Literature DB >> 21732911

Characterization of a novel angiogenic model based on stable, fluorescently labelled endothelial cell lines amenable to scale-up for high content screening.

Natalie L Prigozhina1, Andrew Heisel, Ke Wei, Roberta Noberini, Edward A Hunter, Diego Calzolari, Jordan R Seldeen, Elena B Pasquale, Pilar Ruiz-Lozano, Mark Mercola, Jeffrey H Price.   

Abstract

BACKGROUND: Blood vessel formation is important for many physiological and pathological processes and is therefore a critical target for drug development. Inhibiting angiogenesis to starve a tumour or promoting 'normalization' of tumour vasculature in order to facilitate delivery of anticancer drugs are both areas of active research. Recapitulation of vessel formation by human cells in vitro allows the investigation of cell-cell and cell-matrix interactions in a controlled environment and is therefore a crucial step in developing HCS (high content screening) and HTS (high throughput screening) assays to search for modulators of blood vessel formation. HUVECs (human umbilical-vein endothelial cells) exemplify primary cells used in angiogenesis assays. However, primary cells have significant limitations that include phenotypic decay and/or senescence by six to eight passages in culture, making stable integration of fluorescent markers and large-scale expansion for HTS problematic. To overcome these limitations for HTS, we developed a novel angiogenic model system that employs stable fluorescent endothelial cell lines based on immortalized HMECs (human microvascular endothelial cell). We then evaluated HMEC cultures, both alone and co-cultured with an EMC (epicardial mesothelial cell) line that contributes vascular smooth muscle cells, to determine the suitability for HTS or HCS.
RESULTS: The endothelial and epicardial lines were engineered to express a panel of nuclear- and cytoplasm-localized fluorescent proteins to be mixed and matched to suit particular experimental goals. HMECs retained their angiogenic potential and stably expressed fluorescent proteins for at least 13 passages after transduction. Within 8 h after plating on Matrigel, the cells migrated and coalesced into networks of vessel-like structures. If co-cultured with EMCs, the branches formed cylindrical-shaped structures of HMECs surrounded by EMC derivatives reminiscent of vessels. Network formation measurements revealed responsiveness to media composition and control compounds.
CONCLUSIONS: HMEC-based lines retain most of the angiogenic features of primary endothelial cells and yet possess long-term stability and ease of culture, making them intriguing candidates for large-scale primary HCS and HTS (of ~10000-1000000 molecules). Furthermore, inclusion of EMCs demonstrates the feasibility of using epicardial-derived cells, which normally contribute to smooth muscle, to model large vessel formation. In summary, the immortalized fluorescent HMEC and EMC lines and straightforward culture conditions will enable assay development for HCS of angiogenesis.

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Year:  2011        PMID: 21732911      PMCID: PMC3538155          DOI: 10.1042/BC20100146

Source DB:  PubMed          Journal:  Biol Cell        ISSN: 0248-4900            Impact factor:   4.458


  37 in total

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Authors:  Ronald E Unger; Vera Krump-Konvalinkova; Kirsten Peters; C James Kirkpatrick
Journal:  Microvasc Res       Date:  2002-11       Impact factor: 3.514

2.  HMEC-1: establishment of an immortalized human microvascular endothelial cell line.

Authors:  E W Ades; F J Candal; R A Swerlick; V G George; S Summers; D C Bosse; T J Lawley
Journal:  J Invest Dermatol       Date:  1992-12       Impact factor: 8.551

3.  Role of epicardial mesothelial cells in the modification of phenotype and function of adult rat ventricular myocytes in primary coculture.

Authors:  H Eid; D M Larson; J P Springhorn; M A Attawia; R C Nayak; T W Smith; R A Kelly
Journal:  Circ Res       Date:  1992-07       Impact factor: 17.367

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Authors:  Rakesh K Jain
Journal:  Science       Date:  2005-01-07       Impact factor: 47.728

5.  Human endothelial cell life extension by telomerase expression.

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6.  Suramin derivatives as inhibitors and activators of protein-tyrosine phosphatases.

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8.  Angiogenic transcriptome of human microvascular endothelial cells: Effect of hypoxia, modulation by atorvastatin.

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9.  Origin of periendothelial cells in microvessels derived from human microvascular endothelial cells.

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  12 in total

1.  Amphiphilic suramin dissolves Matrigel, causing an 'inhibition' artefact within in vitro angiogenesis assays.

Authors:  Natalie L Prigozhina; Andrew J Heisel; Jordan R Seldeen; Nicholas D P Cosford; Jeffrey H Price
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2.  Investigating the effect of hypoxic culture on the endothelial differentiation of human amniotic fluid-derived stem cells.

Authors:  Cai Lloyd-Griffith; Garry P Duffy; Fergal J O'Brien
Journal:  J Anat       Date:  2015-03-31       Impact factor: 2.610

3.  Fluorescent imaging of endothelial cells in bioengineered blood vessels: the impact of crosslinking of the scaffold.

Authors:  Guoguang Niu; Etai Sapoznik; Peng Lu; Tracy Criswell; Aaron M Mohs; Ge Wang; Sang-Jin Lee; Yong Xu; Shay Soker
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Review 4.  Human iPSC modeling of heart disease for drug development.

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6.  Identification of functional progenitor cells in the pulmonary vasculature.

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7.  PEGylation potentiates the effectiveness of an antagonistic peptide that targets the EphB4 receptor with nanomolar affinity.

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Review 8.  Increasing the Content of High-Content Screening: An Overview.

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9.  Notch-independent RBPJ controls angiogenesis in the adult heart.

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10.  Identification of Angiogenesis Inhibitors Using a Co-culture Cell Model in a High-Content and High-Throughput Screening Platform.

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Journal:  SLAS Technol       Date:  2017-09-18       Impact factor: 3.047

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