Support Year
1
Fiscal Year
2011
Total Cost
$201,324
Indirect Cost

  Institution

Name
Stanford University
Department
Engineering (All Types)
Type
Schools of Engineering
DUNS #
009214214
City
Stanford
State
CA
Country
United States
Zip Code
94305

  Publications

Raphel, Jordan; Holodniy, Mark; Goodman, Stuart B et al. (2016) Multifunctional coatings to simultaneously promote osseointegration and prevent infection of orthopaedic implants. Biomaterials 84:301-314
Raphel, Jordan; Karlsson, Johan; Galli, Silvia et al. (2016) Engineered protein coatings to improve the osseointegration of dental and orthopaedic implants. Biomaterials 83:269-82
Romano, Nicole H; Madl, Christopher M; Heilshorn, Sarah C (2015) Matrix RGD ligand density and L1CAM-mediated Schwann cell interactions synergistically enhance neurite outgrowth. Acta Biomater 11:48-57
Ferreira, Meghaan M; Dewi, Ruby E; Heilshorn, Sarah C (2015) Microfluidic analysis of extracellular matrix-bFGF crosstalk on primary human myoblast chemoproliferation, chemokinesis, and chemotaxis. Integr Biol (Camb) 7:569-79
Romano, Nicole H; Lampe, Kyle J; Xu, Hui et al. (2015) Microfluidic gradients reveal enhanced neurite outgrowth but impaired guidance within 3D matrices with high integrin ligand densities. Small 11:722-30
Wang, Huiyuan; Heilshorn, Sarah C (2015) Adaptable hydrogel networks with reversible linkages for tissue engineering. Adv Mater 27:3717-36
Xu, Hui; Ferreira, Meghaan M; Heilshorn, Sarah C (2014) Small-molecule axon-polarization studies enabled by a shear-free microfluidic gradient generator. Lab Chip 14:2047-56
Cai, Lei; Heilshorn, Sarah C (2014) Designing ECM-mimetic materials using protein engineering. Acta Biomater 10:1751-60
Wang, Huiyuan; Cai, Lei; Paul, Alexandra et al. (2014) Hybrid elastin-like polypeptide-polyethylene glycol (ELP-PEG) hydrogels with improved transparency and independent control of matrix mechanics and cell ligand density. Biomacromolecules 15:3421-8
Maška, Martin; Ulman, Vladimír; Svoboda, David et al. (2014) A benchmark for comparison of cell tracking algorithms. Bioinformatics 30:1609-17

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