Publication:
Effect of human β-globin bacterial artificial chromosome transgenesis on embryo cryopreservation in mouse models

dc.contributor.authorBoonkusol D.
dc.contributor.authorDinnyes A.
dc.contributor.authorFaisaikarm T.
dc.contributor.authorSangsuwan P.
dc.contributor.authorPratipnatalang N.
dc.contributor.authorSa-Ardrit M.
dc.contributor.authorSaikhun K.
dc.contributor.authorSvasti S.
dc.contributor.authorVadolas J.
dc.contributor.authorWinichagoon P.
dc.contributor.authorFucharoen S.
dc.contributor.authorKitiyanant Y.
dc.date.accessioned2021-04-05T03:36:39Z
dc.date.available2021-04-05T03:36:39Z
dc.date.issued2010
dc.date.issuedBE2553
dc.description.abstractThe purpose of the present study was to investigate the efficiency of embryo cryopreservation for four transgenic (TG) thalassaemic mouse strains, which is a key element of the ongoing gene banking efforts for these highvalue animals. Heterozygous TG embryos were produced by breeding four lines of TG males to wild-type (WT) females (C57BL/6J). Intact two-cell embryos were cryopreserved by vitrification in straws using 35% ethylene glycol. Survival rates of cryopreserved embryos ranged between 91.1% (102/112) and 93.6% (176/188) without significant differences between the lines. In contrast, the paternal line had a significant effect on the development of these embryos to the blastocyst stage, which ranged from 50.6% (92/182) to 77.5% (79/102). This effect was also noted following embryo transfers, with implantation rates varying from 17.3% (19/110) to 78.1% (35/45). The results demonstrate that the in vivo developmental potential is significantly influenced byTG line and reveal a specific line effect on cryosurvival. All bacterial artificial chromosome transgenic fetuses developed from vitrified-warmed embryos showed expression of the human β-globin transgene. In conclusion, the present study shows a strongTG line effect on developmental competence following cryopreservation and the vitrification method was successful to bank the human β-globin TG-expressing mouse strains. © 2010 CSIRO.
dc.format.mimetypeapplication/pdf
dc.identifier.citationReproduction, Fertility and Development. Vol 22, No.5 (2010), p.788-795
dc.identifier.doi10.1071/RD09128
dc.identifier.issn10313613
dc.identifier.other2-s2.0-77951784898
dc.identifier.urihttps://hdl.handle.net/20.500.14740/7582
dc.rights.holderScopus
dc.subject.otherBeta globin
dc.subject.otherEthylene glycol
dc.subject.otherAnimal experiment
dc.subject.otherAnimal tissue
dc.subject.otherArticle
dc.subject.otherBacterial artificial chromosome
dc.subject.otherBlastocyst
dc.subject.otherBreeding line
dc.subject.otherControlled study
dc.subject.otherCryopreservation
dc.subject.otherEmbryo
dc.subject.otherEmbryo cryopreservation
dc.subject.otherEmbryo development
dc.subject.otherEmbryo transfer
dc.subject.otherFemale
dc.subject.otherGene expression
dc.subject.otherHeterozygote
dc.subject.otherIn vivo study
dc.subject.otherMale
dc.subject.otherMouse
dc.subject.otherMouse embryo
dc.subject.otherNidation
dc.subject.otherNonhuman
dc.subject.otherSurvival rate
dc.subject.otherTransgene
dc.subject.otherTransgenics
dc.subject.otherVitrification
dc.subject.otherWild type
dc.subject.otherAnimals
dc.subject.otherBeta-Globins
dc.subject.otherChromosomes, Artificial, Bacterial
dc.subject.otherCryopreservation
dc.subject.otherEmbryo Culture Techniques
dc.subject.otherEmbryo Transfer
dc.subject.otherEmbryo, Mammalian
dc.subject.otherFemale
dc.subject.otherGene Expression
dc.subject.otherGene Transfer Techniques
dc.subject.otherHeterozygote
dc.subject.otherHumans
dc.subject.otherMale
dc.subject.otherMice
dc.subject.otherMice, Inbred C57BL
dc.subject.otherMice, Inbred ICR
dc.subject.otherMice, Knockout
dc.subject.otherMice, Transgenic
dc.subject.otherThalassemia
dc.subject.otherAnimalia
dc.subject.otherBacteria (microorganisms)
dc.titleEffect of human β-globin bacterial artificial chromosome transgenesis on embryo cryopreservation in mouse models
dc.typeArticle
dspace.entity.typePublication
swu.datasource.scopushttps://www.scopus.com/inward/record.uri?eid=2-s2.0-77951784898&doi=10.1071%2fRD09128&partnerID=40&md5=aa76013bb9105ffd5bf468b8b3828a30

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