Global ETD Search

31	An Observation of Immunological Effect, a Diet Enhanced with Spirulina and Treatment with Fractalkine in Models of Parkinson's Disease Pabón, Mibel 31 May 2011 (has links) In my dissertation research we used use human wild type α-synuclein gene expression using an adeno-associated viral vector (AAV9) that induced a slowly progressive loss of dopamine (DA) neurons in the Substantia nigra (SN) as one of our animal model of Parkinson’s disease (PD). It is our hypothesis that neuroinflammation predisposes the brain to susceptibility to neurodegenerative diseases. Thus we examined the progression of a PD lesion and examined the manipulations of the immune system to understand further the inflammatory role when we administered exogenous soluble fractalkine. The specific etiology of neurodegeneration in PD is unknown, but the inflammatory mechanisms and free radicals have been postulated to play a central role. α-synuclein is believed to be the one of the main characteristic associated with PD. It has been found inside saclike structures, called lewy bodies. α-synuclein is believed to activate resident microglia worsening the degeneration of the nigrostriatal pathway due to its aggregation. Aggregation increases the production of reactive oxygen species (ROS) released from microglia. The constant release of these factors and prolonged activation of microglia could be the cause that leads to neurodegeneration in the SN. Spirulina, a blue - green algae, has been shown to have anti-oxidant and anti-inflammatory properties. For example, when rats received an intrastriatal injection of 6-OHDA and were fed a spirulina enriched diet for 4 weeks, there was a significant increase in regeneration of DA terminals into the Tyrosine Hydroxylase (TH) -negative zone of the striatum. This regeneration was accompanied by a decrease in microglia activation as determined by immunohistochemistry of major histo compatibility class II (MHC) (OX-6). This suggests that decreases in microglia activation modulate the beneficial effects of spirulina. Another important therapeutic tool we used was fractalkine as an anti-inflammatory treatment. It is known that fractalkine levels are reduced in the brain during aging. For this reason we administered exogenous fractalkine to 6-OHDA model of PD to test the hypothesis that it improved the microenvironment by reducing microglial activation. Microglia AAV9 nutraceuticals CX3CR1 Tyrosine Hydroxylase American Studies Arts and Humanities Molecular Biology Public Health
32	Zebrafish as a Model for the Study of Parkinson’s Disease Xi, Yanwei 09 May 2011 (has links) Parkinson’s disease (PD) is a common neurodegenerative disorder that is characterized by the degeneration of dopaminergic (DA) neurons in the substantia nigra and motor deficits. Although the majority of PD cases are sporadic, several genetic defects in rare familial cases have been identified. Animal models of these genetic defects have been created and have provided unique insights into the molecular mechanisms of the pathogenesis of PD. However, the etiology of PD is still not well understood. Here, taking advantage of the unique features offered by zebrafish, I characterized the functions of PINK1 (PTEN-induced kinase 1) gene, which is associated with recessive familial PD, in the development and survival of DA neurons. In zebrafish, antisense morpholino knockdown of pink1 did not cause a large loss of DA neurons in the ventral diencephalon (vDC), but the patterning of these neurons and their projections were perturbed. The pink1 morphants also showed impaired response to touch stimuli and reduced swimming behaviour. Moreover, the pink1 knockdown caused a significant reduction in the number of mitochondria, as well as mitochondrial morphological defects such as smaller size or loss of cristae, thus affecting mitochondrial function. These results suggest that zebrafish pink1 plays conserved important roles in the development of DA neurons and in the mitochondrial morphology and function. To better follow DA neurons after injury or administration of toxins, I generated a transgenic zebrafish line, Tg(dat:EGFP), in which the green fluorescent protein (GFP) is expressed under the control of cis-regulatory elements of dopamine transporter (dat). In Tg(dat:EGFP) fish, all major groups of DA neurons are correctly labeled with GFP, especially the ones in the vDC, which are analogous to the ascending midbrain DA neurons in mammals. In addition, we observed that the DA neurons in the vDC could partially be replaced after severe laser cell ablation. This suggests that zebrafish may have the unique capacity of regenerating DA neurons after injury. Taken together, my studies suggested that zebrafish could be a useful alternative animal model for the study of the molecular mechanisms underlying PD and for the screening of potential therapeutic compounds for PD. Zebrafish Parkinson's disease PINK1 dopaminergic neuron dopamine transporter morpholino tyrosine hydroxylase MPTP regeneration
33	Efeito de diferentes dietas sobre a modulação do comportamento alimentar em vias homeostáticas e hedônicas em ratas fêmeas Laureano, Daniela Pereira January 2013 (has links) Introdução: A exposição crônica a diferentes tipos de dieta altera o metabolismo hipotalâmico e mesolímbico, podendo causar alterações no comportamento alimentar do indivíduo. O BDNF, fator de crescimento neuronal, pode atuar na modulação do comportamento alimentar tanto em vias hedônicas quanto homeostáticas. O objetivo do estudo foi investigar como o BDNF atua na modulação do comportamento alimentar em vias homeostáticas e hedônicas em ratas fêmeas com diferentes perfis metabólicos. Materiais e métodos: Ratas Wistar fêmeas adultas randomizadas por peso foram divididas em: dieta controle (C) contendo 22% de proteína e 4% de lipídios; dieta hipoproteica (LP) 8% de proteína ou dieta hiperlipídica (HF) 45% de lipídios, ad libitum, por 5 semanas, sendo o consumo medido a cada 72 horas e o peso semanalmente. O trabalho foi dividido em duas partes. Na primeira parte, após as 5 semanas de dieta os animais ficaram em jejum por 4 horas e foram expostos ao alimento doce (Froot Loops®), previamente pesado, por 1 hora, a fim de verificar o consumo de alimento palatável em ratas com diferentes perfis metabólicos. Imediatamente após coletou-se sangue e cérebro, assim como, o peso da gordura abdominal foi mensurado. Na segunda parte do estudo, após as 5 semanas de dieta, os animais ficaram durante 7 dias no BioDAQ®, um sistema computadorizado de análise do comportamento alimentar, para avaliar o consumo da dieta habitual em ratas com diferentes perfis metabólicos. O consumo foi mensurado através de mordidas (diferença de 0,1 g na balança) e refeições (conjunto de porções por um tempo igual ou menor a 15 min, porções são mordidas ininterruptas). No dia 10 foi realizado o teste de preferência alimentar no qual o animal poderia escolher entre a dieta habitual (dieta que eles receberam por 5 semanas) ou a dieta hipersacarídica (HP) (contendo 34% lipídios, 30,2% carboidratos, 14% proteínas, 20% sacarose), com duração de 20 horas. Após 1 semana, foi coletado sangue, cérebro e mensurada a gordura abdominal. Foi realizado western blotting para tirosina hidroxilase (TH) e fosfo- tirosina hidroxilase (pTH) no núcleo accumbens, STAT3 e fosfo-STAT3 (pSTAT3) no hipotálamo. Adicionalmente, foi mensurado BDNF no soro, no núcleo do trato solitário (NTS), área tegmentar ventral (VTA) e glicemia no soro. Resultados: Nas 5 semanas de tratamento, em relação ao ganho de peso dos animais não houve diferenças significativas entre os grupos, não houve interação, apenas apresentaram efeito do tempo (p< 0,001). A gordura abdominal foi maior nas ratas HF (p= 0,002) e LP (p= 0,023) em relação aos controles. Os animais que receberam dieta HF comeram menos gramas de Froot Loops® do que os animais controle (p= 0,003). Durante a habituação ao BioDAQ® não houve diferença significativa no consumo de dieta entre os grupos. Na análise do comportamento alimentar no BioDAQ®, comparando os grupos controle versus hiperlídica (C x HF), animais HF tiveram o tamanho da refeição (g) (p=0,049), número de porções (p= p< 0,001), tamanho da refeição ciclo escuro (p= 0,002), número de porções ciclo escuro (p < 0,001) menor do que os controles e tamanho da porção ciclo escuro (p=0,006) maior do que os controles. Na análise do comportamento alimentar, comparando os grupos controle versus hipoproteica (C x LP) foram encontradas diferenças significativas nos seguintes parâmetros: média do tamanho da porção (g) (p= 0,004), média do tamanho da porção no ciclo claro (g) (p= 0,042), média do tamanho da refeição no ciclo escuro (g) (p= 0,035), média do tamanho da porção no ciclo escuro (g) (p= 0,006). Em todos os parâmetros os animais LP tiveram uma média maior do que os animais controle. No teste de preferência alimentar, os animais HF apresentaram uma média inferior aos animais controle nos seguintes parâmetros: consumo de dieta hipersacarídica (Kcal) (p= 0,034), número de refeições de dieta hipersacarídica (p= 0,016), número de porções de dieta hipersacarídica (p= 0,001). Os animais HF apresentaram médias superiores aos animais C em relação ao tamanho da porção de dieta hipersacarídica (g) (p= 0,023), PMI (intervalo entre refeições) total de dieta hipersacarídica (p= 0,022), saciedade total de dieta hipersacarídica (p= 0,008). Durante o teste de preferência alimentar comparando-se controle versus hipoproteica (C x LP), os animais (LP) apresentaram o consumo de dieta hipersacarídica (kcal) (p= 0,030) e o número de porções de dieta hipersacarídica (p= 0,003) menor que os animais controles. Os animais LP apresentaram saciedade total de dieta hipersacarídica (p= 0,046) maior do que os controles. Não houve diferenças significativas nos níveis de glicemia no soro entre os grupos. Os animais HF apresentaram as médias de pSTAT3 maior do que os controles (p= 0,013) e fosfo-tirosina hidroxilase menor do que os controles (p= 0,05). Os animais LP apresentaram STAT3 menor do que os animais controle (p= 0,035) e tiveram resultados de BDNF próximos da significância (p=0,053), tendo apresentado uma média inferior aos animais controle. Conclusões: A exposição aos diferentes tipos de dieta muda os padrões de alimentação bem como a estrutura corpórea. Tanto animais expostos a dieta HF quanto a LP apresentam alterações compatíveis com um estado de pré-resistência à leptina. O BDNF parece modular as vias homeostáticas e hedônicas do comportamento alimentar, no entanto mais estudos são necessários para entendermos melhor esses mecanismos. / Introduction: The chronic exposure to different types of diet modifies the hypothalamic and mesolimbic metabolism, what can lead to changes in the individual feeding behavior. BDNF, a neuronal growing factor, can act modulating feeding behavior in hedonic as well as in homeostatic pathways. The aim of this study was to investigate how BDNF acts modulating feeding behavior regarding hedonic and homeostatic pathways in female rats with different metabolic profiles. Materials and methods: Female adult Wistar rats randomized by weight were divided in: control diet (C) with 22% of protein and 4% of lipids; low-protein diet (LP) with 8% of protein or high fat diet (HF) with 45% of lipids, ad libitum, for 5 weeks, with the diet consumption verified every 72 hours and the weight verified weekly. The study was divided in two parts. In the first part, after 5 weeks receiving diet, animals were submitted to 4 hours of fasting and then were exposed to sweet food (Froot Loops®), previously weighted, for 1 hour to verify the palatable food consumption in rats with different metabolic profiles. Immediately after, blood and brain were collected and the abdominal fat weight was verified. In the second part of the study, after 5 weeks receiving diet, the animals were submitted to the BioDAQÒ, a computer system of feeding behavior analyses, to evaluate the habitual diet consumption in rats with different metabolic profiles for 7 days. The consumption was measured through bites (0.1g of difference in the scale) and meals (a group of portions for a period of time less or equal than 15min, portions are uninterrupted bites). On day 10 the food preference test was done and the animals could choose between the habitual diet (the one they have received for 5 weeks) and the high sucrose palatable diet (HP) (with 34% of lipids, 30.2% of carbohydrates, 14% of protein, 20% of sucrose) for a period of 20 hours. After one week, blood and brain were collected and abdominal fat was measured. Western blotting was used to verify the content of tyrosine hydroxylase (TH) and phospho-tyrosine hydroxylase (pTH) in the nucleus accumbens, STAT3 and phospho-STAT3 (pSTAT3) in the hypothalamus. Additionally, BDNF was measured in the serum, in the solitary tract nucleus (NTS) and in the ventral tegmental area (VTA) and glycemia was also verified. Results: Considering the 5 weeks of treatment regarding animals weight gain there was no significant difference between groups and no interaction, only an effect of time (p<0.001). Abdominal fat was higher in HF (p=0.002) and LP (p=0.023) rats comparing to controls. Animals that received HF diet ate less grams of Froot Loopsâ than controls (p=0.003). During the habituation to the BioDAQÒ no significant difference was seen in the consumption of the diet between the groups. When analyzing feeding behavior in the BioDAQÒ, comparing control against high fat groups (C x HF), HF animals had a decrease in the size of the meal (g) (p=0.049), number of portion (p<0.001), meal size in the dark phase (p=0.002), number of portions in the dark phase (p<0.001) compared to controls while the size of the portion in the dark phase (p=0.006) was bigger than controls. Analyzing feeding behavior comparing control against low-protein groups (C x LP) a significant difference was observed in the following parameters: average of the size of the portion (g) (p=0.004), average of the size of the portion in the light phase (g) (p=0.042), average of the size of the meal in the dark phase (g) (p=0.035), average of the size of the portion in the dark phase (g) (p=0.006). LP animals showed a higher average than controls in all parameters. In the food preference test, HF animals showed a lower average than controls in the following parameters: consumption of high sucrose palatable diet (Kcal) (p=0.034), number of meals of high sucrose palatable diet (p=0.016), number of portions of high sucrose palatable diet (p=0.001). HF animals showed higher averages than controls regarding the size of the portion of the high sucrose palatable diet (g) (p=0.023), total PMI (post interval meal) of high sucrose palatable diet (p=0.022) and total satiety of high sucrose palatable diet (p=0.008). In the food preference test comparing controls against low-protein groups (C x LP), LP animals showed a lower consumption of high sucrose palatable diet (Kcal) (p=0.030) and a lower number of portions of high sucrose palatable diet (p=0.003) than control animals. LP animals showed total satiety of high sucrose palatable diet (p=0.046) bigger than controls. There was no significant difference in the glycemia levels between groups. HF animals had pSTAT3 averages higher than controls (p=0.013) and phospho-tyrosine hydroxylase lower than controls (p=0.05). LP animals showed STAT3 lower than control animals (p=0.035) and had BDNF results close to the significance (p=0.053), showing a lower average than control animals. Conclusion: The exposure to different types of diets changes the feeding patterns as well as the body structure. Animals exposed to HF diet as well as those exposed to LP diet showed changes related to a leptin pre-resistant state. BDNF seems to modulate homeostatic and hedonic feeding behavior pathways, however more studies are necessary to a better understanding of the mechanisms. Comportamento alimentar Dieta Dopamina Tirosina hidroxilase Feeding behavior Dopamine Tyrosine hydroxylase BDNF
34	Efeito de diferentes dietas sobre a modulação do comportamento alimentar em vias homeostáticas e hedônicas em ratas fêmeas Laureano, Daniela Pereira January 2013 (has links) Introdução: A exposição crônica a diferentes tipos de dieta altera o metabolismo hipotalâmico e mesolímbico, podendo causar alterações no comportamento alimentar do indivíduo. O BDNF, fator de crescimento neuronal, pode atuar na modulação do comportamento alimentar tanto em vias hedônicas quanto homeostáticas. O objetivo do estudo foi investigar como o BDNF atua na modulação do comportamento alimentar em vias homeostáticas e hedônicas em ratas fêmeas com diferentes perfis metabólicos. Materiais e métodos: Ratas Wistar fêmeas adultas randomizadas por peso foram divididas em: dieta controle (C) contendo 22% de proteína e 4% de lipídios; dieta hipoproteica (LP) 8% de proteína ou dieta hiperlipídica (HF) 45% de lipídios, ad libitum, por 5 semanas, sendo o consumo medido a cada 72 horas e o peso semanalmente. O trabalho foi dividido em duas partes. Na primeira parte, após as 5 semanas de dieta os animais ficaram em jejum por 4 horas e foram expostos ao alimento doce (Froot Loops®), previamente pesado, por 1 hora, a fim de verificar o consumo de alimento palatável em ratas com diferentes perfis metabólicos. Imediatamente após coletou-se sangue e cérebro, assim como, o peso da gordura abdominal foi mensurado. Na segunda parte do estudo, após as 5 semanas de dieta, os animais ficaram durante 7 dias no BioDAQ®, um sistema computadorizado de análise do comportamento alimentar, para avaliar o consumo da dieta habitual em ratas com diferentes perfis metabólicos. O consumo foi mensurado através de mordidas (diferença de 0,1 g na balança) e refeições (conjunto de porções por um tempo igual ou menor a 15 min, porções são mordidas ininterruptas). No dia 10 foi realizado o teste de preferência alimentar no qual o animal poderia escolher entre a dieta habitual (dieta que eles receberam por 5 semanas) ou a dieta hipersacarídica (HP) (contendo 34% lipídios, 30,2% carboidratos, 14% proteínas, 20% sacarose), com duração de 20 horas. Após 1 semana, foi coletado sangue, cérebro e mensurada a gordura abdominal. Foi realizado western blotting para tirosina hidroxilase (TH) e fosfo- tirosina hidroxilase (pTH) no núcleo accumbens, STAT3 e fosfo-STAT3 (pSTAT3) no hipotálamo. Adicionalmente, foi mensurado BDNF no soro, no núcleo do trato solitário (NTS), área tegmentar ventral (VTA) e glicemia no soro. Resultados: Nas 5 semanas de tratamento, em relação ao ganho de peso dos animais não houve diferenças significativas entre os grupos, não houve interação, apenas apresentaram efeito do tempo (p< 0,001). A gordura abdominal foi maior nas ratas HF (p= 0,002) e LP (p= 0,023) em relação aos controles. Os animais que receberam dieta HF comeram menos gramas de Froot Loops® do que os animais controle (p= 0,003). Durante a habituação ao BioDAQ® não houve diferença significativa no consumo de dieta entre os grupos. Na análise do comportamento alimentar no BioDAQ®, comparando os grupos controle versus hiperlídica (C x HF), animais HF tiveram o tamanho da refeição (g) (p=0,049), número de porções (p= p< 0,001), tamanho da refeição ciclo escuro (p= 0,002), número de porções ciclo escuro (p < 0,001) menor do que os controles e tamanho da porção ciclo escuro (p=0,006) maior do que os controles. Na análise do comportamento alimentar, comparando os grupos controle versus hipoproteica (C x LP) foram encontradas diferenças significativas nos seguintes parâmetros: média do tamanho da porção (g) (p= 0,004), média do tamanho da porção no ciclo claro (g) (p= 0,042), média do tamanho da refeição no ciclo escuro (g) (p= 0,035), média do tamanho da porção no ciclo escuro (g) (p= 0,006). Em todos os parâmetros os animais LP tiveram uma média maior do que os animais controle. No teste de preferência alimentar, os animais HF apresentaram uma média inferior aos animais controle nos seguintes parâmetros: consumo de dieta hipersacarídica (Kcal) (p= 0,034), número de refeições de dieta hipersacarídica (p= 0,016), número de porções de dieta hipersacarídica (p= 0,001). Os animais HF apresentaram médias superiores aos animais C em relação ao tamanho da porção de dieta hipersacarídica (g) (p= 0,023), PMI (intervalo entre refeições) total de dieta hipersacarídica (p= 0,022), saciedade total de dieta hipersacarídica (p= 0,008). Durante o teste de preferência alimentar comparando-se controle versus hipoproteica (C x LP), os animais (LP) apresentaram o consumo de dieta hipersacarídica (kcal) (p= 0,030) e o número de porções de dieta hipersacarídica (p= 0,003) menor que os animais controles. Os animais LP apresentaram saciedade total de dieta hipersacarídica (p= 0,046) maior do que os controles. Não houve diferenças significativas nos níveis de glicemia no soro entre os grupos. Os animais HF apresentaram as médias de pSTAT3 maior do que os controles (p= 0,013) e fosfo-tirosina hidroxilase menor do que os controles (p= 0,05). Os animais LP apresentaram STAT3 menor do que os animais controle (p= 0,035) e tiveram resultados de BDNF próximos da significância (p=0,053), tendo apresentado uma média inferior aos animais controle. Conclusões: A exposição aos diferentes tipos de dieta muda os padrões de alimentação bem como a estrutura corpórea. Tanto animais expostos a dieta HF quanto a LP apresentam alterações compatíveis com um estado de pré-resistência à leptina. O BDNF parece modular as vias homeostáticas e hedônicas do comportamento alimentar, no entanto mais estudos são necessários para entendermos melhor esses mecanismos. / Introduction: The chronic exposure to different types of diet modifies the hypothalamic and mesolimbic metabolism, what can lead to changes in the individual feeding behavior. BDNF, a neuronal growing factor, can act modulating feeding behavior in hedonic as well as in homeostatic pathways. The aim of this study was to investigate how BDNF acts modulating feeding behavior regarding hedonic and homeostatic pathways in female rats with different metabolic profiles. Materials and methods: Female adult Wistar rats randomized by weight were divided in: control diet (C) with 22% of protein and 4% of lipids; low-protein diet (LP) with 8% of protein or high fat diet (HF) with 45% of lipids, ad libitum, for 5 weeks, with the diet consumption verified every 72 hours and the weight verified weekly. The study was divided in two parts. In the first part, after 5 weeks receiving diet, animals were submitted to 4 hours of fasting and then were exposed to sweet food (Froot Loops®), previously weighted, for 1 hour to verify the palatable food consumption in rats with different metabolic profiles. Immediately after, blood and brain were collected and the abdominal fat weight was verified. In the second part of the study, after 5 weeks receiving diet, the animals were submitted to the BioDAQÒ, a computer system of feeding behavior analyses, to evaluate the habitual diet consumption in rats with different metabolic profiles for 7 days. The consumption was measured through bites (0.1g of difference in the scale) and meals (a group of portions for a period of time less or equal than 15min, portions are uninterrupted bites). On day 10 the food preference test was done and the animals could choose between the habitual diet (the one they have received for 5 weeks) and the high sucrose palatable diet (HP) (with 34% of lipids, 30.2% of carbohydrates, 14% of protein, 20% of sucrose) for a period of 20 hours. After one week, blood and brain were collected and abdominal fat was measured. Western blotting was used to verify the content of tyrosine hydroxylase (TH) and phospho-tyrosine hydroxylase (pTH) in the nucleus accumbens, STAT3 and phospho-STAT3 (pSTAT3) in the hypothalamus. Additionally, BDNF was measured in the serum, in the solitary tract nucleus (NTS) and in the ventral tegmental area (VTA) and glycemia was also verified. Results: Considering the 5 weeks of treatment regarding animals weight gain there was no significant difference between groups and no interaction, only an effect of time (p<0.001). Abdominal fat was higher in HF (p=0.002) and LP (p=0.023) rats comparing to controls. Animals that received HF diet ate less grams of Froot Loopsâ than controls (p=0.003). During the habituation to the BioDAQÒ no significant difference was seen in the consumption of the diet between the groups. When analyzing feeding behavior in the BioDAQÒ, comparing control against high fat groups (C x HF), HF animals had a decrease in the size of the meal (g) (p=0.049), number of portion (p<0.001), meal size in the dark phase (p=0.002), number of portions in the dark phase (p<0.001) compared to controls while the size of the portion in the dark phase (p=0.006) was bigger than controls. Analyzing feeding behavior comparing control against low-protein groups (C x LP) a significant difference was observed in the following parameters: average of the size of the portion (g) (p=0.004), average of the size of the portion in the light phase (g) (p=0.042), average of the size of the meal in the dark phase (g) (p=0.035), average of the size of the portion in the dark phase (g) (p=0.006). LP animals showed a higher average than controls in all parameters. In the food preference test, HF animals showed a lower average than controls in the following parameters: consumption of high sucrose palatable diet (Kcal) (p=0.034), number of meals of high sucrose palatable diet (p=0.016), number of portions of high sucrose palatable diet (p=0.001). HF animals showed higher averages than controls regarding the size of the portion of the high sucrose palatable diet (g) (p=0.023), total PMI (post interval meal) of high sucrose palatable diet (p=0.022) and total satiety of high sucrose palatable diet (p=0.008). In the food preference test comparing controls against low-protein groups (C x LP), LP animals showed a lower consumption of high sucrose palatable diet (Kcal) (p=0.030) and a lower number of portions of high sucrose palatable diet (p=0.003) than control animals. LP animals showed total satiety of high sucrose palatable diet (p=0.046) bigger than controls. There was no significant difference in the glycemia levels between groups. HF animals had pSTAT3 averages higher than controls (p=0.013) and phospho-tyrosine hydroxylase lower than controls (p=0.05). LP animals showed STAT3 lower than control animals (p=0.035) and had BDNF results close to the significance (p=0.053), showing a lower average than control animals. Conclusion: The exposure to different types of diets changes the feeding patterns as well as the body structure. Animals exposed to HF diet as well as those exposed to LP diet showed changes related to a leptin pre-resistant state. BDNF seems to modulate homeostatic and hedonic feeding behavior pathways, however more studies are necessary to a better understanding of the mechanisms. Comportamento alimentar Dieta Dopamina Tirosina hidroxilase Feeding behavior Dopamine Tyrosine hydroxylase BDNF
35	Zebrafish as a Model for the Study of Parkinson’s Disease Xi, Yanwei January 2011 (has links) Parkinson’s disease (PD) is a common neurodegenerative disorder that is characterized by the degeneration of dopaminergic (DA) neurons in the substantia nigra and motor deficits. Although the majority of PD cases are sporadic, several genetic defects in rare familial cases have been identified. Animal models of these genetic defects have been created and have provided unique insights into the molecular mechanisms of the pathogenesis of PD. However, the etiology of PD is still not well understood. Here, taking advantage of the unique features offered by zebrafish, I characterized the functions of PINK1 (PTEN-induced kinase 1) gene, which is associated with recessive familial PD, in the development and survival of DA neurons. In zebrafish, antisense morpholino knockdown of pink1 did not cause a large loss of DA neurons in the ventral diencephalon (vDC), but the patterning of these neurons and their projections were perturbed. The pink1 morphants also showed impaired response to touch stimuli and reduced swimming behaviour. Moreover, the pink1 knockdown caused a significant reduction in the number of mitochondria, as well as mitochondrial morphological defects such as smaller size or loss of cristae, thus affecting mitochondrial function. These results suggest that zebrafish pink1 plays conserved important roles in the development of DA neurons and in the mitochondrial morphology and function. To better follow DA neurons after injury or administration of toxins, I generated a transgenic zebrafish line, Tg(dat:EGFP), in which the green fluorescent protein (GFP) is expressed under the control of cis-regulatory elements of dopamine transporter (dat). In Tg(dat:EGFP) fish, all major groups of DA neurons are correctly labeled with GFP, especially the ones in the vDC, which are analogous to the ascending midbrain DA neurons in mammals. In addition, we observed that the DA neurons in the vDC could partially be replaced after severe laser cell ablation. This suggests that zebrafish may have the unique capacity of regenerating DA neurons after injury. Taken together, my studies suggested that zebrafish could be a useful alternative animal model for the study of the molecular mechanisms underlying PD and for the screening of potential therapeutic compounds for PD. Zebrafish Parkinson's disease PINK1 dopaminergic neuron dopamine transporter morpholino tyrosine hydroxylase MPTP regeneration
36	Covalent modification and inhibition of tyrosine hydroxylase by 3,4-dihydroxyphenylacetaldehyde, an endogenously produced neurotoxin relevant to Parkinson's disease Vermeer, Lydia Maria Mexas 01 July 2012 (has links) Parkinson's disease (PD) is a prevalent neurodegenerative disorder which affects over a million people in the United States. This disease is marked by the selective loss of dopaminergic neurons in the substantia nigra, leading to a decrease in the important neurotransmitter dopamine (DA), which is essential for the initiation and execution of coordinated movement. Currently, the pathogenesis behind PD is unknown, but there is evidence that both exogenous causes, such as pesticides and metals, as well as endogenous causes, such as reactive oxygen species or reactive metabolism intermediates, may play a role in the onset and progression of the disease. DA is catabolized by monoamine oxidase to 3,4-dihydroxyphenylacetaldehyde (DOPAL), which is further metabolized by aldehyde dehydrogenase and aldehyde reductase to the acid and alcohol products, respectively. Studies have demonstrated the reactivity of DOPAL with peptides and proteins, leading to covalent modification which may be detrimental to protein action. Furthermore, studies have shown that DOPAL is toxic, leading to a decrease in cell viability. Due to this, it was of interest to further study DOPAL and how it may play a role in the onset and progression of PD. It was of particular interest to determine protein targets of DOPAL modification. Until recently, no protein targets were identified and the cellular consequence of elevated DOPAL had not been fully studied. It has been previously shown that the important enzyme, tyrosine hydroxylase (TH) is inhibited by other catechols, including DA. This enzyme catalyzes the rate-limiting step in DA synthesis, oxidizing tyrosine to L-DOPA which is further metabolized to DA. Therefore, it was of interest to determine the effect of DOPAL on TH activity. It was hypothesized that DOPAL modifies and inhibits TH, leading to a decrease in the production of L-DOPA and DA. This work employed the use of a dopaminergic cell model (PC6-3 cells), to positively identify TH as a protein target of DOPAL modification. It also used both cell lysate as well as PC6-3 cell studies to investigate the effect of DOPAL modification on TH activity. Mass spectrometry was also utilized to determine sites of protein modification on TH. Results show that TH is potently inhibited by DOPAL modification, leading to a significant decrease in both L-DOPA and DA. Furthermore, DOPAL inhibition appears to be slowly-irreversible, with enzyme activity showing a time- and concentration dependent in recovery after preincubation with DOPAL. A novel cloning and purification procedure was used to clone human recombinant TH, which was used in mass spectrometry studies in which five sites of DOPAL modification were discovered. Furthermore, a real-time assay for TH activity was developed using a plate reader to spectrophotometrically observe the formation of L-DOPA over time. These data demonstrate the toxicity and potent enzyme inhibition by DOPAL and implicate DOPAL as a neurotoxin relevant in the pathogenesis of PD. Cellular toxicity DOPAL Enzyme inhibition Oxidative Stress Parkinson's disease Tyrosine hydroxylase Pharmacy and Pharmaceutical Sciences
37	The Catecholaminergic RCSN-3 Cell Line: A Model to Study Dopamine Metabolism Paris, Irmgard, Lozano, Jorge, Cardenas, Sergio, Perez-Pastene, Carolina, Saud, Katherine, Fuentes, Patricio, Caviedes, Pablo, Dagnino-Ubiabre, Alexie, Raisman-Vozari, Rita, Shimahara, Takeshi, Kostrzewa, John P., Chi, David, Kostrzewa, Richard M., Caviedes, Raúl, Segura-Aguilar, Juan 01 September 2008 (has links) RCSN-3 cells are a cloned cell line derived from the substantia nigra of an adult rat. The cell line grows in monolayer and does not require differentiation to express catecholaminergic traits, such as (i) tyrosine hydroxylase; (ii) dopamine release; (iii) dopamine transport; (iv) norepinephrine transport; (v) monoamine oxidase (MAO)-A expression, but not MAO-B; (vi) formation of neuromelanin; (vii) vesicular monoamine transporter-2 (VMAT-2) expression. In addition, this cell line expresses serotonin transporters, divalent metal transporter, DMT1, dopamine receptor 1 mRNA under proliferating conditions, and dopamine receptor 5 mRNA after incubation with dopamine or dicoumarol. Expression of dopamine receptors D2, D3 and D4 mRNA were not detected in proliferating cells or when the cells were treated with dopamine, CuSO4, dicoumarol or dopamine-copper complex. Angiotensin II receptor mRNA was also found to be expressed, but it underwent down regulation in the presence of aminochrome. Total quinone reductase activity corresponded 94% to DT-diaphorase. The cells also express antioxidant enzymes such as superoxide dismutase, catalase and glutathione peroxidase. This cell line is a suitable in vitro model for studies of dopamine metabolism, since under proliferating conditions the cells express all the pertinent markers. cell dopamine neuromelanin PC12 SH-SY5Y tyrosine hydroxylase VMAT-2 Biomedical Sciences
38	KISS-1 Expression and Metastin-Like Immunoreactivity in the Rat Brain Brailoiu, G. Cristina, Dun, Siok L., Ohsawa, Masahiro, Yin, Deling, Yang, Jun, Jaw, Kang Chang, Brailoiu, Eugen, Dun, Nae J. 17 January 2005 (has links) Metastin, the gene product of metastasis suppressor gene KiSS-1, is the endogenous ligand for the G-protein-coupled receptor GPR54 (or AXOR12, or OT7T175). The expression of KiSS-1 gene and peptide and the distribution of metastin were studied in the rat central nervous system by reverse transcriptase-polymerase chain reaction, Western blotting, and immunohistochemical methods. KiSS-1 gene and peptide expression was higher in the hypothalamus than in the brainstem and spinal cord. In the brain, metastin-like immunoreactivity (irMT) was found mainly in three groups of cells: dorsomedial hypothalamic nucleus, nucleus of the solitary tract, and caudal ventrolateral medulla. Immunoreactive fibers of varying density were noted in bed nucleus of stria terminalis, septal nuclei, nucleus accumbens, caudate putamen, diagonal band, amygdala, hypothalamus, zona incerta, thalamus, periaqueductal gray, raphe nuclei, lateral parabrachial nucleus, locus coeruleus, spinal trigeminal tract, rostral ventrolateral medulla, and medullary reticular nucleus. Preabsorption of the antiserum with metastin peptide fragment (45-54)-NH2 (1 μg/ml) resulted in no staining in any of the sections. The biological activity of metastin was assessed by monitoring intracellular calcium [Ca2+]i in cultured hippocampal neurons, which are known to express GPR54. Metastin increased [Ca 2+]i in a population of cultured hippocampal neurons. The results show that metastin is biologically active in rat central neurons, and its anatomical distribution suggests a possible role in nociception and autonomic and neuroendocrine functions. caudoventrolateral reticular nucleus dorsal horn hypothalamus nucleus of the solitary tract tyrosine hydroxylase
39	Cocaine- and Amphetamine-Regulated Transcript Peptide-Immunoreactivity in Adrenergic C1 Neurons Projecting to the Intermediolateral Cell Column of the Rat Dun, Siok L., Ng, Yee Kong, Brailoiu, G. Cristina, Ling, Eng Ang, Dun, Nae J. 28 February 2002 (has links) Cocaine- and amphetamine-regulated transcript (CART) peptide-immunoreactivity was detected in neurons of the rostral ventrolateral medulla (RVLM), but few in the caudal ventrolateral medulla (CVLM). Double-labeling the medullary sections with sheep polyclonal phenylethanolamine N-methyltransferase-antiserum (PNMT) or monoclonal tyrosine hydroxylase-antibody and rabbit polyclonal CART peptide-antiserum revealed that nearly all adrenergic cells in the C1 area were CART peptide-positive and vice versa; tyrosine hydroxylase-positive cells in the A1 area were not. In the thoracolumbar spinal cord, neurons in the intermediolateral cell column (IML) and other sympathetic autonomic nuclei were CART peptide-positive; some of these were contacted by immunoreactive fibers arising from the lateral funiculus. By immuno-electron microscopy, axon terminals containing closely packed agranular CART peptide-immunoreactive vesicles appeared to make synaptic contacts with immunoreactive dendrites and soma in the IML, albeit the incidence of such contacts was low. Microinjection of the retrograde tracer Fluorogold into the lateral horn area of the T1-T3 spinal segments labeled a population of neurons in the C1 area, many of which were also CART peptide-positive. The results indicate that CART peptide-immunoreactivity is expressed in C1 adrenergic neurons, some of which project to the thoracolumbar spinal cord. The presence of this novel peptide in C1 adrenergic neurons underscores the multiplicity of putative transmitters that may be involved in signaling between putative cardiovascular neurons in the medulla oblongata and sympathetic preganglionic neurons (SPNs) in the spinal cord. caudal ventrolateral medulla phenylethanolamine-n-methyltransferase prolactin-releasing peptide spinal cord sympathetic preganglionic neurons tyrosine hydroxylase
40	Transcription Factors Phox2a/2b Upregulate Expression of Noradrenergic and Dopaminergic Phenotypes in Aged Rat Brains Fan, Yan, Zeng, Fei, Brown, Russell W., Price, Jennifer B., Jones, Thomas C., Zhu, Meng Yang 01 October 2020 (has links) The present study investigated the effects of forced overexpression of Phox2a/2b, two transcription factors, in the locus coeruleus (LC) of aged rats on noradrenergic and dopaminergic phenotypes in brains. Results showed that a significant increase in Phox2a/2b mRNA levels in the LC region was paralleled by marked enhancement in expression of DBH and TH per se. Furthermore, similar increases in TH protein levels were observed in the substantial nigra and striatum, as well as in the hippocampus and frontal cortex. Overexpression of Phox2 genes also significantly increased BrdU-positive cells in the hippocampal dentate gyrus and NE levels in the striatum. Moreover, this manipulation significantly improved the cognition behavior. The in vitro experiments revealed that norepinephrine treatments may increase the transcription of TH gene through the epigenetic action on the TH promoter. The results indicate that Phox2 genes may play an important role in improving the function of the noradrenergic and dopaminergic neurons in aged animals, and regulation of Phox2 gene expression may have therapeutic utility in aging or disorders involving degeneration of noradrenergic neurons. dopamine dopamine-β-hydroxylase locus coeruleus Morris water maze neurogenesis tyrosine hydroxylase Biological Sciences Biomedical Sciences

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