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2. The epoxiconazole and tebuconazole fungicides impair granulosa cells functions partly through the aryl hydrocarbon receptor (AHR) signalling with contrasted effects in obese, normo-weight and polycystic ovarian syndrome (PCOS) patients

Author

Serra, Loise, Estienne, Anthony, Bongrani, Alice, Ramé, Christelle, Caria, Giovanni, Froger, Claire, Jolivet, Claudy, Henriot, Abel, Amalric, Laurence, Corbin, Emilie, Guérif, Fabrice, Froment, Pascal, and Dupont, Joëlle

Published
2024
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12. Extracellular vesicles are carriers of adiponectin with insulin-sensitizing and anti-inflammatory properties.

Author

Blandin, Alexia, Amosse, Jérémy, Froger, Josy, Hilairet, Grégory, Durcin, Maëva, Fizanne, Lionel, Ghesquière, Valentine, Prieur, Xavier, Chaigneau, Julien, Vergori, Luisa, Dray, Cédric, Pradère, Jean-Philippe, Blandin, Stéphanie, Dupont, Joëlle, Ducluzeau, Pierre-Henri, Dubois, Séverine, Boursier, Jérôme, Cariou, Bertrand, and Le Lay, Soazig

Abstract

Recent evidence supporting that adipose tissue (AT)-derived extracellular vesicles (EVs) carry an important part of the AT secretome led us to characterize the EV-adipokine profile. In addition to evidencing a high AT-derived EV secretion ability that is further increased by obesity, we identify enrichment of oligomeric forms of adiponectin in small EVs (sEVs). This adipokine is mainly distributed at the EV external surface as a result of nonspecific adsorption of soluble adiponectin. EVs also constitute stable conveyors of adiponectin in the blood circulation. Adiponectin-enriched sEVs display in vitro insulin-sensitizing effects by binding to regular adiponectin receptors. Adoptive transfer of adiponectin-enriched sEVs in high-fat-diet-fed mice prevents animals from gaining weight and ameliorated insulin resistance and tissue inflammation, with major effects observed in the AT and liver. Our results therefore provide information regarding adiponectin-related metabolic responses by highlighting EVs as delivery platforms of metabolically active forms of adiponectin molecules. [Display omitted] • Adiponectin is abundantly associated with adipose-tissue-derived sEVs • sEVs constitute stable conveyors of adiponectin in the blood circulation • Adiponectin-enriched sEVs display insulin-sensitizing effects in vitro and in vivo • Adiponectin-enriched sEV injections in mice reduce HFD-induced tissue inflammation Blandin et al. show that adipose-tissue-derived sEVs act as stable conveyors of adiponectin in the blood that relay insulin-sensitizing action of the adipokine. Adoptive transfer of adiponectin-enriched sEVs in mice prevents animals from high-fat-diet weight gain, insulin resistance, and tissue inflammation, highlighting sEVs as delivery platforms of adiponectin active forms. [ABSTRACT FROM AUTHOR]

Published
2023
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13. Ulvan from Ulva armoricana (Chlorophyta) activates the PI3K/Akt signalling pathway via TLR4 to induce intestinal cytokine production.

Author

Berri, Mustapha, Olivier, Michel, Holbert, Sébastien, Dupont, Joëlle, Demais, Hervé, Le Goff, Matthieu, and Collen, Pi Nyvall

Abstract

The biological activities of water-soluble sulfated polysaccharides of green algae (ulvans) have been explored for use as bioactive molecules for the benefit of human and animal health. A purified ulvan fraction was prepared from the green algae Ulva armoricana harvested in the Brittany (France) and tested for its capacity to stimulate the immune response of the gut using an in vitro system of porcine intestinal epithelial (IPEC-1) cells. RT-qPCR and ELISA analyses showed a significant increase in the mRNA and protein expression of cytokines such as CCL20, IL8, and TNFα. Using human embryonic kidney (HEK) 293 reporter cell lines for pattern recognition receptors, ulvan was found to primarily stimulate TLR4. We also examined the effect of the ulvan fraction on different signalling pathways involved in the activation of cytokine gene expression. Western blot analyses of ulvan-treated HEK293-TLR4 cells showed an increase in the phosphorylation of Akt and the p65 subunit of nuclear factor-κB. Inhibition of Akt phosphorylation with the specific inhibitor abrogated the ulvan-mediated enhancement of IL-8 secretion. The overall results showed that ulvan is an immunostimulatory compound by itself, and furthermore, it could be used to effectively complex and deliver TLR ligands to relevant immune cells in vaccination strategies. [ABSTRACT FROM AUTHOR]

Published
2017
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14. Nutritional signals and reproduction.

Author

Dupont, Joëlle, Reverchon, Maxime, Bertoldo, Michael J., and Froment, Pascal

Subjects
*HYPOTHALAMIC-pituitary-thyroid axis, *NUTRITION, *HUMAN reproduction, *KINASES, *HORMONES
Abstract

Highlights: [•] Nutrition influences male and female reproductive functions. [•] The hypothalamus–pituitary–gonadal axis is equipped of nutrient sensors. [•] Nutrient sensors include hormones but also kinases, transporters and receptors. [ABSTRACT FROM AUTHOR]

Published
2014
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16. The infusion of glucose in ewes during the luteal phase increases the number of follicles but reduces oestradiol production and some correlates of metabolic function in the large follicles

Author

Gallet, Claire, Dupont, Joëlle, Campbell, Bruce K., Monniaux, Danielle, Guillaume, Daniel, and Scaramuzzi, Rex J.

Subjects
*DRUG infusion pumps, *GLUCOSE, *EWES, *LUTEAL phase, *ESTRADIOL, *AROMATASE, *PHOSPHORYLATION
Abstract

Abstract: Short-term nutritional supplementation stimulates folliculogenesis in ewes probably by insulin-mediated actions of glucose in the follicle. The aim of this study was to determine the effect of glucose on follicle number and granulosa levels of Aromatase P450 and phosphorylated Akt and AMPK. Twelve Ile-de-France ewes were allocated to two groups; one (n =7) infused with saline and the other (n =5) with glucose (10mM/h) for 72h in the luteal phase. At the end of infusion, ovaries were collected and all follicles >1mm in diameter were dissected to recover granulosa cells. Aromatase P450 and phosphorylated Akt and AMPK were analysed by Western blotting of granulosa cell lysates. Blood plasmas collected before and during the infusions were analysed for progesterone, oestradiol, LH, FSH, glucose, insulin and IGF-I. The infusion of glucose significantly increased follicle number but, significantly reduced Aromatase P450 and phosphorylated Akt and AMPK in granulosa cells. The circulating concentration of glucose rose significantly 3h after the start of the glucose infusion and remained elevated until 27h then fell; the circulating concentration of insulin rose significantly by 3h and remained elevated. The circulating concentration of oestradiol fell significantly by 32h and remained low; the circulating concentrations of LH and FSH were unaffected. These data show that short-term infusion of glucose stimulated follicular growth but decreased Aromatase P450 in granulosa cells. The reduced levels of phosphorylated Akt and AMPK suggest that the phosphatidylinositol 3-kinase pathway has been inhibited by high concentrations of glucose. These data also suggest that there may be functional cross-talk between FSH and insulin signalling in granulosa cells. [Copyright &y& Elsevier]

Published
2011
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17. Leucine supplementation in rats induced a delay in muscle IR/PI3K signaling pathway associated with overall impaired glucose tolerance

Author

Balage, Michèle, Dupont, Joëlle, Mothe-Satney, Isabelle, Tesseraud, Sophie, Mosoni, Laurent, and Dardevet, Dominique

Subjects
*DIETARY supplements, *LEUCINE, *MUSCLE proteins, *LABORATORY rats, *CELLULAR signal transduction, *GLUCOSE tolerance tests, *RAPAMYCIN, *PROTEIN synthesis
Abstract

Abstract: Although activation of the mammalian target of rapamycin complex/p70 S6 kinase (S6K1) pathway by leucine is efficient to stimulate muscle protein synthesis, it can also exert inhibition on the early steps of insulin signaling leading to insulin resistance. We investigated the impact of 5-week leucine supplementation on insulin signaling and sensitivity in 4-month old rats fed a 15% protein diet supplemented (LEU) or not (C) with 4.5% leucine. An oral glucose tolerance test was performed in each rat at the end of the supplementation and glucose transport was measured in vitro using isolated epitrochlearis muscles incubated with 2-deoxy-d-[3H]-glucose under increasing insulin concentrations. Insulin signaling was assessed on gastrocnemius at the postabsorptive state or 30 and 60 min after gavage with a nutrient bolus. Tyrosine phosphorylation of IRβ, IRS1 and PI3 kinase activity were reduced in LEU group 30 min after feeding (−36%, −36% and −38% respectively, P<.05) whereas S6K1, S6rp and 4EBP1 phosphorylations were similar. Overall glucose tolerance was reduced in leucine-supplemented rats and was associated with accumulation of perirenal adipose tissue (+27%, P<.05). Conversely, in vitro insulin-response of muscle glucose transport tended to be improved in leucine-supplemented rats. In conclusion, dietary leucine supplementation in adult rats induced a delay in the postprandial stimulation in the early steps of muscle insulin signaling without muscle resistance on insulin-induced glucose uptake. However, it resulted in overall glucose intolerance linked to increased local adiposity. Further investigations are necessary to clearly define the beneficial and/or deleterious effects of chronic dietary leucine supplementation in healthy subjects. [Copyright &y& Elsevier]

Published
2011
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18. FSH-stimulated PTEN activity accounts for the lack of FSH mitogenic effect in prepubertal rat Sertoli cells

Author

Dupont, Joëlle, Musnier, Astrid, Decourtye, Jérémy, Boulo, Thomas, Lécureuil, Charlotte, Guillou, Hervé, Valet, Sophie, Fouchécourt, Sophie, Pitetti, Jean-Luc, Nef, Serge, Reiter, Eric, and Crépieux, Pascale

Subjects
*FOLLICLE-stimulating hormone, *SERTOLI cells, *LABORATORY rats, *LEYDIG cells, *PHOSPHOINOSITIDES, *PHOSPHATASES, *CHROMOSOMES
Abstract

Abstract: Follicle-stimulating hormone (FSH) controls the proliferation and differentiation of Sertoli cells of the testis. FSH binds a G protein-coupled receptor (GPCR) to stimulate downstream effectors of the phosphoinositide-3 kinase (PI3K)-dependent pathway, without enhancing PI3K activity. To clarify this paradox, we explored the activity of phosphatase and tensin homolog deleted in chromosome 10 (PTEN), the PI3K major regulator, in primary cultures of rat Sertoli cells. We show that, within minutes, FSH increases PTEN neo-synthesis, requiring the proteasomal degradation of an unidentified intermediate, as well as PTEN enzymatic activity. Importantly, introducing an antisense cDNA of PTEN into differentiating Sertoli cells restores FSH-dependent cell proliferation. In conclusion, these results provide a new mechanism of PTEN regulation, which could serve to block entry into S phase of Sertoli cells, while they are proceeding through differentiation in prepubertal animals. [Copyright &y& Elsevier]

Published
2010
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19. Molecular and ultrastructural characterization of two ascomycetes found on sunken wood off Vanuatu Islands in the deep Pacific Ocean

Author

Dupont, Joëlle, Magnin, Sandrine, Rousseau, Florence, Zbinden, Magali, Frebourg, Ghislaine, Samadi, Sarah, Richer de Forges, Bertrand, and Gareth Jones, E.B.

Subjects
*ASCOMYCETES, *MARINE fungi, *FUNGAL molecular biology, *FUNGAL ultrastructure, *FUNGI classification
Abstract

Abstract: A new genus of a deep-sea ascomycete with one new species, Alisea longicolla, is described based on analyses of 18S and 28S rDNA sequences and morphological characters. A. longicolla was found together with Oceanitis scuticella, on small twigs and sugar cane debris trawled from the bottom of the Pacific Ocean off Vanuatu Islands. Molecular and morphological characters indicate that both fungi are members of Halosphaeriaceae. Within this family, O. scuticella is phylogenetically related to Ascosalsum and shares similar ascospore morphology and appendage ontogeny. The genus Ascosalsum is considered congeneric with Oceanitis and Ascosalsum cincinnatulum, Ascosalsum unicaudatum and Ascosalsum viscidulum are transferred to Oceanitis, an earlier generic name. [Copyright &y& Elsevier]

Published
2009
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20. Phylogenetic analysis of the Aspergillus niger aggregate in relation to feruloyl esterase activity

Author

Giraud, Frédéric, Dupont, Joëlle, Haon, Mireille, Bouzid, Ourdia, Alibeu, Olivier, Navarro, David, Sage, Lucile, Seigle-Murandi, Françoise, Asther, Marcel, and Lesage-Meessen, Laurence

Subjects
*ASPERGILLUS niger, *MICROCLUSTERS, *SUGAR beets, *TUBULINS
Abstract

Abstract: Species of the Aspergillus niger aggregate are known to produce feruloyl esterases, enzymes involved in the degradation of cell wall polymers. However, species delineation is difficult in these fungi. We combined AFLP analysis with ITS rDNA and β-tubulin sequencing to characterize the isolates of this aggregate in terms of feruloyl esterase production. A preliminary re-examination of isolates based on comparison of ITS rDNA and β-tubulin sequences with those of typical taxa deposited in international collections led us to re-identify the isolates as members of the species A. niger, A. foetidus and A. tubingensis. Molecular clustering based on β-tubulin data and AFLP analysis showed that the strains of A. niger formed a homogenous phylogenetic group distinguished by either zero or type A feruloyl esterase activity, while strains A. foetidus and A. tubingensis exhibited type B feruloyl esterase activity when grown on sugar beet pulp. [Copyright &y& Elsevier]

Published
2007
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22. Phosphatase PTEN in chicken muscle is regulated during ontogenesis

Author

Vaudin, Pascal, Dupont, Joëlle, Duchêne, Sophie, Audouin, Estelle, Crochet, Sabine, Berri, Cécile, and Tesseraud, Sophie

Subjects
*PHOSPHATASES, *ONTOGENY, *CHICKEN diseases, *PECTORALIS muscle
Abstract

Abstract: The phosphatase and TENsin homolog deleted on chromosome 10 (PTEN) is a lipid and protein phosphatase able to inhibit significant actors of cell signaling (i.e. phosphatidylinositol-3′kinase and mitogen-activated protein kinase pathways). The aim of this study was to characterize PTEN and to investigate its regulation during ontogenesis in chicken muscle. Pectoralis major muscle was sampled on day 18 of the embryonic period (E18), at hatching (d0) and in fed chickens at 2, 7 and 43 days after hatching (d2, d7 and d43). We first cloned the totality of chicken PTEN cDNA; its translation into a putative protein showed more than 95% sequence identity with that characterized in mammals (humans, mice). PTEN was expressed under two major transcripts in the majority of tissues, including muscles where the expression of PTEN mRNA increased with age (P <0.05). Surprisingly, the protein levels of PTEN (protein characterized with an apparent molecular weight of 55kDa) and its activity were considerably decreased between the E18 and d43 stages (approximately 8–10-fold reduction, P <0.001). An association between these decreases and higher phosphorylation levels of two potential indirect downstream targets of phosphatase (i.e. AKT and ERK) was observed only in the early growth phases. It was concluded that phosphatase PTEN was expressed in chicken muscle and that its expression was regulated during ontogenesis. [Copyright &y& Elsevier]

Published
2006
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23. Early steps of insulin receptor signaling in chicken and rat: apparent refractoriness in chicken muscle

Author

Dupont, Joëlle, Dagou, Carine, Derouet, Michel, Simon, Jean, and Taouis, Mohammed

Subjects
*INSULIN, *TYROSINE, *PHOSPHORYLATION, *PROTEINS
Abstract

The early steps of insulin receptor (IR) signaling (tyrosine phosphorylation of IR β-subunit, IRS-1 and Shc and PI 3′-kinase activity) have been characterized in two target tissues in the chicken: liver and muscle. The signaling cascade appeared to depend on nutritional status in the liver, but not in muscle (with a possible exception for a minor tyrosine phosphorylation of the 52 kDa Shc isoform). In this study, we compared the responses of the liver and muscle to exogenous insulin (10 or 1000 mU/kg) in chickens and rats. In the liver, IRS-1 and Shc proteins were present in smaller amounts and the regulatory subunit p85 of PI 3′-kinase was present in larger amounts in chickens than in rats. In the basal state (saline injection), the level of tyrosine phosphorylation of IR was lower, and that of Shc higher, in chickens than in rats. PI 3′-kinase activity in chickens was half that in rats. Insulin activated all components of the cascade in a dose-dependent manner in both species. A different pattern was observed in the muscle. In the basal state, the levels of tyrosine phosphorylation of IR and of PI 3′-kinase activity were much higher in chickens than in rats (by factors of 2 and 30, respectively). Insulin strongly activated all components of the cascade in rats (but with no significant increase in the phosphorylation of Shc). No activation was observed in chickens (with only a slight but significant increase in the tyrosine phosphorylation of Shc). The insulin cascade therefore appears to respond normally in chicken liver but to be refractory in chicken muscle. The large amount of p85 and high levels of PI 3′-kinase activity in muscle may contribute to this situation, making chicken muscle an interesting model of insulin resistance. [Copyright &y& Elsevier]

Published
2004
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24. The Cyclin-dependent Kinase Inhibitor p21[sup CIP/WAF] Is a Positive Regulator of Insulin-like Growth Factor I-induced Cell Proliferation in MCF-7 Human Breast Cancer Cells.

Author

Dupont, Joëlle, Karas, Michael, and LeRoith, Derek

Subjects
*SOMATOMEDIN, *CELL cycle, *BREAST cancer, *BIOCHEMISTRY
Abstract

Studies the role of insulin-like growth factor (IGF)-I receptor signaling on cell cycle events utilizing MCF-7 breast cancer cells. Physiological concentrations of IGF-I; Reduction of the IGF-I effect on the amount of p21 [sup CIP/WAF] protein in MCF-7 cells; MCF-7 cells transiently overexpressing p21.

Published
2003
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26. Vitamin E alleviates glyphosate-based herbicide-induced progesterone secretion inhibition and oxidative stress increase in chicken primary granulosa cells.

Author

Fréville, Mathias, Bernardi, Ophélie, Ramé, Christelle, Froment, Pascal, and Dupont, Joëlle

Subjects
*OXIDANT status, *GRANULOSA cells, *ENDOCRINE disruptors, *CHICKENS, *ENDOCRINE glands, *VITAMIN E
Abstract

Glyphosate-based herbicides (GBH) are the most extensively used herbicides worldwide. Despite a presumed nondangerousness for animals, several studies reported negative effects after a GBH exposure in several animal models including birds, notably on reproductive functions. Several studies concerning the advantages of Vitamin E (VE) for antioxidant activity but also growth and reproduction have been reported in birds. However, it remains unclear whether VE could alleviate the negative effect of GBHs on chicken ovarian cells. Here we exposed chicken primary granulosa cells (GCs) from F1 and F3/4 follicles to growing doses of GBH (0.036, 0.36, 3.6, and 36 gly eq/L), with or without VE supplementation (1 mg/L) and investigated cell viability, proliferation, oxidative stress and steroidogenesis. GBH exposure did not affect F1 and F3 GCs viability but it increased cell proliferation only in F1 GCs and this effect was not altered by VE. In both F1 and F3/4 GCs, GBH exposure increased total oxidant status (TOS), reduced total antioxidant status (TAS) and consequently increased index of oxidative stress (OSI) in dose dependent manner. This latter effect for GBH 36 mg eq gly/L was totally abolished in response to VE. In both F1 and F3/4 GCs, GBH exposure reduced progesterone secretion in a dose dependent manner and this effect with GBH 0.36 and 1.8 mg eq glyphosate/L was alleviated by VE. However, we did not observe any effect of GBH and VE on the gene expression of several components of the steroidogenesis process. Taken together, these results show that GBH may have endocrine disruptor effects, and that these effects might be alleviated by antioxidant VE supplementation. [ABSTRACT FROM AUTHOR]

Published
2024
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27. Molecular mechanisms involved in LH release by the ovine pituitary cells

Author

Yang, Dominique, Caraty, Alain, and Dupont, Joëlle

Subjects
*LUTEINIZING hormone, *LUTEINIZING hormone releasing hormone, *GLYCOPROTEIN hormones, *GONADOTROPIN
Abstract

Abstract: The luteinizing hormone-releasing hormone (LHRH) is a hypothalamic decapeptide and main positive regulator of luteinizing hormone (LH) secretion from pituitary cells. Insulin-like growth factor-I (IGF-1) also stimulates LH release and enhances the effect of LHRH. However, the molecular mechanisms involved in the interactions between LHRH and IGF-1 are unclear. Here, we first determined the effect of various types of LHRH [I (mammalian), II (chicken), III (lamprey), hyp9 and salmon] on both LH secretion and activation of MAPK (ERK1/2 and p38) in ovine pituitary cells. After 3h of treatment, LH secretion was significantly higher for LHRH-I than for the other LHRH tested. Interestingly, LHRH-III had no effect at any concentration used on the LH release by ovine pituitary cells. The phosphorylation of both MAPK ERK1/2 and p38 was also significantly higher after treatment with LHRH-I than LHRH-II, salmon LHRH or hyp9. These MAPKs were not activated or only very weakly activated by LHRH-III. We then used pharmacological inhibitors to show that MAPK ERK1/2 and PKCδ participate in the LH release by ovine pituitary cells in response to LHRH-I. We identified the main substrates and signaling pathways [PI3K/Akt and MAPK (ERK1/2, p38 and JNK1/2] of IGF-1R and investigated the effect of IGF-1 on the stimulation of ovine pituitary cell LH secretion by the various LHRH. IGF-1 increases LH secretion in response to LHRH-I, LHRH-II, hyp9 and salmon LHRH but not the secretion after treatment with LHRH-III. Using specific inhibitors, we found that the MAPK ERK1/2 but not the PI3K/Akt signaling pathway is involved in the LH secretion in response to IGF-1. This is the first description of a common molecular mechanism, involving the MAPK ERK1/2, by which LHRH-R and IGF-1-R induce LH secretion in ovine pituitary cells. [Copyright &y& Elsevier]

Published
2005
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28. Evaluation of acute toxicity of Scabiosa artropurperea var.maritima aqueous extracts in Swiss mice.

Author

Niama, Wijden, Ben Said, Samia, Rame, Christelle, Aroua, Mohamed, Mahouachi, Mokhtar, Froment, Pascal, and Dupont, Joëlle

Subjects
*LABORATORY mice, *TOXICITY testing, *ORAL drug administration, *SEMINAL vesicles, *SPERM motility, *INGESTION, *PHYTOCHEMICALS, *FOOD consumption
Abstract

Scabiosa artropurperea var.maritima is a plant widely distributed in the Mediterranean region and used as a traditional medicine. The present study evaluated the biochemical composition and the potential toxicity of aqueous extract of whole Scabiosa artropurperea var.maritima through acute toxicity oral administration in male mice. Phytochemical analysis of the Scabiosa artropurperea var.maritima revealed high levels of reductor sugars and significant flavonoid and total phenol content. The aqueous extract of Scabiosa artropurperea var.maritima was daily oral administered to mice at doses of 300 (group 1), 2000 (group 2) and 4000 (group 3) mg/kg body weight per day for 14 days. We observed no significant difference in the consumption of food, body weight and relative organ weights except for an increase in the seminal vesicles weight in group 3. Hematological parameters revealed the non-adverse effects of prolonged oral consumption of Scabiosa artropurperea var.maritima except for a slight increase but significant of percentage of hematocrit in group 1 and 3 and a decrease in percentage of granulocytes in group 2. The histopathologic examination did not show any differences in vital organs. We also observed non-adverse effects on the reproductive parameters including testosterone concentration, spermatozoa motility and morphologies. Based on our findings, the aqueous extract of Scabiosa artropurperea var.maritima could be considered safe for oral medication in animals. [Display omitted] • Scabiosa artropurperea var.maritima (SAVM) contain reducter sugars and flavanoids. • Oral administration of SAVM has no effect on food intake and body weight in male mice. • SAVM has no effects on haematological parameters except for hematocrit and granulocytes. • SAVM exerts no negative effects on reproductive parameters. • Aqueous extract of SAVM could be considered safe for oral medication in animals. [ABSTRACT FROM AUTHOR]

Published
2024
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29. Chemerin concentration in egg white in layer and broiler hens during the laying period for 2 successive generations.

Author

Bernardi, Ophélie, Fréville, Mathias, Ramé, Christelle, Reverchon, Maxime, and Dupont, Joëlle

Subjects
*HENS, *CHEMERIN, *EGG whites, *EGGS, *EGG yolk, *EGG quality, *OVIDUCT
Abstract

The genetic selection progress in layers and broilers makes poultry production one of the fastest growing industries. Objectives of the breeding companies are the stability or the increase in the laying rate and the production of viable chicks. New biomarkers are necessary to improve reproductive and egg performances. Chemerin (Chem) produced by oviduct accumulates in egg white (EW). Here, we hypothesized that EW Chem concentration was dependent on the stage of laying and on the breed (layer vs. broiler). In addition, they could be associated to laying performance and fertility parameters. In breeding companies, we collected during 2 successive generations (G0 (mother) and G1 (daughter)) eggs from 100 layers and 100 broilers hens during 5 d at 3 stages: before, after laying peak and at the end of laying period. For each egg, the EW was sampled to measure Chem concentration by ELISA assay. In each generation at the end of laying period, magnums from oviduct, where the EG is formed, were collected in layers and broilers in order to investigate Chem differential expression by RT-qPCR between both breeds. Chem concentration in EW was dependent on the time of laying period and its profile was differently regulated in layers and broilers. Indeed, it increased at the end of laying in layers whereas it decreased after the laying peak in broilers. At the end of laying period, Chem concentration in EW was almost 2-fold higher in layers than in broilers and this was confirmed in both G0 and G1 generations at the Chem mRNA and protein levels in the magnum. For the 2 successive generations, Chem concentration in EW was negatively correlated with the laying rate and the fertility parameter in broiler hens whereas it was negatively correlated with the egg quality (weight of whole egg and weight of albumen) and positively with the fertility rate at some time of laying in layer hens. Taken together, the Chem concentration in EW could be a potential predictive tool for reproductive parameters in genetic selection. [ABSTRACT FROM AUTHOR]

Published
2024
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30. Expression of chemerin and its receptors in extra-embryonic annexes and role of chemerin and its GPR1 receptor in embryo development in layer and broiler hens.

Author

Bernardi, Ophélie, Ramé, Christelle, Reverchon, Maxime, and Dupont, Joëlle

Subjects
*CHICKEN embryos, *AMNIOTIC liquid, *CHEMERIN, *AMNION, *EMBRYOS, *HENS, *BLOOD plasma
Abstract

Intensive genetic selection of broiler breeders and layer hens resulted in differences in the mechanisms of growth and also in cell metabolism during embryogenesis. Previous research has shown that an adipokine named chemerin and one of these receptors, CMKLR1 were potentially involved in broiler embryo development. Here, our objectives were 1) to compare the expression of chemerin and its receptors CMKLR1, GPR1, and CCRL2 and chemerin concentration in extra-embryonic annexes (allantoic and amniotic membranes and fluids and plasma) in broiler and layer fertile eggs during the development (embryonic day (ED) 7, 14, and 18) by RT-qPCR and specific chicken ELISA and 2) to investigate the role of chemerin and one of its receptors GPR1 in embryo development after in ovo injections of neutralizing antibodies against chicken chemerin and GPR1. We found that chemerin expression in amniotic membranes was higher in layer than broiler eggs at ED7 and ED14 whereas the expression of the 3 receptors was higher in layer than broiler in the allantoic membranes at ED14 and ED18. Chemerin concentration was more important in layer than broiler at ED14 and ED18 in amniotic liquid and at all the studied stages in blood plasma. We also showed positive correlation between amniotic chemerin concentration and chemerin amniotic membrane expression, chemerin plasma concentration and embryo body weight in both breeds. Finally, in ovo injection of chicken chemerin and GPR1 neutralizing antibodies increased embryo mortality in both layer and broiler eggs. Taken together, even if chemerin concentration and chemerin system expression in embryonic membranes are mainly higher expressed in layer than in broiler, chemerin potentially through GPR1 could promote embryo development in both breeds. [ABSTRACT FROM AUTHOR]

Published
2024
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31. Adipokines expression in reproductive tract, egg white and embryonic annexes in hen.

Author

Bernardi, Ophélie, Bourdon, Guillaume, Estienne, Anthony, Brossaud, Adeline, Ramé, Christelle, Reverchon, Maxime, and Dupont, Joëlle

Subjects
*GENITALIA, *ADIPOKINES, *EGG whites, *AMNIOTIC liquid, *CHICKEN embryos, *WHITE adipose tissue, *FALLOPIAN tubes, *CHEMERIN, *FEMALE reproductive organs
Abstract

In mammals, molecules mainly secreted by white adipose tissue named adipokines are also synthetized locally in the reproductive tract and are able to influence reproductive functions. In avian species, previous studies indicated that the adipokine chemerin is highly abundant in the albumen, compared to the yolk and this was associated to high chemerin expression in the magnum. In addition, the authors observed that chemerin and its receptors are expressed by allantoic and amniotic membranes and chemerin is present in fluids during the embryo development. Here, we studied other adipokines, including adiponectin, visfatin, apelin, and adipolin in egg white and their known receptors in the active (egg-laying hen) and regressed (hen not laying) oviduct and embryonic annexes during embryo development. By using Western blot, RT-qPCR analysis and immunohistochemistry, we demonstrated the expression of different adipokines in the egg albumen (visfatin) and the reproductive tract (adiponectin, visfatin, apelin, adipolin, and their cognate receptors) according the position of egg in the oviduct. We showed that the expression of adipokines and adipokines receptors was strongly reduced in the regressed oviducts (arrested laying hen). Results indicated that visfatin and adiponectin appeared at ED11 to 14 and increased until ED18 in amniotic fluid whereas it was found from ED7 and was unchanged during embryo development in allantoic fluid. Taken together, adipokines and their receptors are expressed in the egg white, the reproductive tract and the embryonic annexes. Data obtained suggest important functions of theses metabolic hormones during the chicken embryo development. Thus, adipokines could be potential biomarkers to improve the embryo development. [ABSTRACT FROM AUTHOR]

Published
2023
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32. Chronic dietary exposure to a glyphosate-based herbicide in broiler hens has long-term impacts on the progeny metabolism.

Author

Estienne, Anthony, Fréville, Mathias, Bernardi, Ophélie, Ramé, Christelle, Calandreau, Ludovic, Cornilleau, Fabien, Ganier, Patrice, Chahnamian, Marine, Froment, Pascal, and Dupont, Joëlle

Subjects
*GLYPHOSATE, *HERBICIDES, *ABDOMINAL adipose tissue, *MONOUNSATURATED fatty acids, *UNSATURATED fatty acids, *HENS, *CHICKS
Abstract

Glyphosate-based herbicides (GBH) are the most commonly used herbicides in agriculture. Several studies reported possible adverse effects on human and animal models after a GBH exposure. However, the effects of a temporary maternal exposure on the progeny have been poorly documented, especially in avian models. We investigated the effects of a hen chronic dietary exposure to a GBH on the progeny, obtained during the period following the withdrawal of GBH from the diet. Hens were exposed to a GBH via their food for 6 wk, after which the GBH was removed from their food. Eggs from these hens were collected 3 wk after the GBH was withdrawn for 1 wk. We monitored the growth performances, metabolic parameters, and behavior from the progeny of the hens (Ex-GBH chicks, n = 186) and compared them with those of unexposed control-hen progeny (CT chicks, n = 213). Ex-GBH chicks were more likely to explore their new environment than CT chicks during the open-field test. In addition, they had an increased fattening and blood triglycerides level, whereas their food consumption was similar to CT chicks. Quantitative PCR on the chemerin system and FASN in chicks livers indicate a transcriptional activity in favor of fatty acid synthesis, and lipidomic analysis on chicks abdominal adipose tissue reveal a global increase in monounsaturated fatty acid and a global decrease in polyunsaturated fatty acids. Seven genes involved in the synthesis of fatty acids were identified with the open access LIPIDMAP software, and their disturbance in Ex-GBH chicks was confirmed via qPCR. Taken together, these results suggest that the progeny of hens temporarily exposed to a GBH are more likely to fatten, even with a balanced diet. The removal of GBH from their contaminated environment would therefore not be sufficient to completely restore their health, has it could induce transgenerational effects. [ABSTRACT FROM AUTHOR]

Published
2023
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33. The role of type I interferons (IFNs) in the regulation of chicken macrophage inflammatory response to bacterial challenge.

Author

Garrido, Damien, Alber, Andreas, Kut, Emmanuel, Chanteloup, Nathalie K., Lion, Adrien, Trotereau, Angélina, Dupont, Joëlle, Tedin, Karsten, Kaspers, Bernd, Vervelde, Lonneke, Trapp, Sascha, Schouler, Catherine, and Guabiraba, Rodrigo

Subjects
*INTERFERONS, *MACROPHAGES, *CHICKEN diseases, *PHAGOCYTES, *INFLAMMATION
Abstract

Mammalian type I interferons (IFNα/β) are known to modulate inflammatory processes in addition to their antiviral properties. Indeed, virus-induced type I interferons regulate the mammalian phagocyte immune response to bacteria during superinfections. However, it remains unresolved whether type I IFNs similarly impact the chicken macrophage immune response. We first evidenced that IFNα and IFNβ act differently in terms of gene expression stimulation and activation of intracellular signaling pathways in chicken macrophages. Next, we showed that priming of chicken macrophages with IFNα increased bacteria uptake, boosted bacterial-induced ROS/NO production and led to an increased transcriptional expression or production of NOS2 /NO, IL1B /IL-1β and notably IFNB /IFNβ. Neutralization of IFNβ during bacterial challenge limited IFNα-induced augmentation of the pro-inflammatory response. In conclusion, we demonstrated that type I IFNs differently regulate chicken macrophage functions and drive a pro-inflammatory response to bacterial challenge. These findings shed light on the diverse functions of type I IFNs in chicken macrophages. [ABSTRACT FROM AUTHOR]

Published
2018
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34. Screening of wheat endophytes as biological control agents against Fusarium head blight using two different in vitro tests.

Author

Comby, Morgane, Gacoin, Marie, Robineau, Mathilde, Rabenoelina, Fanja, Ptas, Sébastien, Dupont, Joëlle, Profizi, Camille, and Baillieul, Fabienne

Subjects
*WHEAT, *ENDOPHYTES, *PHYSIOLOGICAL control systems, *FUSARIUM, *TISSUES
Abstract

In order to find biological control agents (BCAs) for the management of Fusarium head blight (FHB), a major disease on wheat crops worldwide, 86 microorganisms isolated from inner tissues of wheat plants were discriminated for their ability to inhibit the growth of Fusarium graminearum and Fusarium culmorum by in vitro dual culture assays. A group of 22 strains appeared very effective to inhibit F. graminearum (inhibition of 30–51%) and they were also globally effective in controlling F. culmorum (inhibition of 15–53%). Further evaluation of a subselection of strains by screening on detached spikelets in vitro confirmed three species, namely Phoma glomerata , Aureobasidium proteae and Sarocladium kiliense , that have not yet been reported for their efficacy against Fusarium spp., indicating that looking for BCAs toward FHB among wheat endophytes proved to be promising. The efficacy of some strains turned out different between both in vitro screening approaches, raising the importance of finding the most appropriate screening approach for the search of BCAs. This study pointed out the interest of the test on detached wheat spikelets that provided information about a potential pathogenicity, the growth capacity and efficacy of the endophyte strains on the targeted plant, before testing them on whole plants. [ABSTRACT FROM AUTHOR]

Published
2017
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35. Effect of a long-chain n-3 polyunsaturated fatty acid-enriched diet on adipose tissue lipid profiles and gene expression in Holstein dairy cows.

Author

Elis, Sebastien, Desmarchais, Alice, Freret, Sandrine, Maillard, Virginie, Labas, Valérie, Cognié, Juliette, Briant, Eric, Hivelin, Celine, Dupont, Joëlle, and Uzbekova, Svetlana

Subjects
*UNSATURATED fatty acids, *FISH oils, *ADIPOSE tissues, *LIPIDS, *GENE expression, *COWS, *ANIMAL health
Abstract

The objective of this study was to determine whether fish oil supplement has an effect on adipose tissue lipid profiles and gene expression in postpartum dairy cows. Holstein cows were supplemented with either long-chain n-3 polyunsaturated fatty acid (PUFA; protected fish oil) or control PUFA (n-6; toasted soybeans) for 2 mo after calving (n = 23 per diet). These cows showed no difference in milk production or metabolic parameters, but exhibited a tendency toward a decrease in early embryo mortality rate after artificial insemination. We hypothesized that, in addition to this effect, modifications in adipose tissue (AT) gene expression and lipid profiles would occur in response to diet. Subcutaneous AT samples were thus collected from the dewlaps of n-3 and n-6 dairy cows at 1 mo antepartum, and 1 wk, 2 mo, and 5 mo postpartum for the analysis of lipids and gene expression. Lipid profiles were obtained by matrix-assisted laser desorption/ionization time-offlight mass spectrometry in both positive and negative modes. We found 37 lipid species in the 200 to 1,200 m/z range, which differed between the n-3 and control groups, suggesting that the n-3 supplement affected the lipid composition through the enrichment of lipids integrating long-chain PUFA from fish oil sources: eicosapentaenoic and docosahexaenoic acid. Moreover, a decrease in triacylglycerolipids was observed in AT of n-3 supplemented cows. The expression of 44 genes involved in fatty acid metabolism and the adipokine system was assessed by real-time reverse-transcription PCR. Hierarchical clustering, according to either postpartum stage or diet, enabled us to group genes exhibiting similar kinetic properties during lactation or by those that varied in similar ways after n-3 supplementation, respectively. Among the genes exhibiting a dietary effect, FABP4, LIPE, CD36, and PLIN1 were overexpressed in n-3 AT samples compared with the control, suggesting an increase in lipolysis due to n-3 supplementation, which was reflected on lipolytic activity at the protein level (i.e., protein expression of fatty acid binding protein 4, phosphorylated perilipin 1, and phosphorylated hormone-sensitive lipase). This increase in lipolysis is relevant to the decrease in triglycerides observed in these samples. Gene expression analyses between n-3 and control AT samples also suggested that the n-3 diet could modulate the secretory functions of AT, possibly by affecting adipokine expression; however, this has to be confirmed at the protein level. [ABSTRACT FROM AUTHOR]

Published
2016
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36. The influence of selection in wild pheasant (Phasianus colchicus) breeding on reproduction and the involvement of the chemerin system.

Author

Estienne, Anthony, Bernardi, Ophélie, Ramé, Christelle, Reverchon, Maxime, Tricoire, Serge, Froment, Pascal, and Dupont, Joëlle

Subjects
*CHEMERIN, *EGGS, *GENITALIA, *PHEASANTS, *AMNION, *ALBUMINS
Abstract

Chemerin is a hormone produced mainly by adipose tissue and liver. We have recently shown that it is locally produced in the reproductive tract in hens, particularly at the magnum level, leading to its accumulation in the egg albumen. We have also determined that chemerin is necessary for egg fertilization, embryo development, and angiogenesis within the chorio-allantoic membrane in chicken species. We, therefore, hypothesize that chemerin, widely present in various gallinacean species, could be a marker of egg fertility in this animal order. To demonstrate this, we used a model close to the hen: the pheasant. By RT-qPCR, we have shown that chemerin and its three receptors CMKLR1, GPR1, and CCRL2 are expressed in the reproductive tract of females. In addition, chemerin is also produced predominantly in the magnum and accumulates in the egg albumen as determined by immunoblot. We then compared two lines of pheasants with different reproductive characteristics: the F11 and F22 breeds. F22 lays more eggs than F11, but have significantly lower fertility and hatchability rates. In addition, F22 exhibit a significantly lower amount of chemerin protein in their magnum (P < 0.01) and in the egg albumen (P < 0.0001) compared to F11. Finally, we observed a positive correlation between the chemerin amount in the albumen of F11 eggs and the hatching rate of the eggs (r = 0.5; P = 0.04) as well as a negative correlation between the chemerin quantity in the albumen of F22 eggs and the rate of unfertilized eggs (r = −0.37; P = 0.04). Finally, chemerin system (ligand and receptors) is also expressed within embryo annexes (chorioallantoic and amniotic membranes) during incubation. These data demonstrate an interspecies conservation of chemerin production in the magnum, its accumulation in the egg albumen and its possible use as a marker for determining the quality of eggs in term of fertility and embryo development. [ABSTRACT FROM AUTHOR]

Published
2023
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37. Specific deletion of AMP-activated protein kinase (α1AMPK) in mouse Sertoli cells modifies germ cell quality.

Author

Bertoldo, Michael J., Guibert, Edith, Faure, Melanie, Guillou, Florian, Ramé, Christelle, Nadal-Desbarats, Lydie, Foretz, Marc, Viollet, Benoit, Dupont, Joëlle, and Froment, Pascal

Subjects
*ADENOSINE monophosphate, *LABORATORY mice, *SERTOLI cells, *GERM cells, *BIOMARKERS
Abstract

The AMP-activated protein kinase (AMPK) is an important regulator of cellular energy homeostasis which plays a role in fertility. Complete disruption of the AMPK catalytic subunit α1 gene (α1AMPK KO) in male mice results in a decrease in litter size which is associated with the production of altered sperm morphology and motility. Because of the importance of Sertoli cells in the formation of germ cells, we have chosen to selectively disrupt α1AMPK only in the Sertoli cells in mice (Sc-α1AMPK-KO mice). Specific deletion of the α1AMPK gene in Sertoli cells resulted in a 25% reduction in male fertility associated with abnormal spermatozoa with a thin head. No clear alterations in testis morphology or modification in the number of Sertoli cells in vivo were observed, but a dysregulation in energy metabolism in Sertoli cells occurred. We have reported an increase in lactate production, in lipid droplets, and a reduction in ATP production in Sc-α1AMPK-KO Sertoli cells. These perturbations were associated with lower expression of mitochondrial markers (cytochrome c and PGC1 -α ). In addition another metabolic sensor, the deacetylase SIRT1, had a reduction in expression which is correlated with a decline in deacetylase activity. Finally, expression and localization of junctions forming the blood-testis barrier between Sertoli cells themselves and with germ cells were deregulated in Sc-α1AMPK-KO. In conclusion, these results suggest that dysregulation of the energy sensing machinery exclusively through disruption of α1AMPK in Sertoli cells translates to a reduction in the quality of germ cells and fertility. [ABSTRACT FROM AUTHOR]

Published
2016
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38. A hemocyanin-derived antimicrobial peptide from the penaeid shrimp adopts an alpha-helical structure that specifically permeabilizes fungal membranes.

Author

Petit, Vanessa W., Rolland, Jean-Luc, Blond, Alain, Cazevieille, Chantal, Djediat, Chakib, Peduzzi, Jean, Goulard, Christophe, Bachère, Evelyne, Dupont, Joëlle, Destoumieux-Garzón, Delphine, and Rebuffat, Sylvie

Subjects
*HEMOCYANIN, *ANTIMICROBIAL peptides, *PENAEIDAE, *SHRIMPS, *HELICAL structure, *PERMEABILITY, *FUNGAL membranes
Abstract

Background Hemocyanins are respiratory proteins with multiple functions. In diverse crustaceans hemocyanins can release histidine-rich antimicrobial peptides in response to microbial challenge. In penaeid shrimp, strictly antifungal peptides are released from the C-terminus of hemocyanins. Methods The three-dimensional structure of the antifungal peptide PvHCt from Litopenaeus vannamei was determined by NMR. Its mechanism of action against the shrimp pathogen Fusarium oxysporum was investigated using immunochemistry, fluorescence and transmission electron microscopy. Results PvHCt folded into an amphipathic α-helix in membrane-mimicking media and displayed a random conformation in aqueous environment. In contact with F. oxysporum , PvHCt bound massively to the surface of fungal hyphae without being imported into the cytoplasm. At minimal inhibitory concentrations, PvHCt made the fungal membrane permeable to SYTOX-green and fluorescent dextran beads of 4 kDa. Higher size beads could not enter the cytoplasm. Therefore, PvHCt likely creates local damages to the fungal membrane. While the fungal cell wall appeared preserved, gradual degeneration of the cytoplasm most often resulting in cell lysis was observed in fungal spores and hyphae. In the remaining fungal cells, PvHCt induced a protective response by the formation of daughter hyphae. Conclusion The massive accumulation of PvHCt at the surface of fungal hyphae and subsequent insertion into the plasma membrane disrupt its integrity as a permeability barrier, leading to disruption of internal homeostasis and fungal death. General significance The histidine-rich antimicrobial peptide PvHCt derived from shrimp hemocyanin is a strictly antifungal peptide, which adopts an amphipathic α-helical structure, and selectively binds to and permeabilizes fungal cells. [ABSTRACT FROM AUTHOR]

Published
2016
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39. Cell proliferation and progesterone synthesis depend on lipid metabolism in bovine granulosa cells.

Author

Elis, Sebastien, Desmarchais, Alice, Maillard, Virginie, Uzbekova, Svetlana, Monget, Philippe, and Dupont, Joëlle

Subjects
*PROGESTERONE, *GRANULOSA cells, *CELL proliferation, *LIPID metabolism, *ESTRADIOL, *CARNITINE palmitoyltransferase, *FATTY acid synthases
Abstract

In dairy cows, lipids are essential to support energy supplies for all biological functions, especially during early lactation. Lipid metabolism is crucial for sustaining proper reproductive function. Alteration of lipid metabolism impacts follicular development and affects oocyte developmental competence. Indeed, nonesterified fatty acids are able to decrease granulosa cell (GC) proliferation and affect estradiol synthesis, thus potentially affecting follicular growth and viability. The objective of this study was to assess the impact of lipid metabolism on bovine GCs, through the use of the lipid metabolism inhibitors etomoxir, an inhibitor of fatty acid (FA) oxidation through inhibition of carnitine palmitoyl transferase 1 (CPT1), and C75, an inhibitor of FA synthesis through inhibition of fatty acid synthase. We showed that etomoxir and C75 significantly inhibited DNA synthesis in vitro ; C75 also significantly decreased progesterone synthesis. Both inhibitors significantly reduced AMPK (5′ adenosine monophosphate–activated protein kinase) and acetyl-CoA carboxylase phosphorylation. Etomoxir also affected the AKT (protein kinase B) signaling pathway. Combined, these data suggest that both FA oxidation and synthesis are important for the bovine GCs to express a proliferative and steroidogenic phenotype and, thus, for sustaining follicular growth. Despite these findings, it is important to note that the changes caused by the inhibitors of FA metabolism on GCs in vitro are globally mild, suggesting that lipid metabolism is not as critical in GCs as was observed in the oocyte–cumulus complex. Further studies are needed to investigate the detailed mechanisms by which lipid metabolism interacts with GC functions. [ABSTRACT FROM AUTHOR]

Published
2015
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40. Expression of adipokine and lipid metabolism genes in adipose tissue of dairy cows differing in a female fertility quantitative trait locus.

Author

Elis, Sebastien, Coyral-Castel, Stephanie, Freret, Sandrine, Cognié, Juliette, Desmarchais, Alice, Fatet, Alice, Rame, Christelle, Briant, Eric, Maillard, Virginie, and Dupont, Joëlle

Subjects
*ADIPOKINES, *LIPID metabolism, *DAIRY cattle genetics, *CATTLE fertility, *ADIPONECTIN, *DAIRY cattle reproduction
Abstract

We have previously characterized 2 haplotypes (Fertil+ and Fertil-) of Holstein dairy cows differing in 1 female fertility quantitative trait locus (QTL) located on chromosome 3 (QTL-Fert-F-BTA3) between positions 9.8 and 13.5 cM. This QTL is composed of 124 genes, some of them being involved in metabolism or reproduction. Primiparous Fertil+ and Fertil- cows exhibited 69 and 39% pregnancy rate at first service, respectively. A difference in plasma nonesterified fatty acid concentrations observed between both haplotypes might indicate a difference in adipose tissue mobilization. We compared adipose tissue gene expression in Fertil+ and Fertil- cows during their second lactation, at 2 physiological stages, implying either intense lipid mobilization (1 wk postpartum) or fat storage (5 mo of gestation). We investigated by reverse-transcription quantitative PCR the mRNA gene expression of 5 positional candidate genes located in the QTL-Fert-FBTA3, as well as 18 other functional candidate genes encoding proteins involved in lipid metabolism and several adipokines. Among them, genes involved in either lipolysis or lipogenesis were chosen as controls because they were previously described in dairy cow adipose tissue. A hierarchical clustering was performed to group genes according to their expression pattern, allowing 2 clusters to be determined. Cluster 1 was composed of genes that were overexpressed during mobilization (ADIPOQ, ADIPOR2, LIPE, FABP4, PLIN1, RARRES, LEPR, and CPT1A) and cluster 2 of genes overexpressed during reconstitution of body reserves (ACACA, FASN, and SCD). Genes belonging to cluster 1 (LIPE, FABP4, PLIN1, and CPT1A) are known to be involved in lipolysis and fatty acid oxidation, and genes belonging to cluster 2 (ACACA, FASN, and SCD) are known to be involved in fatty acid synthesis. The expression of 5 genes from cluster 1 was correlated to plasma nonesterified fatty acid levels and thus to mobilization of body reserves in dairy cows (ADIPOQ, ADIPOR2, LIPE, PLIN1, and FABP4). During the mobilization stage, none of the positional candidate genes belonging to QTL-Fert-F-BTA3 (ADAR, MTX1, SHC1, SPTA1, and PAQR6) showed a difference in expression between the 2 haplotypes. Interestingly, ADIPOQ and ADIPOR2 were the only genes showing a significant mRNA overexpression in Fertil- cows at the mobilization stage. Further studies focusing on plasma adiponectin level and adipokine actions on the ovary are needed to investigate its potential role in dairy cow fertility. [ABSTRACT FROM AUTHOR]

Published
2013
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41. Resistin decreases insulin-like growth factor l-induced steroid production and insulin-like growth factor I receptor signaling in human granulosa cells.

Author

Reverchon, Maxime, Cornuau, Marion, Ramé, Christelle, Guerif, Fabrice, Royère, Dominique, and Dupont, Joëlle

Subjects
*OVARIAN follicle, *GRANULOSA cells, *RESISTIN, *PROGESTERONE, *ESTRADIOL, *REVERSE transcriptase polymerase chain reaction, *IMMUNOBLOTTING, *IMMUNOHISTOCHEMISTRY, *RADIOIMMUNOASSAY, *CELL proliferation, *STEROIDOGENIC acute regulatory protein
Abstract

Objective: To identify resistin in human ovarian follicles and investigate the effect and the molecular mechanisms associated with resistin on steroidogenesis in human granulosa cells (GCs). Design: The effects of recombinant human resistin on the secretion of progesterone (P) and estradiol (E2) by cultured human GCs were investigated. Setting: Academic institutions Patient(s): Twenty infertile and healthy women undergoing IVF. Intervention(s): Primary human GC cultures stimulated with recombinant human resistin (10 ng/mL). Main Outcome Measure(s): Determination of messenger RNA (mRNA) and protein expression of resistin in fresh human GCs by reverse transcriptase-polymerase chain reaction (RT-PCR), immunoblot and immunohistochemistry, respectively; measurement of P and E2 levels in the conditioned media by radioimmunoassay; determination of cell proliferation by tritiated thymidine incorporation; and analysis of signaling pathways activation by immunoblot analysis. Result(s): Human GCs and theca cells express resistin. In primary human GCs, resistin decreases P and E2 secretion in response to insulin-like growth factor I (IGF-I). This was associated with a reduction in the P450 aromatase and P450scc (cholesterol side-chain cleavage cytochromes P450) (P450scc) protein levels but not those of 3/3-hydroxysteroid dehydrogenase (3/3-HSD) or steroidogenic acute regulatory protein (StAR) and with a decrease in IGF-I-induced IGF-I receptor and mitogen-activated protein kinase (MAPK.) extracellular signal-regulated kinase 1/2 (ERK1/2) phosphorylation. Resistin treatment does not affect IGF-I-induced cell proliferation and basal steroidogenesis (there is no IGF-I or follicle-stimulating hormone stimulation). In the basal state, resistin rapidly stimulates Akt and MAPK ERK1/2 and p38 phosphorylation in primary human GCs Conclusion(s): Resistin is present in human GCs and theca cells. It decreases P and E2 secretion, P450scc and P4S0 aromatase protein levels, and IGF-IR signaling in response to IGF-I in primary human GCs. [ABSTRACT FROM AUTHOR]

Published
2013
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42. Geographic locality greatly influences fungal endophyte communities in Cephalotaxus harringtonia

Author

Langenfeld, Aude, Prado, Soizic, Nay, Bastien, Cruaud, Corine, Lacoste, Sandrine, Bury, Edith, Hachette, François, Hosoya, Tsuyoshi, and Dupont, Joëlle

Subjects
*ENDOPHYTIC fungi, *CEPHALOTAXACEAE, *BIODIVERSITY, *PHYTOPATHOGENIC fungi in host plants, *RIBOSOMAL DNA, *NIGROSPORA, *SEQUENCE alignment
Abstract

Abstract: Although endophytes of conifers have been extensively studied, few data are available on Cephalotaxaceae. We examined foliar and stem endophytes of Cephalotaxus harringtonia, within its natural range in Japan and outside its natural range in France to study the effect of geography on endophyte community composition. In Japan, rapidly growing endophytes were dominant and may have masked the real diversity, in comparison to France where most endophytes were growing slowly. Analyses of ITS rDNA revealed 104 different Blast Groups among 554 isolates. Almost no overlap between endophyte assemblages of C. harringtonia from the two countries was observed. It seems that Japanese C. harringtonia trees, which should be well adapted to their native site, would host a specific, endemic endophyte community, while trees that have been introduced recently to a foreign site, in France, should have captured existing cosmopolitan and more generalist taxa. In Japan the majority of xylariaceous taxa, which dominated the communities, were unknown and, although closely related to Asian taxa, may be new to science. Dothideomycetes were more prevalent in France. Locally, urban environment, particularly in Japan, may have introduced some perturbations in the native endophyte community of C. harringtonia, with an abundance of generalist fungi such as Nigrospora and Colletotrichum. [Copyright &y& Elsevier]

Published
2013
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43. A taxonomic and ecological overview of cheese fungi

Author

Ropars, Jeanne, Cruaud, Corinne, Lacoste, Sandrine, and Dupont, Joëlle

Subjects
*CHEESE microbiology, *PENICILLIUM camemberti, *PENICILLIUM roqueforti, *ASCOMYCETES, *RIBOSOMAL DNA, *HYPOCREALES, *PROTEINS, *FUNGAL ecology
Abstract

Abstract: Cheese is made from milk by a succession of microbes (bacteria, yeasts and fungi) that determine the consistency and flavor of the cheese. Apart from the emblematic species, Penicillium camemberti and Penicillium roqueforti, cheese fungi are not well known. Here we present a taxonomic and phylogenetic overview of the most important filamentous cheese Ascomycota based on 133 isolates provided by the producers of cheese and cheese starter cultures and 97 isolates from culture collections. We checked the congruence of different gene genealogies to circumscribe cheese species and our results allow us to propose molecular targets for their identification. To study their phylogenetic affiliation, we used LSU rDNA and showed that cheese fungi are found in two classes, the Eurotiomycetes with Penicillium species (Eurotiales) and Sporendonema casei/Sphaerosporium equinum (Onygenales), and the Sordariomycetes with Scopulariopsis species (Microascales) and Fusarium domesticum (Hypocreales). Some of these fungi, such as, P. camemberti, F. domesticum, Scopulariopsis flava and S. casei, are only known from cheeses and are probably adapted to this particular habitat, which is extremely rich in protein and fat. Other cheese fungi are ubiquitous, such as, P. roqueforti, Scopulariopsis candida and Scopulariopsis fusca. [Copyright &y& Elsevier]

Published
2012
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44. Effect of PUFA on embryo cryoresistance, gene expression and AMPKα phosphorylation in IVF-derived bovine embryos

Author

Al Darwich, Abdulrahman, Perreau, Christine, Petit, Marie Hélène, Papillier, Pascal, Dupont, Joëlle, Guillaume, Daniel, Mermillod, Pascal, and Guignot, Florence

Subjects
*UNSATURATED fatty acids, *GENE expression, *ADENOSINE monophosphate, *PHOSPHORYLATION, *EMBRYOS, *CONTROL groups
Abstract

Abstract: The objectives of the present study were to evaluate the effect of conjugated linoleic acid (CLA t10, c12, C18:2), linolenic acid (C18:3) and docosahexaenoic acid (DHA, C22:6) supplementation on in vitro bovine embryo development, embryo survival after cryopreservation, gene expression and AMPKα phosphorylation. Control groups with modified synthetic oviduct fluid (mSOF)±100μM β-mercaptoethanol (β-ME) were performed. The effects of co-culture with bovine oviduct epithelial cell (Boec) monolayers, serum supplementation and embryo development in the ewe oviduct, on gene expression were also examined. Experiments 1 and 2: a lower d 7 embryo survival was found with 100μM C22:6 and 100μM C18:2 supplementation compared to 1μM C22:6 and 100μM β-ME supplementation (P <0.05). C18:3 supplementation had no effect on d 7 embryo survival, but 100μM C18:3 increased d 8 embryo survival compared to 100μM β-ME supplementation (P <0.05). Experiments 3 and 4: stearoyl-CoA desaturase 1 (SCD1) and sterol regulatory element-binding transcription factor 1 (SREBP1) mRNA decreased after 10μM C22:6 supplementation compared to all other supplementations (P <0.05). A lower fatty acid desaturase 2 (FADS2) transcript level was found with 100μM C18:2, 10μM C22:6 and 10μM C18:3 supplementations compared to groups without fatty acid supplementation (P <0.05). Acetyl-CoA-carboxylase (ACC), fatty acid synthase (FAS), adipose differentiation-related protein (ADRP), acyl-CoA synthetase long-chain family member 1 (ACSL1), diacylglycerol O-acyltransferase 1 (DGAT1), carnitin palmitoyltransferase-II (CPT-II) mRNAs expression and AMPKα phosphorylation were not modified with PUFA supplementation. Experiment 5: SCD1 and FAS mRNA decrease in Boec group compared to serum supplementation, as SCD1 mRNA in ewe oviduct group (P <0.05). In conclusion, this study showed that a PUFA supplementation with C18:2, C18:3 or C22:6 in bovine culture development for 6 days and co-culture with Boec down-regulate mRNA expression of proteins involved in lipid metabolism in d 7–8 embryo (SCD1 and FADS2 desaturases), probably through SREBP1 mRNA regulation after 10μM C22:6 supplementation, indicating a modification of saturated/unsaturated fatty acid balance in bovine blastocyst. [Copyright &y& Elsevier]

Published
2010
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45. Microsatellite loci to recognize species for the cheese starter and contaminating strains associated with cheese manufacturing

Author

Giraud, Frédéric, Giraud, Tatiana, Aguileta, Gabriela, Fournier, Elisabeth, Samson, Robert, Cruaud, Corine, Lacoste, Sandrine, Ropars, Jeanne, Tellier, Aurélien, and Dupont, Joëlle

Subjects
*MICROSATELLITE repeats, *LOCUS (Genetics), *CHEESE industry, *BACTERIAL starter cultures, *GENETIC markers, *FOOD contamination, *PENICILLIUM, *PHYLOGENY, *GENETIC polymorphisms, *GENE amplification
Abstract

Abstract: We report the development of 17 microsatellite markers in the cheese fungi Penicillium camemberti and P. roqueforti, using an enrichment protocol. Polymorphism and cross-amplification were explored using 23 isolates of P. camemberti, 26 isolates of P. roqueforti, and 2 isolates of each of the P. chrysogenum and P. nalgiovense species, used to produce meat fermented products. The markers appeared useful for differentiating species, both using their amplification sizes and the sequences of their flanking regions. The microsatellite locus PC4 was particularly suitable for distinguishing contaminant species closely related to P. camemberti and for clarifying the phylogenetic relationship of this species with its supposed ancestral form, P. commune. We analyzed 22 isolates from different culture collections assigned to the morphospecies P. commune, most of them occurring as food spoilers, mainly from the cheese environment. None of them exhibited identical sequences with the ex-type isolate of the species P. commune. They were instead distributed into two other distinct lineages, corresponding to the old species P. fuscoglaucum and P. biforme, previously synonymised respectively with P. commune and P. camemberti. The ex-type isolate of P. commune was strictly identical to P. camemberti at all the loci examined. P. caseifulvum, a non toxinogenic species described as a new candidate for cheese fermentation, also exhibited sequences identical to P. camemberti. The microsatellite locus PC4 may therefore be considered as a useful candidate for the barcode of these economically important species. [Copyright &y& Elsevier]

Published
2010
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46. Adiponectin increases insulin-like growth factor I-induced progesterone and estradiol secretion in human granulosa cells

Author

Chabrolle, Christine, Tosca, Lucie, Ramé, Christelle, Lecomte, Pierre, Royère, Dominique, and Dupont, Joëlle

Subjects
*RECOMBINANT proteins, *SOMATOMEDIN, *PROGESTERONE, *ESTRADIOL, *SECRETION, *CELL receptors, *HUMAN in vitro fertilization, *HEALTH outcome assessment, *MESSENGER RNA, *CELLULAR signal transduction
Abstract

Objective: To identify adiponectin and its receptors (AdipoR1 and AdipoR2) in human granulosa cells (GC) and to study the effects of recombinant human adiponectin on P and E2 secretion from these cells. Design: The effects of recombinant human adiponectin on the secretion of P and E2 by cultured human GCs were investigated. Setting: Academic institutions. Patient(s): Seventeen infertile and healthy women undergoing IVF. Intervention(s): Primary human GC cultures stimulated with human recombinant adiponectin (5 μg/mL). Main Outcome Measure(s): Determination of messenger RNA (mRNA) and protein expression of adiponectin and its receptors AdipoR1 and AdipoR2 in fresh human GCs by reverse transcriptase-polymerase chain reaction (RT-PCR) and immunoblot, respectively. Measurement of P and E2 levels in the conditioned media by RIA and determination of cell proliferation by tritied thymidine incorporation. Result(s): Human GCs express adiponectin receptors AdipoR1 and AdipoR2 but not adiponectin. In primary human GCs, adiponectin increases P and E2 secretion in response to insulin-like growth factor I (IGF-I). This was associated with an increase in the p450 aromatase protein level but not those of p450scc, 3βHSD, or StAR. Adiponectin treatment does not affect IGF-1-induced cell proliferation and basal steroidogenesis (no IGF-1 or FSH stimulation). Adiponectin rapidly stimulates MAPK ERK1/2 and p38 phosphorylation in primary human GCs. Conclusion(s): Adiponectin receptors AdipoR1 and AdipoR2, but not adiponectin, are present in human GCs. Adiponectin increases IGF-1-induced P and E2 secretion in primary human GCs. [Copyright &y& Elsevier]

Published
2009
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47. IGF-1 receptor signaling pathways and effects of AMPK activation on IGF-1-induced progesterone secretion in hen granulosa cells

Author

Tosca, Lucie, Chabrolle, Christine, Crochet, Sabine, Tesseraud, Sophie, and Dupont, Joëlle

Subjects
*PROGESTERONE receptors, *INSULIN-like growth factor-binding proteins, *BIOLOGICAL transport, *TYROSINE
Abstract

Abstract: IGF-1 plays a key role in the proliferation and differentiation of granulosa cells. However, the molecular mechanism of IGF-1 action in avian granulosa cells during follicle maturation is unclear. Here, we first studied IGF-1 receptor (IGF-1R) expression, IGF-1-induced progesterone production and some IGF-1R signaling pathways in granulosa cells from different follicles. IGF-1R (mRNA and protein) was higher in fresh or cultured granulosa cells from the largest follicles (F1 or F2) than in those from smaller follicles (F3 or F4). In vitro, IGF-1 treatment (10−8 M, 36h) increased progesterone secretion by four-fold in mixed F3 and F4 (F3/4) granulosa cells and by 1.5-fold in F1 granulosa cells. IGF-1 (10−8 M, 30min)-induced increases in tyrosine phosphorylation of IGF-1R beta subunit and phosphorylation of ERK were higher in F1 than in F3/4 granulosa cells. Interestingly, IGF-1 stimulation (10−8 M, 10min) decreased the level of AMPK Thr172 phosphorylation in F1 and F3/4 granulosa cells. We have recently showed that AMPK (AMP-activated protein kinase) is a protein kinase involved in the steroidogenesis in chicken granulosa cells. We then studied the effects of AMPK activation by AICAR (5-aminoimidazole-4-carboxamide ribonucleoside), an activator of AMPK, on IGF-1-induced progesterone secretion by F3/4 and F1 granulosa cells. AICAR treatment (1mM, 36h) increased IGF-1-induced progesterone secretion, StAR protein levels and decreased ERK phosphorylation in F1 granulosa cells. Opposite data were observed in F3/4 granulosa cells. Adenovirus-mediated expression of dominant negative AMPK totally reversed the effects of AICAR on IGF-1-induced progesterone secretion, StAR protein production and ERK phosphorylation in both F3/4 and F1 granulosa cells. Thus, a variation of energy metabolism through AMPK activation could modulate differently IGF-1-induced progesterone production in F1 and F3/4 granulosa cells. [Copyright &y& Elsevier]

Published
2008
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48. Involvement of the ERK1/2 MAPK pathway in insulin-induced S6K1 activation in avian cells

Author

Duchêne, Sophie, Audouin, Estelle, Crochet, Sabine, Duclos, Michel J., Dupont, Joëlle, and Tesseraud, Sophie

Subjects
*HYPOGLYCEMIC agents, *HORMONES, *PROTEIN kinases, *MUSCLE cells
Abstract

Abstract: In mammals, insulin regulates S6K1, a key enzyme involved in the control of protein synthesis, via the well-documented phosphoinositide-3′kinase (PI3K) pathway. Conversely, S6K1 is activated by insulin in avian muscle despite the relative insulin insensitivity of the PI3K pathway in this tissue. Mitogen-activated protein kinase (MAPK) cascade is another insulin sensitive pathway. The aim of this study was to explore the potential involvement of the ERK1/2 MAPK pathway in the control of p70 S6 kinase (S6K1) in avian species. Firstly, we characterized ERK1/2 MAPK in various chicken tissues. ERK2 was the only isoform detected in avian species whatever the tissue studied. We also showed that ERK2 is activated in vivo by insulin in chicken muscle. The regulation and the role of ERK2 in insulin signaling were next investigated in chicken hepatoma cells (LMH) and primary myoblasts. Insulin stimulation led to ERK2 and S6K1 phosphorylation, and concomitantly increased kinase activity. U0126, an inhibitor of the ERK MAPK pathway, completely abolished insulin-induced S6K1 phosphorylation and activity in chicken myoblasts, whereas its effect was only partial in LMH cells. In conclusion, these results show that ERK1/2 MAPK is involved in the control of S6K1 by insulin in chicken cells, particularly myoblasts. [Copyright &y& Elsevier]

Published
2008
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49. Refeeding and insulin activate the AKT/p70S6 kinase pathway without affecting IRS1 tyrosine phosphorylation in chicken muscle

Author

Duchêne, Sophie, Métayer, Sonia, Audouin, Estelle, Bigot, Karine, Dupont, Joëlle, and Tesseraud, Sophie

Subjects
*HYPOGLYCEMIC agents, *HORMONES, *CHEMICAL reactions, *PROTEIN kinases
Abstract

Abstract: p70 S6 kinase (p70S6K) is a key enzyme involved in the control of protein synthesis. We have previously shown that this kinase is insulin sensitive in chicken muscle despite a relative insulin resistance in the early steps of insulin receptor signaling in this tissue, particularly with no change in tyrosine phosphorylation of the insulin receptor substrate 1 (IRS1). The aim of the present study is to further study the p70S6K pathway in chicken muscle. By analyzing in silico several kinases involved in the protein kinase B (PKB also called AKT)/target of rapamycin (TOR)/p70S6K pathway in the chicken, we showed that the amino acid sequence of the proteins exhibited a very high identity with their homologs in mammalian species and Drosophila. We investigated the regulation of these kinases in vivo or in vitro. Refeeding and insulin treatment significantly (P <0.05) increased the phosphorylation and/or activity of kinases upstream of p70S6K such as AKT and TOR. Similarly, refeeding and insulin increased the phosphorylation of p70S6K on key residues (i.e. T389, T229 and T421/S424) and the phosphorylation of a p70S6K downstream target, the ribosomal protein S6 (by 3–10-fold, P <0.05). Interestingly, we also showed an increase in the phosphorylation level of IRS1 on S632/S635, sites involved in insulin resistance. In conclusion, the AKT/TOR/p70S6K pathway is activated by refeeding and insulin injection, which might negatively regulate IRS1 tyrosine phosphorylation. These results indicate some particularities of the insulin signaling in chicken muscle and suggest the involvement of p70S6K in these features. [Copyright &y& Elsevier]

Published
2008
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50. Expression of adiponectin and its receptors (AdipoR1 and AdipoR2) in chicken ovary: Potential role in ovarian steroidogenesis

Author

Chabrolle, Christine, Tosca, Lucie, Crochet, Sabine, Tesseraud, Sophie, and Dupont, Joëlle

Subjects
*MESSENGER RNA, *ORGANS (Anatomy), *BIOLOGICAL transport, *PITUITARY hormones
Abstract

Abstract: Adiponectin and its receptors (AdipoR1 and AdipoR2) mRNAs are expressed in various chicken tissues including ovary. However, the cellular expression and the role of adiponectin system have never been investigated in chicken ovary. Here, we have shown that the level of adiponectin mRNA is about 10- to 30-fold higher (p <0.001) in theca cells than in granulosa cells from each hierarchical yellow follicle studied (F4–F1). In contrast, the level of AdipoR1 mRNA expression was about two-fold lower in theca cells than in granulosa cells (p <0.05) whereas those of AdipoR2 was similar in both ovarian cells. Whereas expression of adiponectin mRNA increased with follicular differentiation in theca cells, it decreased in granulosa cells. In contrast, mRNA expression of AdipoR1 and AdipoR2 in both theca and granulosa cells remained stable during yellow follicle development. To determine whether adiponectin is involved in the ovarian steroidogenesis, LH (100ng/ml)-, FSH (100ng/ml)- and IGF-1 (100ng/ml)-induced progesterone production was measured in absence or presence of human recombinant adiponectin (10μg/ml) for 36h in cultured granulosa cells from F1, F2 and mixed F3 and F4 follicles. In absence of LH, FSH and IGF-1, adiponectin treatment had no effects on progesterone production whatever vitollegenic follicle studied. However, it increased by about two-fold IGF-1-induced progesterone secretion in F2 and F3/4 follicles whereas it halved progesterone production in response to gonadotropins (LH and FSH) in F3/4 follicles. Thus, in chicken, adiponectin, mainly expressed in theca cells, could exert paracrine or autocrine effect on the ovarian steroidogenesis. [Copyright &y& Elsevier]

Published
2007
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