Successful pregnancy after SrCl<sub>2</sub>oocyte activation in couples with repeated low fertilization rates following calcium ionophore treatment

Kim, Junwoo; Kim, Sang‐Don; Yang, Seong-Ho; Yoon, San-Hyun; Jung, Jaehoon; Lim, Jin‐Ho

doi:10.3109/19396368.2014.900832

“…In contrast, the efficiency of Sr 2+ in activating human oocytes is still debatable (Yanagida et al 2006, Kim et al 2015. Several authors described the efficiency of Sr 2+ in 'rescuing' human oocytes that failed to fertilize after ICSI (Kyono et al 2008, Kim et al 2014. On the contrary, other authors did not find that Sr 2+ stimulated Ca 2+ oscillations even after several hours of measurements (Rogers et al 2004, Lu 2015.…”

Section: +mentioning

confidence: 82%

Single Ca2+ transients vs oscillatory Ca2+ signaling for assisted oocyte activation: limitations and benefits

Ferrer-Buitrago

¹

,

Bonte

²

,

Sutter

³

et al. 2018

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“…To date, Sr 2+ has been applied as an AOA method to overcome FF or low fertilization rates (Kyono et al , 2008; Kim et al , 2012, 2014) in several IVF centers. However, the efficiency and the exact mechanism of Sr 2+ as an activation agent in human oocytes remains largely unknown.…”

Section: Discussionmentioning

confidence: 99%

“…Thereafter, the technology of assisted oocyte activation (AOA) is frequently applied during ICSI, with the principle of inducing a Ca 2+ increase within the FF oocytes. Thus far, a number of physical, mechanical and chemical AOA methods have been evaluated, with successful oocyte activation and development to term after applying electrical pulses (Egashira et al , 2009), modified ICSI procedures (Tesarik et al , 2002), Ca 2+ ionophores (Heindryckx et al , 2008; Ebner et al , 2012; Vanden Meerschaut et al , 2014) and strontium chloride (SrCl 2 ) (Kim et al , 2012, 2014).…”

Section: Introductionmentioning

confidence: 99%

“…Despite several studies reporting successful pregnancies obtained following AOA treatment with Sr 2+ (Yanagida et al , 2006; Kyono et al , 2008; Kim et al , 2012, 2014), the efficiency of Sr 2+ as an activating agent for human oocytes is still under debate. In contrast to mice and rats oocytes studies, in which repetitive Ca 2+ transients are observed when Sr 2+ is used (Whittingham and Siracusa, 1978; Roh et al , 2003), there is a lack of evidence supporting the same for human oocytes (Versieren et al , 2010).…”

Section: Introductionmentioning

confidence: 99%

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Strontium fails to induce Ca2+ release and activation in human oocytes despite the presence of functional TRPV3 channels

Yang

¹

,

Reddy

²

,

Buitrago

³

et al. 2018

Human Reproduction Open

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STUDY QUESTION Are the transient receptor potential cation channels vanilloid 3 (TRPV3) present and able to mediate strontium (Sr 2+ ) induced artificial activation in human oocytes? SUMMARY ANSWER Sr 2+ did not induce Ca 2+ rises or provoke activation in human oocytes, however, mRNA for the TRPV3 channel was present in metaphase II (MII) human oocytes after IVM and TRPV3 agonists induced Ca 2+ rises and oocyte activation, demonstrating the channels were functional. WHAT IS KNOWN ALREADY Selective activation of TRPV3 by agonists induces Ca 2+ entry and promotes mouse oocyte activation, and the absence of TRPV3 channels in mouse oocytes prevents Sr 2+ mediated artificial activation. Sr 2+ is sometimes used to overcome fertilization failure after ICSI in the clinic, but its efficiency is still controversial and the mechanism(s) of how it mediates the Ca 2+ flux has not been studied yet in human. STUDY DESIGN, SIZE, DURATION The protein distribution ( n = 10) and mRNA expression level ( n = 19) of the TRPV3 channels was investigated in human MII oocytes after IVM. The Sr 2+ (10 mM) and TRPV3 agonists (200 μM 2-aminoethoxydiphenyl borate [2-APB] and 200 μM carvacrol)-induced Ca 2+ response was analyzed in human ( n = 15, n = 16 and n = 16, respectively) and mouse oocytes ( n = 15, n = 19 and n = 26, respectively). The subsequent embryonic developmental potential following the parthenogenetic activation using these three agents was recorded in human ( n = 10, n = 9 and n = 9, respectively) and mouse ( n = 20 per agent) oocytes, by determining pronucleus, or 2-cell and blastocyst formation rates. PARTICIPANTS/MATERIALS, SETTING, METHODS MII oocytes from B6D2F1 mice (6–10 weeks old) as well as human IVM oocytes and IVO oocytes (from patients aged 25–38 years old) with aggregates of smooth endoplasmic reticulum clusters were used. The expression of TRPV3 channels was determined by immunofluorescence staining with confocal microscopy and RT-PCR, and the temporal evolution of intracellular Ca 2+ concentration was measured by time-lapse imaging after exposure to Sr 2+ and TRPV3 agonists (2-APB and carvacrol). Artificial activation efficiency was assessed using these agents. MAIN RESULTS AND THE ROLE OF CHANCE S...

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“…Various methods have been employed to induce artificial calcium oscillations in mammalian oocytes in vitro and thereby provoke oocyte activation and embryo development. Electrical pulses [18], calcium ionophore [19], and strontium [20] are typically used as parthenogenetic agents, and it has been demonstrated that electrical pulses and calcium ionophore generate a single calcium elevation, whereas multiple calcium oscillations are induced by normal fertilization or strontium [20]. Moreover, there is some evidence that procaine is able to disregulate cytoplasmic calcium rise(s) in female gametes.…”

Section: Introductionmentioning

confidence: 98%

Procaine Induces Cytokinesis in Horse Oocytes via a pH-Dependent Mechanism1

Leemans

¹

,

Gadella

²

,

Stout

³

et al. 2015

Biology of Reproduction

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Coincubating equine gametes in the presence of procaine has been reported to facilitate in vitro fertilization, with cleavage rates exceeding 60%. We report that while procaine does trigger sperm hyperactivation, it independently induces cleavage of equine oocytes. First, we found that procaine (1-5 mM) did not facilitate stallion sperm penetration of equine oocytes but instead induced sperm-independent oocyte cytokinesis in the absence of the second polar body extrusion. Indeed, 56 ± 4% of oocytes cleaved within 2.5 days of exposure to 2.5 mM procaine regardless of sperm presence. However, the cleaved oocytes did not develop beyond 8 to 16 cells, and the daughter cells either lacked nuclei or contained aberrant, condensed DNA fragments. By contrast, intracytoplasmic sperm injection (ICSI) was followed by second polar body extrusion and formation of normal blastocysts. Moreover, neither the calcium oscillations detectable using fura-2 AM staining nor the cortical granule reaction visualized by LCA-FITC staining, after oocyte activation induced by ICSI or ionomycin treatment, were detected after exposing oocytes to 2.5 mM procaine. Instead, procaine initiated an ooplasmic alkalinization, detectable by BCECF-AM staining that was not observed after other treatments. This alkalinization was followed, after an additional 18 h of incubation, by cortical F-actin depolymerization, as demonstrated by reduced actin phalloidin-FITC staining intensity, that resembled preparation for cytokinesis in ICSI-fertilized zygotes. Overall, we conclude that procaine induces cytokinesis in equine oocytes accompanied by aberrant chromatin condensation and division; this explains why embryos produced after exposing equine oocytes to procaine fail to develop beyond the 8- to 16-cell stage.

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Successful pregnancy after SrCl₂oocyte activation in couples with repeated low fertilization rates following calcium ionophore treatment

Cited by 33 publications

References 39 publications

Single Ca2+ transients vs oscillatory Ca2+ signaling for assisted oocyte activation: limitations and benefits

Single Ca2+ transients vs oscillatory Ca2+ signaling for assisted oocyte activation: limitations and benefits

Strontium fails to induce Ca2+ release and activation in human oocytes despite the presence of functional TRPV3 channels

Procaine Induces Cytokinesis in Horse Oocytes via a pH-Dependent Mechanism1

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Successful pregnancy after SrCl2oocyte activation in couples with repeated low fertilization rates following calcium ionophore treatment

Cited by 33 publications

References 39 publications

Single Ca2+ transients vs oscillatory Ca2+ signaling for assisted oocyte activation: limitations and benefits

Single Ca2+ transients vs oscillatory Ca2+ signaling for assisted oocyte activation: limitations and benefits

Strontium fails to induce Ca2+ release and activation in human oocytes despite the presence of functional TRPV3 channels

Procaine Induces Cytokinesis in Horse Oocytes via a pH-Dependent Mechanism1

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Successful pregnancy after SrCl₂oocyte activation in couples with repeated low fertilization rates following calcium ionophore treatment