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Rho-dependent agonist-induced spatio-temporal change in myosin phosphorylation in smooth muscle cells

dc.contributor.authorMiyazaki, Koji
dc.contributor.authorYano, Takeo
dc.contributor.authorSchmidt, David J.
dc.contributor.authorTokui, Toshiya
dc.contributor.authorShibata, Masao
dc.contributor.authorLifshitz, Lawrence M.
dc.contributor.authorKimura, Satoshi
dc.contributor.authorTuft, Richard A.
dc.contributor.authorIkebe, Mitsuo
dc.date2022-08-11T08:10:03.000
dc.date.accessioned2022-08-23T16:53:54Z
dc.date.available2022-08-23T16:53:54Z
dc.date.issued2001-10-24
dc.date.submitted2008-08-04
dc.identifier.citationJ Biol Chem. 2002 Jan 4;277(1):725-34. Epub 2001 Oct 22. <a href="http://dx.doi.org/10.1074/jbc.M108568200">Link to article on publisher's site</a>
dc.identifier.issn0021-9258 (Print)
dc.identifier.doi10.1074/jbc.M108568200
dc.identifier.pmid11673466
dc.identifier.urihttp://hdl.handle.net/20.500.14038/42379
dc.description.abstractAgonist-induced translocation of RhoA and the spatio-temporal change in myosin regulatory light chain (MLC20) phosphorylation in smooth muscle was clarified at the single cell level. We expressed green fluorescent protein-tagged RhoA in the differentiated tracheal smooth muscle cells and visualized the translocation of RhoA in a living cell with three-dimensional digital imaging analysis. The stimulation of the cells by carbachol initiated the translocation of green fluorescent protein-tagged wild type RhoA to the plasma membrane within a minute. The change in MLC20 phosphorylation level after carbachol stimulation was monitored by using phospho-Ser-19-specific antibody recognizing the phosphorylated MLC20 in single cells. Cells expressing the dominant negative form (T19N) of RhoA significantly suppressed sustained MLC20 phosphorylation during the prolonged phase (>300 s), whereas the maximum phosphorylation level (reached at 10 s after stimulation) of these cells was not significantly different from the control cells. The kinetics of RhoA translocation was consistent with that of sustained myosin phosphorylation, suggesting the involvement of a RhoA pathway. Carbachol stimulation increased myosin phosphorylation within a minute both at the cortical and the central region. On the other hand, during prolonged phase, myosin phosphorylation was sustained at the cortical region of the cells but not at the central fibers. A myosin light chain kinase-specific inhibitor, ML-9, diminished myosin phosphorylation at the central region of the cells after the stimulation but not at the cortical area. On the other hand, Y-27632, a Rho kinase-specific inhibitor, diminished myosin phosphorylation at the cortical region but not the central region. The results clearly show that the myosin light chain kinase pathway and the Rho pathway distinctly change myosin phosphorylation in smooth muscle cells in both a temporal and spatial manner.
dc.language.isoen_US
dc.relation<a href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=pubmed&cmd=Retrieve&list_uids=11673466&dopt=Abstract">Link to Article in PubMed</a>
dc.relation.urlhttp://dx.doi.org/10.1074/jbc.M108568200
dc.subjectAnimals
dc.subjectBiological Transport
dc.subjectCOS Cells
dc.subjectCarbachol
dc.subjectCells, Cultured
dc.subjectMuscle, Smooth
dc.subjectMyosin-Light-Chain Kinase
dc.subjectMyosins
dc.subjectPhosphorylation
dc.subjectSwine
dc.subjectTrachea
dc.subjectrhoA GTP-Binding Protein
dc.subjectLife Sciences
dc.subjectMedicine and Health Sciences
dc.titleRho-dependent agonist-induced spatio-temporal change in myosin phosphorylation in smooth muscle cells
dc.typeJournal Article
dc.source.journaltitleThe Journal of biological chemistry
dc.source.volume277
dc.source.issue1
dc.identifier.legacycoverpagehttps://escholarship.umassmed.edu/oapubs/733
dc.identifier.contextkey564648
html.description.abstract<p>Agonist-induced translocation of RhoA and the spatio-temporal change in myosin regulatory light chain (MLC20) phosphorylation in smooth muscle was clarified at the single cell level. We expressed green fluorescent protein-tagged RhoA in the differentiated tracheal smooth muscle cells and visualized the translocation of RhoA in a living cell with three-dimensional digital imaging analysis. The stimulation of the cells by carbachol initiated the translocation of green fluorescent protein-tagged wild type RhoA to the plasma membrane within a minute. The change in MLC20 phosphorylation level after carbachol stimulation was monitored by using phospho-Ser-19-specific antibody recognizing the phosphorylated MLC20 in single cells. Cells expressing the dominant negative form (T19N) of RhoA significantly suppressed sustained MLC20 phosphorylation during the prolonged phase (>300 s), whereas the maximum phosphorylation level (reached at 10 s after stimulation) of these cells was not significantly different from the control cells. The kinetics of RhoA translocation was consistent with that of sustained myosin phosphorylation, suggesting the involvement of a RhoA pathway. Carbachol stimulation increased myosin phosphorylation within a minute both at the cortical and the central region. On the other hand, during prolonged phase, myosin phosphorylation was sustained at the cortical region of the cells but not at the central fibers. A myosin light chain kinase-specific inhibitor, ML-9, diminished myosin phosphorylation at the central region of the cells after the stimulation but not at the cortical area. On the other hand, Y-27632, a Rho kinase-specific inhibitor, diminished myosin phosphorylation at the cortical region but not the central region. The results clearly show that the myosin light chain kinase pathway and the Rho pathway distinctly change myosin phosphorylation in smooth muscle cells in both a temporal and spatial manner.</p>
dc.identifier.submissionpathoapubs/733
dc.contributor.departmentDepartment of Physiology and Biomedical Imaging Group
dc.source.pages725-34


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