Nuclear transfer in cattle with non‐transfected and transfected fetal or cloned transgenic fetal and postnatal fibroblasts

Zakhartchenko, Valeri; Mueller, Sigrid; Alberio, Ramiro; Schernthaner, Wolfgang; Stojković, Miodrag; Wenigerkind, Hendrik; Wanke, Rüdiger; Lassnig, Caro; Mueller, Mathias; Wolf, Eckhard; Brem, Gottfried

doi:10.1002/mrd.1098

Cited by 89 publications

(57 citation statements)

References 30 publications

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“…Iguma et al [25], Forsberg et al [26] and Zakhartchenko et al [27] reported that in the case of cattle, genetic modification of donor cells influences the number of cloned calves born. An increase in chromosomal aberration, such as mutation and deletion due to a long culturing period, is considered one of the causes.…”

Section: Discussionmentioning

confidence: 99%

Effects of Recloning on the Efficiency of Production of .ALPHA.1,3-Galactosyltransferase Knockout Pigs

Fujimura¹,

Murakami²,

Kurome

et al. 2008

Journal of Reproduction and Development

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Abstract. Obtaining sufficient transgenic cells via selective cultivation of genetically manipulated somatic cells is difficult due to the limited number of cell divisions. Additionally, if irreversible mutations in a cell's chromosomes occur during selective cultivation and the cell is used as the nuclear donor, somatic cell nuclear transfer (SCNT) embryos often exhibit abnormal development. On the other hand, a SCNT method in which fetal cells derived from SCNT embryos are used as the nuclear donor (recloning method) is an effective technique for obtaining large quantities of transgenic cells. In this study, we compared the in vivo development rate of SCNT embryos produced from porcine α1-3 galactosyltransferase gene knockout (GTKO) cells by a recloning method with that of SCNT embryos produced without recloning from porcine GTKO cells (direct method). In the direct method, 557 and 462 cloned embryos were produced using two types of activation methods, the two-step activation (TA) method and the delayed activation (DA) method, and then transferred into 6 and 4 recipients, respectively, but no piglets were born from these recipients. In the recloning method, 956 and 1038 cloned embryos were produced using the TA and DA methods, respectively, and then transferred to 8 and 7 recipients, respectively. Two piglets were born from one recipient in the TA group and 6 piglets were born from 3 recipients in the DA group. This report indicates that the recloning method improved the developmental capacity of SCNT embryos reconstructed with gene-targeted somatic cells.

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Section: Discussionmentioning

confidence: 99%

Effects of Recloning on the Efficiency of Production of .ALPHA.1,3-Galactosyltransferase Knockout Pigs

Fujimura¹,

Murakami²,

Kurome

et al. 2008

Journal of Reproduction and Development

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“…47 However, somatic cells have a limited life span in in vitro culture, and the decrease in developmental rates for modified cells has been attributed to the extended culture periods associated with the transfection and selection procedures before SCNT. 48 Studies using different approaches aimed at increasing the efficiency for the generation of viable clones have been performed. The methods investigated include recloning, autologous SCNT, impeding Xist expression from the active X chromosome, treatment with trichostatin A after SCNT and histone deacetylase inhibitors, among others.…”

Section: Strategies For the Generation Of Transgenic Cattlechallengesmentioning

confidence: 99%

Transgenic bovine as bioreactors: Challenges and perspectives

et al. 2016

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The use of recombinant proteins has increased in diverse commercial sectors. Various systems for protein production have been used for the optimization of production and functional protein expression. The mammary gland is considered to be a very interesting system for the production of recombinant proteins due to its high level of expression and its ability to perform post-translational modifications. Cows produce large quantities of milk over a long period of lactation, and therefore this species is an important candidate for recombinant protein expression in milk. However, transgenic cows are more difficult to generate due to the inefficiency of transgenic methodologies, the long periods for transgene detection, recombinant protein expression and the fact that only a single calf is obtained at the end of each pregnancy. An increase in efficiency for transgenic methodologies for cattle is a big challenge to overcome. Promising methodologies have been proposed that can help to overcome this obstacle, enabling the use of transgenic cattle as bioreactors for protein production in milk for industry.

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“…The integrated gene can be examined before proceeding to nuclear transfer. This method is without contest more attractive than microinjection for sheep [35], goats [19,32] and cows [2,43].…”

Section: Gene Additionmentioning

confidence: 99%

Transgenesis for the study and the control of lactation

Houdebiné

Rival

Pantano³

et al. 2002

Reprod. Nutr. Dev.

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-The study and the control of milk synthesis are required to decipher the mechanisms of gene expression, to improve milk production, to modify milk composition, to induce a resistance to diseases in the mammary gland and to produce recombinant proteins of pharmaceutical interest. Transgenesis has become a mandatory tool to reach these goals. The use of transgenesis is still limited by the difficulty of adding foreign genes in farm animals and mainly by replacing genes by homologous recombination. Transgene expression is also often ill-controlled. The present paper summarizes the current progress in this field with a particular emphasis on expression vectors for transgenes. lactation / transgenesis / expression vectorsRésumé -La transgénèse pour l'étude et le contrôle de la lactation. L'étude et le contrôle de la synthèse du lait sont nécessaires pour décrypter les mécanismes de l'expression de gènes, pour amé-liorer la production de lait, pour modifier la composition du lait, pour induire une résistance de la glande mammaire contre des maladies infectieuses et pour produire des protéines recombinantes d'intérêt pharmaceutique. La transgénèse est devenue un outil indispensable pour mener à bien ces projets. La mise en oeuvre de la transgénèse est encore limitée par la difficulté d'ajouter des gènes étrangers chez les animaux d'élevage et surtout de remplacer des gènes par recombinaison homologue. L'expression des transgènes est par ailleurs souvent mal contrôlée. Cet article se propose de faire le point dans ce domaine en développant plus particulièrement la mise au point de vecteurs d'expression pour les transgènes. lactation / transgénèse / vecteurs d'expression

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Nuclear transfer in cattle with non‐transfected and transfected fetal or cloned transgenic fetal and postnatal fibroblasts

Cited by 89 publications

References 30 publications

Effects of Recloning on the Efficiency of Production of .ALPHA.1,3-Galactosyltransferase Knockout Pigs

Effects of Recloning on the Efficiency of Production of .ALPHA.1,3-Galactosyltransferase Knockout Pigs

Transgenic bovine as bioreactors: Challenges and perspectives

Transgenesis for the study and the control of lactation

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