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In vivo comparison of Edwardsiella ictaluri survival in kidneys of vaccinated and naÏve rag1-/- zebrafishVarner, Casey Janine 07 August 2010 (has links)
This study used rag1-/- mutant zebrafish, which lack functional T and B lymphocytes, to investigate whether innate immune cells from vaccinated mutant zebrafish demonstrate enhanced survival compared to phagocytes from naïve mutant fish. Edwardsiella ictaluri, an economically significant aquatic pathogen and the causative agent of enteric septicemia of catfish (ESC), was used for the trials. Quantification of live bacteria from sampled kidneys was accomplished via colony counts, luminescence readings, and differential DNA extractions using Ethidium Monoazide (EMA) and Propidium Monoazide (PMA) followed by qPCR. There was a general trend of less bacteria in vaccinated mutant fish. Additionally, the mortality in the vaccinated fish was less than the naïve group, suggesting that the vaccinated fish are better able to withstand the bacteria load. Giemsa-stained cytospins showed E. ictaluri exclusively within macrophages from sampled kidneys, suggesting that the macrophages are the critical site of pathogenesis in rag1-/- zebrafish.
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DEVELOPMENTAL ENVIRONMENT ALTERS CONDITIONAL AGGRESSION IN ZEBRAFISHMarks, Christopher P. 05 October 2006 (has links)
No description available.
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Zebrafish Asd Discovery Models for Epileptic Mutations of Scn2a and Scn8aMilder, Patrick 12 1900 (has links)
Indiana University-Purdue University Indianapolis (IUPUI) / Approximately 30% of patients with epilepsy do not achieve adequate seizure control through current anti-seizure drugs (ASD) and treatment methods. Therefore, a critical need exists to efficiently screen ASDs to enhance our ability to tailor treatment protocols and improve patient outcomes. The zebrafish pentylenetetrazol (PTZ) seizure model has become an increasingly popular screening paradigm for novel ASDs. Here, we present an optimized PTZ assay to improve reliability and reproducibility based on work in our laboratory. This optimized assay improves robustness in our screening of anti-seizure drugs (topiramate, lamotrigine, carbamazepine and GS967). These findings show that electroencephalogram (EEG) and calcium sensitive GFP from fusion protein (GCaMP) assays largely correlate with the behavioral findings, helping us connect physiological and behavioral responses to ASDs. Genetic epilepsy syndromes, like voltage gated sodium channel SCN2A and SCN8A pathogenic variants, are often poorly controlled by current medications. Our optimized assay relied on a fast and precise zebrafish seizure model using mRNA overexpression of hSCN2A and hSCN8A variants including: hSCN2A R1882Q and R853Q and hSCN8A R1872Q. All three pathogenic variants increased seizure activity, and the ASDs significantly decreased this seizure activity. This mRNA overexpression assay can be used to quickly evaluate seizure activity induced by pathogenic variants in voltage gated sodium channel genes and test ASDs to determine efficacy. In a separate study, we tested if the addition of the human SCN2A sodium channel could potentially rescue the loss of the zebrafish scn1Lab gene. Our GCaMP assay data indicates that this loss was successfully rescued. Cumulatively, these findings can be used to improve the screening of novel ASDs and treatments for patients with refractory epilepsy.
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Characterization of an Enhancer Upstream of Msx3 and its Role in Development of the Neural Tube of Embryonic and Larval ZebrafishKeil, Shea 03 April 2023 (has links)
The vertebrate nervous system arises during embryogenesis from an epithelial sheet of cells called the neural plate that subsequently folds to become a rod of cells called the neural tube. Several signaling pathways act on the neural progenitors of the neural tube to give rise to the diverse set of neurons and glia that will make up the spinal cord and brain in adulthood. In vertebrates, Muscle segment homeobox (Msx) genes are expressed in the dorsal neural tube during development, and pattern dorsal neural progenitors to give rise to dorsal neuronal subtypes. Additionally, Msx genes are involved in the regulation of neurogenesis and proliferation in the neural tube. In zebrafish, three msx genes are expressed in the neural tube: msx1a, msx1b, and msx3. The Akimenko lab has identified a potential enhancer of msx3 called Fragment C that drives expression in the dorsal neural tube. We hypothesized that Fragment C is a bona fide enhancer of msx3 specifically in the neural tube, and that this enhancer contributes toward proper patterning and neurogenesis/proliferation in the developing neural tube of zebrafish. To test this hypothesis, I have generated zebrafish mutants with a deletion of the Fragment C enhancer using CRISPR/Cas9 that also have a transgenic Fragment C enhancer driving reporter expression of enhanced green fluorescent protein (Egfp). The deletion of Fragment C abolishes msx3 expression in the neural tube excluding the dorsal-most cells likely corresponding to the roof plate. The spatial domain in which msx3 is lost corresponds to where Fragment C drives expression in the neural tube, suggesting that Fragment C contains an enhancer of msx3. This domain of expression corresponds to where dorsal neural progenitors reside. Analysis of markers for the cells with Fragment C-driven Egfp expression shows that at least some of these cells are indeed neural progenitors, many of which give rise to neurons during embryonic and larval development. The deletion of Fragment C and loss of msx3 expression in neural progenitors did not affect the numbers of neurons or neural progenitors amongst cells with Fragment C-driven expression, nor did it affect the dorsoventral location of cells in the neural tube. Taken together, we conclude that Fragment C-driven msx3 expression does not contribute to the dorso-ventral position of neural progenitors nor the balance of proliferation and neurogenesis in the developing neural tube. However, a role for msx3 in regulating neural progenitor identity along the dorso-ventral axis without affecting progenitor position cannot be ruled out.
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Leptin Expression in Male and Female Raffishness (Danio Reri)Riley, Caitlin L. 20 September 2013 (has links)
No description available.
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Developmental Toxicity of Dextromethorphan and Acetaminophen in Zebrafish Embryos/Larvae: Relevance of SULT-mediated Dextromethorphan/Acetaminophen SulfationXu, Zheng 14 June 2010 (has links)
No description available.
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Characterization of Actinodin 1 and Actinodin 2 Loss-of-function Mutations in ZebrafishBaird, Connor 11 January 2024 (has links)
Zebrafish (Danio rerio) are ray-finned fish of the teleost class, whose fins consist of an
exoskeletal domain and an endoskeletal domain. The exoskeletal domain of the fins contains
the fin rays and originate from embryonic fin folds that elongate as the fins are growing. The
elongation of the fin fold is supported by two parallel sets of rigid fibrils oriented along the
proximal-distal axis, called actinotrichia. Actinotrichia fibrils are composed of two primary
components, a collagenous component and actinodin proteins. The actinodin proteins are
encoded for by the actinodin (and) family of genes which are found in the genomes of finned
fish while absent in limbed tetrapods. CRISPR/Cas9 was used to create loss-of-function
deletions in the and1 and and2 genes, resulting in the absence of actinotrichia in the zebrafish
double mutants. We hypothesised that the loss of actinotrichia during zebrafish development
would result in developmental defects leading to fin ray defects in the adult zebrafish. The
and1/2 mutants that lack actinotrichia presented with fin fold and cell migration defects during
development that persisted into adulthood and resulted in shorter fins, disturbed fin ray
patterning, and a decrease in ray number. In addition, an unexpected fusion between the
hypurals of the caudal fin endoskeleton revealed an additional function of the actinotrichia
fibrils in caudal fin endoskeletal patterning. During zebrafish development, actinotrichia fibrils
play a vital role in ensuring normal fin development, normal patterning and formation of the
fin rays, and the normal development of the caudal fin endoskeleton.
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CARBAMAZEPINE & GEMFIBROZIL AFFECT ZEBRAFISH REPRODUCTION / LONG TERM ADVERSE EFFECTS OF CARBAMAZEPINE AND GEMFIBROZIL ON MALE ZEBRAFISH (Danio rerio) REPRODUCTIONFraz, Shamaila 20 December 2017 (has links)
Pharmaceuticals are emerging surface water contaminants, and are manufactured, used, and released into environment in considerable amounts. Concerns have been raised due to the inherent potency and bioactivity of these molecules, which makes effects at low concentrations more likely. The ubiquitous presence and stability of pharmaceuticals brings up concerns about the frequency and length of exposures. However, the distribution and fate of these compounds in surface water bodies is not clear. There is limited information about the potential effects in non-target, especially aquatic, species vulnerable to cumulative or lifelong exposures. Carbamazepine (CBZ) and gemfibrozil (GEM) are two of the most frequently detected pharmaceuticals in surface water. This thesis examined sub-lethal adverse reproductive effects of chronic direct exposure of CBZ and GEM to F0 zebrafish and several generations of unexposed offspring; the effects of exposure on testicular steroidogenesis were also examined. Chronic exposure of zebrafish to CBZ and GEM reduced ex vivo production of 11KT in testes. In vivo, CBZ decreased reproductive output, 11-ketotestosterone (11KT), male courtship and aggression behaviours, and sperm morphology in F0 parents. The F1, F2 and F3 offspring of CBZ exposed males had lower reproductive output, altered courtship, aggression, sperm morphology and lower 11KT compared to fish from the unexposed lineage. The adverse effects persisted into the F3 generation which suggested transgenerational paternal effects. GEM decreased reproductive output in F0 parents and a reduction in 11KT, altered male courtship, aggression and sperm morphology. Unexposed F1 male offspring, but not other generations, had sub-lethal toxic effects from parental exposure. We therefore suggest that CBZ and GEM act as endocrine disruptors in fish and that chronic exposure may reduce male reproductive fitness. / Dissertation / Doctor of Philosophy (PhD) / Human pharmaceuticals reach aquatic environments through municipal wastewater. The bioactivity of pharmaceuticals at low concentrations has raised concerns about undesired effects in aquatic species like fish, which can experience chronic exposures. This thesis examined adverse reproductive effects of direct chronic exposure of carbamazepine and gemfibrozil to parental zebrafish and their un-exposed offspring for multiple generations. Exposure to both compounds reduced androgens and reproduction and altered behaviour, and sperm quality in males. Effects persisted in the unexposed offspring. Parental carbamazepine exposure impacted multiple generations. We suggest that carbamazepine and gemfibrozil may reduce male reproductive fitness by reducing male sex steroids.
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Studies on the Fibrinolytic Pathway in ZebrafishGill, Jaspreet Kaur 08 1900 (has links)
Fibrinolysis pathway is an important mechanism for dissolution of fibrin clot by the action of plasmin which is formed from plasminogen, a zymogen via the action of plasminogen activators, i.e. tissue plasminogen activator and urinary plasminogen activator. The regulation of fibrinolysis system in vivo is maintained by plasminogen activators and natural inhibitors i.e. α2-antiplasmin, α2-macroglobulin, Thrombin-activatable fibrinolysis inhibitor (TAFI) and plasminogen activator inhibitor 1 and 2 (PAI-1and PAI-2). There are several fibrinolytic assays developed for human plasma but there are no reports describing fibrinolytic assay using zebrafish plasma. In this study, a fibrinolytic assay via using small amount of zebrafish plasma was developed. This assay was performed under different conditions; one by the addition of exogenous tissue plasminogen activator alone to the pooled zebrafish plasma along with calcium chloride and thromboplastin, second Dade ACTIN was used instead of tissue plasminogen activator and third Dade ACTIN along with thromboplastin was used. Epsilon amino caproic acid (EACA), a synthetic antifibrinolytic agent was used at different concentrations to inhibit fibrinolysis successfully. Similar experiments were performed on human plasma as well to check the applicability of the assay to humans and positive results were obtained. Furthermore, knockdown of tissue plasminogen activator and plasminogen genes was performed and the prolongation of peak time, the time taken for the maximal formation of fibrin was observed, similar to the EACA inhibition. In conclusion, a fibrinolysis assay using miniscule amount of plasma was developed and applied to study knockdown of fibrinolytic pathway genes. The assay developed here may have clinical utility.
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Avaliação do efeito ambiental do inseticida Kraft 36EC® (abamectina) e do fungicida Score 250EC® (difenoconazol) por meio de análises ecotoxicológicas em diferentes estágios de vida do Danio rerio / Analysis of the environmental effect of the insecticide Kraft 36EC® (abamectin) and the fungicide Score 250EC® (difenoconazole) by means of ecotoxicological analyzes in different Danio rerio life stagesSanches, Ana Letícia Madeira 29 June 2018 (has links)
O Kraft 36EC® (i.a. abamectina) e o Score 250EC® (i.a. difenoconazol) são agrotóxicos intensamente utilizados nas culturas de morango em regiões de clima tropical, embora sejam compostos classificados como extremamente tóxicos e muito perigosos ao ambiente. Misturas de agrotóxicos são aplicadas nas culturas agrícolas e a presença destes compostos na água pode potencializar os efeitos tóxicos a organismos aquáticos não alvos. A ocorrência do escorrimento superficial (runoff) contaminado com agrotóxico e a contaminação por aspersão direta (spray drift) em ecossistemas tropicais próximo aos corpos hídricos também podem comprometer o ecossistema aquático local devido à toxicidade desses compostos a organismos não alvos. Considerando os riscos ecológicos inerentes ao uso destes agrotóxicos, o objetivo principal desta pesquisa foi avaliar o efeito ambiental dos praguicidas Kraft 36EC® e Score 250EC® e de seus princípios ativos, abamectina e difenoconazol, respectivamente. Foram realizados testes de toxicidade aguda em laboratório a partir de exposições dos compostos isolados e em misturas utilizando como organismo teste embriões e adultos de Danio rerio. Experimentos in situ (mesocosmos) foram realizados a fim de avaliar os efeitos do runoff e spray drift contaminados com os agrotóxicos Kraft 36EC® e Score 250EC®, isolados e em misturas. Tanto nos mesocosmos quanto em experimentos de laboratório analisou-se, além da mortalidade, biomarcadores bioquímicos. Pelos resultados obtidos verifica-se que não foram observadas diferenças significativas entre a toxicidade isolada dos ingredientes ativos e suas respectivas formulações comerciais em testes agudos. Nos testes de toxicidade com as misturas dos ingredientes ativos, observou-se que a mistura de abamectina + difenoconazol promoveu um efeito tóxico sinérgico a adultos de Danio rerio em exposições agudas. Observou-se também a ausência do mesmo efeito nas exposições com as misturas das formulações comerciais neste mesmo estágio de vida. A exposição dos embriões às misturas de Kraft 36EC® e Score 250EC® mostrou um efeito antagônico nas baixas concentrações e efeito sinérgico nas mais altas. Verificou-se um aumento significativo na atividade da enzima de biotransformação 7-etóxiresorufina-0-deetilase (EROD) e nos níveis de malondialdeído MDA nas brânquias de peixes expostos à formulação comercial da abamectina. Houve um aumento na atividade da glutationa-S-transferase (GST), glutationa peroxidase (GPx) e níveis de MDA, e diminuição da glutationa redutase (GR) nas brânquias dos peixes expostos ao difenoconazol e sua formulação comercial. Também foi observado um aumento nas respostas dos biomarcadores analisados nas brânquias dos organismos expostos às misturas tanto dos princípios ativos quanto das formulações comerciais. A exposição ao Kraft 36EC® spray drift em campo promoveu os maiores efeitos deletérios no metabolismo de Danio rerio, seguido das exposições ao runoff contaminado com Kraft 36EC® e Score 250EC®. As formulações comerciais Kraft 36EC® e Score 250EC® e as misturas das mesmas promoveram alterações significativas no metabolismo de detoxificação, e causam estresse oxidativo em peixes. Diferenças no padrão de respostas dos biomarcadores entre os experimentos realizados em mesocosmos e em laboratório ficam evidentes devido à influência das concentrações utilizadas, das interações ecológicas entre as comunidades presentes no meio e das variáveis ambientais nos experimentos em mesocosmos. A avaliação da toxicidade de agrotóxicos, especialmente em países tropicais, e indicações para futuras pesquisas são discutidos. / Kraft 36EC® (a.s. abamectin) and Score 250EC® (a.s. difenoconazole) are intensely used pesticides in strawberry crops in tropical regions, even though they are classified as extremely toxic and very dangerous to the environment. Mixtures of agrochemicals are applied to agricultural crops and the presence of these compounds in water may potentiate toxic effects to non-target aquatic organisms. The contamination of edge-of-field water bodies through runoff and spray drift may compromise the local aquatic ecosystem due to the toxicity of these compounds to non-target organisms. Considering the potential ecological risks related with the use of these pesticides, the main objective of this research was to evaluate the environmental effects of the pesticides Kraft 36EC® and Score 250EC® and its active ingredients abamectin and difenoconazole, respectively. Acute toxicity tests were performed in the laboratory with the isolated compounds and their mixtures using zebrafish (Danio rerio) embryos and adults as test organism. A mesocosm experiment was also performed to evaluate the effects of simulated runoff and spray drift containing Kraft 36EC® and Score 250EC® individually and in mixtures. Besides lethality, selected biomarkers were also evaluated in the fish from the mesocosm and laboratory experiments. No significant differences were observed in effects of the active ingredients and their respective commercial formulations in acute fish tests after single exposure to each test compound. The acute mixture toxicity tests with the active ingredients showed that this mixture exerts a synergistic toxic effect to adult fish. The absence of the synergistic effect on exposures with the commercial formulations mixtures was also observed. Embryo exposure to Kraft 36EC® and Score 250EC® mixtures showed an antagonistic effect at low concentrations and synergistic effect at the highest. A significant increase was observed in the activity of the EROD biotransformation enzyme and in the levels of MDA in fish gills after exposure to Kraft 36EC®. An increase in GST activity, GPx and MDA levels, and a decrease of GR in fish gills was noted after fish exposure to difenoconazole and its commercial formulation. An increase in the responses of the biomarkers analyzed in the gills of the organisms exposed to the mixtures of both the active ingredients and the commercial formulations as compared to single-compound exposure was also observed. Exposure to simulated spray drift of Kraft 36EC® in the mesocosms promotes the greatest deleterious effects on metabolism of Danio rerio followed by exposures to the runoff contaminated with a Kraft 36EC® and Score 250EC® mixture. The commercial formulations Kraft 36EC® and Score 250EC® and their mixtures lead to significant changes in the detoxification metabolism resulting in oxidative stress to fish. Differences in biomarkers responses between the experiments performed in the mesocosms and the laboratory were noted and are due to the different concentrations tested; the ecological interactions between the communities present in the mesocosms and differences in environmental variables. The need and indications for future research related with the evaluation of pesticide toxicity, especially in tropical countries, are discussed.
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