Synthesis of scaffold-free, three dimensional, osteogenic constructs following culture of skeletal osteoprogenitor cells on glass surfaces

Latifa Alghfeli; Divyasree Parambath; Shaista Manzoor; Helmtrud I. Roach; Richard O.C. Oreffo; Ahmed T. El-Serafi

Bone Reports (Dec 2021)

Synthesis of scaffold-free, three dimensional, osteogenic constructs following culture of skeletal osteoprogenitor cells on glass surfaces

Latifa Alghfeli,
Divyasree Parambath,
Shaista Manzoor,
Helmtrud I. Roach,
Richard O.C. Oreffo,
Ahmed T. El-Serafi

Affiliations

Latifa Alghfeli: Research Institute for Medical and Health Sciences, University of Sharjah, United Arab Emirates
Divyasree Parambath: Research Institute for Medical and Health Sciences, University of Sharjah, United Arab Emirates
Shaista Manzoor: Research Institute for Medical and Health Sciences, University of Sharjah, United Arab Emirates
Helmtrud I. Roach: Bone and Joint Research Group, Institute of Developmental Sciences, University of Southampton, School of Medicine, UK
Richard O.C. Oreffo: Bone and Joint Research Group, Institute of Developmental Sciences, University of Southampton, School of Medicine, UK
Ahmed T. El-Serafi: Research Institute for Medical and Health Sciences, University of Sharjah, United Arab Emirates; Medical Biochemistry Department, Faculty of Medicine, Suez Canal University, Ismailia, Egypt; Department of Biomedical and Clinical Sciences (BKV), Linköping University, Sweden; Corresponding author at: Hus 462, ingång 71, plan 11, Campus US, Linköping 581 83, Sweden.

Journal volume & issue: Vol. 15
p. 101143

Abstract

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Background: Efficient differentiation of stem cells into three-dimensional (3D) osteogenic construct is still an unmet challenge. These constructs can be crucial for patients with bone defects due to congenital or traumatic reasons. The modulation of cell fate and function as a consequence of interaction with the physical and chemical properties of materials is well known. Methods: The current study has examined the osteogenic differentiation potential of human skeletal populations following culture on glass surfaces, as a monolayer, or in glass tubes as a pellet culture. The 3D prosperities were assessed morphometrically and the differentiation was evaluated through molecular characterization as well as matrix formation. Results: Early temporal expression of alkaline phosphatase expression of skeletal populations was observed following culture on glass surfaces. Skeletal populations seeded on glass tubes, adhered as a monolayer to the tube base and subsequently formed 3D pellets at the air -media interface. The pellets cultured on glass displayed 4.9 ± 1.3 times the weight and 2.9 ± 0.1 the diameter of their counterpart cultured in plastic tubes and displayed enhanced production of osteogenic matrix proteins, such a collagen I and osteonectin. The size and weight of the pellets correlated with surface area in contrast to cell numbers seeded. Global DNA methylation level was decreased in pellets cultured on glass. In contrast, gene expression analysis confirmed upregulation extracellular matrix proteins and osteogenesis-related growth factors. Conclusion: This simple approach to the culture of skeletal cells on glass tubes provides a scaffold-free, 3D construct platform for generating pellets enabling analysis and evaluation of tissue development and integration of multiple constructs with implications for tissue repair and regenerative application on scale-up.

Published in Bone Reports

ISSN: 2352-1872 (Online)
Publisher: Elsevier
Country of publisher: Netherlands
LCC subjects: Medicine: Internal medicine: Specialties of internal medicine: Diseases of the musculoskeletal system
Website: http://www.journals.elsevier.com/bone-reports/

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