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

Grupen, Christopher G.; Nottle, Mark B.; Nagashima, Hiroshi

doi:10.1262/jrd.48.313

Cited by 18 publications

(13 citation statements)

References 213 publications

(323 reference statements)

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“…Ethanol-induced Ca 2+ elevation would inactivate the existing CSF and MPF, and the subsequent exposure to protein phosophorylation inhibitor (6-DMAP) would prevent renewal of CSF synthesis in the oocyte and support the further development. Grupen et al (2002) recorded that the kinetics of MPF activity following 6-DMAP treatment was similar to that found in inseminated oocytes. However, compared to 6-DMAP, CHX prolonged the first and shortened the third cell cycle, though cytoskeleton activity was initialized, a large proportion of CHX embryos was unable to accomplished first cleavage (Holm et al 2003).…”

Section: Discussionsupporting

confidence: 52%

“…Ethanol‐induced Ca 2+ elevation would inactivate the existing CSF and MPF, and the subsequent exposure to protein phosophorylation inhibitor (6‐DMAP) would prevent renewal of CSF synthesis in the oocyte and support the further development. Grupen et al. (2002) recorded that the kinetics of MPF activity following 6‐DMAP treatment was similar to that found in inseminated oocytes.…”

Section: Discussionmentioning

confidence: 53%

“…These authors reported that ethanol activation followed by 6-DMAP gave better results in terms of activation, higher cleavage rate and higher proportion of oocytes developing into morula-blastocysts compared with buffalo oocytes activated in ionomycin followed by 6-DMAP. Ethanol promotes a single intracellular Ca 2+ increase of greater and longer amplitude (Grupen et al 2002), and originates both from extracellular entry of Ca 2+ and mobilization of intracellular stores (Loi et al 1998). Ethanol-induced Ca 2+ elevation would inactivate the existing CSF and MPF, and the subsequent exposure to protein phosophorylation inhibitor (6-DMAP) would prevent renewal of CSF synthesis in the oocyte and support the further development.…”

Section: Discussionmentioning

confidence: 99%

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Morphology of Dromedary Camel Oocytes and their Ability to Spontaneous and Chemical Parthenogenetic Activation

Abdoon

Kandil

Berisha

et al. 2007

Reprod Domestic Animals

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The present work was conducted to examine (1) the morphology of dromedary cumulus-oocytes complexes (COCs), (2) to study the incidence of spontaneous development of oocytes in vivo and (3) to assess the ability of in vitro matured dromedary oocytes to chemical parthenogenetic activation compared with in vitro fertilized (IVF) oocytes. COCs were recovered from dromedary ovaries classified according to their morphology into six categories. Oocyte diameter was measured using eye piece micrometer. For chemical activation, COCs with at least three layers of cumulus-cells were in vitro matured (IVM) in TCM 199 + 10 microg/ml FSH + 10 IU hCG/ml + 10% FCS + 50 microg/ml gentamycin. COCs were incubated for 40 h at 38.5 degrees C under 5% CO2 in humidified air. After IVM, matured oocytes with first polar body (first Pb) were divided into two groups. Group 1: activated in 7% ethanol (E) for 5 min followed by culture in 2 mM 6-dimethylaminopurin (6-DMAP, E D, subgroup 1) or 10 microg/ml cycloheximide (CHX, E CHX, subgroup 2) for 3.5 h at 38.5 degrees C under 5% CO2. In group 2, oocytes were activated using 50 microM Ca A23187 (Ca A) for 5 min followed by culture in 2 mM 6-DMAP (Ca D, subgroup 3) or 10 microg/ml CHX(Ca CHX, subgroup 4) for 3.5 h at 38.5 degrees C under 5% CO2. For control group, IVM oocytes were fertilized using frozen-thawed camel spermatozoa separated by swim-up method then suspended in Fert-TALP medium supplemented with 6 mg/ml BSA (FAF) + 10 microg/ml heparin. In all groups, oocytes were in vitro cultured in SOFaa medium + 5% FCS and 5 microg/ml insulin + 50 microg/ml gentamycin. Cleavage rate and embryo development were checked on Days 2, 5 and 8. An average of 11.3 +/- 0.3 COCs were recovered/dromedary ovary. Categories 1 and 2 represented 33.1% and 34.8%, respectively, and were significantly higher (p < 0.01) than the other categories (19.1, 9.2 and 2.6% for categories 3-5, respectively). Category 6 (embryo-like structures) represented 1.2% of the recovered oocytes, staining of these embryo-like structures with orcien dye indicated the presence of divided cells with condensed nuclei. Dromedary oocytes averaged 166.2 +/- 2.6 microm in diameter with black cytoplasm. Chemical activation of IVM dromedary oocyte with first Pb in 7% ethanol or 50 microM Ca A followed by culture in 2 mM 6-DMAP showed significantly higher (p < 0.01) cleavage and developmental rates to the morula stage than oocytes activated using 7% ethanol or 50 microM Ca A followed by 10 microg/ml CHX or in vitro fertilized control group. Higher (p < 0.01) proportion of oocytes sequentially cultured in 10 microg/ml CHX or that in vitro fertilized were arrested at the 2-4-cell stage compared with that cultured in 6-DMAP.

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Section: Discussionsupporting

confidence: 52%

Section: Discussionmentioning

confidence: 53%

Section: Discussionmentioning

confidence: 99%

See 1 more Smart Citation

Morphology of Dromedary Camel Oocytes and their Ability to Spontaneous and Chemical Parthenogenetic Activation

Abdoon

Kandil

Berisha

et al. 2007

Reprod Domestic Animals

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“…While an increase in the intracellular IP3 mediates Ca 2+ release by binding and gating its receptor on the endoplasmic reticulum membrane [22][23][24], DAG may be involved in the regulation of Ca 2+ influx [25,26]. Similarly, it has been shown that parthenogenetic agents activate oocytes also by inducing intracellular Ca 2+ rises [27][28][29][30][31]. Mature rat eggs showed reduced rates of SA when cultured either in calcium-free medium or in calcium-containing medium with L-type calcium channel blocker or IP3 receptor inhibitor [3,32,33].…”

Section: Introductionmentioning

confidence: 99%

Control of Spontaneous Activation of Rat Oocytes by Regulating Plasma Membrane Na+/Ca2+ Exchanger Activities

Cui

Zhang

et al. 2013

Biology of Reproduction

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Inhibiting oocyte spontaneous activation (SA) is essential for successful rat cloning by nuclear transfer (NT). This study tested the hypothesis that activities of the Na(+)/Ca(2+) exchanger (NCX) would decrease with oocyte aging and that SA of rat oocytes could be inhibited if the intraoocyte Ca(2+) rises were prevented by activating the NCX through increasing Na(+) concentrations in the culture medium. Elevating Na(+) levels in culture medium by supplementing NaCl inhibited SA of rat oocytes, while maintaining a constant level of maturation-promoting factor and mitogen-activated protein kinase activities. Experiments using the NCX inhibitor bepridil, the Na(+)/K(+)-ATPase inhibitor ouabain, and an assay for intraoocyte Ca(2+) concentrations showed that extracellular Na(+) inhibited rat oocyte SA by enhancing NCX activity and preventing intracellular Ca(2+) rises. Immunohistochemical quantification indicated that the density of NCX1 decreased significantly in aged oocytes that were prone to SA compared with that in freshly ovulated oocytes whose SA rates were low during in vitro culture. Cumulus cell NT showed that sham enucleation caused marked SA in freshly ovulated rat oocytes and that Na(+) supplementation prevented the manipulation-induced SA and improved the in vitro and in vivo development of rat somatic cell NT embryos. Taken together, the results have confirmed our hypothesis that the NCX is active in rat oocytes and its activity decreases with oocyte aging and that activating the NCX by increasing extracellular Na(+) inhibits SA of rat oocytes and improves the development of rat somatic cell NT embryos. These data are also important for understanding the mechanisms of oocyte aging.

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“…Suss dan Madison (1983) dalam Gordon (1994) mengemukakan bahwa dari beberapa oosit yang dimaturasi kirakira sekitar 50% diantaranya menunjukkan adanya PB dengan konfigurasi kromosom pada MII. (Grupen et al, 2002) selanjutnya menurun pada saat sel masuk fase anafase I dan fase telofase I tetapi meningkat kembali pada saat sel masuk dalam fase metafase II sebagaimana halnya seperti yang dialami pada saat metafase I. Sementara itu, cyclin B disintesa dan terakumulasi ketika p34 cdc2 ada dalam sitoplasma yaitu pada saat interfase (Solomon et al, 1990dalam Mayes, 2002) dan terdegradasi oleh ubiquitin-dependent proteolysis. Sebaliknya kadar p34 cdc2 tidak berubah selama meiosis (Choi et al, 1991).…”

Section: Hasil Penelitian Dan Pembahasanunclassified

Evaluasi Oosit Kambing Hasil Ivm Sebagai Salah Satu Faktor Penentu Keberhasilan Dalam Aktivasi Partenogenesis

Holil

2012

el–Hayah

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Abstrak PENDAHULUANHafez (2000) mengemukakan bahwa oosit secara umum dalam kehidupannya mengalami 2 periode yaitu periode pertumbuhan (period of growth) dan periode pematangan (period of maturation). Pada periode pertumbuhan oosit tumbuh sempurna pada saat berada pada waktu pembentukan antrum sampai pada saat pembentukan cumulus oophorus sudah dalam kondisi kuat. Sedangkan periode pematangan terjadi pada saat meiosis yaitu pada saat fetal ovary dan pada saat sebelum lahir (tahap diploten) yang kemudian terhenti dan berlanjut kembali sampai oosit siap untuk melakukan fertilisasi. Pada kondisi ini oosit ada dalam fase metafase II (MII).Dalam periode pematangan, oosit mengalami 2 hal yaitu maturasi inti (nuclear maturation) dan maturasi sitoplasma (cytoplasmic maturation). Pada maturasi inti, oosit mengalami berbagai proses yaitu dimulai dari proses munculnya germinal vesicle break down (GVBD), kondensasi kromosom, proses pembentukan spindel pada metafase I, proses pemisahan kromosom homolog dengan ekstruksi polar body II sampai pada saat MII (Kubelka et al., 1995). Sedangkan maturasi sitoplasma menyangkut perubahan morfologi dan ultrastruktur dari organel-organel penyusun oosit. Kruip et al., (1983) dalam Mayes, (2002) mengemukakan bahwa terjadinya perubahan morfologi dan ultrastruktur pada maturasi sitoplasma secara tidak langsung menyangkut kemampuan dalam hal untuk bisa berfertilisasi secara normal, cleavage dan berkembang menjadi blastosis (Kruip et al., 1983 dalam Mayes, 2002.Contoh penting terjadinya perubahan ultrastruktur selama maturasi oosit tersebut dapat dilihat pada keberadaan sel-sel kumulus sebagai pemberi makan bagi oosit dan sebagai penyedia produk kunci developmental competence. Kadar glutathion rendah pada oosit immature dan meningkat selama maturasi dan turun pada tahap awal perkembangan embrio. Perreault et al., (1988) dalam Mayes,

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

Cited by 18 publications

References 213 publications

Morphology of Dromedary Camel Oocytes and their Ability to Spontaneous and Chemical Parthenogenetic Activation

Morphology of Dromedary Camel Oocytes and their Ability to Spontaneous and Chemical Parthenogenetic Activation

Control of Spontaneous Activation of Rat Oocytes by Regulating Plasma Membrane Na+/Ca2+ Exchanger Activities

Evaluasi Oosit Kambing Hasil Ivm Sebagai Salah Satu Faktor Penentu Keberhasilan Dalam Aktivasi Partenogenesis

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