Artificial activation of porcine oocytes matured in vitro

Prather, Randall S.; Eichen, P. A.; Nicks, Diane; Peters, M.S.

doi:10.1002/mrd.1080280413

Cited by 48 publications

(23 citation statements)

References 14 publications

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“…Application of one or more electric pulses has been s h o w n t o i n d u c e m e i o t i c r e s u m p t i o n a n d pronuclear formation in mouse [123,129], rabbit [8,124], sheep [130], cattle [6,131], pig [125,126,[132][133][134] and marmoset [135] oocytes. Furthermore, electrically activated rabbit [8], cattle [6] and pig [126,132,133,[136][137][138] oocytes undergo cleavage and parthenogenetic development to the blastocyst stage.…”

Section: Calcium Ionsmentioning

confidence: 99%

Calcium Release at Fertilization: Artificially Mimicking the Oocyte's Response to Sperm.

Grupen¹,

Nottle²,

Nagashima

2002

Journal of Reproduction and Development

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Abstract. The mechanism of sperm-induced calcium release has been the subject of many studies since the development in the late 1950s of in vitro culture systems that support mammalian fertilization. Despite efforts to elucidate the nature of the signal from the sperm that triggers both the early and late events of oocyte activation, the precise mechanism remains unresolved. Now, with the advent of somatic nuclear transfer technologies, the need to better understand this unique process has been recognised. Nuclear transfer embryos must be induced to commence development artificially because the activating signal from the sperm is absent. The primary activating stimulus is a large increase in the concentration of intracellular-free calcium and numerous physical and chemical treatments have been found to induce calcium changes that initiate the events of oocyte activation. Although live cloned offspring have been produced in a number of species, the overall efficiencies of the nuclear transfer procedures described thus far are unacceptably low and phenotypic anomalies are common. With the aim of improving these efficiencies, researchers are developing artificial activation treatments which induce oocyte responses that mimic those induced by fertilizing sperm. One strategy is to replicate the pattern of calcium change more closely. Another strategy is to couple an activating stimulus with treatments that inhibit maturation (or M-phase) promoting factor (MPF) activity, which regulates meiotic progression in oocytes. This paper reviews what is understood of calcium release at fertilization and describes the treatments that have been used to induce oocyte activation artificially in parthenogenetic and nuclear transfer studies. The relative effectiveness of the strategies employed to mimic the oocyte's response to sperm are discussed. Key words: Oocyte activation, Fertilization, Parthenogenesis, Nuclear transfer (J. Reprod. Dev. 48: 2002) o produce a viable embryo at fertilization, the s p e r m n o t o n l y p r o v i d e s t h e m a l e chromosomal complement, but also the stimulus that initiates development. The mechanism by which the activating signal is transmitted from the sperm to the oocyte is not fully clarified, but it is clear that this signal triggers a large increase in the concentration of intracellular-free calcium. In fertilized sea urchin and Xenopus eggs, the calcium increase takes the form of a propagating wave that originates at the point of sperm attachment and traverses the egg at a velocity of 5 to 10 µm/sec

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Section: Calcium Ionsmentioning

confidence: 99%

Calcium Release at Fertilization: Artificially Mimicking the Oocyte's Response to Sperm.

Grupen¹,

Nottle²,

Nagashima

2002

Journal of Reproduction and Development

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“…This ability allows different manipulations with the zygote such as the creation of parthenogenetic (monoparental) embryos, and nuclear/pronuclear transfer, including interspecies transfer (Chang et al, 2003;Hammer et al, 2001;Liu et al, 2004b;McGrath and Solter, 1983;McGrath and Solter, 1984;McGrath and Solter, 1986). The mature oocyte, awaiting the fertilization at metaphase II, gets activated by the penetrating sperm, but it also can be artificially activated in vitro by chemicals, or even by temperature and pH shifts (Meo et al, 2004;Nagai, 1987;Prather et al, 1991). After activation or fertilization, the oocyte completes meiosis II and one set of maternal chromosomes is extruded as second polar body.…”

Section: Introductionmentioning

confidence: 99%

DNA methylation reprogramming and DNA repair in the mouse zygote

Lepikhov

Wossidlo²,

Arand³

et al. 2010

Int. J. Dev. Biol.

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Here, we summarize current knowledge about epigenetic reprogramming during mammalian preimplantation development, as well as the potential mechanisms driving these processes. We will particularly focus on changes taking place in the zygote, where the paternally derived DNA and chromatin undergo the most striking alterations, such as replacement of protamines by histones, histone modifications and active DNA demethylation. The putative mechanisms of active paternal DNA demethylation have been studied for over a decade, accumulating a lot of circumstantial evidence for enzymatic activities provided by the oocyte, protection of the maternal genome against such activities and possible involvement of DNA repair. We will discuss the various facets of dynamic epigenetic changes related to DNA methylation with an emphasis on the putative involvement of DNA repair in DNA demethylation.

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“…The sperm activation stimulus can be simulated artificially, ie parthenogenetically, via, for example by Ca 2+ ionophore A23187 (Ware et al, 1989), protein synthesis inhibitors (First et al, 1992) or ethanol (Nagai, 1987) and also by an electric pulse. It has been demonstrated that electrically activated oocytes exhibit similar characteristics to penetrated eggs: establishment of zona pellucida block prevents polyspermic penetration (Gwatkin et al, 1973;Behalova et al, 1992), completion of meiosis, chromatin decondensation and pronuclear formation (Landa and Hdjkovd, 1989;Prochazka et al, 1992), cleavage (Tarkowski et al, 1970;Kaufman et al, 1975; Prather et al, 1991;Prochazka et al, 1993) and in particular cases limited postimplantation development (Ozil, 1990). Although the kinetics of pronucleus formation in activated bovine oocytes has been monitored (Landa and Hajkova, 1989;Powell and Barnes, 1992) (Xu et al, 1986).…”

Section: Introductionmentioning

confidence: 99%

Pronucleus formation in bovine oocytes activated by a single electric pulse

Behalová

Smith²,

Hyttel³

et al. 1993

Reprod. Nutr. Dev.

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Summary ― Bovine oocytes matured in vitro were stimulated by a single pulse of direct current (DC), then cultured for 0.5-6 h and evaluated by light (LM) and transmission electron microscopy (TEM). At the light microscopic level, the beginning of oocyte chromatin decondensation was first observed 3 h post-activation (14%). A well-developed pronucleus with evenly granulated nucleoplasm surrounded by nuclear membrane was found in 12, 61 and 81% oocytes at 4, 5 and 6 h postactivation, respectively. The TEM evaluation revealed that nuclear membrane vesicules were first visible at 0.5 h post-activation and became even more prominent at 1 h. Based on these observations, it is concluded that a nuclear membrane starts to form immediately after oocyte activation, while a well-developed pronucleus appears at 4-6 h. oocyte / activation / nuclear envelope / pronucleus / bovine species Résumé ― Formation du pronoyau dans les ovocytes bovins activés par un choc électrique unique. Des ovocytes bovins maturés in vitro ont été stimulés par un seul choc électrique (courant continu), cultivés de 0,5 à 6 h et observés en microscopie optique et électronique à transmission (MET). Au microscope photonique, le début de la décondensation de la chromatine est observable 3 h après l'activation (14%). Un pronoyau bien développé avec un nucléoplasme régulièrement granulaire, entouré d'une membrane, est retrouvé dans 12, 61 et 81 % des ovocytes, 4, 5 et 6 h après activation. La MET révèle que les vésicules formant l'enveloppe nucléaire apparaissent une demiheure après activation et deviennent plus évidentes après 1 h. D'après ces observations, on peut conclure qu'une enveloppe nucléaire commence à se former immédiatement après l'activation de l'ovocyte tandis qu'un pronoyau bien formé n'apparaît qu'après 4 à 6 h.

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Artificial activation of porcine oocytes matured in vitro

Cited by 48 publications

References 14 publications

Calcium Release at Fertilization: Artificially Mimicking the Oocyte's Response to Sperm.

Calcium Release at Fertilization: Artificially Mimicking the Oocyte's Response to Sperm.

DNA methylation reprogramming and DNA repair in the mouse zygote

Pronucleus formation in bovine oocytes activated by a single electric pulse

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