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3. Insights into Species Preservation: Cryobanking of Rabbit Somatic and Pluripotent Stem Cells

Author

Gavin-Plagne, Lucie, Perold, Florence, Osteil, Pierre, Voisin, Sophie, Moreira, Synara Cristina, Combourieu, Quitterie, Saïdou, Véronique, Mure, Magali, Louis, Gérard, Baudot, Anne, Buff, Samuel, Joly, Thierry, Afanassieff, Marielle, VetAgro-Sup (UPSP ICE), Institut cellule souche et cerveau (U846 Inserm - UCBL1), Institut National de la Recherche Agronomique (INRA)-Université Claude Bernard Lyon 1 (UCBL), Université de Lyon-Université de Lyon-Institut National de la Santé et de la Recherche Médicale (INSERM), Laboratoire de Recherche Vasculaire Translationnelle (LVTS (UMR_S_1148 / U1148)), Université Paris 13 (UP13)-Université Paris Diderot - Paris 7 (UPD7)-Institut National de la Santé et de la Recherche Médicale (INSERM), ISARA-Lyon, French National Research Agency (ANR)ANR-12-RPIB-0013Infrastructures Nationales en Biologie et Sante CRB-Anim ANR-11-INBS-0003INGESTEM ANR-11-INBS-0009Laboratoires d'Excellence Revive ANR-10-LABX-73DEVweCAN ANR-10-LABX-006, AFANASSIEFF, Marielle, and Isara

Subjects
Cryopreservation, Male, Pluripotent Stem Cells, Induced Pluripotent Stem Cells, cryobanking, rabbit, dimethyl sulfoxide, Cell Differentiation, Ear, [SDV.BDLR]Life Sciences [q-bio]/Reproductive Biology, Article, synthetic medium, lcsh:Chemistry, Blastocyst, Cryoprotective Agents, lcsh:Biology (General), lcsh:QD1-999, Animals, pluripotent stem cell, somatic cell, Rabbits, lcsh:QH301-705.5, [SDV.BDLR] Life Sciences [q-bio]/Reproductive Biology, Biological Specimen Banks
Abstract

Induced pluripotent stem cells (iPSCs) are obtained by genetically reprogramming adult somatic cells via the overexpression of specific pluripotent genes. The resulting cells possess the same differentiation properties as blastocyst-stage embryonic stem cells (ESCs) and can be used to produce new individuals by embryonic complementation, nuclear transfer cloning, or in vitro fertilization after differentiation into male or female gametes. Therefore, iPSCs are highly valuable for preserving biodiversity and, together with somatic cells, can enlarge the pool of reproductive samples for cryobanking. In this study, we subjected rabbit iPSCs (rbiPSCs) and rabbit ear tissues to several cryopreservation conditions with the aim of defining safe and non-toxic slow-freezing protocols. We compared a commercial synthetic medium (STEM ALPHA.CRYO3) with a biological medium based on fetal bovine serum (FBS) together with low (0&ndash, 5%) and high (10%) concentrations of dimethyl sulfoxide (DMSO). Our data demonstrated the efficacy of a CRYO3-based medium containing 4% DMSO for the cryopreservation of skin tissues and rbiPSCs. Specifically, this medium provided similar or even better biological results than the commonly used freezing medium composed of FBS and 10% DMSO. The results of this study therefore represent an encouraging first step towards the use of iPSCs for species preservation.

Published
2020
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4. Laparoscopic insemination method in sheep allows the use of an animal protein-free and inexpensive freezing medium

Author

Gavin-Plagne, Lucie, Boyer, Lionel, Baudot, Anne, Guedes Teixeira, Magda, Louis, Gérard, Commin, Loris, Buff, Samuel, Joly, Thierry, IMV-Technologies, Union de coopérative FEDATEST, Paysat Bas, Université Paris Descartes - Paris 5 (UPD5), Laboratoire de Recherche Vasculaire Translationnelle (LVTS (UMR_S_1148 / U1148)), Université Paris 13 (UP13)-Université Paris Diderot - Paris 7 (UPD7)-Institut National de la Santé et de la Recherche Médicale (INSERM), Interactions Cellules Environnement - UR (ICE), VetAgro Sup - Institut national d'enseignement supérieur et de recherche en alimentation, santé animale, sciences agronomiques et de l'environnement (VAS), ISARA-Lyon, International Embryo Technology Society, ANR-11-INBS-0003,CRB-Anim,Réseau de Centres de Ressources Biologiques pour les animaux domestiques(2011), ISARA-LYON (ISARA-LYON), and ANR-11-INBS-0003/11-INBS-0003,CRB-Anim,Réseau de Centres de Ressources Biologiques pour les animaux domestiques(2011)

Subjects
[SDV.BA.MVSA]Life Sciences [q-bio]/Animal biology/Veterinary medicine and animal Health, [SDV.BIO]Life Sciences [q-bio]/Biotechnology, [PHYS.PHYS.PHYS-BIO-PH]Physics [physics]/Physics [physics]/Biological Physics [physics.bio-ph], [SDV.BDLR.RS]Life Sciences [q-bio]/Reproductive Biology/Sexual reproduction
Abstract

International audience; Animal-derived products are widely used in sperm cryopreservation for their cryoprotective properties. These components, however, must be replaced because of sanitary risks. STEMALPHA.CRYO3 (Ref. 5617, Stem Alpha), called CRYO3, is a chemically defined preservation medium currently used for freezing human tissue and adult stem cells. The aim of this study was to evaluate the effects of a CRYO3-based medium and of two cooling rates on in vitro parameters and in vivo fertility of ram sperm. Six rams (Blanche du Massif Central) were subjected to sperm collection four times using an artificial vagina. Sperm were split and frozen in three media: an egg yolk and milk-based medium (positive control), a CRYO3-based medium (tested medium), and a medium without additives (negative control). The two cooling rates were related to the distance between the straws and the surface of liquid nitrogen during the freezing process (5 and 20 cm). Sperm membrane integrity (propidium iodide/SYBR-14), acrosome integrity (fluorescein isothiocyanate-peanut agglutinin/propidium iodide; FITC-PNA/PI), and mitochondrial membrane potential (JC-1) were assessed using flow cytometry, whereas functional membrane integrity was assessed using a hypo-osmotic swelling test and motion characteristics were evaluated using computer-assisted sperm analysis. Pregnancy rate, parturition rate, and prolificacy were evaluated after performing laparoscopic inseminations (n ¼ 75 ewes). Moreover, we characterised the freezing media thermodynamically using a differential scanning calorimeter. Statistical analyses were performed using R software. In vitro parameters were assessed using a mixed model including the time and the medium as fixed effects and the ram as a random effect. Pregnancy and parturition rates, following a binomial distribution, and prolificacy, assumed to follow a Poisson distribution, were analysed using generalised linear models, including the medium as a fixed effect and the ram as a random effect. Differences with P , 0.05 were considered statistically significant. The cooling rates had no significant effect except on the wobble motion parameter. The positive control medium showed significantly higher results than the CRYO3-based medium and the negative control medium for all in vitro parameters except for straightness motion parameter. Conversely, field trials showed no significant difference between the media for pregnancy rate (71, 64, and 74%), parturition rate (68, 61, and 74%) and prolificacy (2.0, 2.1, and 1.7), for the positive control, CRYO3-based medium, and the negative control, respectively. This study showed that the product, CRYO3, cannot replace egg yolk and milk in freezing extenders. Moreover, we showed that laparoscopic inseminations allowed a 74% parturition rate due to an easy and inexpensive medium comprising only a Tris buffer and glycerol. Although it could not be used on a large scale, this medium remains an option for international transport or long-term storage of genetic diversity.

Published
2020
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5. Long-term antibiotic-free preservation of rainbow trout milt (oncorhynchus mykiss)

Author

Gavin-Plagne, Lucie, Na, Li, Goardon, Lionel, Labbé, Laurent, Schmitt, Eric, Leboucher, Richard, IMV Technologies, Pisciculture Expérimentale INRA des Monts d'Arrée (PEIMA), and Institut National de la Recherche Agronomique (INRA)

Subjects
endocrine system, animal structures, trout sperm, motility standardization, milt activation, urogenital system, animal diseases, [SDV]Life Sciences [q-bio], education, liquid preservation, CASA system, sperm velocity
Abstract

Long-term antibiotic-free preservation of rainbow trout milt (oncorhynchus mykiss). 7. International Workshop on the Biology of Fish Gametes

Published
2019

6. Changes in sperm cryopreservation procedure for industrial needs

Author

Labbé, Catherine, Delhomme, Guy, Depince, Alexandra, Gavin-Plagne, Lucie, Goardon, Lionel, Kica, Stéphanie, Leboucher, Richard, Morvezen, Romain, Na, Li, Laboratoire de Physiologie et Génomique des Poissons (LPGP), Institut National de la Recherche Agronomique (INRA)-Structure Fédérative de Recherche en Biologie et Santé de Rennes ( Biosit : Biologie - Santé - Innovation Technologique ), IMV Technologies, Pisciculture Expérimentale INRA des Monts d'Arrée (PEIMA), Institut National de la Recherche Agronomique (INRA), Syndicat des Sélectionneurs Avicoles et Aquacoles Français (SYSAAF), Work funded by the FEAMP BIOGERM project and by the PIA CRB Anim (ANR-11-INBS-0003), ANR-11-INBS-0003,CRB-Anim,Réseau de Centres de Ressources Biologiques pour les animaux domestiques(2011), Syndicat des Sélectionneurs Avicoles et Aquacoles Français, and Work funded by the FEAMP BIOGERM (2017, mesure 49) project and by the PIA CRB Anim (ANR-11-INBS-0003

Subjects
Cryoconservation, raft, urogenital system, [SDV]Life Sciences [q-bio], education, MeOH, Poisson, Digitcool, Rainbow trout, Cryoconservation du sperme, neomale, Oncorhynchus mykiss, Sperme, sense organs, skin and connective tissue diseases, DMSO, health care economics and organizations
Abstract

Changes in sperm cryopreservation procedure for industrial needs. 7. International Workshop on the Biology of Fish Gametes

Published
2019

7. Advancing Cryobank strategies: Innovations and Challenges in Fish Genetic Preservation.

Author

Gavin-Plagne, Lucie

Subjects
GERMPLASM conservation, GERMPLASM, AQUATIC resources, FISH farming, AQUATIC biodiversity
Abstract

As global biodiversity faces unprecedented threats, the conservation of genetic diversity has become a priority in preserving ecosystems and species. Fish genetic preservation, a critical component of aquatic biodiversity conservation, has seen significant advancements through cryobanking strategies. This communication provides an overview of the different cryobank strategies and discusses the practical applications and challenges of cryopreservation in fish genetic resources. For years, cryopreservation in fish production was primarily used for genetic resource storage, beginning in the 1990s. It became essential for breeding programs, especially with advancements in genomics and the selection for disease resistance. However, the application of cryopreservation was largely limited to off-site facilities until 2016, when IMV Technologies introduced production-based laboratories directly into fish hatcheries. This shift allowed cryopreservation to become a more integrated part of fish farming operations. Today, various organizational models for cryopreservation services exist worldwide. In the United States and Denmark, public institutes offer off-site cryopreservation services. In France, cooperatives provide similar support, while in Chile and Norway, private companies handle these services. IMV Technologies offers an innovative on-site service model, setting up laboratories within farms. This enables farmers to collect, freeze, and store sperm on-site, providing them with more flexibility and control over their genetic resources. These developments in cryobanking strategies highlight the need for significant European and national funding to expand and optimize cryobank infrastructure. Establishing and maintaining cryobanks requires substantial resources, and financial support is crucial to fully realize the potential of these technologies. Adequate funding would not only facilitate broader adoption of cryopreservation but also improve the management of genetic resources, ultimately contributing to the sustainability of fish populations. In conclusion, while significant progress has been made in fish genetic preservation, ongoing research and collaboration are essential to overcome existing barriers and ensure the long-term sustainability of aquatic genetic resources. This communication serves as a call to action for researchers, policymakers, and conservationists to prioritize and invest in the development of robust cryobank strategies as part of global efforts to safeguard our planet's aquatic heritage. [ABSTRACT FROM AUTHOR]

Published
2024

8. Comparison Between an Animal-Derived Product Medium and a Chemically Defined Medium for Ram Sperm Cryopreservation.

Author

Gavin-Plagne, Lucie, Commin, Loris, Bruyère, Pierre, Buff, Samuel, and Joly, Thierry

Abstract

Animal-derived products are widely used in sperm cryopreservation for their cryoprotective properties. These components, however, tend to be replaced because of sanitary risks. STEMALPHA.CRYO3 (Ref. 5617; Stem Alpha, Saint-Genis-l'Argentière, France), called "CRYO3," is a chemically defined preservation medium currently used for freezing human tissue and adult stem cells. The aim of this study was to evaluate the effect of a CRYO3-based medium on ram sperm freezing regarding in vitro parameters and in vivo fertility. Semen from nine Charolais rams was collected using an artificial vagina, then split and frozen using two media: a CRYO3-based medium or a control medium containing egg yolk (10%) and milk (45%). Sperm membrane integrity (propidium iodide [PI]/SYBR-14 and calcein AM/ethidium homodimer-1), acrosome integrity (FITC-PNA/PI), and mitochondrial membrane potential (JC-1) were assessed using flow cytometry, while functional membrane integrity was assessed using a hypo-osmotic swelling test and motility parameters, evaluated by computer-assisted sperm analysis. Pregnancy rates, prolificacy, and the average daily weight gain (DWG) of lambs were evaluated after performing 195 laparoscopic inseminations. The control medium showed significantly higher results than CRYO-based medium for all in vitro parameters, except for linearity and straightness (motions parameters). Conversely, field trials showed no significant difference between the control medium and the CRYO3-based medium for pregnancy rates (72.2% and 67.9%, respectively), prolificacy (1.8 and 1.6, respectively), and the DWG (0.34 and 0.35 kg/d, respectively). This preliminary study showed that CRYO3 cannot replace egg yolk and milk in freezing extenders for commercial purposes. However, as laparoscopic inseminations allowed a 67% pregnancy rate, CRYO3-based medium remains an option for international transport or long-term storage of genetic diversity. [ABSTRACT FROM AUTHOR]

Published
2019
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11. INRA96 Supplemented With Phospholipids Liposomes, A Promising Approach for Stallion Sperm Chilling.

Author

Eterpi, Mickael, Magistrini, Michele, Couty, Isabelle, Gavin-Plagne, Lucie, Aguirre-Lavin, Tiphaine, Schmitt, Eric, and Carion, Olivier

Abstract

• INRA96 extender supplemented with liposomes of egg yolk phospholipids improves significantly motility parameters Among biotechnologies of reproduction in the equine species, artificial insemination remains the most used technology especially for cooled transported sperm. Although the use of INRA96 extender has demonstrated its efficiency for long-term sperm storage at 4°C or 15°C, some stallions ("bad coolers") are excluded from such technology. Some years ago, we demonstrated that liposomes produced from egg yolk (EY) phospholipids could be an alternative to egg yolk plasma in stallion freezing extenders. To develop a new extender for sperm chilling, we evaluated the protective effect of liposomes produced from EY phospholipids on stallion sperm storage at 4°C. The sperm of stallions from two studs was diluted in INRA96 extender (as control) or an experimental extender (EE) composed of INRA96 supplemented with liposomes of EY phospholipids. After 24H (D1), 72H (D3), and 6 days (D6) or 7 days (D7), motility parameters were evaluated using Computer Assisted Semen Analyzer. Our results demonstrated that total and progressive motility decreased significantly after dilution and storage in INRA96 between D1 and D3 (P <.05) while no significant decrease was observed between D1 and D3 with EE. Regarding VAP parameter, no significant difference was observed between extenders except at D7 in stud 2. Moreover, total and progressive motility were maintained at a significantly higher level (D3, D6, D7) when sperm was stored in EE compared to INRA96. These promising results demonstrate that the supplementation of INRA96 extender with egg-yolk phospholipids liposomes allows a higher protection to stallion sperm cells. [ABSTRACT FROM AUTHOR]

Published
2022
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12. The effect of adjusting settings within a Computer-Assisted Sperm Analysis (CASA) system on bovine sperm motility and morphology results.

Author

O'Meara C, Henrotte E, Kupisiewicz K, Latour C, Broekhuijse M, Camus A, Gavin-Plagne L, and Sellem E

Abstract

Semen motility is the most widely recognized semen quality parameter used by Artificial Insemination (AI) centers. With the increasing worldwide export of semen between AI centers there is an increasing need for standardized motility assessment methods. Computer-Assisted Sperm Analysis (CASA) technology is thought to provide an objective motility evaluation; however, results can still vary between laboratories. The aim of present study was to verify the impact of different setting values of the CASA IVOS II on motility, concentration, and morphology of bovine semen samples frozen in an extender with or without egg yolk and then decide on optimal settings for a further validation step across AI centers. Semen straws from 30 different bulls were analyzed using IVOS II with twelve modified settings. No significant changes were observed in semen concentration, percentage of motile sperm or kinetic results for either extender type. However, increasing settings for both STR and VAP progressive (%) from Low, Medium, and High cut-off values significantly (p<0.05) reduced the percentage of detected progressive spermatozoa, in egg yolk extender from 49.5±15.2, 37.2±11.9 to 11.9±5.3%, and in clear extender from 51.9±9.1, 35.8±7.3 to 10.0±2.4%, respectively. In clear extender only, the modification of droplet proximal head length significantly affected the detection of normal sperm percentages (88.0± 4.7 to 95.0±0.6 and 96.0±0.6%) and of the percentage of detected proximal droplets (12.2±4.7, 2.5±2.7 to 0.6±0.2%) for Low, Medium and High values respectively (p<0.05). The identification of sensitivity within the CASA system to changes in set parameters then led to the determination of an optimal IVOS II setting. The existing variability among centers for these phenotypes was reduced when the standardized settings were applied across different CASA units. The results clearly show the importance of applied settings for the final CASA results and emphasize the need for standardized settings to obtain comparable data., Competing Interests: Conflicts of interest: The authors have no conflict of interest to declare.

Published
2022
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