A method for the production of complex cell‐laden structures is reported, which allows high‐levels of spatial control over mechanical and chemical properties. The potential of this method for producing complicated tissues is demonstrated by manufacturing a complex hard/soft tissue interface and demonstrating that cell phenotype can be maintained over four weeks of culture.
The lack of in vitro tissue and organ
models capable of mimicking
human physiology severely hinders the development and clinical translation
of therapies and drugs with higher in vivo efficacy. Bioprinting allow
us to fill this gap and generate 3D tissue analogues with complex
functional and structural organization through the precise spatial
positioning of multiple materials and cells. In this review, we report
the latest developments in terms of bioprinting technologies for the
manufacturing of cellular constructs with particular emphasis on material
extrusion, jetting, and vat photopolymerization. We then describe
the different base polymers employed in the formulation of bioinks
for bioprinting and examine the strategies used to tailor their properties
according to both processability and tissue maturation requirements.
By relating function to organization in human development, we examine
the potential of pluripotent stem cells in the context of bioprinting
toward a new generation of tissue models for personalized medicine.
We also highlight the most relevant attempts to engineer artificial
models for the study of human organogenesis, disease, and drug screening.
Finally, we discuss the most pressing challenges, opportunities, and
future prospects in the field of bioprinting for tissue engineering
(TE) and regenerative medicine (RM).
Brain extracellular matrix (ECM) is complex, heterogeneous and often poorly replicated in traditional 2D cell culture systems. The development of more physiologically relevant 3D cell models capable of emulating the native ECM is of paramount importance for the study of human induced pluripotent stem cell (iPSC)-derived neurons. Due to its structural similarity with hyaluronic acid, a primary component of brain ECM, alginate is a potential biomaterial for 3D cell culture systems. However, a lack of cell adhesion motifs within the chemical structure of alginate has limited its application in neural culture systems. This study presents a simple and accessible method of incorporating collagen fibrils into an alginate hydrogel by physical mixing and controlled gelation under physiological conditions and tests the hypothesis that such a substrate could influence the behaviour of human neurons in 3D culture. Regulation of the gelation process enabled the penetration of collagen fibrils throughout the hydrogel structure as demonstrated by transmission electron microscopy. Encapsulated human iPSC-derived neurons adhered to the blended hydrogel as evidenced by the increased expression of α1, α2 and β1 integrins. Furthermore, immunofluorescence microscopy revealed that encapsulated neurons formed complex neural networks and matured into branched neurons expressing synaptophysin, a key protein involved in neurotransmission, along the neurites. Mechanical tuning of the hydrogel stiffness by modulation of the alginate ionic crosslinker concentration also influenced neuron-specific gene expression. In conclusion, we have shown that by tuning the physicochemical properties of the alginate/collagen blend it is possible to create different ECM-like microenvironments where complex mechanisms underpinning the growth and development of human neurons can be simulated and systematically investigated.
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