Fundamental Technologies and Recent Advances of Cell-Sheet-Based Tissue Engineering

Chikahiro Imashiro; Tatsuya Shimizu

doi:10.3390/ijms22010425

Fundamental Technologies and Recent Advances of Cell-Sheet-Based Tissue Engineering

International Journal of Molecular Sciences ◽

10.3390/ijms22010425 ◽

2021 ◽

Vol 22 (1) ◽

pp. 425

Author(s):

Chikahiro Imashiro ◽

Tatsuya Shimizu

Keyword(s):

Tissue Engineering ◽

Ex Vivo ◽

Cell Sheet ◽

Tissue Cell ◽

Culture Methods ◽

Recent Advances ◽

A Cell ◽

Cell Sheet Technology

Tissue engineering has attracted significant attention since the 1980s, and the applications of tissue engineering have been expanding. To produce a cell-dense tissue, cell sheet technology has been studied as a promising strategy. Fundamental techniques involving tissue engineering are mainly introduced in this review. First, the technologies to fabricate a cell sheet were reviewed. Although temperature-responsive polymer-based technique was a trigger to establish and spread cell sheet technology, other methodologies for cell sheet fabrication have also been reported. Second, the methods to improve the function of the cell sheet were investigated. Adding electrical and mechanical stimulation on muscle-type cells, building 3D structures, and co-culturing with other cell species can be possible strategies for imitating the physiological situation under in vitro conditions, resulting in improved functions. Finally, culture methods to promote vasculogenesis in the layered cell sheets were introduced with in vivo, ex vivo, and in vitro bioreactors. We believe the present review that shows and compares the fundamental technologies and recent advances for cell-sheet-based tissue engineering should promote further development of tissue engineering. The development of cell sheet technology should promote many bioengineering applications.

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Collagen fibrous scaffolds for sustained delivery of growth factors for meniscal tissue engineering

Nanomedicine ◽

10.2217/nnm-2021-0313 ◽

2022 ◽

Author(s):

Jihye Baek ◽

Kwang Il Lee ◽

Ho Jong Ra ◽

Martin K Lotz ◽

Darryl D D'Lima

Keyword(s):

Tissue Engineering ◽

Growth Factors ◽

Sustained Release ◽

Ex Vivo ◽

Synovial Cell ◽

Growth Factor Delivery ◽

Meniscal Tissue ◽

A Cell

Aim: To mimic the ultrastructural morphology of the meniscus with nanofiber scaffolds coupled with controlled growth factor delivery to modulate cellular performance for tissue engineering of menisci. Methods: The authors functionalized collagen nanofibers by conjugating heparin to the following growth factors for sustained release: PDGF-BB, TGF-β1 and CTGF. Results: Incorporating growth factors increased human meniscal and synovial cell viability, proliferation and infiltration in vitro, ex vivo and in vivo; upregulated key genes involved in meniscal extracellular matrix synthesis; and enhanced generation of meniscus-like tissue. Conclusion: The authors' results indicate that functionalizing collagen nanofibers can create a cell-favorable micro- and nanoenvironment and can serve as a system for sustained release of bioactive factors.

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Regulation of cilia abundance in multiciliated cells

eLife ◽

10.7554/elife.44039 ◽

2019 ◽

Vol 8 ◽

Cited By ~ 18

Author(s):

Rashmi Nanjundappa ◽

Dong Kong ◽

Kyuhwan Shim ◽

Tim Stearns ◽

Steven L Brody ◽

...

Keyword(s):

Progenitor Cells ◽

Surface Area ◽

Ex Vivo ◽

Compensatory Mechanism ◽

Multiciliated Cells ◽

Culture Model ◽

A Cell ◽

Dependent Mechanism

Multiciliated cells (MCC) contain hundreds of motile cilia used to propel fluid over their surface. To template these cilia, each MCC produces between 100-600 centrioles by a process termed centriole amplification. Yet, how MCC regulate the precise number of centrioles and cilia remains unknown. Airway progenitor cells contain two parental centrioles (PC) and form structures called deuterosomes that nucleate centrioles during amplification. Using an ex vivo airway culture model, we show that ablation of PC does not perturb deuterosome formation and centriole amplification. In contrast, loss of PC caused an increase in deuterosome and centriole abundance, highlighting the presence of a compensatory mechanism. Quantification of centriole abundance in vitro and in vivo identified a linear relationship between surface area and centriole number. By manipulating cell size, we discovered that centriole number scales with surface area. Our results demonstrate that a cell-intrinsic surface area-dependent mechanism controls centriole and cilia abundance in multiciliated cells.

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Fabrication of hyaline-like cartilage constructs using mesenchymal stem cell sheets

Scientific Reports ◽

10.1038/s41598-020-77842-0 ◽

2020 ◽

Vol 10 (1) ◽

Author(s):

Hallie Thorp ◽

Kyungsook Kim ◽

Makoto Kondo ◽

David W. Grainger ◽

Teruo Okano

Keyword(s):

Chondrogenic Differentiation ◽

Cell Sheet ◽

Cartilage Regeneration ◽

Cell Sheets ◽

Chondrogenic Potential ◽

Cell Sheet Technology ◽

Cell Functionality ◽

Articular Cartilage Regeneration

AbstractCell and tissue engineering approaches for articular cartilage regeneration increasingly focus on mesenchymal stem cells (MSCs) as allogeneic cell sources, based on availability and innate chondrogenic potential. Many MSCs exhibit chondrogenic potential as three-dimensional (3D) cultures (i.e. pellets and seeded biomaterial scaffolds) in vitro; however, these constructs present engraftment, biocompatibility, and cell functionality limitations in vivo. Cell sheet technology maintains cell functionality as scaffold-free constructs while enabling direct cell transplantation from in vitro culture to targeted sites in vivo. The present study aims to develop transplantable hyaline-like cartilage constructs by stimulating MSC chondrogenic differentiation as cell sheets. To achieve this goal, 3D MSC sheets are prepared, exploiting spontaneous post-detachment cell sheet contraction, and chondrogenically induced. Results support 3D MSC sheets’ chondrogenic differentiation to hyaline cartilage in vitro via post-contraction cytoskeletal reorganization and structural transformations. These 3D cell sheets’ initial thickness and cellular densities may also modulate MSC-derived chondrocyte hypertrophy in vitro. Furthermore, chondrogenically differentiated cell sheets adhere directly to cartilage surfaces via retention of adhesion molecules while maintaining the cell sheets’ characteristics. Together, these data support the utility of cell sheet technology for fabricating scaffold-free, hyaline-like cartilage constructs from MSCs for future transplantable articular cartilage regeneration therapies.

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Cartilage Regeneration Characteristics of Human and Goat Auricular Chondrocytes

Frontiers in Bioengineering and Biotechnology ◽

10.3389/fbioe.2021.766363 ◽

2021 ◽

Vol 9 ◽

Author(s):

Mengjie Hou ◽

Baoshuai Bai ◽

Baoxing Tian ◽

Zheng Ci ◽

Yu Liu ◽

...

Keyword(s):

Culture System ◽

Cell Sheet ◽

Cartilage Regeneration ◽

Chondrogenic Medium ◽

Culture Time ◽

Medium System ◽

A Cell ◽

Seed Cells

Although cartilage regeneration technology has achieved clinical breakthroughs, whether auricular chondrocytes (AUCs) represent optimal seed cells to achieve stable cartilage regeneration is not clear. In this study, we systematically explore biological behaviors of human- and goat-derived AUCs during in vitro expansion as well as cartilage regeneration in vitro and in vivo. To eliminate material interference, a cell sheet model was used to evaluate the feasibility of dedifferentiated AUCs to re-differentiate and regenerate cartilage in vitro and in vivo. We found that the dedifferentiated AUCs could re-differentiate and regenerate cartilage sheets under the chondrogenic medium system, and the generated chondrocyte sheets gradually matured with increased in vitro culture time (2, 4, and 8 weeks). After the implantation of cartilage sheets with different in vitro culture times in nude mice, optimal neocartilage was formed in the group with 2 weeks in vitro cultivation. After in vivo implantation, ossification only occurred in the group with goat-regenerated cartilage sheet of 8 weeks in vitro cultivation. These results, which were confirmed in human and goat AUCs, suggest that AUCs are ideal seed cells for the clinical translation of cartilage regeneration under the appropriate culture system and culture condition.

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Building neuromuscular junctions in vitro

Development ◽

10.1242/dev.193920 ◽

2020 ◽

Vol 147 (22) ◽

pp. dev193920

Author(s):

Susie Barbeau ◽

Julie Tahraoui-Bories ◽

Claire Legay ◽

Cécile Martinat

Keyword(s):

Human Disease ◽

Molecular Mechanisms ◽

Neuromuscular Junctions ◽

Ex Vivo ◽

Culture Methods ◽

Recent Developments ◽

Chemical Synapses ◽

And Function

ABSTRACTThe neuromuscular junction (NMJ) has been the model of choice to understand the principles of communication at chemical synapses. Following groundbreaking experiments carried out over 60 years ago, many studies have focused on the molecular mechanisms underlying the development and physiology of these synapses. This Review summarizes the progress made to date towards obtaining faithful models of NMJs in vitro. We provide a historical approach discussing initial experiments investigating NMJ development and function from Xenopus to mice, the creation of chimeric co-cultures, in vivo approaches and co-culture methods from ex vivo and in vitro derived cells, as well as the most recent developments to generate human NMJs. We discuss the benefits of these techniques and the challenges to be addressed in the future for promoting our understanding of development and human disease.

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Prospects and Challenges of Translational Corneal Bioprinting

Bioengineering ◽

10.3390/bioengineering7030071 ◽

2020 ◽

Vol 7 (3) ◽

pp. 71 ◽

Cited By ~ 2

Author(s):

Matthias Fuest ◽

Gary Hin-Fai Yam ◽

Jodhbir S. Mehta ◽

Daniela F. Duarte Campos

Keyword(s):

Tissue Engineering ◽

Ex Vivo ◽

Corneal Transplantation ◽

Human Cornea ◽

Corneal Tissue ◽

Full Thickness ◽

Future Directions ◽

Spatial Control

Corneal transplantation remains the ultimate treatment option for advanced stromal and endothelial disorders. Corneal tissue engineering has gained increasing interest in recent years, as it can bypass many complications of conventional corneal transplantation. The human cornea is an ideal organ for tissue engineering, as it is avascular and immune-privileged. Mimicking the complex mechanical properties, the surface curvature, and stromal cytoarchitecure of the in vivo corneal tissue remains a great challenge for tissue engineering approaches. For this reason, automated biofabrication strategies, such as bioprinting, may offer additional spatial control during the manufacturing process to generate full-thickness cell-laden 3D corneal constructs. In this review, we discuss recent advances in bioprinting and biomaterials used for in vitro and ex vivo corneal tissue engineering, corneal cell-biomaterial interactions after bioprinting, and future directions of corneal bioprinting aiming at engineering a full-thickness human cornea in the lab.

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The fate of methylmercury through the formation of bismethylmercury sulfide as an intermediate in mice

Scientific Reports ◽

10.1038/s41598-021-96579-y ◽

2021 ◽

Vol 11 (1) ◽

Author(s):

Yumi Abiko ◽

Yusuke Katayama ◽

Wenyang Zhao ◽

Sawako Horai ◽

Kenji Sakurai ◽

...

Keyword(s):

Ex Vivo ◽

Intraperitoneal Administration ◽

Distal Colon ◽

The Body ◽

Gas Chromatography Mass Spectrometry ◽

Dependent Manner ◽

Free System ◽

A Cell

AbstractA previous study by our group indicated that methylmercury (MeHg) is biotransformed to bismethylmercury sulfide [(MeHg)2S)] by interaction with reactive sulfur species (RSS) produced in the body. In the present study, we explored the transformation of MeHg to (MeHg)2S in the gut and the subsequent fate of (MeHg)2S in vitro and in vivo. An ex vivo experiment suggested the possibility of the extracellular transformation of MeHg to (MeHg)2S in the distal colon, and accordingly, the MeHg sulfur adduct was detected in the intestinal contents and feces of mice administered MeHg, suggesting that (MeHg)2S is formed through reactions between MeHg and RSS in the gut. In a cell-free system, we found that (MeHg)2S undergoes degradation in a time-dependent manner, resulting in the formation of mercury sulfide and dimethylmercury (DMeHg), as determined by X-ray diffraction and gas chromatography/mass spectrometry, respectively. We also identified DMeHg in the expiration after the intraperitoneal administration of (MeHg)2S to mice. Thus, our present study identified a new fate of MeHg through (MeHg)2S as an intermediate, which leads to conversion of volatile DMeHg in the body.

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Recent advances in gold nanoparticle-based bioengineering applications

Journal of Materials Chemistry B ◽

10.1039/c5tb01292a ◽

2015 ◽

Vol 3 (43) ◽

pp. 8433-8444 ◽

Cited By ~ 31

Author(s):

Eun Young Kim ◽

Dinesh Kumar ◽

Gilson Khang ◽

Dong-Kwon Lim

Keyword(s):

Drug Delivery ◽

Tissue Engineering ◽

Gold Nanoparticle ◽

Drug Delivery Systems ◽

Delivery Systems ◽

Recent Advances

The recently developed gold nanoparticle-based bioengineering technologies for biosensors,in vitroandin vivobioimaging, drug delivery systems for improved therapeutics and tissue engineering are discussed.

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PEG-Plasma Hydrogels Increase Epithelialization Using a Human Ex Vivo Skin Model

International Journal of Molecular Sciences ◽

10.3390/ijms19103156 ◽

2018 ◽

Vol 19 (10) ◽

pp. 3156 ◽

Cited By ~ 5

Author(s):

Randolph Stone II ◽

John T. Wall ◽

Shanmugasundaram Natesan ◽

Robert J. Christy

Keyword(s):

Wound Healing ◽

Ex Vivo ◽

Smooth Muscle Actin ◽

Cellular Migration ◽

Natural Setting ◽

Ex Vivo Model ◽

Alpha Smooth Muscle Actin ◽

Culture Methods

In vitro cell culture methods are used extensively to study cellular migration, proliferation, and differentiation, which play major roles in wound healing but the results often do not translate to the in vivo environment. One alternative would be to establish an ex vivo model utilizing human discarded skin to evaluate therapies in a more natural setting. The purpose of this study was to institute such a model by creating ‘wounds’ in the center of a piece of discarded skin and treating them with three different biomaterials: collagen, polyethylene glycol (PEG)-fibrin, or PEG-platelet free plasma (PFP). Explants were cultured for 14 days with supernatant and microscopy images collected every 3 days to assess cytotoxicity and epithelialization. After 14 days, the explants were fixed, sectioned, and stained for cytokeratin-10 (CK-10), alpha-smooth muscle actin (α-SMA), and wheat germ (WG). Compared to controls, similar levels of cytotoxicity were detected for 12 days which decreased slightly at day 14. The PEG-PFP hydrogel-treated wounds epithelialized faster than other treatments at days 6 to 14. A 6-8 cell layer thick CK-10+ stratified epidermis had developed over the PEG-PFP hydrogel and cells co-stained by WG and α-SMA were observed within the hydrogel. An ex vivo model was established that can be used practically to screen different therapies exploring wound healing.

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Regulation of Cilia Abundance in Multiciliated Cells

10.1101/478297 ◽

2018 ◽

Cited By ~ 1

Author(s):

Rashmi Nanjundappa ◽

Dong Kong ◽

Kyuhwan Shim ◽

Tim Stearns ◽

Steven L. Brody ◽

...

Keyword(s):

Surface Area ◽

Direct Relationship ◽

Ex Vivo ◽

Multiciliated Cells ◽

Culture Model ◽

A Cell ◽

Total Complement ◽

Dependent Mechanism

AbstractMulticiliated cells (MCC) are specialized epithelia that contain hundreds of motile cilia used to propel fluid over the surface of the cell. To template these cilia, each MCC produces hundreds of centrioles by a process termed centriole amplification. Airway progenitor cells initially contain two parental centrioles that nucleate multiple centrioles at once, and structures called deuterosomes that assemble the vast majority of centrioles during amplification. Remarkably, how each cell regulates the precise number of its centrioles and cilia remains unknown. Here, we investigate mechanisms that establish centriole number in MCC using an ex vivo airway culture model. We show that ablation of parental centrioles, via inhibition of Plk4 kinase, does not perturb deuterosome formation and centriole amplification, nor alter the total complement of centrioles per cell. Airway MCC vary in size and surface area, and exhibit a broad range in centriole number. Quantification of centriole abundance in vitro and in vivo identified a direct relationship between cell-surface area and centriole number. By manipulating cell size and shape, we discovered that centriole number scales with increasing surface area. Collectively, our results demonstrate that parental centrioles and Plk4 are dispensable for deuterosome formation, centriole amplification, and establishment of centriole number. Instead, a cell-intrinsic surface area-dependent mechanism controls centriole and cilia abundance in multiciliated cells.

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