Microarray analyses to quantify advantages of 2D and 3D hydrogel culture systems in maintaining the native valvular interstitial cell phenotype

Mabry, Kelly M.; Payne, Samuel Z.; Anseth, Kristi S.

doi:10.1016/j.biomaterials.2015.09.035

Cited by 111 publications

(80 citation statements)

References 54 publications

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“…Other approaches for reducing aSMA expression have involved 3D VIC culture in soft hydrogels. 10,[23][24][25] Interestingly, VIC encapsulation in synthetic hydrogels decorated with peptides derived from collagen I led to the lowest percentage of aSMA-positive VICs compared with fibronectinand elastinderived peptides. 23 In many of these cases, the ability to induce the quiescent phenotype has been hypothesized to depend on the soft mechanical properties of these materials.…”

Section: Discussionmentioning

confidence: 99%

Robust Generation of Quiescent Porcine Valvular Interstitial Cell Cultures

Porras

Engeland

Marchbanks

et al. 2017

JAHA

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BackgroundValvular interstitial cells (VICs) in the healthy aortic valve leaflet exhibit a quiescent phenotype, with <5% of VICs exhibiting an activated phenotype. Yet, in vitro culture of VICs on tissue culture polystyrene surfaces in standard growth medium results in rapid transformation to an activated phenotype in >90% of cells. The inability to preserve a healthy VIC phenotype during in vitro studies has hampered the elucidation of mechanisms involved in calcific aortic valve disease. This study describes the generation of quiescent populations of porcine VICs in 2‐dimensional in vitro culture and their utility in studying valve pathobiology.Methods and ResultsWithin 4 days of isolation from fresh porcine hearts, VICs cultured in standard growth conditions were predominantly myofibroblastic (activated VICs). This myofibroblastic phenotype was partially reversed within 4 days, and fully reversed within 9 days, following application of a combination of a fibroblast media formulation with culture on collagen coatings. Specifically, culture in this combination significantly reduced several markers of VIC activation, including proliferation, apoptosis, α‐smooth muscle actin expression, and matrix production, relative to standard growth conditions. Moreover, VICs raised in a fibroblast media formulation with culture on collagen coatings exhibited dramatically increased sensitivity to treatment with transforming growth factor β1, a known pathological stimulus, compared with VICs raised in either standard culture or medium with a fibroblast media formulation.ConclusionsThe approach using a fibroblast media formulation with culture on collagen coatings generates quiescent VICs that more accurately mimic a healthy VIC population and thus has the potential to transform the study of the mechanisms of VIC activation and dysfunction involved in the early stages of calcific aortic valve disease.

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Section: Discussionmentioning

confidence: 99%

Robust Generation of Quiescent Porcine Valvular Interstitial Cell Cultures

Porras

Engeland

Marchbanks

et al. 2017

JAHA

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“…Others and we demonstrated that three‐dimensional (3D) matrix‐embedding influences the phenotype and genotype of a variety of human cells mimicking the in vivo cell type to a greater extent than simply 2D tissue culture plating (Baharvand, Hashemi, Kazemi Ashtiani, & Farrokhi, ; Benya & Shaffer, ; Luca et al, ; Mabry, Payne, & Anseth, ; Methe et al, ; Nelson & Bissell, ). 3D cell culture systems have gained increasing interest in drug discovery and tissue engineering due to their evident advantages in providing more physiologically relevant information and more predictive data for in vivo tests (Edmondson, Broglie, Adcock, & Yang, ).…”

Section: Introductionmentioning

confidence: 92%

3D matrix‐embedding inhibits cycloheximide‐mediated sensitization to TNF‐alpha‐induced apoptosis of human endothelial cells

Saemisch

Nickmann²,

Riesinger

et al. 2017

J Tissue Eng Regen Med

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The programmed form of cell death (apoptosis) is essential for normal development of multicellular organisms. Dysregulation of apoptosis has been linked with embryonal death and is involved in the pathophysiology of various diseases. Others and we previously demonstrated endothelial biology being intertwined with biochemical and structural composition of the subendothelial basement membrane. We now demonstrate that a three-dimensional growing environment significantly shields endothelial cells from cytokine-induced apoptosis. Detailed analysis reveals differences in intracellular signaling pathways in naive endothelial cells and cytokine-stimulated endothelial cells when cells are grown within a three-dimensional collagen-based matrix compared to cells grown on two-dimensional tissue culture plates. Main findings are significantly reduced p53 expression and level of p38-phosphorylation in three-dimensional grown endothelial cells. Despite similar concentrations of focal adhesion kinase three-dimensional matrix embedded endothelial cells express significantly less tyrosine-phosphorylated focal adhesion kinase. Pretreatment with antibodies against integrin αvβ3 partially reversed the protective effect of three-dimensional matrix-embedding on endothelial apoptosis. Our findings provide detailed insights into the mechanisms of endothelial apoptosis with respect to the spatial matrix environment. These results enhance our understanding of endothelial biology and may otherwise help in the design of tissue-engineered materials. Furthermore, findings on focal adhesion kinase phosphorylation might enhance our understanding of clinical studies with tyrosine kinase inhibitors.

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“…6,33,[37][38][39][40] The amount of fibrillar F-actin in cells cultured on the 2D hydrogels was much lower in both cell lines than on TCPS (Figure 3c). [41][42] Comparing the 2D hydrogels by qualitative visual inspection, we observed that more cells could adhere to the "collagen-rich" substrate over the collagen I only substrate for both MDA-MB-231 and Hs578T cell lines. This result is likely due to the variety of integrin-binding sites provided by the protein mixture.…”

Section: Lap Is An Efficient Photoinitiator To Synthesize 2d Peg-pc Hmentioning

confidence: 99%

Complementary, Semi-automated Methods for Creating Multi-dimensional, PEG-based Biomaterials

Brooks

Jansen

Gencoglu

et al. 2017

Preprint

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Tunable biomaterials that mimic selected features of the extracellular matrix (ECM), such as its stiffness, protein composition, and dimensionality, are increasingly popular for studying how cells sense and respond to ECM cues. In the field, there exists a significant trade-off for how complex and how well these biomaterials represent the in vivo microenvironment, versus how easy they are to make and how adaptable they are to high-throughput fabrication techniques. To address this need to integrate more complex biomaterials design with high-throughput screening approaches, we present several methods to fabricate synthetic biomaterials in 96-well plates and demonstrate that they can be adapted to existing liquid handling robotics. These platforms include 1) glass bottom plates with covalently attached ECM proteins, and 2) hydrogels with tunable stiffness and protein composition with either cells seeded on the surface, or 3) laden within the three-dimensional hydrogel matrix. This study includes proof-of-concept results demonstrating control over breast cancer cell line phenotypes via these ECM cues in a highthroughput fashion. We foresee the use of these methods as a mechanism to bridge the gap between high-throughput cell-matrix screening and engineered ECM-mimicking biomaterials.

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Microarray analyses to quantify advantages of 2D and 3D hydrogel culture systems in maintaining the native valvular interstitial cell phenotype

Cited by 111 publications

References 54 publications

Robust Generation of Quiescent Porcine Valvular Interstitial Cell Cultures

Robust Generation of Quiescent Porcine Valvular Interstitial Cell Cultures

3D matrix‐embedding inhibits cycloheximide‐mediated sensitization to TNF‐alpha‐induced apoptosis of human endothelial cells

Complementary, Semi-automated Methods for Creating Multi-dimensional, PEG-based Biomaterials

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