Identification of Fluorescent Compounds with Non-Specific Binding Property via High Throughput Live Cell Microscopy

dc.contributor.author Nath, Sangeeta
dc.contributor.author Spencer, Virginia
dc.contributor.author Han, Ju
dc.contributor.author Chang, Hang
dc.contributor.author Zhang, Kai
dc.contributor.author Fontenay, Gerald
dc.contributor.author Anderson, Charles
dc.contributor.author Hyman, Joel
dc.contributor.author Nilsen-Hamilton, Marit
dc.contributor.author Chang, Young-Tae
dc.contributor.author Parvin, Bahram
dc.contributor.department Roy J. Carver Department of Biochemistry, Biophysics and Molecular Biology (CALS)
dc.date 2018-02-17T10:56:05.000
dc.date.accessioned 2020-06-29T23:47:03Z
dc.date.available 2020-06-29T23:47:03Z
dc.date.copyright Sun Jan 01 00:00:00 UTC 2012
dc.date.issued 2012-01-01
dc.description.abstract <p><h2>Abstract</h2> <h3>Introduction</h3></p> <p>Compounds exhibiting low non-specific intracellular binding or non-stickiness are concomitant with rapid clearing and in high demand for live-cell imaging assays because they allow for intracellular receptor localization with a high signal/noise ratio. The non-stickiness property is particularly important for imaging intracellular receptors due to the equilibria involved. <h3>Method</h3></p> <p>Three mammalian cell lines with diverse genetic backgrounds were used to screen a combinatorial fluorescence library via high throughput live cell microscopy for potential ligands with high in- and out-flux properties. The binding properties of ligands identified from the first screen were subsequently validated on plant root hair. A correlative analysis was then performed between each ligand and its corresponding physiochemical and structural properties. <h3>Results</h3></p> <p>The non-stickiness property of each ligand was quantified as a function of the temporal uptake and retention on a cell-by-cell basis. Our data shows that (i) mammalian systems can serve as a pre-screening tool for complex plant species that are not amenable to high-throughput imaging; (ii) retention and spatial localization of chemical compounds vary within and between each cell line; and (iii) the structural similarities of compounds can infer their non-specific binding properties. <h3>Conclusion</h3></p> <p>We have validated a protocol for identifying chemical compounds with non-specific binding properties that is testable across diverse species. Further analysis reveals an overlap between the non-stickiness property and the structural similarity of compounds. The net result is a more robust screening assay for identifying desirable ligands that can be used to monitor intracellular localization. Several new applications of the screening protocol and results are also presented.</p>
dc.description.comments <p>This is an article from <em>PLOS ONE</em> 7 (2012): 1, <a href="http://dx.doi.org/10.1371/journal.pone.0028802%20" target="_blank">doi:10.1371/journal.pone.0028802</a>. Posted with permission.</p>
dc.format.mimetype application/pdf
dc.identifier archive/lib.dr.iastate.edu/bbmb_ag_pubs/30/
dc.identifier.articleid 1043
dc.identifier.contextkey 8031714
dc.identifier.s3bucket isulib-bepress-aws-west
dc.identifier.submissionpath bbmb_ag_pubs/30
dc.identifier.uri https://dr.lib.iastate.edu/handle/20.500.12876/10760
dc.language.iso en
dc.source.bitstream archive/lib.dr.iastate.edu/bbmb_ag_pubs/30/2012_Nilsen_IdentificationFluorescent.pdf|||Fri Jan 14 23:27:16 UTC 2022
dc.source.uri 10.1371/journal.pone.0028802
dc.subject.disciplines Biochemistry, Biophysics, and Structural Biology
dc.title Identification of Fluorescent Compounds with Non-Specific Binding Property via High Throughput Live Cell Microscopy
dc.type article
dc.type.genre article
dspace.entity.type Publication
relation.isAuthorOfPublication c84e6eba-3eab-4cce-8d1e-80e67584729b
relation.isOrgUnitOfPublication c70f85ae-e0cd-4dce-96b5-4388aac08b3f
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