Mosaic Gene Expression in Nuclear Transfer-Derived Embryos and the Production of Cloned Transgenic Pigs from Ear-Derived Fibroblasts1

Park, Kwang-Wook; Lai, Liangxue; Cheong, Hyeonsook; Cabot, Ryan; Sun, Qing‐Yuan; Wu, Guangming; Rucker, Edmund B.; Durtschi, David C.; Bonk, Aaron J.; Samuel, Melissa; Rieke, August; Day, Bill; Murphy, Clifton N.; Carter, D.B.; Prather, Randall S.

doi:10.1095/biolreprod66.4.1001

Cited by 127 publications

(89 citation statements)

References 30 publications

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“…Retro-and lentiviral vectors are established potent tools for stable modification of porcine somatic donor cells for SCNT Park et al 2001;Park et al 2002) and have been successfully used for transgene delivery to porcine embryos (Cabot et al 2001;Hofmann et al 2003;Whitelaw et al 2004). SB-directed transgenesis combined with SCNT and HMC represents a nonviral alternative that offers insertion of a defined genetic unit, strong systemic transgene expression, and possibilities of multicopy transgene insertion.…”

Section: Discussionmentioning

confidence: 99%

“…Permanent genetic modification of somatic donor cells for SCNT has been achieved by random genomic insertion of plasmid DNA (Hyun et al 2003;Kragh et al 2009;Kragh et al 2004;Watanabe et al 2005) or by genomic integration of transduced retroviral or lentiviral vectors Park et al 2001;Park et al 2002). In both non-viral and viral approaches inclusion of a drug resistance gene in the transgene-encoding vectors allows selection for cells containing the integrated vector.…”

Section: Introductionmentioning

confidence: 99%

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Pig transgenesis by Sleeping Beauty DNA transposition

Jakobsen

Kragh

et al. 2010

Transgenic Res

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Modelling of human disease in genetically engineered pigs provides unique possibilities in biomedical research and in studies of disease intervention. Establishment of methodologies that allow efficient gene insertion by non-viral gene carriers is an important step towards development of new disease models. In this report, we present transgenic pigs created by Sleeping Beauty DNA transposition in primary porcine fibroblasts in combination with somatic cell nuclear transfer by handmade cloning. Göttingen minipigs expressing green fluorescent protein are produced by transgenesis with DNA transposon vectors carrying the transgene driven by the human ubiquitin C promoter. These animals carry multiple copies (from 8 to 13) of the transgene and show systemic transgene expression. Transgene-expressing pigs carry both transposase-catalyzed insertions and at least one copy of randomly inserted plasmid DNA. Our findings illustrate critical issues related to DNA transposon-directed transgenesis, including coincidental plasmid insertion and relatively low Sleeping Beauty transposition activity in porcine fibroblasts, but also provide a platform for future development of porcine disease models using the Sleeping Beauty gene insertion technology.

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Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Pig transgenesis by Sleeping Beauty DNA transposition

Jakobsen

Kragh

et al. 2010

Transgenic Res

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“…This phenomenon could be due to higher cell numbers from the beginning of embryo culture, or to an epigenetic combination within each embryo that compensates for inefficient cellular reprogramming of individual embryos, or to a combination of both hypotheses. The epigenetic combination obtained after the aggregation of two genetically identical reconstructed embryos that were reprogrammed differently (Boiani et al 2002, Park et al 2002, could compensate for defective individual embryos enhancing developmental competence of aggregates (Eckardt & McLaughlin 2004, Balbach et al 2012. In this manner, aggregation could make the development of a complete embryo possible, even if one of the two contributing embryos may not have been competent alone.…”

Section: Effect Of Iscnt and Aggregation On In Vitro Development Of Dmentioning

confidence: 99%

“…As a result of the donor nucleus and recipient ooplast state, each reconstructed embryo is unique in terms of epigenetic marks and gene expression (Park et al 2002). This characteristic affects embryo quality and consequently cloning success.…”

Section: Introductionmentioning

confidence: 99%

Cheetah interspecific SCNT followed by embryo aggregation improves in vitro development but not pluripotent gene expression

Moro¹,

Hiriart²,

Buemo³

et al. 2015

Reproduction

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The aim of this study was to evaluate the capacity of domestic cat (Dc, Felis silvestris) oocytes to reprogram the nucleus of cheetah (Ch, Acinonyx jubatus) cells by interspecies SCNT (iSCNT), by using embryo aggregation. Dc oocytes were in vitro matured and subjected to zona pellucida free (ZP-free) SCNT or iSCNT, depending on whether the nucleus donor cell was of Dc or Ch respectively. ZP-free reconstructed embryos were then cultured in microwells individually (Dc1X and Ch1X groups) or in couples (Dc2X and Ch2X groups). Embryo aggregation improved in vitro development obtaining 27.4, 47.7, 16.7 and 28.3% of blastocyst rates in the Dc1X, Dc2X, Ch1X and Ch2X groups, respectively (P!0.05). Moreover, aggregation improved the morphological quality of blastocysts from the Dc2X over the Dc1X group. Gene expression analysis revealed that Ch1X and Ch2X blastocysts had significantly lower relative expression of OCT4, CDX2 and NANOG than the Dc1X, Dc2X and IVF control groups. The OCT4, NANOG, SOX2 and CDX2 genes were overexpressed in Dc1X blastocysts, but the relative expression of these four genes decreased in the Dc2X, reaching similar relative levels to those of Dc IVF blastocysts. In conclusion, Ch blastocysts were produced using Dc oocytes, but with lower relative expression of pluripotent and trophoblastic genes, indicating that nuclear reprogramming could be still incomplete. Despite this, embryo aggregation improved the development of Ch and Dc embryos, and normalized Dc gene expression, which suggests that this strategy could improve full-term developmental efficiency of cat and feline iSCNT embryos.Reproduction (2015) 150 1-10

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“…Continuation of reprogramming during cleavage stages may either be mediated by maternal factors remaining from the ooplasm or via novel gene expression from a partially reprogrammed somatic nucleus. Observations such as mosaic gene expression in murine and porcine blastocyst stage clones could indicate either differential reprogramming between blastomeres or a differential failure of gene expression (Boiani et al 2002, Park et al 2002. Differential reprogramming between blastomeres would require that modifications occur subsequent to the first cleavage.…”

Section: Introductionmentioning

confidence: 99%

Differential reprogramming of somatic cell nuclei after transfer into mouse cleavage stage blastomeres

Eckardt

Leu²,

Kurosaka³

et al. 2005

Reproduction

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Mammalian somatic cell cloning requires factors specific to the oocyte for reprogramming to succeed. This does not exclude that reprogramming continues during the zygote and cleavage stages. The capacity or role of zygotic and cleavage stages to reprogram somatic cell nuclei is difficult to assess due to the limited development of somatic cell nuclei transplanted into cytoplasts of these stages. Alternatively, tetraploid embryos have been used to study reprogramming and can be assessed for their contribution to extra-embryonic lineages. When mouse cumulus cell nuclei transgenic for Oct4-green fluorescent protein (GFP) were injected into intact two-and four-cell stage blastomeres, manipulated embryos developed into blastocysts with expression of Oct4-GFP as observed in embryos produced by nuclear transfer into metaphase II oocytes. However, only the latter contributed to extra-embryonic tissues in day 10.5 conceptuses, with the exclusion of the somatic genome in cells originating from transfer into blastomeres already at 5.5 days post conception. Somatic nuclei transferred into cleavage stage blastomeres reinitiated expression of an embyronic-specific transgene, but lacked the extent of reprogramming required for contribution to post-implantation development, even when complemented by an embryonic genome.

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Mosaic Gene Expression in Nuclear Transfer-Derived Embryos and the Production of Cloned Transgenic Pigs from Ear-Derived Fibroblasts1

Cited by 127 publications

References 30 publications

Pig transgenesis by Sleeping Beauty DNA transposition

Pig transgenesis by Sleeping Beauty DNA transposition

Cheetah interspecific SCNT followed by embryo aggregation improves in vitro development but not pluripotent gene expression

Differential reprogramming of somatic cell nuclei after transfer into mouse cleavage stage blastomeres

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