Your search keyword '"Pedro J. Díaz‐Payno"' showing total 17 results

1. Emergent collective organization of bone cells in complex curvature fields

Author

Sebastien J. P. Callens, Daniel Fan, Ingmar A. J. van Hengel, Michelle Minneboo, Pedro J. Díaz-Payno, Molly M. Stevens, Lidy E. Fratila-Apachitei, and Amir A. Zadpoor

Subjects

Science

Abstract

It remains unclear how cells respond to complex extracellular geometries at the mesoscale. Here, the authors study the organization of bone cells in landscapes with varying curvatures, observing a preference for local concavities, multicellular bridging, and collective stress fiber orientation.

Published

2023

2. Mechanotransduction in high aspect ratio nanostructured meta-biomaterials: The role of cell adhesion, contractility, and transcriptional factors

Author

Khashayar Modaresifar, Mahya Ganjian, Pedro J. Díaz-Payno, Maria Klimopoulou, Marijke Koedam, Bram C.J. van der Eerden, Lidy E. Fratila-Apachitei, and Amir A. Zadpoor

Subjects

High aspect ratio nanopillars, Osteogenic response, Mechanotransduction, Focal adhesion kinase, Rho-associated protein kinase, Yes-associated protein, Medicine (General), R5-920, Biology (General), QH301-705.5

Abstract

Black Ti (bTi) surfaces comprising high aspect ratio nanopillars exhibit a rare combination of bactericidal and osteogenic properties, framing them as cell-instructive meta-biomaterials. Despite the existing data indicating that bTi surfaces induce osteogenic differentiation in cells, the mechanisms by which this response is regulated are not fully understood. Here, we hypothesized that high aspect ratio bTi nanopillars regulate cell adhesion, contractility, and nuclear translocation of transcriptional factors, thereby inducing an osteogenic response in the cells. Upon the observation of significant changes in the morphological characteristics, nuclear localization of Yes-associated protein (YAP), and Runt-related transcription factor 2 (Runx2) expression in the human bone marrow-derived mesenchymal stem cells (hMSCs), we inhibited focal adhesion kinase (FAK), Rho-associated protein kinase (ROCK), and YAP in separate experiments to elucidate their effects on the subsequent expression of Runx2. Our findings indicated that the increased expression of Runx2 in the cells residing on the bTi nanopillars compared to the flat Ti is highly dependent on the activity of FAK and ROCK. A mechanotransduction pathway is then postulated in which the FAK-dependent adhesion of cells to the extreme topography of the surface is in close relation with ROCK to increase the endogenous forces within the cells, eventually determining the cell shape and area. The nuclear translocation of YAP may also enhance in response to the changes in cell shape and area, resulting in the translation of mechanical stimuli to biochemical factors such as Runx2.

Published

2022

3. Promoting endogenous articular cartilage regeneration using extracellular matrix scaffolds

Author

David C. Browe, Ross Burdis, Pedro J. Díaz-Payno, Fiona E. Freeman, Jessica M. Nulty, Conor T. Buckley, Pieter A.J. Brama, and Daniel J. Kelly

Subjects

Cartilage repair, ECM scaffold, Large animal model, Microfracture, Fixation device, Medicine (General), R5-920, Biology (General), QH301-705.5

Abstract

Articular cartilage defects fail to heal spontaneously, typically progressing to osteoarthritis. Bone marrow stimulation techniques such as microfracture (MFX) are the current surgical standard of care; however MFX typically produces an inferior fibro-cartilaginous tissue which provides only temporary symptomatic relief. Here we implanted solubilised articular cartilage extracellular matrix (ECM) derived scaffolds into critically sized chondral defects in goats, securely anchoring these implants to the joint surface using a 3D-printed fixation device that overcame the need for sutures or glues. In vitro these ECM scaffolds were found to be inherently chondro-inductive, while in vivo they promoted superior articular cartilage regeneration compared to microfracture. In an attempt to further improve the quality of repair, we loaded these scaffolds with a known chemotactic factor, transforming growth factor (TGF)-β3. In vivo such TGF-β3 loaded scaffolds promoted superior articular cartilage regeneration. This study demonstrates that ECM derived biomaterials, either alone and particularly when combined with exogenous growth factors, can successfully treat articular cartilage defects in a clinically relevant large animal model.

Published

2022

4. Bioprinting of a Zonal-Specific Cell Density Scaffold: A Biomimetic Approach for Cartilage Tissue Engineering

Author

Angeliki Dimaraki, Pedro J. Díaz-Payno, Michelle Minneboo, Mahdiyeh Nouri-Goushki, Maryam Hosseini, Nicole Kops, Roberto Narcisi, Mohammad J. Mirzaali, Gerjo J. V. M. van Osch, Lidy E. Fratila-Apachitei, and Amir A. Zadpoor

Subjects

bioprinting, biofabrication, tissue engineering, articular cartilage, human chondrocytes, cell density, Technology, Engineering (General). Civil engineering (General), TA1-2040, Biology (General), QH301-705.5, Physics, QC1-999, Chemistry, QD1-999

Abstract

The treatment of articular cartilage defects remains a significant clinical challenge. This is partially due to current tissue engineering strategies failing to recapitulate native organization. Articular cartilage is a graded tissue with three layers exhibiting different cell densities: the superficial zone having the highest density and the deep zone having the lowest density. However, the introduction of cell gradients for cartilage tissue engineering, which could promote a more biomimetic environment, has not been widely explored. Here, we aimed to bioprint a scaffold with different zonal cell densities to mimic the organization of articular cartilage. The scaffold was bioprinted using an alginate-based bioink containing human articular chondrocytes. The scaffold design included three cell densities, one per zone: 20 × 106 (superficial), 10 × 106 (middle), and 5 × 106 (deep) cells/mL. The scaffold was cultured in a chondrogenic medium for 25 days and analyzed by live/dead assay and histology. The live/dead analysis showed the ability to generate a zonal cell density with high viability. Histological analysis revealed a smooth transition between the zones in terms of cell distribution and a higher sulphated glycosaminoglycan deposition in the highest cell density zone. These findings pave the way toward bioprinting complex zonal cartilage scaffolds as single units, thereby advancing the translation of cartilage tissue engineering into clinical practice.

Published

2021

5. Gremlin-1 Suppresses Hypertrophy of Engineered Cartilage In Vitro but Not Bone Formation In Vivo

Author

Pedro J. Díaz-Payno, David C. Browe, Fiona E. Freeman, Jessica Nulty, Ross Burdis, and Daniel J. Kelly

Subjects

Biomaterials, Biomedical Engineering, Bioengineering, Biochemistry

Published

2022

6. Bilayered extracellular matrix derived scaffolds with anisotropic pore architecture guide tissue organization during osteochondral defect repair

Author

David C. Browe, Pedro J. Díaz-Payno, Fiona E. Freeman, Rossana Schipani, Ross Burdis, Daniel P. Ahern, Jessica M. Nulty, Selcan Guler, Lindsey D. Randall, Conor T. Buckley, Pieter A.J. Brama, and Daniel J. Kelly

Subjects

Cartilage, Articular, History, Tissue Engineering, Tissue Scaffolds, Polymers and Plastics, Biomedical Engineering, Biocompatible Materials, General Medicine, Biochemistry, Industrial and Manufacturing Engineering, Extracellular Matrix, Biomaterials, Animals, Collagen, Business and International Management, Chondrogenesis, Molecular Biology, Biotechnology

Abstract

While some clinical advances in cartilage repair have occurred, osteochondral (OC) defect repair remains a significant challenge, with current scaffold-based approaches failing to recapitulate the complex, hierarchical structure of native articular cartilage (AC). To address this need, we fabricated bilayered extracellular matrix (ECM)-derived scaffolds with aligned pore architectures. By modifying the freeze-drying kinetics and controlling the direction of heat transfer during freezing, it was possible to produce anisotropic scaffolds with larger pores which supported homogenous cellular infiltration and improved sulfated glycosaminoglycan deposition. Neo-tissue organization in vitro could also be controlled by altering scaffold pore architecture, with collagen fibres aligning parallel to the long-axis of the pores within scaffolds containing aligned pore networks. Furthermore, we used in vitro and in vivo assays to demonstrate that AC and bone ECM derived scaffolds could preferentially direct the differentiation of mesenchymal stromal cells (MSCs) towards either a chondrogenic or osteogenic lineage respectively, enabling the development of bilayered ECM scaffolds capable of spatially supporting unique tissue phenotypes. Finally, we implanted these scaffolds into a large animal model of OC defect repair. After 6 months in vivo, scaffold implantation was found to improve cartilage matrix deposition, with collagen fibres preferentially aligning parallel to the long axis of the scaffold pores, resulting in a repair tissue that structurally and compositionally was more hyaline-like in nature. These results demonstrate how scaffold architecture and composition can be spatially modulated to direct the regeneration of complex interfaces such as the osteochondral unit, enabling their use as cell-free, off-the-shelf implants for joint regeneration. STATEMENT OF SIGNIFICANCE: The architecture of the extracellular matrix, while integral to tissue function, is often neglected in the design and evaluation of regenerative biomaterials. In this study we developed a bilayered scaffold for osteochondral defect repair consisting of tissue-specific extracellular matrix (ECM)-derived biomaterials to spatially direct stem/progenitor cell differentiation, with a tailored pore microarchitecture to promote the development of a repair tissue that recapitulates the hierarchical structure of native AC. The use of this bilayered scaffold resulted in improved tissue repair outcomes in a large animal model, specifically the ability to guide neo-tissue organization and therefore recapitulate key aspects of the zonal structure of native articular cartilage. These bilayer scaffolds have the potential to become a new therapeutic option for osteochondral defect repair.

Published

2022

7. Affinity-bound growth factor within sulfated interpenetrating network bioinks for bioprinting cartilaginous tissues

Author

Jessica Nulty, Pedro J. Díaz-Payno, Daniel J. Kelly, Fiona E. Freeman, Bin Wang, David C. Browe, and Ross Burdis

Subjects

Cartilage, Articular, Swine, 0206 medical engineering, Biomedical Engineering, Mice, Nude, 02 engineering and technology, Biochemistry, Regenerative medicine, law.invention, Biomaterials, Extracellular matrix, Transforming Growth Factor beta3, Tissue engineering, law, Cartilaginous Tissue, Animals, Molecular Biology, Mice, Inbred BALB C, 3D bioprinting, Tissue Engineering, Tissue Scaffolds, Sulfates, Chemistry, Regeneration (biology), Mesenchymal stem cell, Bioprinting, General Medicine, 021001 nanoscience & nanotechnology, Chondrogenesis, 020601 biomedical engineering, Cell biology, Printing, Three-Dimensional, 0210 nano-technology, Biotechnology

Abstract

3D bioprinting has emerged as a promising technology in the field of tissue engineering and regenerative medicine due to its ability to create anatomically complex tissue substitutes. However, it still remains challenging to develop bioactive bioinks that provide appropriate and permissive environments to instruct and guide the regenerative process in vitro and in vivo. In this study alginate sulfate, a sulfated glycosaminoglycan (sGAG) mimic, was used to functionalize an alginate-gelatin methacryloyl (GelMA) interpenetrating network (IPN) bioink to enable the bioprinting of cartilaginous tissues. The inclusion of alginate sulfate had a limited influence on the viscosity, shear-thinning and thixotropic properties of the IPN bioink, enabling high-fidelity bioprinting and supporting mesenchymal stem cell (MSC) viability post-printing. The stiffness of printed IPN constructs greatly exceeded that achieved by printing alginate or GelMA alone, while maintaining resilience and toughness. Furthermore, given the high affinity of alginate sulfate to heparin-binding growth factors, the sulfated IPN bioink supported the sustained release of transforming growth factor-β3 (TGF-β3), providing an environment that supported robust chondrogenesis in vitro, with little evidence of hypertrophy or mineralization over extended culture periods. Such bioprinted constructs also supported chondrogenesis in vivo, with the controlled release of TGF-β3 promoting significantly higher levels of cartilage-specific extracellular matrix deposition. Altogether, these results demonstrate the potential of bioprinting sulfated bioinks as part of a 'single-stage' or 'point-of-care' strategy for regenerating cartilaginous tissues. STATEMENT OF SIGNIFICANCE: This study highlights the potential of using sulfated interpenetrating network (IPN) bioink to support the regeneration of phenotypically stable articular cartilage. Construction of interpenetrating networks in the bioink enables unique high-fidelity bioprinting and provides synergistic increases in mechanical properties. The presence of alginate sulfate enables the capacity of high affinity-binding of TGF-β3, which promoted robust chondrogenesis in vitro and in vivo.

Published

2021

8. 3D printing of fibre-reinforced cartilaginous templates for the regeneration of osteochondral defects

Author

Eamon J. Sheehy, Pedro J. Díaz-Payno, Eben Alsberg, Pieter A.J. Brama, Daniel J. Kelly, Gráinne M. Cunniffe, Susan E. Critchley, Simon F. Carroll, and Oju Jeon

Subjects

Cartilage, Articular, Bone Regeneration, 0206 medical engineering, Biomedical Engineering, Mice, Nude, 02 engineering and technology, Biochemistry, Biomaterials, Mice, Tissue engineering, medicine, Animals, Molecular Biology, Endochondral ossification, Tissue Engineering, Tissue Scaffolds, Infrapatellar fat pad, Chemistry, Goats, Regeneration (biology), Cartilage, Mesenchymal stem cell, General Medicine, 021001 nanoscience & nanotechnology, Chondrogenesis, 020601 biomedical engineering, medicine.anatomical_structure, Printing, Three-Dimensional, 0210 nano-technology, Biotechnology, Biofabrication, Biomedical engineering

Abstract

Successful osteochondral defect repair requires regenerating the subchondral bone whilst simultaneously promoting the development of an overlying layer of articular cartilage that is resistant to vascularization and endochondral ossification. During skeletal development articular cartilage also functions as a surface growth plate, which postnatally is replaced by a more spatially complex bone-cartilage interface. Motivated by this developmental process, the hypothesis of this study is that bi-phasic, fibre-reinforced cartilaginous templates can regenerate both the articular cartilage and subchondral bone within osteochondral defects created in caprine joints. To engineer mechanically competent implants, we first compared a range of 3D printed fibre networks (PCL, PLA and PLGA) for their capacity to mechanically reinforce alginate hydrogels whilst simultaneously supporting mesenchymal stem cell (MSC) chondrogenesis in vitro. These mechanically reinforced, MSC-laden alginate hydrogels were then used to engineer the endochondral bone forming phase of bi-phasic osteochondral constructs, with the overlying chondral phase consisting of cartilage tissue engineered using a co-culture of infrapatellar fat pad derived stem/stromal cells (FPSCs) and chondrocytes. Following chondrogenic priming and subcutaneous implantation in nude mice, these bi-phasic cartilaginous constructs were found to support the development of vascularised endochondral bone overlaid by phenotypically stable cartilage. These fibre-reinforced, bi-phasic cartilaginous templates were then evaluated in clinically relevant, large animal (caprine) model of osteochondral defect repair. Although the quality of repair was variable from animal-to-animal, in general more hyaline-like cartilage repair was observed after 6 months in animals treated with bi-phasic constructs compared to animals treated with commercial control scaffolds. This variability in the quality of repair points to the need for further improvements in the design of 3D bioprinted implants for joint regeneration. STATEMENT OF SIGNIFICANCE: Successful osteochondral defect repair requires regenerating the subchondral bone whilst simultaneously promoting the development of an overlying layer of articular cartilage. In this study, we hypothesised that bi-phasic, fibre-reinforced cartilaginous templates could be leveraged to regenerate both the articular cartilage and subchondral bone within osteochondral defects. To this end we used 3D printed fibre networks to mechanically reinforce engineered transient cartilage, which also contained an overlying layer of phenotypically stable cartilage engineered using a co-culture of chondrocytes and stem cells. When chondrogenically primed and implanted into caprine osteochondral defects, these fibre-reinforced bi-phasic cartilaginous grafts were shown to spatially direct tissue development during joint repair. Such developmentally inspired tissue engineering strategies, enabled by advances in biofabrication and 3D printing, could form the basis of new classes of regenerative implants in orthopaedic medicine.

Published

2020

9. The identification of articular cartilage and growth plate extracellular matrix-specific proteins supportive of either osteogenesis or stable chondrogenesis of stem cells

Author

Daniel J. Kelly, Pedro J. Díaz-Payno, David C. Browe, and Gráinne M. Cunniffe

Subjects

Cartilage, Articular, 0301 basic medicine, Swine, Biophysics, Stimulation, Biochemistry, Regenerative medicine, Extracellular matrix, 03 medical and health sciences, 0302 clinical medicine, Osteogenesis, medicine, Animals, Growth Plate, Molecular Biology, Extracellular Matrix Proteins, biology, Chemistry, Cartilage, S100A10, Lectin, Mesenchymal Stem Cells, Hypertrophy, Cell Biology, Chondrogenesis, 3. Good health, Cell biology, 030104 developmental biology, medicine.anatomical_structure, 030220 oncology & carcinogenesis, biology.protein, Stem cell

Abstract

Tissue-specific extracellular matrix (ECM) proteins can play a key role in regulating the fate of stem cells and can potentially be utilized for therapeutic applications. Realising this potential requires further characterization of the diversity of biomolecules present in tissue-specific ECMs and an evaluation of their role as regulatory cues for regenerative medicine applications. The goal of this study was to identify specific soluble factors within the ECM of articular cartilage (AC) and growth plate (GP) that may impart chondro-inductivity or osteo-inductivity respectively. To this end, the significantly different proteins between both matrisomes were searched against the STRING database platform, from which C-type lectin domain family-11 member-A (CLEC11A) and S100 calcium-binding protein-A10 (S100A10) were identified as potential candidates for supporting osteogenesis, and Gremlin-1 (GREM1) and TGF-β induced gene human clone-3 (βIGH3) were identified as potential candidates for supporting stable chondrogenesis. Stimulation of chondrogenically-primed bone marrow-derived stem cells (BMSCs) with the AC-specific proteins GREM1 and βIGH3 had no noticeable effect on the deposition of collagen-II, a marker of chondrogenesis, but appeared to suppress the production of the hypertrophic marker collagen-X, particularly for higher concentrations of GREM1. Stimulation with GREM1 was also found to suppress the direct osteoblastic differentiation of BMSCs. In contrast, stimulation with the GP-specific factors CLEC11A and S100A10 was found to enhance osteogenesis of BMSCs, increasing the levels of mineralization, particularly for higher concentration of CLEC11A. Together these results demonstrate that AC- and GP-specific proteins may play a key role in developing novel strategies for engineering phenotypically stable articular cartilage or enhancing the regeneration of critically-sized bone defects.

Published

2020

10. Swelling-Dependent Shape-Based Transformation of a Human Mesenchymal Stromal Cells-Laden 4D Bioprinted Construct for Cartilage Tissue Engineering

Author

Pedro J. Díaz‐Payno, Maria Kalogeropoulou, Iain Muntz, Esther Kingma, Nicole Kops, Matteo D'Este, Gijsje H. Koenderink, Lidy E. Fratila‐Apachitei, Gerjo J. V. M. van Osch, Amir A. Zadpoor, Orthopedics and Sports Medicine, and Otorhinolaryngology and Head and Neck Surgery

Subjects

Biomaterials, 4D bioprinting, biofabrication, tissue engineering, shape-change, Biomedical Engineering, Pharmaceutical Science, smart bioinks

Abstract

3D bioprinting is usually implemented on flat surfaces, posing serious limitations in the fabrication of multilayered curved constructs. 4D bioprinting, combining 3D bioprinting with time-dependent stimuli-induced transformation, enables the fabrication of shape-changing constructs. Here, a 4D biofabrication method is reported for cartilage engineering based on the differential swelling of a smart multi-material system made from two hydrogel-based materials: hyaluronan and alginate. Two ink formulations are used: tyramine-functionalized hyaluronan (HAT, high-swelling) and alginate with HAT (AHAT, low-swelling). Both inks have similar elastic, shear-thinning, and printability behavior. The inks are 3D printed into a bilayered scaffold before triggering the shape-change by using liquid immersion as stimulus. In time (4D), the differential swelling between the two zones leads to the scaffold's self-bending. Different designs are made to tune the radius of curvature and shape. A bioprinted formulation of AHAT and human bone marrow cells demonstrates high cell viability. After 28 days in chondrogenic medium, the curvature is clearly present while cartilage-like matrix production is visible on histology. A proof-of-concept of the recently emerged technology of 4D bioprinting with a specific application for the design of curved structures potentially mimicking the curvature and multilayer cellular nature of native cartilage is demonstrated.

Published

2022

11. Biomimetic Approaches for the Design and Fabrication of Bone-to-Soft Tissue Interfaces

Author

Pedro J. Díaz-Payno, Niko Eka Putra, Sara Panahkhahi, Amir A. Zadpoor, Carlos Pitta Kruize, Mohammad J. Mirzaali, and Gerjo J.V.M. van Osch

Subjects

Materials science, Fabrication, Gradual transition, Natural user interface, business.industry, Regeneration (biology), Biomedical Engineering, Soft tissue, 3D printing, Nanotechnology, Biomaterials, Biomimetics, business, Interlocking

Abstract

Bone-to-soft tissue interfaces are responsible for transferring loads between tissues with significantly dissimilar material properties. The examples of connective soft tissues are ligaments, tendons, and cartilages. Such natural tissue interfaces have unique microstructural properties and characteristics which avoid the abrupt transitions between two tissues and prevent formation of stress concentration at their connections. Here, we review some of the important characteristics of these natural interfaces. The native bone-to-soft tissue interfaces consist of several hierarchical levels which are formed in a highly specialized anisotropic fashion and are composed of different types of heterogeneously distributed cells. The characteristics of a natural interface can rely on two main design principles, namely by changing the local microarchitectural features (e.g., complex cell arrangements, and introducing interlocking mechanisms at the interfaces through various geometrical designs) and changing the local chemical compositions (e.g., a smooth and gradual transition in the level of mineralization). Implementing such design principles appears to be a promising approach that can be used in the design, reconstruction, and regeneration of engineered biomimetic tissue interfaces. Furthermore, prominent fabrication techniques such as additive manufacturing (AM) including 3D printing and electrospinning can be used to ease these implementation processes. Biomimetic interfaces have several biological applications, for example, to create synthetic scaffolds for osteochondral tissue repair.

Published

2021

12. Regeneration of Osteochondral Defects Using Developmentally Inspired Cartilaginous Templates

Author

Rossana Schipani, Jung-Youn Shin, Aidan McAlinden, Daniel J. Kelly, Pedro J. Díaz-Payno, Daniel Withers, Eben Alsberg, Gráinne M. Cunniffe, Susan E. Critchley, and Adam O'Reilly

Subjects

Cartilage, Articular, 0206 medical engineering, Biomedical Engineering, Bioengineering, 02 engineering and technology, Biology, Mesenchymal Stem Cell Transplantation, Biochemistry, Bone and Bones, Biomaterials, 03 medical and health sciences, Tissue engineering, Animals, Regeneration, Endochondral ossification, 030304 developmental biology, 0303 health sciences, Regeneration (biology), Mesenchymal stem cell, Mesenchymal Stem Cells, Chondrogenesis, 020601 biomedical engineering, Cell biology, Female, Rabbits

Abstract

Successfully treating osteochondral defects involves regenerating both the damaged articular cartilage and the underlying subchondral bone, in addition to the complex interface that separates these tissues. In this study, we demonstrate that a cartilage template, engineered using bone marrow-derived mesenchymal stem cells, can enhance the regeneration of such defects and promote the development of a more mechanically functional repair tissue. We also use a computational mechanobiological model to understand how joint-specific environmental factors, specifically oxygen levels and tissue strains, regulate the conversion of the engineered template into cartilage and bone in vivo.

Published

2019

13. Tissue-specific extracellular matrix scaffolds for the regeneration of spatially complex musculoskeletal tissues

Author

Tanya J. Levingstone, Fergal J. O'Brien, Eamon J. Sheehy, Conor J. Moran, Daniel J. Kelly, Olwyn R. Mahon, Pedro J. Díaz-Payno, Pierluca Pitacco, Aisling Dunne, Pieter A.J. Brama, Simon F. Carroll, Gráinne M. Cunniffe, Robert T. Brady, Susan E. Critchley, and Henrique V. Almeida

Subjects

Cartilage, Articular, Scaffold, Swine, Cellular differentiation, Biophysics, Biocompatible Materials, Bioengineering, 02 engineering and technology, Biomaterials, Extracellular matrix, 03 medical and health sciences, Osteogenesis, medicine, Animals, Regeneration, Growth Plate, Cells, Cultured, 030304 developmental biology, 0303 health sciences, Tissue Engineering, Tissue Scaffolds, Hyaline cartilage, Chemistry, Goats, Cartilage, Regeneration (biology), Soft tissue, Cell Differentiation, Mesenchymal Stem Cells, 021001 nanoscience & nanotechnology, Extracellular Matrix, Cell biology, medicine.anatomical_structure, Mechanics of Materials, Ceramics and Composites, 0210 nano-technology, Chondrogenesis, Adult stem cell

Abstract

Biological scaffolds generated from tissue-derived extracellular matrix (ECM) are commonly used clinically for soft tissue regeneration. Such biomaterials can enhance tissue-specific differentiation of adult stem cells, suggesting that structuring different ECMs into multi-layered scaffolds can form the basis of new strategies for regenerating damaged interfacial tissues such as the osteochondral unit. In this study, mass spectrometry is used to demonstrate that growth plate (GP) and articular cartilage (AC) ECMs contain a unique array of regulatory proteins that may be particularly suited to bone and cartilage repair respectively. Applying a novel iterative freeze-drying method, porous bi-phasic scaffolds composed of GP ECM overlaid by AC ECM are fabricated, which are capable of spatially directing stem cell differentiation in vitro, promoting the development of graded tissues transitioning from calcified cartilage to hyaline-like cartilage. Evaluating repair 12-months post-implantation into critically-sized caprine osteochondral defects reveals that these scaffolds promote regeneration in a manner distinct to commercial control-scaffolds. The GP layer supports endochondral bone formation, while the AC layer stimulates the formation of an overlying layer of hyaline cartilage with a collagen fiber architecture better recapitulating the native tissue. These findings support the use of a bi-layered, tissue-specific ECM derived scaffolds for regenerating spatially complex musculoskeletal tissues.

Published

2019

14. Affinity-Bound Growth Factor within Sulfated Interpenetrate Network Bioinks for Bioprinting Cartilaginous Tissues

Author

Pedro J. Díaz-Payno, Jessica Nulty, Bin Wang, Ross Burdis, Daniel J. Kelly, David C. Browe, and Fiona E. Freeman

Subjects

Extracellular matrix, 3D bioprinting, Tissue engineering, Chemistry, law, Mesenchymal stem cell, Cartilaginous Tissue, Chondrogenesis, Controlled release, Regenerative medicine, Cell biology, law.invention

Abstract

3D bioprinting has emerged as a promising technology in the field of tissue engineering and regenerative medicine due to its ability to create anatomically complex tissue substitutes. However, it still remains challenging to develop bioactive bioinks that provide appropriate and permissive environments to instruct and guide the regenerative process in vitro and in vivo. In this study alginate sulfate, a sulfated glycosaminoglycan (sGAG) mimic, was used to functionalize an alginate-gelatin methacryloyl (GelMA) interpenetrating network (IPN) bioink to enable the bioprinting of cartilaginous tissues. The inclusion of alginate sulfate had a limited influence on the viscosity, shear-thinning and thixotropic properties of the IPN bioink, enabling high-fidelity bioprinting and supporting mesenchymal stem cell (MSC) viability post-printing. The stiffness of printed IPN constructs greatly exceeded that achieved by printing alginate or GelMA alone, while maintaining resilience and toughness. Furthermore, given the high affinity of alginate sulfate to heparin-binding growth factors, the sulfated IPN bioink supported the sustained release of transforming growth factor-β3 (TGF-β3), providing an environment that supported robust chondrogenesis in vitro, with little evidence of hypertrophy or mineralization over extended culture periods. Such bioprinted constructs also supported chondrogenesis in vivo, with the controlled release of TGF-β3 promoting significantly higher levels of cartilage-specific extracellular matrix deposition. Altogether, these results demonstrate the potential of bioprinting sulfated bioinks as part of a ‘single-stage’ or ‘point-of-care’ strategy for regenerating cartilaginous tissues.

Published

2020

15. Extracellular matrix scaffolds derived from different musculoskeletal tissues drive distinct macrophage phenotypes and direct tissue-specific cellular differentiation

Author

Olwyn R. Mahon, Pedro J. Díaz-Payno, Kyle T. Cunningham, Kingston H. G. Mills, Aisling Dunne, Pierluca Pitacco, Daniel J. Kelly, and David C. Browe

Subjects

0301 basic medicine, Stromal cell, Chemistry, Regeneration (biology), Cellular differentiation, 0206 medical engineering, Mesenchymal stem cell, 02 engineering and technology, M2 Macrophage, 020601 biomedical engineering, Cell biology, Extracellular matrix, 03 medical and health sciences, 030104 developmental biology, Macrophage, Stem cell

Abstract

The host immune response, specifically macrophage function, is a critical determinant of biomaterial success or failure post-implantation. Extracellular matrix (ECM) derived scaffolds have been shown to promote a pro-regenerative macrophage phenotype and a more constructive remodelling outcome. Here we demonstrate that macrophages adopt distinct phenotypes when exposed to articular cartilage (AC), ligament (LIG) and growth plate (GP) derived ECM scaffolds. Macrophages were generally unresponsive to LIG-derived ECM, adopted an M2-like phenotype when exposed to AC-derived ECM, and a hybrid M1-M2 phenotype when exposed to GP-ECM. Furthermore, macrophages expressed higher levels of pro-chondrogenic factors, such as FGF2, when exposed to AC-ECM, and higher levels of angiogenic and pro-osteogenic factors, such as VEGF, IL-6 and TNF, when exposed to GP-ECM. In addition, we observed that they can differentially direct the differentiation of skeletal stem cells, whereby AC-ECM promotes the chondrogenic differentiation and GP-ECM the osteogenic differentiation of multipotent stem/stromal cells (MSCs). In vivo characterisation of immune cell subsets following scaffold implantation into a large bone defect demonstrated that AC-ECM drives an M2 macrophage phenotype, while GP-ECM containing scaffolds promoted a hybrid M1-M2 phenotype and enhanced vascularisation and vessel maturation. This distinct response to the implantation of GP-ECM containing scaffolds was associated with increased CD45+ leukocyte and CD3+ T cell infiltration, accompanied by elevated concentrations of IFN-γ and IL-17. Taken together this work demonstrates that the source tissue of ECM scaffolds plays a key role in regulating the phenotype of both macrophages and skeletal stem cells. Furthermore, these ECMs can direct the cellular differentiation and production of growth factors essential for the regeneration of their source tissue. This work highlights the need for a more thorough characterisation of innate immune cell subsets post-biomaterial implantation.

Published

2021

16. Growth plate extracellular matrix-derived scaffolds for large bone defect healing

Author

J S Ramey, Fergal J. O'Brien, Gráinne M. Cunniffe, Aisling Dunne, Emmet M. Thompson, Daniel J. Kelly, Pedro J. Díaz-Payno, and Olwyn R. Mahon

Subjects

Male, 0301 basic medicine, Bone Regeneration, lcsh:Diseases of the musculoskeletal system, extracellular matrix, Sus scrofa, Long bone, lcsh:Surgery, 02 engineering and technology, Matrix (biology), scaffold, Bone and Bones, Extracellular matrix, 03 medical and health sciences, Osteogenesis, medicine, Animals, Humans, Bone regeneration, Endochondral ossification, Glycosaminoglycans, Wound Healing, Tissue Scaffolds, Chemistry, Macrophages, Regeneration (biology), Skull, Biomaterial, X-Ray Microtomography, lcsh:RD1-811, 021001 nanoscience & nanotechnology, Rats, Inbred F344, Cell biology, Phenotype, 030104 developmental biology, medicine.anatomical_structure, large bone defect regeneration, Intramembranous ossification, Cytokines, Growth plate, lcsh:RC925-935, 0210 nano-technology, Chondrogenesis, Porosity

Abstract

Limitations associated with demineralised bone matrix and other grafting materials have motivated the development of alternative strategies to enhance the repair of large bone defects. The growth plate (GP) of developing limbs contain a plethora of growth factors and matrix cues which contribute to long bone growth, suggesting that biomaterials derived from its extracellular matrix (ECM) may be uniquely suited to promoting bone regeneration. The goal of this study was to generate porous scaffolds from decellularised GP ECM and to evaluate their ability to enhance host mediated bone regeneration following their implantation into critically-sized rat cranial defects. The scaffolds were first assessed by culturing with primary human macrophages, which demonstrated that decellularisation resulted in reduced IL-1β and IL-8 production. In vitro, GP derived scaffolds were found capable of supporting osteogenesis of mesenchymal stem cells via either an intramembranous or an endochondral pathway, demonstrating the intrinsic osteoinductivity of the biomaterial. Furthermore, upon implantation into cranial defects, GP derived scaffolds were observed to accelerate vessel in-growth, mineralisation and de novo bone formation. These results support the use of decellularised GP ECM as a scaffold for large bone defect regeneration.

Published

2017

17. Glyoxal cross-linking of solubilized extracellular matrix to produce highly porous, elastic, and chondro-permissive scaffolds for orthopedic tissue engineering

Author

Nina Cassidy, Ivan Dudurych, Conor T. Buckley, Daniel J. Kelly, Olwyn R. Mahon, David C. Browe, Pedro J. Díaz-Payno, and Aisling Dunne

Subjects

Cartilage, Articular, Scaffold, Materials science, Swine, 0206 medical engineering, Biomedical Engineering, Type II collagen, 02 engineering and technology, Biomaterials, Extracellular matrix, chemistry.chemical_compound, Chondrocytes, Tissue engineering, medicine, Animals, Humans, Decellularization, Tissue Engineering, Tissue Scaffolds, Cartilage, Macrophages, Metals and Alloys, Biomaterial, Glyoxal, 021001 nanoscience & nanotechnology, 020601 biomedical engineering, Elasticity, Extracellular Matrix, medicine.anatomical_structure, Cross-Linking Reagents, Orthopedics, chemistry, Solubility, Ceramics and Composites, Biophysics, Cytokines, Female, 0210 nano-technology, Chondrogenesis, Porosity

Abstract

Extracellular matrix (ECM)-derived implants hold great promise for tissue repair, but new strategies are required to produce efficiently decellularized scaffolds with the necessary porosity and mechanical properties to facilitate regeneration. In this study, we demonstrate that it is possible to produce highly porous, elastic, articular cartilage (AC) ECM-derived scaffolds that are efficiently decellularized, nonimmunogenic, and chondro-permissive. Pepsin solubilized porcine AC was cross-linked with glyoxal, lyophilized and then subjected to dehydrothermal treatment. The resulting scaffolds were predominantly collagenous in nature, with the majority of sulphated glycosaminoglycan (sGAG) and DNA removed during scaffold fabrication. Four scaffold variants were produced to examine the effect of both ECM (10 or 20 mg/mL) and glyoxal (5 or 10 mM) concentration on the mechanical and biological properties of the resulting construct. When seeded with human infrapatellar fat pad-derived stromal cells, the scaffolds with the lowest concentration of both ECM and glyoxal were found to promote the development of a more hyaline-like cartilage tissue, as evident by increased sGAG and type II collagen deposition. Furthermore, when cultured in the presence of human macrophages, it was found that these ECM-derived scaffolds did not induce the production of key proinflammatory cytokines, which is critical to success of an implantable biomaterial. Together these findings demonstrate that the novel combination of solubilized AC ECM and glyoxal crosslinking can be used to produce highly porous scaffolds that are sufficiently decellularized, highly elastic, chondro-permissive and do not illicit a detrimental immune response when cultured in the presence of human macrophages.

Published

2019