Please use this identifier to cite or link to this item: http://hdl.handle.net/11452/21599
Full metadata record
DC FieldValueLanguage
dc.contributor.authorBağış, Haydar-
dc.contributor.authorMercan, Hande Odaman-
dc.contributor.authorDinnyés, András-
dc.date.accessioned2021-09-01T10:19:49Z-
dc.date.available2021-09-01T10:19:49Z-
dc.date.issued2004-02-
dc.identifier.citationBağış, H. vd. (2004). “Vitrification of pronuclear-stage mouse embryos on solid surface (SSV) versus in cryotube: Comparison of the effect of equilibration time and different sugars in the vitrification solution”. Molecular Reproduction and Development, 67(2), 186-192.en_US
dc.identifier.issn1040-452X-
dc.identifier.urihttps://doi.org/10.1002/mrd.10388-
dc.identifier.urihttps://onlinelibrary.wiley.com/doi/10.1002/mrd.10388-
dc.identifier.urihttp://hdl.handle.net/11452/21599-
dc.description.abstractThe cryopreservation of pronuclear-stage embryos has particular importance in transgenic technology and human assisted reproductive technology (ART). The objective of this study was to improve the efficiency of cryopreservation of pronuclear-stage mouse embryos. Two vitrification methods (solid surface vitrification (SSV) vs. vitrification in cryotube) have been compared with special emphasis on the effect of the exposure of the embryos to the solutions for various times and the sugar content (trehalose, sucrose, or raffinose) of the vitrification solutions. Pronuclear-stage embryos were either exposed to I M dimethyl sulfoxide (DMSO)+1 M propylene-glycol (PG) solution for 2, 5, 10, or 15 min or not exposed to this "equilibration" solution. The vitrification solutions consisted of 2.75 M DMSO and 2.75 M PG in M2 medium supplemented with 1 M trehalose (DPT), 1 M sucrose (DPS), or 1 M raffinose (DPR). In the cryotube method, groups of 15-25 embryos were transferred into a 1.8 ml cryotube containing 30 mul of DPT, DPS, or DPR. After 30 sec, the cryotubes were directly plunged into liquid nitrogen (LN2) and stored for 1 day to I month. Vitrified samples were warmed by immersing the cryotubes in a 40degreesC water bath and then immediately diluted with 300 mul of 0.3 M trehalose, sucrose, or raffinose in M2. In the SSV method, after equilibration 15-20 embryos were exposed to DPT, DPS, or DPR solutions for around 20 sec before being dropped in 2-mul drops onto a pre-cooled (-150 to -180degreesC) metal surface. Vitrified droplets were stored in cryovials in LN2. Warming was performed by transferring the vitrified droplets into 0.3 M solutions of trehalose, sucrose, or raffinose at 37degreesC, respectively. Results showed that both SSV and cryotube vitrification methods can result in high rates of in vitro blastocyst development (up to 58.3 and 68.5% with DPR, respectively), not statistically different from that of the controls (58.3 and 64.4%). Even without the equilibration step prior to vitrification, relatively high-survival rates have been achieved, except for the DPS solution. In conclusion, vitrification of pronuclear-stage mouse embryos can result in high rates of in vitro development to blastocyst, and the use of raffinose in the vitrification solution is advantageous to improve cryosurvival.en_US
dc.language.isoenen_US
dc.publisherWileyen_US
dc.rightsinfo:eu-repo/semantics/closedAccessen_US
dc.subjectBiochemistry & molecular biologyen_US
dc.subjectCell biologyen_US
dc.subjectDevelopmental biologyen_US
dc.subjectReproductive biologyen_US
dc.subjectSugarcane streak virusen_US
dc.subjectMiceen_US
dc.subjectPronuclear-stage embryosen_US
dc.subjectRaffinoseen_US
dc.subjectTrehaloseen_US
dc.subjectVitrificationen_US
dc.subjectIn-vitro fertilizationen_US
dc.subjectEthylene-glycolen_US
dc.subjectTransgenic miceen_US
dc.subjectBovine oocytesen_US
dc.subjectDevelopmental stageen_US
dc.subjectLow toxicityen_US
dc.subjectRapid methoden_US
dc.subjectCryopreservationen_US
dc.subjectSurvivalen_US
dc.subject.meshAnimalsen_US
dc.subject.meshBlastocysten_US
dc.subject.meshCarbohydratesen_US
dc.subject.meshCleavage stage, ovumen_US
dc.subject.meshCryopreservationen_US
dc.subject.meshCryoprotective agentsen_US
dc.subject.meshEmbryonic developmenten_US
dc.subject.meshMiceen_US
dc.subject.meshMice, inbred BALB Cen_US
dc.subject.meshMice, inbred C57BLen_US
dc.subject.meshRaffinoseen_US
dc.subject.meshSolutionsen_US
dc.subject.meshSucroseen_US
dc.subject.meshSurface propertiesen_US
dc.subject.meshTime factorsen_US
dc.subject.meshTrehaloseen_US
dc.titleVitrification of pronuclear-stage mouse embryos on solid surface (SSV) versus in cryotube: Comparison of the effect of equilibration time and different sugars in the vitrification solutionen_US
dc.typeArticleen_US
dc.identifier.wos000187889100008tr_TR
dc.identifier.scopus2-s2.0-0346728810tr_TR
dc.relation.publicationcategoryMakale - Uluslararası Hakemli Dergitr_TR
dc.contributor.departmentUludağ Üniversitesi/Veteriner Fakültesi.tr_TR
dc.identifier.startpage186tr_TR
dc.identifier.endpage192tr_TR
dc.identifier.volume67tr_TR
dc.identifier.issue2tr_TR
dc.relation.journalMolecular Reproduction and Developmenten_US
dc.contributor.buuauthorSağırkaya, Hakan-
dc.contributor.researcheridAAH-8821-2021tr_TR
dc.relation.collaborationYurt dışıen_US
dc.relation.collaborationYurt içien_US
dc.identifier.pubmed14694434tr_TR
dc.subject.wosBiochemistry & molecular biologyen_US
dc.subject.wosCell biologyen_US
dc.subject.wosDevelopmental biologyen_US
dc.subject.wosReproductive biologyen_US
dc.indexed.wosSCIEen_US
dc.indexed.scopusScopusen_US
dc.indexed.pubmedPubmeden_US
dc.wos.quartileQ2 (Reproductive biology)en_US
dc.wos.quartileQ3 (Cell biology)en_US
dc.wos.quartileQ2 (Biochemistry & molecular biology)en_US
dc.wos.quartileQ3 (Developmental biology)en_US
dc.contributor.scopusid6602400461tr_TR
dc.subject.scopusOocyte Vitrification; Cryoprotectants; Cryopreservationen_US
dc.subject.emtreeCryoprotective agenten_US
dc.subject.emtreeDimethyl sulfoxideen_US
dc.subject.emtreeLiquid nitrogenen_US
dc.subject.emtreePropylene glycolen_US
dc.subject.emtreeRaffinoseen_US
dc.subject.emtreeSucroseen_US
dc.subject.emtreeTrehaloseen_US
dc.subject.emtreeAnimal experimenten_US
dc.subject.emtreeAnimal tissueen_US
dc.subject.emtreeBlastocysten_US
dc.subject.emtreeControlled studyen_US
dc.subject.emtreeCryopreservationen_US
dc.subject.emtreeCryotubeen_US
dc.subject.emtreeEmbryoen_US
dc.subject.emtreeEmbryo developmenten_US
dc.subject.emtreeFemaleen_US
dc.subject.emtreeIn vitro studyen_US
dc.subject.emtreeIntermethod comparisonen_US
dc.subject.emtreeMaleen_US
dc.subject.emtreeMouseen_US
dc.subject.emtreeNonhumanen_US
dc.subject.emtreePriority journalen_US
dc.subject.emtreePronucleusen_US
dc.subject.emtreeSolid surface vitrificationen_US
dc.subject.emtreeSuperovulationen_US
dc.subject.emtreeSurvival rateen_US
dc.subject.emtreeVitrificationen_US
Appears in Collections:Scopus
Web of Science

Files in This Item:
There are no files associated with this item.


Items in DSpace are protected by copyright, with all rights reserved, unless otherwise indicated.