Comparison of Uncultured Marrow Mononuclear Cells and Culture-Expanded Mesenchymal Stem Cells in 3D Collagen-Chitosan Microbeads for Orthopedic Tissue Engineering

Wise, Joel K.; Alford, Andrea I.; Goldstein, Steven A.; Stegemann, Jan P.

doi:10.1089/ten.tea.2013.0151

Cited by 45 publications

(60 citation statements)

References 88 publications

(115 reference statements)

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“…113 Recently, a chitosan-collagen hydrogel microbead was reported as a vehicle for culture and delivery of cultured-expanded mesenchymal stem cells or fresh bone marrow mononuclear cells. 117 The microbeads were fabricated via a two-step process. Chitosan, collagen and β-glycerophosphate were mixed in solution and bead formation was achieved using a water-in-oil emulsion system followed by thermally induced gelation at physiological temperature.…”

Section: Advances In Chitosan-based Scaffolds For Bone Tissue Engimentioning

confidence: 99%

Chitosan-based scaffolds for bone tissue engineering

2014

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Bone defects requiring grafts to promote healing are frequently occurring and costly problems in health care. Chitosan, a biodegradable, naturally occurring polymer, has drawn considerable attention in recent years as scaffolding material in tissue engineering and regenerative medicine. Chitosan is especially attractive as a bone scaffold material because it supports the attachment and proliferation of osteoblast cells as well as formation of mineralized bone matrix. In this review, we discuss the fundamentals of bone tissue engineering and the unique properties of chitosan as a scaffolding material to treat bone defects for hard tissue regeneration. We present the common methods for fabrication and characterization of chitosan scaffolds, and discuss the influence of material preparation and addition of polymeric or ceramic components or biomolecules on chitosan scaffold properties such as mechanical strength, structural integrity, and functional bone regeneration. Finally, we highlight recent advances in development of chitosan-based scaffolds with enhanced bone regeneration capability.

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Section: Advances In Chitosan-based Scaffolds For Bone Tissue Engimentioning

confidence: 99%

Chitosan-based scaffolds for bone tissue engineering

2014

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“…19,20 Cell collections containing bone marrow-derived mononucleated cells (BMNCs)-a small fraction of which are BMSCs-are seeded within biomaterials for 3D isolation, expansion, and subsequent differentiation. 20,21 Cell seeding density is a transplantation variable that has not been evaluated in detail to date for either 2D-or 3D-expanded BMSCs. Healthy articular cartilage naturally contains 9.6 × 10 6 chondrocytes/cm 3 .…”

Section: Introductionmentioning

confidence: 99%

Optimal Seeding Densities for In Vitro Chondrogenesis of Two- and Three-Dimensional-Isolated and -Expanded Bone Marrow-Derived Mesenchymal Stromal Stem Cells Within a Porous Collagen Scaffold

Bornes

Jomha

Mulet‐Sierra

et al. 2016

Tissue Engineering Part C: Methods

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Bone marrow-derived mesenchymal stromal stem cells (BMSCs) are a promising cell source for treating articular cartilage defects. The objective of this study was to assess the impact of cell seeding density within a collagen I scaffold on in vitro BMSC chondrogenesis following isolation and expansion in two-dimensional (2D) and three-dimensional (3D) environments. It was hypothesized that both expansion protocols would produce BMSCs capable of hyaline-like chondrogenesis with an optimal seeding density of 10 × 10 6 cells/cm 3 . Ovine BMSCs were isolated in a 2D environment by plastic adherence, expanded to passage two in flasks containing an expansion medium, and seeded within collagen I scaffolds at densities of 50, 10, 5, 1, and 0.5 × 10 6 BMSCs/cm 3 . For 3D isolation and expansion, aspirates containing known quantities of mononucleated cells (bone marrow-derived mononucleated cells [BMNCs]) were seeded on scaffolds at 50, 10, 5, 1, and 0.5 × 10 6 BMNCs/cm 3 and cultured in the expansion medium for an equivalent duration to 2D expansion. Constructs were differentiated in vitro in the chondrogenic medium for 21 days and assessed with reverse-transcription quantitative polymerase chain reaction, safranin O staining, histological scoring using the Bern Score, collagen immunofluorescence, and glycosaminoglycan (GAG) quantification. Two-dimensional-expanded BMSCs seeded at all densities were capable of proteoglycan production and displayed increased expressions of aggrecan and collagen II messenger RNA (mRNA) relative to pre-differentiation controls. Collagen II deposition was apparent in scaffolds seeded at 0.5-10 × 10 6 BMSCs/cm 3 . Chondrogenesis of 2D-expanded BMSCs was most pronounced in scaffolds seeded at 5-10 × 10 6 BMSCs/cm 3 based on aggrecan and collagen II mRNA, safranin O staining, Bern Score, total GAG, and GAG/deoxyribonucleic acid (DNA). For 3D-expanded BMSC-seeded scaffolds, increased aggrecan and collagen II mRNA expressions relative to controls were noted with all densities. Proteoglycan deposition was present in scaffolds seeded at 0.5-50 × 10 6 BMNCs/cm 3 , while collagen II deposition occurred in scaffolds seeded at 10-50 × 10 6 BMNCs/cm 3 . The

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“…A two-paddle impeller stirred the mixture at 700 rpm for 6 min at 37 °C and then for 30 min on ice to gel the resulting microbeads. Previous work has shown that use of FBS acts as a surfactant that facilitates the separation of the beads from the oil phase during production, and also aids in maintaining high cell viability [17, 21]. …”

Section: Methodsmentioning

confidence: 99%

Distributed vasculogenesis from modular agarose-hydroxyapatite-fibrinogen microbeads

et al. 2017

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Critical limb ischemia impairs circulation to the extremities, causing pain, disrupted wound healing, and potential tissue necrosis. Therapeutic angiogenesis seeks to repair the damaged microvasculature directly to restore blood flow. In this study, we developed modular, micro-scale constructs designed to possess robust handling qualities, allow in vitro pre-culture, and promote microvasculature formation. The microbead matrix consisted of an agarose (AG) base to prevent aggregation, combined with cell-adhesive components of fibrinogen (FGN) and/or hydroxyapatite (HA). Microbeads encapsulating a co-culture of human umbilical vein endothelial cells (HUVEC) and fibroblasts were prepared and characterized. Microbeads were generally 80–100 microns in diameter, and the size increased with the addition of FGN and HA. Addition of HA increased the yield of microbeads, as well as the homogeneity of distribution of FGN within the matrix. Cell viability was high in all microbead types. When cell-seeded microbeads were embedded in fibrin hydrogels, HUVEC sprouting and inosculation between neighboring microbeads were observed over seven days. Pre-culture of microbeads for an additional seven days prior to embedding in fibrin resulted in significantly greater HUVEC network length in AG+HA+FGN microbeads, as compared to AG, AG+HA or AG+FGN microbeads. Importantly, composite microbeads resulted in more even and widespread endothelial network formation, relative to control microbeads consisting of pure fibrin. These results demonstrate that AG+HA+FGN microbeads support HUVEC sprouting both within and between adjacent microbeads, and can promote distributed vascularization of an external matrix. Such modular microtissues may have utility in treating ischemic tissue by rapidly re-establishing a microvascular network.

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Comparison of Uncultured Marrow Mononuclear Cells and Culture-Expanded Mesenchymal Stem Cells in 3D Collagen-Chitosan Microbeads for Orthopedic Tissue Engineering

Cited by 45 publications

References 88 publications

Chitosan-based scaffolds for bone tissue engineering

Chitosan-based scaffolds for bone tissue engineering

Optimal Seeding Densities for In Vitro Chondrogenesis of Two- and Three-Dimensional-Isolated and -Expanded Bone Marrow-Derived Mesenchymal Stromal Stem Cells Within a Porous Collagen Scaffold

Distributed vasculogenesis from modular agarose-hydroxyapatite-fibrinogen microbeads

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