Expression et effets des WNTs sur l’expansion du cumulus et la maturation de l’ovocyte chez la vache

Diaw, Mouhamadou

12 1900

Les WNTs sont une famille de glycoprotéines qui, secrétées dans le milieu extracellulaire, jouent un rôle important dans l’embryogenèse. Chez l’adulte, leur dérégulation va entrainer diverses affections incluant des troubles du développement accompagnés ou non de malformations mais aussi des cancers. Au niveau de l’ovaire, le rôle des WNTs demeure peu défini même si des études chez l’humain et la souris prouvent l’implication de certains membres de cette famille dans le développement ovarien ainsi que dans les processus de maturation folliculaire et d’ovulation. Dans ce contexte, nous avons voulu évaluer l’expression de quelques membres de la famille des WNTs (-2, -2b, -4, -5a et -5b) durant l’expansion des cellules du cumulus et évaluer l’effet de certains d’entre eux sur le COC ainsi que la maturation de l’ovocyte chez la vache. Les COCs bovins étaient placés dans une solution de maturation in vitro pendant 0, 6, 12 et 22h et les niveaux d’ARNm mesurés par PCR en temps réel. L’abondance de l’ARNm pour WNT-2b était significativement plus élevée après 6h de maturation comparée aux COCs immatures (à 0h), alors que l’ARNm codant pour WNT-2, -4, -5a et -5b n’augmentait qu’en fin de culture. L’addition d’EGF provoquait l’expansion du COC et la progression de l’ovocyte vers la métaphase II (MII) comme nous l’espérions mais, à notre grande surprise, l’ajout de WNT-2b au milieu de maturation provoquait également l’expansion du COC (82% et 69% pour EGF et WNT-2b respectivement) et la progression de l’ovocyte vers le stade MII (62% et 56% EGF et WNT-2b respectivement). La combinaison d’EGF et WNT-2b n’a pas produit de meilleurs résultats. Notre étude met en lumière l’implication des WNTs dans la maturation du COC chez la vache. Leurs voies d’activation restent toutefois à déterminer. / The Wnts comprise a large family of secreted glycoproteins which, when secreted in the extracellular space, play a key role in embryonic development. In adults, Wnts play a role in homeostasis and their deregulation likely causes several problems including developmental abnormalities with or without deformities, and cancer. The role of Wnts in the ovaries is not clearly defined although studies in humans and mice show the involvement of some Wnts in ovarian development, follicular maturation and in the process of ovulation. In this study, we tested the hypothesis that members of the Wnt family are involved in oocyte maturation in cattle. The specific objectives were to measure the expression of key Wnts (Wnt-2, -2b, -4, -5a and -5b) in cumulus cells during expansion, and to assess the effect of select Wnt proteins on expansion of the cumulus oocyte complex (COC) and oocyte maturation. Bovine COCs were placed into IVM medium for 0, 6, 12 and 22 h and mRNA levels measured by real-time PCR. The abundance of Wnt-2b mRNA in the cumulus cells was significantly higher at 6 h of maturation compared to immature (time 0) COCs, whereas mRNAs encoding Wnt-2, -4, -5a and -5b did not increase until the end of culture. The addition of EGF induced COC expansion and progression of the oocyte to meiosis II (MII) as expected but, unexpectedly, addition of Wnt-2b also induced expansion and (82% and 69%, EGF and Wnt2b, respectively) and progression to MII (62% and 56%, EGF and Wnt2b, respectively); a combination of WNT-2b and EGF did not improve the rates over either alone. Our study provides new evidence for a role for Wnts in the maturation of the COC in cattle. The Wnt signalling pathways are still unknown and more studies are needed.

Maturation COC

WNTs

EGF

vache

COC maturation

EGF

cow

Effets de la reprogrammation sur le gène empreinté H19 chez les équins

Poirier, Mikhael

08 1900

Lors de la fécondation, le génome subit des transformations épigénétiques qui vont guider le développement et le phénotype de l’embryon. L'avènement des techniques de reprogrammation cellulaire, permettant la dédifférenciation d'une cellule somatique adulte, ouvre la porte à de nouvelles thérapies régénératives. Par exemple, les procédures de transfert nucléaire de cellules somatique (SCNT) ainsi que la pluripotence par induction (IP) visent à reprogrammer une cellule somatique adulte différentiée à un état pluripotent similaire à celui trouvé durant la fécondation chez l'embryon sans en impacter l'expression génique vitale au fonctionnement cellulaire. Cependant, la reprogrammation partielle est souvent associée à une mauvaise méthylation de séquences géniques responsables de la régulation des empreintes géniques. Ces gènes, étudiés chez la souris, le bovin et l'humain, sont exprimés de manière monoallélique, parent spécifique et sont vitaux pour le développement embryonnaire. Ainsi, nous avons voulu définir le statut épigénétique du gène empreinté H19 chez l'équin, autant chez le gamètes que les embryons dérivés de manière in vivo, SCNT ainsi que les cellules pluripotentes induites (iPSC). Une région contrôle empreinté (ICR) riche en îlots CpG a été observée en amont du promoteur. Couplé avec une analyse de transcrit parent spécifique du gène H19, nous avons confirmé que l'empreinte du gène H19 suit le modèle insulaire décrit chez les autres mammifères étudiés et résiste à la reprogrammation induite par SCNT ou IP. La déméthylation partielle de l'ICR observée chez certains échantillons reprogrammés n'était pas suffisante pour induire une expression biallélique, suggérant un contrôle des empreintes chez les équins durant la reprogrammation. / After fertilization, the animal genome undergoes a complex epigenetic remodeling that dictates the growth and phenotypic signature of the animal. The development of reprogramming methods using adult differentiated cells as the primordial genetic source has opened the door to new regenerative therapies for animals. Somatic cell nuclear transfer (SCNT) and induced pluripotency are two techniques which aim to reprogram a cell from its adult differentiated state to an embryonic-like pluripotency level, without impairing the expression of genes vital for the cellular function. Albeit promising, the mechanisms involved in these techniques remain only moderately understood. Partial reprogramming is frequently associated with irregular methylation of DNA sequences responsible for imprint regulation. These imprinted genes, mostly studied in rodents, cattle and humans, are expressed in a monoallelic parent-specific fashion and are vital for embryo growth. Hence, we aim to define the equine H19 imprinting control region (ICR) in gametes, in vivo and in SCNT derived embryos, as well as in induced pluripotent stem cells (iPSC). A CpG rich ICR was characterized upstream of the promotor using bisulfite treated DNA sequencing. Coupled with parent-specific gene expression analysis, we confirmed that the imprinted gene H19 is resistant to cellular reprogramming, and that partial demethylation of its ICR does not result in biallelic expression, suggesting that equine species have rigorous imprint maintenance during cellular reprogramming.

Épigénétique

Reprogrammation

SCNT

iPSC

H19

Équin

ICR

Epigenetics

Reprogramming

Equine

L'hepcidine : un possible lien entre l'inflammation chronique et le métabolisme du fer dans les maladies rénales chroniques félines

Javard, Romain

08 1900

Le rôle de l'inflammation dans le développement et la progression des maladies rénales chroniques (MRC) chez le chat a été peu étudié. L'hepcidine est une protéine de la phase aigue (PPA) de l'inflammation qui contribue au développement des anémies lors de MRC chez l'homme. Les objectifs de cette étude sont de comparer les concentrations en PPAs, en erythropoietine (EPO) ainsi que le statut en fer entre un groupe de chats sains et en MRC. 18 chats sains et 38 chats en MRC ont été recrutés de façon prospective. Les examens réalisés incluaient hématologie, biochimie, analyse d'urine, Serum amyloid A (SAA), haptoglobine (HAP), EPO, hepcidine,fer, TIBC et ferritinne. Nous avons observé une augmentation significative des concentrations en SAA et en hepcidine ainsi qu'une diminution significative du fer et du TIBC dans le groupe MRC (P < .05). Une corrélation positive entre la créatinine et certaines PPAs (SAA and hepcidin; P < .05) était présente. L'augmentation de SAA et hepcidine était significativement associé avec une diminution du TIBC et de l'hématocrite dans le groupe MRC. Les 14 (37%) chats anémiques du groupe MRC avaient une concentration significativement plus basse en fer et en TIBC (P < .05), changements compatibles avec une déficience fonctionelle en fer. Aucun chat n'avait un panel de fer compatible avec une carence en fer absolue. En conclusion, les résultats de cette étude suggèrent que les MRC chez le chat sont des conditions pro-inflammatoires, ayant un impact sur le métabolisme du fer. / The role of inflammation in the development and progression of feline chronic kidney disease (CKD) is not well characterized. Hepcidin, a recently discovered acute phase protein (APP) contributes to the development of anemia in human patients with CKD. The objectives of our study was to compare plasma APP including hepcidin, iron status, and erythropoietin (EPO) concentrations between healthy and cats with naturally occurring CKD. Eighteen healthy control cats and 38 cats with CKD were prospectively recruited. Complete physical examination along with hematology, biochemistry, plasma amyloid A (SAA), haptoglobine (HAP), EPO, iron, TIBC and ferritin were performed using routine laboratory analyses and commercially available feline ELISA-assays. Hepcidin-25 concentration was assessed with a human ELISA kit (DRG® Diagnostics). We found that mean SAA and hepcidin concentration were significantly higher and mean total iron and TIBC were significantly lower in the CKD group (P < .05). There was a significant positive correlation between creatinine and APPs (SAA and hepcidin; P < .05). Increase in SAA and hepcidin was also significantly associated with decrease of TIBC and PCV in the CKD group. The 14 (37%) anaemic cats with CKD had significantly and lower iron, TIBC, consistent with functional iron deficiency (P < .05). There were no patients with an iron profile suggestive of a true iron deficiency. There was no association with survival. In conclusion, our data suggest that feline CKD is a pro-inflammatory state, having significant impact on iron metabolism. With further validation, hepcidin may help better characterize these interactions.

Serum Amyloid A

érythropoïétine

ferritine

anémie

hepcidine

Erythropoietin

Ferritin

anemia

Hepcidin

Immunosuppressive properties of Wharton's jelly derived mesenchymal stromal cells in the treatment of graft versus host disease in rat model

Lopez Rodriguez, Yelica Virginia

January 1900

Doctor of Philosophy / Department of Anatomy and Physiology / Mark L. Weiss / Graft Versus Host Disease (GVHD) is the major complication following hematopoietic stem cell transplantation. GVHD is activated by immunocompetent T cells presented in the donor grafted tissue. Due to the increased use of bone marrow transplantation to treat diverse malignancies, the incidence of GVHD has shown a notable increase. Depending of the degree of immunological mismatch between donor and host, 50-70% of patients develop GVHD after allogeneic Bone Marrow Transplantation (BMT). Once GVHD develops, mortality reaches up to 50% in humans. Several studies using Mesenchymal Stromal Cells (MSCs) to prevent and treat GVHD have produced controversial results. It is thought that distinct MSCs sources used in those studies might be an important factor that produces different outcomes. For cellular therapy, the most attractive characteristics of MSCs are their reduced immunogenic potential, and their abilities to modulate immune responses. This dissertation addressed the hypothesis that Wharton’s jelly cells (WJCs) would prevent the pathology and death associated with GVHD after BMT. To accomplish this, I created a clinically relevant model of GVHD by transplanting allogeneic bone marrow across minor histocompatibility antigen (HA) barriers in the rat. To enhance alloreactive T-cell stimulation, bone marrow (BM) was co-administered with a fraction of CD8[superscript]+ cells magnetically selected from spleen to induce GVHD. Bone marrow tissue was isolated from a donor rat Fischer 344 (F344, RT1lv) and transplanted into lethally irradiated (10 Gray) Lewis rat (LEW, RT1l). Once GVHD was induced, MSCs derived from umbilical cord WJCs were either co-transplanted at day 0 with bone marrow, or given on day 2 post-BMT intravenously. The prophylactic potential of WJCs in an in vivo GVHD model was assessed as survival time, clinical symptomatology occurrence, and histopathology injuries in target tissues. Results indicate that while co-administration of WJCs with hematopoietic cells on day 0 failed to alleviate GVHD associated symptomatology and mortality. WJCs administered on day 2 post-induction ameliorated GVHD-associated symptomatology, improved engraftment and survival.

Graft versus host disease

Umbilical cord mesenchymal stromal cells

Wharton's jelly cells

GVHD rat model

Veterinary Medicine (0778)

Effects of chlortetracycline and copper supplementation on levels of antimicrobial resistance in the feces of weaned pigs

Agga, Getahun Ejeta

January 1900

Doctor of Philosophy / Department of Diagnostic Medicine and Pathobiology / Harvey Morgan Scott / The use of antibiotics in food animals is of major concern as a purported cause of antimicrobial resistance (AMR) in human pathogens; as a result, alternatives to in-feed antibiotics such as heavy metals have been proposed. The effect of copper and CTC supplementation in weaned pigs on AMR in the gut microbiota was evaluated. Four treatment groups: control, copper, chlortetracycline (CTC), and copper plus CTC were randomly allocated to 32 pens with five pigs per pen. Fecal samples (n = 576) were collected weekly from three pigs per pen over six weeks and two Escherichia coli isolates per sample were tested phenotypically for antimicrobial and copper susceptibilities and genotypically for the presence of tetracycline (tet), copper (pcoD) and ceftiofur bla[subscript]C[subscript]M[subscript]Y₋₂) resistance genes. CTC-supplementation significantly increased tetracycline resistance and susceptibility to copper when compared with the control group. Copper supplementation decreased resistance to most of the antibiotics, including cephalosporins, over all treatment periods. However, copper supplementation did not affect minimum inhibitory concentrations of copper or detection of pcoD. While tetA and bla[subscript]C[subscript]M[subscript]Y₋₂ genes were associated with a higher multi-drug resistance (MDR), tetB and pcoD were associated with lower MDR. Supplementations of CTC or copper alone were associated with increased tetB prevalence; however, their combination was paradoxically associated with reduced prevalence. These studies indicate that E. coli isolates from the weaned pigs studied exhibit high levels of antibiotic resistance with diverse multi-resistant phenotypic profiles. In a related study, total fecal community DNA (n = 569) was used to detect 14 tet genes and to quantify gene copies of tetA, tetB, pcoD and bla[subscript]C[subscript]M[subscript]Y₋₂. CTC and copper plus CTC supplementation increased both the prevalence and gene copies of tetA, while decreasing both the prevalence and gene copies of tetB, when compared with the control group. The diversity of tet genes were reduced over time in the gut bacterial community. The roles of copper supplementation in pig production and pco-mediated copper resistance in E. coli need to be further explored since a strong negative association of pcoD, with both tetA and bla[subscript]C[subscript]M[subscript]Y₋₂, suggests there exist opportunities to select for a more innocuous resistance profile.

Pigs

Antimicrobial and copper resistance

E. coli

Ceftiofur

Tetracycline

Epidemiology (0766)

Microbiology (0410)

Veterinary Medicine (0778)

The epidemiology of tetracycline and ceftiofur resistance in commensal Escherichia coli

McGowan, Matthew Thomas

January 1900

Master of Science / Department of Biomedical Science / H. Morgan Scott / The modern phenomenon of increasing prevalence of antibiotic resistance in clinically relevant bacteria threatens humanity’s ability to use antibiotics to treat infection in both humans and animals. Despite the marked complexity of bacterial evolution, there is tremendous importance in unfolding the process by which antibiotic resistance genes emerge, disperse, and persist in the natural world. This thesis investigates certain aspects of this process in two experimental studies that differ primarily by scale but also by methodology. The first study examined the long-term annual prevalence of ceftiofur and tetracycline resistance in Canadian beef cattle from 2002 to 2011 at both phenotypic and genotypic levels. Ceftiofur was present at a very low prevalence (<4%) that did not statistically increase over the decade (p<0.05). Relative proportions of tetracycline genes tet(A), tet(B), and tet(C) also did not significantly change over the observation period. However, it was surprising that almost 20% of isolates recovered from nonselective agar harbored tet(C) given that current literature generally indicates that tet(C) is significantly less prevalent than tet(A) or tet(B). The usage of historical samples in addition to parallel selective plating using agar supplemented with antibiotics provided insight into systemic bias present in common microbial approaches. Long-term sample freezing significantly diminished the recoverability of E. coli over time. Additionally the usage of selective MacConkey agar containing tetracycline biased the proportions of tetracycline genes to over-represent the tet(B) gene in commensal E. coli compared to nonselective MacConkey agar. The second study attempted to explain the short-term selection effects of antibiotic treatment on the overall ecological fitness of commensal E. coli using bacterial growth parameters estimated from spectrophotometric growth curves as a simple surrogate of general fitness. Treating cattle with either tetracycline or ceftiofur was found to not only select in favor of tetracycline resistant bacteria, but also increased the overall fitness among the tetracycline resistant population. However, growth curves were unable able to explain why transiently selected resistant bacteria were eventually replaced by susceptible bacteria once the selection pressure was removed.

Antimicrobial resistance

Growth curves

Tetracycline resistance

Ceftiofur resistance

Beef cattle

Epidemiology (0766)

Microbiology (0410)

Veterinary Medicine (0778)

In vitro effects of canine Wharton’s jelly mesenchymal stromal cells and nanoparticles on canine osteosarcoma D17 cell viability.

Reeds, Kimberly

January 1900

Master of Science / Department of Clinical Sciences / Mary Lynn Higginbotham / Objectives – To isolate and maintain canine Wharton’s jelly mesenchymal stromal cells (WJMSCs) in culture, to determine the effects of micellar nanoparticles containing doxorubicin (DOX) on WJMSCs and canine osteosarcoma (OSA) D17 cell viability, and to determine the effects of conditioned media from WJMSCs loaded with micellar nanoparticles containing DOX on OSA D17 cell viability. Sample Population – Canine WJMSCs containing various concentrations of DOX micelles and canine OSA D17 cells. Procedures – WJMSCs were isolated from canine umbilical cords. Micellar nanoparticles containing DOX were prepared and added to culture plates containing canine OSA D17 cells to determine micelle effects on cell growth and viability. Conditioned media from culture plates containing canine WJMSCs incubated with various DOX micelle concentrations was added to OSA D17 cells for conditioned media experiments. A 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) assay was performed to assess OSA D17 cell viability. A trypan blue stain was also utilized to perform cell counts to determine the effect of the DOX micelles on stromal cell growth. Results – WJMSCs were successfully isolated and maintained in culture. Micellar nanoparticles containing DOX decreased OSA D17 cell viability. OSA D17 cell viability was also decreased following incubation with conditioned media from canine WJMSCs loaded with micellar nanoparticles containing DOX. Significant decreases with the conditioned media of canine WJMSCs loaded with 10μM micelles occurred at 48 hours (p < 0.005) and at 72 and 96 hours (p < 0.0001). Significant decreases were also observed with the 1 μM DOX micelles at 72 hours (p < 0.005) and 96 hours (p < 0.0001). WJMSC numbers decreased in a dose dependent manner following incubation with DOX micelles. Changes in WJMSC number was not caused by increased cell death as all variables produced similar percentages of dead cells. Conclusions – Canine WJMSCs were successfully isolated and maintained in culture. Stromal cells containing DOX micellar nanoparticles induced OSA D17 cell cytotoxicity while inducing an anti-proliferative, rather than cytotoxic effect, on the WJMSC. These data support future in vivo experiments utilizing canine WJMSCs and micellar nanoparticles.

Osteosarcoma

Doxorubicin

Nanoparticles

Polymeric micelles

Nanoscience (0565)

Oncology (0992)

Veterinary Medicine (0778)

Validation of the Fung double tube to enumerate Clostridium perfringens from the intestinal contents of broiler chickens raised on different diets

Barrios Godoy, Miguel Alejandro

January 1900

Master of Science / Department of Animal Science / R. Scott Beyer / Daniel Y.C. Fung / Clostridium perfringens causes necrotic enteritis (NE), resulting in decreased feed efficiency and increased mortality, costing the poultry industry USD 2 billion a year worldwide. The objective of the first trial was to validate the Fung Double Tube (FDT) to detect and enumerate C. perfringens in chicken intestines. Two methods (FDT and petri plates) and three media (Shahidi Ferguson Perfringens [SFP] with egg supplement, polymyxin B [p], and kanamycin [k; E]; SFP with p and k [P]; and SFP with cycloserine [C]) were arranged in a 2 x 3 factorial, resulting in six treatments. The FDT with medium C (5.35 log CFU/g) had significantly (P<0.05) higher C. perfringens counts than any other media/method combination. The objective of the second and third trials was to determine the effect of diet type on the population of C. perfringens in broiler intestines using the FDT. Trial 2 tested: corn-soybean meal (SBM), low-crude protein (19.8%)/high synthetic amino acids (SAA), and barley (56%)-fishmeal (4%; BF). Diets in Trial 3 included: corn-SBM, barley (7.46%), fishmeal (4%), and BF. Diets in Trial 2 contained an antibiotic and a coccidiostat; diets in Trial 3 did not. After 21 days, birds in Trial 2 fed BF had significantly higher (P<0.05) counts (5.96 log CFU/g) of C. perfringens, as compared to all other diets. Both, corn-SBM and SAA diets resulted in 3.89 log CFU/g. In Trial 3, birds fed the corn-SBM diet (2.7 log CFU/g) had significantly lower (P<0.05) counts than broilers fed BF (4.15 log CFU/g). When broilers were fed fishmeal (3.583 log CFU/g) and barley (3.577 log CFU/g) separately, C. perfringens counts were numerically higher compared to the corn-SBM diet, but numerically lower than birds fed BF. Barley and fishmeal inclusion increased the incidence of C. perfringens, and their combination resulted in a cumulative effect. The FDT method is able to detect C. perfringens at higher levels than the conventional petri plate method (P<0.001) and it also proved to be an effective method to detect differences in C. perfringens counts from the intestines of chickens fed different diet.

Fung double tube

Clostridium perfringens

Broilers

Barley

Fishmeal

Anaerobic method

Animal Diseases (0476)

Animal Sciences (0475)

Veterinary Medicine (0778)

In vitro and in vivo effects of deoxynivalenol (DON) mycotoxin on porcine reproductive and respiratory syndrome virus (PRRSV) in piglets

Pinilla, Vicente

04 1900

Les récoltes de céréales sont souvent contaminées par des moisissures qui se développent pendant la récolte et l’entreposage et produisent des métabolites secondaires appelés mycotoxines. Le porc est reconnu pour être sensible au déoxynivalénol (DON). L’infection virale la plus importante chez le porc est causée par le virus du syndrome reproducteur et respiratoire porcin (VSRRP). Celui-ci provoque un syndrome grippal et des troubles de reproduction. L’objectif du présent projet était de déterminer l'effet in vitro de DON sur la réplication du VSRRP dans de lignées cellulaires permissives, MARC-145 et PAM, et déterminer in vivo l'impact de DON dans des aliments naturellement contaminés sur l’infection au VSRRP chez le porcelet. Tout d’abord, les cellules ont été incubées avec des doses croissantes de DON et ont été infectées avec du VSRRP pour évaluer la viabilité et la mortalité cellulaire, la réplication virale et l’expression de cytokines. Les résultats ont montré que les concentrations de DON de 560ng/ml et plus affectaient significativement la survie des cellules MARC-145 et PAM infectées par le VSRRP. En revanche, il y avait une augmentation significative de la viabilité et une réduction de la mortalité cellulaire à des concentrations de DON de 140 à 280 ng/ml pour les cellules PAM et de 70 à 280 ng/ml pour les cellules MARC-145 avec une réduction de l'effet cytopathique provoqué parle VSRRP. Au niveau in vivo, 30 porcelets divisés en 3 groupes de 10 porcelets et nourris pendant 2 semaines avec 3 différentes diètes naturellement ont été contaminées avec DON (0; 2,5 et 3,5 mg/kg). Les porcelets ont été subdivisés en 6 groupes, 3 groupes de 6 porcelets et ont été exposés au DON pendant 2 semaines et infectés par voie intratrachéale et intramusculaire avec le virus. Les 3 autres groupes de 4 porcelets servaient de contrôle non infectés. Les signes cliniques ont été enregistrés pendant 21 jours. La virémie a été évaluée par PCR. À la fin de l’expérimentation, les porcelets ont été euthanasiés et les lésions pulmonaires ont été évaluées. Les résultats ont montré que l’ingestion de DON à 3,5 mg/kg a augmenté l’effet du VSRRP sur la sévérité des signes cliniques, les lésions pulmonaires et la mortalité. L’ingestion de DON à 2,5 mg/kg a entrainé une augmentation de la virémie au jour 3 après l’infection mais sans impact sur les signes cliniques et les lésions pulmonaires. Mot clés: DON, VSRRP, MARC-145, PAM, effet cytopathique, cytokines, PCR / Cereal crops are often contaminated with moulds that grow during harvest and storage and produce secondary metabolites called mycotoxins. Pig is known to be sensitive to deoxynivalenol (DON). On the other hand, infection by porcine reproductive and respiratory syndrome virus (PRRSV) causes a flu-like syndrome and reproductive disorders. The objectives of this project were to determine the in vitro effect of DON on the replication of PRRSV in permissive cell lines, MARC-145 and PAM and the in vivo impact of DON-naturally contaminated feed on PRRSV infection in piglets. Firstly, cells were incubated with gradually increasing doses of DON and were infected with PRRSV to evaluate cytopathic effect and to assess cell viability, virus replication and cytokine mRNA expression on infected and uninfected cells. Results showed that DON concentrations of 560 ng/ml and higher were significantly detrimental to the survival of MARC-145 cells infected with PRRSV. In contrast, there was a significant increase of cell viability and decreased of cell mortality at DON concentrations within 140 to 280 ng/ml for PAM cells and 70 to 280 ng/ml ranges for MARC-145 showing a reduced cytopathic effect (CPE) caused by PRRSV. In vivo study was carried out on 30 piglets divided into 3 groups of 10 piglets fed naturally contaminated diets with different levels of DON; 0, 2.5 and 3.5 mg/kg. After 2 weeks, pigs were further divided into 6 subgroups, 3 subgroups of 6 piglets were infected intra tracheally and intramuscularly with PRRSV. The other 3 subgroups of 4 piglets were used as uninfected controls. Clinical signs were recorded for 21 days post-infection (p.i.). Sera were evaluated for viremia by PCR. At the end of the experiment, piglets were euthanized and pulmonary lesions were evaluated. Results showed that ingestion of diet highly contaminated with DON at 3.5 mg/kg increased the effect of PRRSV infection on the severity of clinical signs, weight loss, lung lesions and mortality. Diet with DON at 2.5 mg/kg showed an increase of viremia at day 3 but had not significant impact on clinical signs and lung lesions. Keywords: DON, PRRSV, MARC-145, PAM, cytopathic effect, cytokines, PCR

DON

VSRRP

MARC-145

PAM

Effet cytopathique

Cytokines

PCR

PRRSV

Cytopathic effect

Évaluation du lactate sanguin chez les chiens atteints de cancer

Touret, Maude

04 1900

Malgré le manque d’études sur ce sujet, le cancer est considéré comme une des principales causes d’hyperlactatémie de type B chez le chien. Les cellules malignes ont une production accrue de lactates secondaire à une glycolyse aérobie accrue, via l’effet Warburg. Les mécanismes ne sont pas encore clairement établis mais certains auteurs suggèrent que le cancer pourrait causer une hyperlactatémie via l’effet Warburg. Cette étude a pour objectif de déterminer si les tumeurs malignes peuvent être associées à une hyperlactatémie cliniquement significative (≥2,5 mmol/L) chez le chien. Trente-sept chiens atteints de tumeurs malignes ont été recrutés (22 atteints de tumeurs hématopoïétiques et 15 de tumeurs non hématopoïétiques). Le diagnostic était confirmé par analyse histologique, ou cytologique en cas de lymphome. Les autres causes possibles d’hyperlactatémie étaient écartées puis la mesure des lactates sanguins était réalisée sur sang veineux jugulaire immédiatement analysé avec le LactatePro®. Aucun chien n’était hyperlactatémique. La concentration moyenne en lactates sanguins était de 1,09 mmol/L. La concentration moyenne en lactates sanguins pour les chiens atteints de tumeurs non hématopoïétiques et hématopoïétiques était respectivement de 0,95 mmol/L et de 1,19 mmol/L. Les chiens atteints de lymphome (n=18) avaient une concentration moyenne en lactates sanguins de 1,15 mmol/L. Les tumeurs malignes ne sont pas associées à une hyperlactatémie de type B cliniquement significative chez le chien. L’hyperlactatémie tumorale est donc une complication rare chez le chien. Son diagnostic devrait conduire à une investigation minutieuse des autres causes d’hyperlactatémie. / Cancer is considered a cause of type B hyperlactatemia in dogs. However, studies evaluating cancer as a cause of clinically relevant type B hyperlactatemia (≥2.5 mmol/L) are lacking. It is well accepted that cancer cells have a higher lactate production due to increased aerobic glycolysis, known as the Warburg effect. The mechanisms through which aerobic glycolysis occurs are not well elucidated but it has been suggested that neoplasia may cause type B hyperlactatemia via this process. The aim of this study is to determine if canine malignant tumors could be associated with a clinically relevant type B hyperlactatemia (≥ 2.5 mmol/L). Thirty-seven dogs with malignant tumors were included: 22 with hematopoietic and 15 with solid tumors. Histology was used to confirm the diagnosis (cytology was considered appropriate for lymphoma). Confounding factors associated with hyperlactatemia were excluded. Lactate measurements were obtained from a free flow jugular whole blood sample and immediately analyzed using the LactatePro®. All dogs had lactate values less than 2.5 mmol/L. The mean blood lactate concentration was 1.09 mmol/L. The mean blood lactate concentration for solid and hematopoietic tumor was 0.95 mmol/L and 1.19 mmol/L respectively. Dogs with lymphoma (n = 18) had a mean blood lactate concentration of 1.15 mmol/L. Malignant tumors were not considered a cause of clinically relevant type B hyperlactatemia. Therefore, cancer related type B hyperlactatemia in dogs with cancer is uncommon and its diagnosis should prompt careful investigation for causes other than cancer.

Lactate

Cancer

Warburg

Hyperlactatémie

Chien

Lactate

Cancer

Warburg

Hyperlactatemia

Dog