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Featured researches published by Delphine Connan.


Human Reproduction | 2013

Lower intracellular concentration of cryoprotectants after vitrification than after slow freezing despite exposure to higher concentration of cryoprotectant solutions

Pierre Vanderzwalmen; Delphine Connan; Luc Grobet; Barbara Wirleitner; Benoit Remy; Sabine Vanderzwalmen; Nicolas H. Zech; Fabien Ectors

STUDY QUESTION What is the intracellular concentration of cryoprotectant (ICCP) in mouse zygotes during vitrification (VIT) and slow-freezing (SLF) cryopreservation procedures? SUMMARY ANSWER Contrary to common beliefs, it was observed that the ICCP in vitrified zygotes is lower than after SLF, although the solutions used in VIT contain higher concentrations of cryoprotectants (CPs). WHAT IS KNOWN ALREADY To reduce the likelihood of intracellular ice crystal formation, which has detrimental effects on cell organelles and membranes, VIT was introduced as an alternative to SLF to cryopreserve embryos and gametes. Combined with high cooling and warming rates, the use of high concentrations of CPs favours an intracellular environment that supports and maintains the transition from a liquid to a solid glass-like state devoid of crystals. Although the up-to-date publications are reassuring in terms of obstetric and perinatal outcomes after VIT, a fear about exposing gametes and embryos to high amounts of CPs that exceed 3-4-fold those found in SLF was central to a debate initiated by advocates of SLF procedures. STUDY DESIGN, SIZE, DURATION Two experimental set-ups were applied. The objective of a first study was to determine the ICCP at the end of the exposure steps to the CP solutions with our VIT protocol (n = 31). The goal of the second investigation was to compare the ICCP between VIT (n = 30) and SLF (n = 30). All experiments were performed in triplicates using mouse zygotes. The study took place at the GIGA-Research Institute of the University of Liège. PARTICIPANTS/MATERIALS, SETTING, METHODS Cell volume is modified by changes in extracellular osmolarity. Hence, we estimated the final ICCP after the incubation steps in the VIT solutions by exposing the cells to sucrose (SUC) solutions with defined molarities. The ICCP was calculated from the SUC concentration that produced no change in cell volume, i.e. when intra- and extracellular osmolarities were equivalent. Cell volume was monitored by microscopic cinematography. ICCP was compared between SLF and VIT based on the principle that a high ICCP lowers the probability of (re)crystallization during warming but increases the probability of over-swelling of the cell due to fast inflow of water. The survival rates of mouse zygotes after SLF or VIT were compared using either (i) various warming rates or (ii) various concentrations of SUC in the warming dilution medium. MAIN RESULTS AND THE ROLE OF CHANCE The ICCP in mouse zygotes during the VIT procedure prior to plunging them in liquid nitrogen was ∼2.14 M, i.e. one-third of the concentration in the VIT solution. After SLF, the warming rate did not affect the zygote survival rate. In contrast, only 3/30 vitrified zygotes survived when warmed slowly but as many as 30/30 zygotes survived when warming was fast (>20 000°C/min). Vitrified zygotes showed significantly higher survival rates than slow-frozen zygotes when they were placed directly in the culture medium or in solutions containing low concentrations of SUC (P < 0.01). These two experiments demonstrate a lower ICCP after VIT than after SLF. LIMITATIONS, REASONS FOR CAUTION The results should not be directly extrapolated to other stages of development or to other species due to possible differences in membrane permeability to water and CPs. WIDER IMPLICATIONS OF THE FINDINGS The low ICCP we observed after VIT removes the concern about high ICCP after VIT, at least in murine zygotes and helps to explain the observed efficiency and lack of toxicity of VIT. STUDY FUNDING / COMPETING INTEREST(S) The study was funded by the FNRS (National Funds for Scientific Research). The authors declare that they have no competing interests.


Stem Cell Research & Therapy | 2015

Tissues from equine cadaver ligaments up to 72 hours of post-mortem: a promising reservoir of stem cells

Mohamad Khir Shikh Alsook; Annick Gabriel; Joëlle Piret; Olivier Waroux; Céline Tonus; Delphine Connan; Etienne Baise; Nadine Antoine


Theriogenology | 2017

Cryopreservation of chicken primordial germ cells by vitrification and slow freezing: A comparative study

Céline Tonus; Delphine Connan; Olivier Waroux; Benoit Vandenhove; Jérome Wayet; Laurent Gillet; Daniel Desmecht; Nadine Antoine; Fabien Ectors; Luc Grobet


Archive | 2018

METHODE DE VITRIFICATION EN UNE ETAPE

Delphine Connan; Fabien Ectors; Pierre Vanderzwalmen; Luc Grobet


Archive | 2018

ONE-STEP VITRIFICATION OF MURINE EMBRYOS CHALLENGES CURRENT PARADIGMS OF CRYOBIOLOGY

Fabien Ectors; Pierre Vanderzwalmen; Nadine Dupuis; Delphine Connan; Luc Grobet


Archive | 2018

VitriCell: The cool way from academic research to company foundation

Delphine Connan; Fabien Ectors; Luc Grobet


Archive | 2017

Surgical co-transfers of genetically engineered pig embryos produced in vitro by ICSI-SMGT

Jessy M'Boumba; Fabien Ectors; Anne-Sophie Van Laere; Delphine Connan; Stefan Deleuze; Kamal Touati; Philippe Delahaut; Daniel Desmecht


Archive | 2016

VITRICELL: new efficient method for cryopreserving cells by vitrification

Delphine Connan; Fabien Ectors; Nadine Antoine; Pierre Vanderzwalmen; Luc Grobet


Archive | 2015

Long term culture, cryopreservation and genetic modification of chicken primordial germ cells

Céline Tonus; Francisco José Garcia Gil; Karine Cloquette; Delphine Connan; Laurent Gillet; Joëlle Piret; Fabien Ectors; Nadine Antoine; Daniel Desmecht; Alain Vanderplasschen; Olivier Waroux; Luc Grobet


Archive | 2015

Equine cadaver ligaments : A new promising source of stem cells

Mohamad Khir Shikh Al Sook; Annick Gabriel; Moustafa Salouci; Joëlle Piret; Elisa Charlier; Céline Tonus; Delphine Connan; Fabien Ectors; Etienne Baise; Nadine Antoine

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