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dc.contributor.authorFilatova, T. S.en
dc.contributor.authorAbramochkin, D. V.en
dc.contributor.authorShiels, H. A.en
dc.date.accessioned2021-08-31T14:56:51Z-
dc.date.available2021-08-31T14:56:51Z-
dc.date.issued2020-
dc.identifier.citationFilatova T. S. Warmer, faster, stronger: Ca2+ cycling in avian myocardium / T. S. Filatova, D. V. Abramochkin, H. A. Shiels. — DOI 10.1242/jeb.228205 // Journal of Experimental Biology. — 2020. — Vol. 223. — Iss. 19. — jeb228205.en
dc.identifier.issn220949-
dc.identifier.otherFinal2
dc.identifier.otherAll Open Access, Bronze3
dc.identifier.otherhttps://www.scopus.com/inward/record.uri?eid=2-s2.0-85092750530&doi=10.1242%2fjeb.228205&partnerID=40&md5=14b0765ee89e4190dcb24b335315c409
dc.identifier.otherhttps://journals.biologists.com/jeb/article-pdf/223/19/jeb228205/1979174/jeb228205.pdfm
dc.identifier.urihttp://elar.urfu.ru/handle/10995/101385-
dc.description.abstractBirds occupy a unique position in the evolution of cardiac design. Their hearts are capable of cardiac performance on par with, or exceeding that of mammals, and yet the structure of their cardiomyocytes resembles those of reptiles. It has been suggested that birds use intracellular Ca2+ stored within the sarcoplasmic reticulum (SR) to power contractile function, but neither SR Ca2+ content nor the cross-talk between channels underlying Ca2+-induced Ca2+ release (CICR) have been studied in adult birds. Here we used voltage clamp to investigate the Ca2+ storage and refilling capacities of the SR and the degree of trans-sarcolemmal and intracellular Ca2+ channel interplay in freshly isolated atrial and ventricular myocytes from the heart of the Japanese quail (Coturnix japonica). A trans-sarcolemmal Ca2+ current (ICa) was detectable in both quail atrial and ventricular myocytes, and was mediated only by L-type Ca2+ channels. The peak density of ICa was larger in ventricular cells than in atrial cells, and exceeded that reported for mammalian myocardium recorded under similar conditions. Steadystate SR Ca2+ content of quail myocardium was also larger than that reported for mammals, and reached 750.6±128.2 μmol lâ'1 in atrial cells and 423.3±47.2 μmol lâ'1 in ventricular cells at 24°C. We observed SR Ca2+-dependent inactivation of ICa in ventricular myocytes, indicating cross-talk between sarcolemmal Ca2+ channels and ryanodine receptors in the SR. However, this phenomenon was not observed in atrial myocytes. Taken together, these findings help to explain the high-efficiency avian myocyte excitation-contraction coupling with regard to their reptilian-like cellular ultrastructure. © 2020 Company of Biologists Ltd. All rights reserved.en
dc.description.sponsorshipThe study was supported by the Russian Foundation for Basic Research (19-34-90142 to D.V.A.).en
dc.format.mimetypeapplication/pdfen
dc.language.isoenen
dc.publisherCompany of Biologists Ltden
dc.rightsinfo:eu-repo/semantics/openAccessen
dc.sourceJ. Exp. Biol.2
dc.sourceJournal of Experimental Biologyen
dc.subjectBIRDen
dc.subjectCOTURNIX JAPONICAen
dc.subjectEXCITATION-CONTRACTION COUPLINGen
dc.subjectHEARTen
dc.subjectL-TYPE CA2+ CURRENTen
dc.subjectSARCOPLASMIC RETICULUMen
dc.subjectCALCIUMen
dc.subjectRYANODINE RECEPTORen
dc.subjectANIMALen
dc.subjectCARDIAC MUSCLEen
dc.subjectCARDIAC MUSCLE CELLen
dc.subjectCOTURNIXen
dc.subjectHEART CONTRACTIONen
dc.subjectHEART VENTRICLEen
dc.subjectMETABOLISMen
dc.subjectSARCOPLASMIC RETICULUMen
dc.subjectANIMALSen
dc.subjectCALCIUMen
dc.subjectCOTURNIXen
dc.subjectHEART VENTRICLESen
dc.subjectMYOCARDIAL CONTRACTIONen
dc.subjectMYOCARDIUMen
dc.subjectMYOCYTES, CARDIACen
dc.subjectRYANODINE RECEPTOR CALCIUM RELEASE CHANNELen
dc.subjectSARCOPLASMIC RETICULUMen
dc.titleWarmer, faster, stronger: Ca2+ cycling in avian myocardiumen
dc.typeArticleen
dc.typeinfo:eu-repo/semantics/articleen
dc.typeinfo:eu-repo/semantics/publishedVersionen
dc.identifier.doi10.1242/jeb.228205-
dc.identifier.scopus85092750530-
local.contributor.employeeFilatova, T.S., Department of Human and Animal Physiology, Lomonosov Moscow State University, Leninskiye Gory, 1, 12, Moscow, 119234, Russian Federation, Pirogov Russian National Research Medical University, Department of Physiology, Ostrovityanova str., 1, Moscow, 117997, Russian Federation
local.contributor.employeeAbramochkin, D.V., Department of Human and Animal Physiology, Lomonosov Moscow State University, Leninskiye Gory, 1, 12, Moscow, 119234, Russian Federation, Pirogov Russian National Research Medical University, Department of Physiology, Ostrovityanova str., 1, Moscow, 117997, Russian Federation, Ural Federal University, Mira 19, Ekaterinburg, 620002, Russian Federation, Laboratory of Cardiac Physiology, Institute of Physiology of Komi Science Centre of Ural Branch of Russian Academy of Sciences, Frc Komi Sc Ub Ras, Pervomayskaya str., 50, Syktyvkar, Komi Republic, 167982, Russian Federation
local.contributor.employeeShiels, H.A., Faculty of Biology,Medicine and, Health,Core Technology Facility, University of Manchester, 46 Grafton Street, Manchester, M13 9NT, United Kingdom
local.issue19-
local.volume223-
dc.identifier.wos000582938000017-
local.contributor.departmentDepartment of Human and Animal Physiology, Lomonosov Moscow State University, Leninskiye Gory, 1, 12, Moscow, 119234, Russian Federation
local.contributor.departmentPirogov Russian National Research Medical University, Department of Physiology, Ostrovityanova str., 1, Moscow, 117997, Russian Federation
local.contributor.departmentUral Federal University, Mira 19, Ekaterinburg, 620002, Russian Federation
local.contributor.departmentLaboratory of Cardiac Physiology, Institute of Physiology of Komi Science Centre of Ural Branch of Russian Academy of Sciences, Frc Komi Sc Ub Ras, Pervomayskaya str., 50, Syktyvkar, Komi Republic, 167982, Russian Federation
local.contributor.departmentFaculty of Biology,Medicine and, Health,Core Technology Facility, University of Manchester, 46 Grafton Street, Manchester, M13 9NT, United Kingdom
local.identifier.pure5d7b0bd3-972e-412c-9091-b9f1c778a64buuid
local.identifier.pure14159752-
local.description.orderjeb228205-
local.identifier.eid2-s2.0-85092750530-
local.fund.rffi19-34-90142-
local.identifier.wosWOS:000582938000017-
local.identifier.pmid32843363-
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