Validation of a High-Content Screening Assay Using Whole-Well Imaging of Transformed Phenotypes

Ramirez, Christina N.; Ozawa, Tatsuya; Takagi, Toshimitsu; Antczak, Christophe; Shum, David; Graves, Robert J.; Holland, Eric C.; Djaballah, Hakim

doi:10.1089/adt.2010.0342

Cited by 14 publications

(16 citation statements)

References 32 publications

(52 reference statements)

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“…Automated imaging has been available for the last 20 years and it has significantly streamlined the process of in vitro drug screening in addition to decreasing the time needed both for high quality image collection and analysis [24], [25]. Naturally fluorescent drugs have, in the past, been evaluated by fluorescent microscopy [26], [27], [28], [29]; however, a phenotypic screen of toxicity in cells using naturally fluorescent compounds has seldom been attempted due to its inherent restrictions.…”

Section: Resultsmentioning

confidence: 99%

“…The reduction is performed by the action of mitochondrial dehydrogenases in metabolically active cells; the amount of formatazan produced is known to be directly proportional to the mitochondrial enzymatic activity and, therefore, to the number of proliferating cells in culture [22], [23], [24], [25]. This assay has been extensively used both to determine cell proliferation, viability and to determine toxicity of potential therapeutic agents [35], [36], [37].…”

Section: Resultsmentioning

confidence: 99%

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High Content Screening as High Quality Assay for Biological Evaluation of Photosensitizers In Vitro

et al. 2013

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A novel single step assay approach to screen a library of photdynamic therapy (PDT) compounds was developed. Utilizing high content analysis (HCA) technologies several robust cellular parameters were identified, which can be used to determine the phototoxic effects of porphyrin compounds which have been developed as potential anticancer agents directed against esophageal carcinoma. To demonstrate the proof of principle of this approach a small detailed study on five porphyrin based compounds was performed utilizing two relevant esophageal cancer cell lines (OE21 and SKGT-4). The measurable outputs from these early studies were then evaluated by performing a pilot screen using a set of 22 compounds. These data were evaluated and validated by performing comparative studies using a traditional colorimetric assay (MTT). The studies demonstrated that the HCS assay offers significant advantages over and above the currently used methods (directly related to the intracellular presence of the compounds by analysis of their integrated intensity and area within the cells). A high correlation was found between the high content screening (HCS) and MTT data. However, the HCS approach provides additional information that allows a better understanding of the behavior of these compounds when interacting at the cellular level. This is the first step towards an automated high-throughput screening of photosensitizer drug candidates and the beginnings of an integrated and comprehensive quantitative structure action relationship (QSAR) study for photosensitizer libraries.

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Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

High Content Screening as High Quality Assay for Biological Evaluation of Photosensitizers In Vitro

et al. 2013

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“…7 The instrument dimensions are [654mm × 1140mm × 605mm (D x W x H)] with a weight of 50 kilograms. The INCA2000 operating software (Build Version 3.0.0.43) runs on a Windows XP operating system.…”

Section: Methodsmentioning

confidence: 99%

Designs and Concept Reliance of a Fully Automated High-Content Screening Platform

et al. 2012

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High content screening (HCS) is becoming an accepted platform in academic and industry screening labs and does require slightly different logistics for execution. To automate our stand alone HCS microscopes, namely an alpha IN Cell Analyzer 3000 (INCA3000) originally a Praelux unit hooked to a Hudson Plate Crane with a maximum capacity of 50 plates per run; and the IN Cell Analyzer 2000 (INCA2000) where up to 320 plates could be fed per run using the Thermo Fisher Scientific Orbitor, we opted for a 4 meter linear track system harboring both microscopes, plate washer, bulk dispensers, and a high capacity incubator allowing us to perform both live and fixed cell based assays while accessing both microscopes on deck. Considerations in design were given to the integration of the alpha INCA3000, a new gripper concept to access the onboard nest, and peripheral locations on deck to ensure a self reliant system capable of achieving higher throughput. The resulting system, referred to as Hestia, has been fully operational since the New Year, has an onboard capacity of 504 plates, and harbors the only fully automated alpha INCA3000 unit in the World.

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“…Images of cells in 384-well microplates were acquired as previously described 13 by using the following two IN Cell Analyzer platforms (GE Healthcare): the automated epifluorescence IN Cell Analyzer 2000 (INCA2000) and the line-scanning confocal automated microscope IN Cell Analyzer 3000 (INCA3000). Imaging on the INCA2000 was performed at 20 · /0.45NA magnification.…”

Section: Image Acquisitionmentioning

confidence: 99%

“…Serial doubling dilutions of compounds were prepared as previously described. 13 Controls consisted of 1% DMSO (v/v) (high control) and 10 mM gefitinib in 1% DMSO (v/v) (low control). The assay was performed according to our optimized workflow ( Table 1).…”

Section: Pilot Screenmentioning

confidence: 99%

Domain-Based Biosensor Assay to Screen for Epidermal Growth Factor Receptor Modulators in Live Cells

Antczak

Bermingham²,

Calder³

et al. 2012

ASSAY and Drug Development Technologies

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Traditional drug discovery efforts have resulted in the approval of a handful of receptor tyrosine kinase (RTK) inhibitors; however, their discovery relied solely on screening recombinant kinases, often with poor cellular activity outcome. The ability to screen RTKs in their natural environment is sought as an alternative approach. We have adapted a novel strategy utilizing a green fluorescent protein-labeled SRC homology 2 domain-based biosensor as a surrogate reporter of endogenous epidermal growth factor receptor (EGFR) activity in A549 cells. Upon activation of the receptor, EGFR function in live cells is measured by the number of green granules that form. Here we describe assay miniaturization and demonstrate specificity for EGFR through its chemical inhibition and RNAi-dependent knockdown resulting in complete abrogation of granule formation. Gefitinib and PD 153035 were identified as hits in a pilot screen. This approach allows for the identification of novel EGFR modulators in high-throughput formats for screening chemical and RNAi libraries.

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Validation of a High-Content Screening Assay Using Whole-Well Imaging of Transformed Phenotypes

Cited by 14 publications

References 32 publications

High Content Screening as High Quality Assay for Biological Evaluation of Photosensitizers In Vitro

High Content Screening as High Quality Assay for Biological Evaluation of Photosensitizers In Vitro

Designs and Concept Reliance of a Fully Automated High-Content Screening Platform

Domain-Based Biosensor Assay to Screen for Epidermal Growth Factor Receptor Modulators in Live Cells

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