Literature DB >> 26554505

Into the depths: Techniques for in vitro three-dimensional microtissue visualization.

Pranita K Kabadi1, Marguerite M Vantangoli1, April L Rodd1, Elizabeth Leary2, Samantha J Madnick1, Jeffrey R Morgan2, Agnes Kane1, Kim Boekelheide1.   

Abstract

Three-dimensional (3-D) in vitro platforms have been shown to closely recapitulate human physiology when compared with conventional two-dimensional (2-D) in vitro or in vivo animal model systems. This confers a substantial advantage in evaluating disease mechanisms, pharmaceutical drug discovery, and toxicity testing. Despite the benefits of 3-D cell culture, limitations in visualization and imaging of 3-D microtissues present significant challenges. Here we optimized histology and microscopy techniques to overcome the constraints of 3-D imaging. For morphological assessment of 3-D microtissues of several cell types, different time points, and different sizes, a two-step glycol methacrylate embedding protocol for evaluating 3-D microtissues produced using agarose hydrogels improved resolution of nuclear and cellular histopathology characteristic of cell death and proliferation. Additional immunohistochemistry, immunofluorescence, and in situ immunostaining techniques were successfully adapted to these microtissues and enhanced by optical clearing. Utilizing the Clear(T2) protocol greatly increased fluorescence signal intensity, imaging depth, and clarity, allowing for more complete confocal fluorescence microscopy imaging of these 3-D microtissues compared with uncleared samples. The refined techniques presented here address the key challenges associated with 3-D imaging, providing new and alternative methods in evaluating disease pathogenesis, delineating toxicity pathways, and enhancing the versatility of 3-D in vitro testing systems in pharmacological and toxicological applications.

Entities:  

Keywords:  clearing; histology; microtissues; spheroids; three-dimensional

Mesh:

Year:  2015        PMID: 26554505      PMCID: PMC4804457          DOI: 10.2144/000114353

Source DB:  PubMed          Journal:  Biotechniques        ISSN: 0736-6205            Impact factor:   1.993


  32 in total

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Review 2.  Implications of the lack of accuracy of the lifetime rodent bioassay for predicting human carcinogenicity.

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3.  Modeling mass transfer in hepatocyte spheroids via cell viability, spheroid size, and hepatocellular functions.

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Review 4.  A decade of tissue microarrays: progress in the discovery and validation of cancer biomarkers.

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Journal:  Exp Neurol       Date:  2012-11-01       Impact factor: 5.330

6.  Toxicity testing in the 21st century: a vision and a strategy.

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Journal:  J Toxicol Environ Health B Crit Rev       Date:  2010-02       Impact factor: 6.393

Review 7.  "In vitro" 3D models of tumor-immune system interaction.

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8.  Scaffold-free three-dimensional cell culture utilizing micromolded nonadhesive hydrogels.

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9.  Engineering a scaffold-free 3D tumor model for in vitro drug penetration studies.

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  13 in total

Review 1.  In vitro models of the cardiac microenvironment to study myocyte and non-myocyte crosstalk: bioinspired approaches beyond the polystyrene dish.

Authors:  Celinda M Kofron; Ulrike Mende
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2.  Morphologic effects of estrogen stimulation on 3D MCF-7 microtissues.

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5.  A 3D fish liver model for aquatic toxicology: Morphological changes and Cyp1a induction in PLHC-1 microtissues after repeated benzo(a)pyrene exposures.

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Journal:  Aquat Toxicol       Date:  2017-02-21       Impact factor: 4.964

6.  Quantitative Live-Cell Confocal Imaging of 3D Spheroids in a High-Throughput Format.

Authors:  Elizabeth Leary; Claire Rhee; Benjamin T Wilks; Jeffrey R Morgan
Journal:  SLAS Technol       Date:  2018-02-07       Impact factor: 3.047

7.  Sample preparation strategies for high-throughput mass spectrometry imaging of primary tumor organoids.

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Review 8.  High Content Imaging (HCI) on Miniaturized Three-Dimensional (3D) Cell Cultures.

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9.  A novel human 3D lung microtissue model for nanoparticle-induced cell-matrix alterations.

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10.  Matrix Metalloproteinase Response of Dendritic Cell, Gingival Epithelial Keratinocyte, and T-Cell Transwell Co-Cultures Treated with Porphyromonas gingivalis Hemagglutinin-B.

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Journal:  Int J Mol Sci       Date:  2018-12-07       Impact factor: 5.923

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