Please use this identifier to cite or link to this item: http://hdl.handle.net/10397/92696
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dc.contributorSchool of Optometryen_US
dc.creatorShan, SWen_US
dc.creatorDo, CWen_US
dc.creatorLam, CTen_US
dc.creatorLi, HLen_US
dc.creatorStamer, DWen_US
dc.creatorTo, CHen_US
dc.date.accessioned2022-05-11T06:23:35Z-
dc.date.available2022-05-11T06:23:35Z-
dc.identifier.issn0146-0404en_US
dc.identifier.urihttp://hdl.handle.net/10397/92696-
dc.descriptionThis is a 2021 ARVO Annual Meeting abstract.en_US
dc.language.isoenen_US
dc.publisherAssociation for Research in Vision and Ophthalmologyen_US
dc.rightsThis work is licensed under a Creative Commons Attribution-NonCommercial-NoDerivatives 4.0 International License (https://creativecommons.org/licenses/by-nc-nd/4.0/).en_US
dc.rightsThe following publication Shan, S. W., Do, C. W., Lam, C. T., Li, H. L., Stamer, D. W., & To, C. H. (2021). The Role of Thrombospondin-1 in Rho-kinase Inhibitor Mediated Changes in Outflow Facility. Investigative Ophthalmology & Visual Science, 62(8), 1631 is available at https://iovs.arvojournals.org/article.aspx?articleid=2775163en_US
dc.titleThe role of thrombospondin-1 in rho-kinase inhibitor mediated changes in outflow facilityen_US
dc.typeOther Conference Contributionsen_US
dc.identifier.volume62en_US
dc.identifier.issue8en_US
dcterms.abstractPurpose : Rho-kinase (ROCK) inhibitors is a novel class of anti-glaucoma agents, which act by increasing the aqueous humor outflow through conventional trabecular meshwork (TM) pathway. The downstream signaling consequences of ROCK inhibition in the TM are not fully understood. In this study, we evaluated the role of thrombospondin-1 (TSP-1) in triggering ROCK inhibitor-mediated increase in outflow facility.en_US
dcterms.abstractMethods : Primary cultures of human TM (hTM) cells were used. Cell migration assay was conducted with or without Y39983 (1μM, a selective ROCK inhibitor), LSKL (a TSP-1 antagonist), and TSP-1 siRNA knockdown. Differential protein expression was quantified by LC-MS/MS using SWATHTM technologies. Expression of TSP-1 protein and mRNA was confirmed by Western blot analysis and qPCR, respectively. Conventional outflow facility was measured in ex vivo mouse eyes.en_US
dcterms.abstractResults : Proteomic analyses identified 20 proteins whose expression were significantly altered after hTM cells were treated with Y39983 for 2 days. Of these, thrombospondin-1 (TSP-1) was downregulated 5-fold following Y39983 treatment. In addition, Y39983 elicited a dose-dependent inhibition of hTM cell migration. Similarly, LSKL and TSP-1 siRNA knockdown significantly reduced TSP-1 gene expression (~50% reduction and ~80% reduction, respectively) and hTM cell migration, respectively. In the presence of Y39983, no further inhibition of cell migration was observed after LSKL treatment and TSP-1 gene silencing. Likewise, LSKL increased the outflow facility in mouse eyes by 74%, similar to that of Y39983 (increase by 82%). There were no additive effects with simultaneous treatment with LSKL and Y39983.en_US
dcterms.abstractConclusions : Y39983 down-regulated the TSP-1 expression in hTM and silencing TSP-1 gene expression improved the outflow facility. Since there was no additive effect with combined treatment of Y39983 and TSP-1 blockade, the results suggests that TSP-1 is a downstream effector of ROCK inhibition that regulates outflow facility.en_US
dcterms.accessRightsopen accessen_US
dcterms.bibliographicCitationInvestigative ophthalmology and visual science, June 2021, v. 62, no. 8, 1631 (Abstract)en_US
dcterms.isPartOfInvestigative ophthalmology and visual scienceen_US
dcterms.issued2021-06-
dc.relation.conferenceARVO Annual Meetingen_US
dc.identifier.eissn1552-5783en_US
dc.identifier.artn1631en_US
dc.description.validate202205 bcfcen_US
dc.description.oaMetadata onlyen_US
dc.identifier.FolderNumberSO-0018-
dc.description.fundingSourceRGCen_US
dc.description.fundingSourceOthersen_US
dc.description.fundingTextPolyU internal grants; Henry G. Leong Endowed Professorship in Elderly Vision Health; Centre for Eye and Vision Research, Hong Kong; Shenzhen Science and Technology Innovation Commissionen_US
dc.description.pubStatusPublisheden_US
dc.identifier.OPUS55430469-
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