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Characterization of heavy metal tolerant bacterial plasmids isolated from a platinum mine tailings dam / by Tladi Abram Mahlatsi.Mahlatsi, Tladi Abram January 2012 (has links)
The development of metal-tolerance and antibiotic resistance in bacteria may be caused by metals polluting a particular environment. During mining and mineral processing activities, large quantities of metals are deposited into the soil. These high concentrations of metals are evolutionary pressures selecting for microorganisms tolerant to these metals. Metaltolerance maybe conferred to these organisms by mobile genetic elements such as plasmids. This study describes the characteristics of plasmids isolated from various bacteria that displayed an ability to withstand high metal concentrations. The isolated plasmids were individually transformed into Escherichia coli JM109. Transformants were then evaluated for metal-tolerant capabilities using a microdilution approach. Plasmids were then isolated from the transformants and the concentration of the plasmid DNA ranged between 11.75 – 118.06 ng/μl. These plasmids were of the same size as the original ones. This demonstrated that successful transformations with plasmid DNA were conducted. In order to determine the compatibility group, plasmids were subjected to PCR amplification using IncQ, IncP-9 and IncW specific primers. Only the IncW provided positive results. To demonstrate that the plasmids were free of genomic DNA, a 16S rDNA PCR test was included. The plasmids that were positive for IncW PCRs were all negative for the rDNA PCRs. Plasmids were stably inherited and at least three, isolated from three different Gram positive species, belonged to the Inc W group of plasmids. These were originally isolated from Paenibacillus ginsingari, Paenibacillus lautus and Bacillus cereus. Minimum inhibition concentrations (MICs) were carried out to determine the ability of transformed E. coli JM109 to tolerate metals at varying concentrations. Results indicated that transformed E. coli JM109 developed ability to grow in the presence of several heavy metals. Some strains were resistant to high concentrations (+10 mM) of Ni2+/Al3+, Pb2+ and Ba2+. The order of metal resistance was Ni/Al=Pb>Ba>Mn>Cr>Cu>Co=Hg. All the x transformants were sensitive to 1 mM of Co2+ and Hg2+. Moreover, protein profiling was used to determine the impact of plasmids on E. coli JM109. Proteins were extracted from both transformed and un-transformed E. coli JM109 using acetone-SDS protocol and subjected to one-dimensional (1D) and two-dimensional (2D) Sodium Dodecyl Sulphate Polyacrylamide Gel Electrophoresis (SDS- PAGE). Transformed E. coli JM109 were grown under the metal stress. One dimension SDS-PAGE illustrated general similarity of the profiles except for two banding positions in the 30 to 35 kDa region where bands were present in the transformants that were grown in the Ni/Al alloy containing media. Twodimensional electrophoresis PAGE analysis showed that some of the proteins were upregulated while others were down-regulated. The largest numbers of proteins were from 15 – 75 kDa. The majority of these proteins had isoelectric points (pI) between 5 and 6. It was concluded that plasmids isolated from various heavy metal-tolerant bacterial species were successfully transformed into E. coli JM109 rendering various new metal-tolerant E. coli JM109 strains. Furthermore, the study showed that metal resistance was due to the presence of the plasmids. Two-dimensional SDS-PAGE resolved more differences in the protein expression profiles. Since the plasmids rendered the E. coli JM109 tolerant to metals tested, it also can be concluded that the change in the protein profiles was due to the effects of the plasmids. Furthermore, plasmids were also re-isolated from the transformants and these plasmids were of the same size as the original ones.. All the plasmids in this study were also stably inherited, a feature associated with IncW plasmids. More detailed genetic characterization of these plasmids is required. Plasmids isolated and characterized in this study may hold biotechnology potential. Such features should be exploited in follow-up experiments. / Thesis (Master of Environmental Sciences)--North-West University, Potchefstroom Campus, 2013.
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Characterization of heavy metal tolerant bacterial plasmids isolated from a platinum mine tailings dam / by Tladi Abram Mahlatsi.Mahlatsi, Tladi Abram January 2012 (has links)
The development of metal-tolerance and antibiotic resistance in bacteria may be caused by metals polluting a particular environment. During mining and mineral processing activities, large quantities of metals are deposited into the soil. These high concentrations of metals are evolutionary pressures selecting for microorganisms tolerant to these metals. Metaltolerance maybe conferred to these organisms by mobile genetic elements such as plasmids. This study describes the characteristics of plasmids isolated from various bacteria that displayed an ability to withstand high metal concentrations. The isolated plasmids were individually transformed into Escherichia coli JM109. Transformants were then evaluated for metal-tolerant capabilities using a microdilution approach. Plasmids were then isolated from the transformants and the concentration of the plasmid DNA ranged between 11.75 – 118.06 ng/μl. These plasmids were of the same size as the original ones. This demonstrated that successful transformations with plasmid DNA were conducted. In order to determine the compatibility group, plasmids were subjected to PCR amplification using IncQ, IncP-9 and IncW specific primers. Only the IncW provided positive results. To demonstrate that the plasmids were free of genomic DNA, a 16S rDNA PCR test was included. The plasmids that were positive for IncW PCRs were all negative for the rDNA PCRs. Plasmids were stably inherited and at least three, isolated from three different Gram positive species, belonged to the Inc W group of plasmids. These were originally isolated from Paenibacillus ginsingari, Paenibacillus lautus and Bacillus cereus. Minimum inhibition concentrations (MICs) were carried out to determine the ability of transformed E. coli JM109 to tolerate metals at varying concentrations. Results indicated that transformed E. coli JM109 developed ability to grow in the presence of several heavy metals. Some strains were resistant to high concentrations (+10 mM) of Ni2+/Al3+, Pb2+ and Ba2+. The order of metal resistance was Ni/Al=Pb>Ba>Mn>Cr>Cu>Co=Hg. All the x transformants were sensitive to 1 mM of Co2+ and Hg2+. Moreover, protein profiling was used to determine the impact of plasmids on E. coli JM109. Proteins were extracted from both transformed and un-transformed E. coli JM109 using acetone-SDS protocol and subjected to one-dimensional (1D) and two-dimensional (2D) Sodium Dodecyl Sulphate Polyacrylamide Gel Electrophoresis (SDS- PAGE). Transformed E. coli JM109 were grown under the metal stress. One dimension SDS-PAGE illustrated general similarity of the profiles except for two banding positions in the 30 to 35 kDa region where bands were present in the transformants that were grown in the Ni/Al alloy containing media. Twodimensional electrophoresis PAGE analysis showed that some of the proteins were upregulated while others were down-regulated. The largest numbers of proteins were from 15 – 75 kDa. The majority of these proteins had isoelectric points (pI) between 5 and 6. It was concluded that plasmids isolated from various heavy metal-tolerant bacterial species were successfully transformed into E. coli JM109 rendering various new metal-tolerant E. coli JM109 strains. Furthermore, the study showed that metal resistance was due to the presence of the plasmids. Two-dimensional SDS-PAGE resolved more differences in the protein expression profiles. Since the plasmids rendered the E. coli JM109 tolerant to metals tested, it also can be concluded that the change in the protein profiles was due to the effects of the plasmids. Furthermore, plasmids were also re-isolated from the transformants and these plasmids were of the same size as the original ones.. All the plasmids in this study were also stably inherited, a feature associated with IncW plasmids. More detailed genetic characterization of these plasmids is required. Plasmids isolated and characterized in this study may hold biotechnology potential. Such features should be exploited in follow-up experiments. / Thesis (Master of Environmental Sciences)--North-West University, Potchefstroom Campus, 2013.
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Molecular studies of the response of Helicobacter hepaticus to bile, and the effect of Helicobacter bilis on human hepatoma cellsOkoli, Arinze Stanley, Medical Sciences, Faculty of Medicine, UNSW January 2009 (has links)
Enterohepatic Helicobacter species (EHS) are emerging infectious disease agents. Infection of the enterohepatobiliary tract of several mammals by this group of bacteria results in various pathological disorders. The availability of the Helicobacter hepaticus sequenced and annotated genome, allowed molecular characterisation of the responses of H. hepaticus to host factors such as bile. The adaptation/responses of the bacterium to bovine, porcine and human bile were investigated using proteomics and transcriptomics. Ninety-one different proteins were identified in the responses of H. hepaticus response to the three types of bile. These proteins participate in several key cellular processes including DNA replication; protein transcription, translation and folding; oxidative stress response; motility; virulence; and metabolism. In particular, the bacteria deployed several strategies such as inhibition of the TCA cycle and the electron transport chain as well as iron sequestration to ensure control of the levels of hydroxyl radicals. The results of this study revealed also the modulation by bile of the expression of H. hepaticus genes involved in response to oxidative stress and virulence. The responses of human HEp-2 and Huh7-derived cell-lines to H. hepaticus and Helicobacter bilis, respectively, were investigated employing proteomics and transcriptomics. One-hundred and twenty different proteins were differentially expressed in the responses of the human cells to the presence of Helicobacter spp. in the cell cultures. These proteins are involved in regulation of cell proliferation and structure; metabolism; protein transcription, translation and modification; stress response; and tumour induction. For example, in co-cultures of Huh7-derived cells and H. bilis, the activation of several mitochondrial and endoplasmic reticulum stress-related proteins and the dysregulation of several apoptosis effectors were suggested as mechanisms that could result in the death of the liver cells. Importantly, the differential expression of several tumour-related proteins by the Huh7 cells supported a possible role for Helicobacter spp. in liver cancer.
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Estudo de biomarcadores de mercúrio em peixes da amazônia por meio da metalômica e análise do estresse oxidativoBittarello, Alis Correia January 2017 (has links)
Orientador: Pedro de Magalhães Padilha / Resumo: O mercúrio é um metal tóxico, de distribuição ubíqua, com capacidade para bioacumulação e biomagnificação, que provoca alterações em biomoléculas importantes no metabolismo e contribui para o estabelecimento do estresse oxidativo em organismos aquáticos. Logo, o presente estudo teve por objetivo identificar e avaliar possíveis biomarcadores proteicos e/ou enzimáticos da toxicidade do mercúrio em peixes da região amazônica, por meio do estudo metaloproteômico e avaliação do estresse oxidativo. Foram utilizadas metodologias de fracionamento e identificação de proteínas por eletroforese bidimensional (2D PAGE) associada à espectrometria de massas (MS), mapeamento do mercúrio, em spots proteicos, por espectrometria de absorção atômica em forno de grafite (GFAAS) e avaliação de marcadores de estresse oxidativo. As espécies utilizadas foram o Plagioscion squamosissimus (corvina) e Colossoma macropomum (tambaqui), coletados na área da Usina Hidrelétrica de Jirau (rio Madeira-RO), que foram selecionadas em função da abundância populacional, interesse para a pesca e posição diferente na cadeia trófica (carnívoro e onívoro, respectivamente). Os tecidos amostrados foram o hepático, renal e muscular. Os resultados obtidos demonstraram maior concentração de mercúrio total no P. squamosissimus, espécie carnívora, e padrão de distribuição deste elemento igual para ambas as espécies (fígado>rim>músculo). Há tendência para maior atividade enzimática nos tecidos hepático e renal da espécie com... (Resumo completo, clicar acesso eletrônico abaixo) / Doutor
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Sledování exprese proteinů v savčích buňkách infikovaných virem klíšťové encefalitidyKOČOVÁ, Pavlína January 2017 (has links)
This study is focused on changes in protein expression in a glioblastoma cell line during infection with tick-borne encephalitis virus. Newly synthesized proteins were distinguished from previously synthesized proteins using bioorthogonal chemistry (BONCAT method) to observe changes in protein synthesis. Labelled proteins were visualized using two-dimensional PAGE and western blotting followed by Click reaction on membrane. Differences in protein pattern between control and infected cells were observed.
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Caracterização, quantificação e expressão de proteínas estruturais e regulatórias do tecido muscular esquelético e suas relações com as características de qualidade da carne de bovinos Nelore (Bos indicus) / Characterization, quantification and expression of structural and regulatory proteins of skeletal muscle tissue and its relationship with meat quality traits in Nellore cattle (Bos indicus)Malheiros, Jessica Moraes 02 March 2018 (has links)
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Previous issue date: 2018-03-02 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES) / Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP) / O presente trabalho teve como objetivo avaliar a associação da expressão gênica e proteômica com a maciez da carne de bovinos da raça Nelore. A partir de uma população de 90 animais foram selecionados três grupos experimentais por meio da análise de força de cisalhamento (FC) e índice de fragmentação miofibrilar (MFI), sendo: carne moderadamente macia, carne moderadamente dura e carne muito dura. A expressão dos genes foi avaliada por meio da análise de PCR em tempo real e a análise proteômica foi realizada com base na separação de proteínas por meio da eletroforese bidimensional (2D-PAGE) e caracterizção por espectrometria de massas com ionização eletrospray (ESI-MS/MS). A expressão da isoforma da calpastatina (CAST2) mostrou-se up regulated (P<0,05) nos grupos de carne moderadamente dura e muito dura. Os genes HSP90AA1, DNAJA1 e HSPB1, os quais representam as proteínas de choque térmico Hsp90, Hsp40 e Hsp27, respectivamente, mostraram expressão down regulated (P<0,05) no grupo de carne moderadamente macia em relação ao grupo de carne muito dura. Na análise proteômica, a expressão do spot protéico das enzimas metabólicas TPI e PGM1, proteína estrutural PFN1 e aminiopeptidase LAP3 se mostraram up regulated (P<0,05) no grupo de carne moderadamente macia, enquanto que a expressão das proteínas estruturais (ACTA1, ACTB, ACTG1 e MLC1), estresse oxidativo (PRDX6, PRDX2, PRDX1 and PARK7), proteínas de choque térmico (HSP90AA1, HSP90AB1, HSPA1A, HSPA1B, HSPA1L, HSPD1 e HSPB1), e co-chaperonas e regulação celular (CD37, STIP1 e ARHGDIA) se mostraram down regulated (P>0,05) no mesmo grupo experimental. Estes resultados fornecem uma visão importante de novos possíveis marcadores biológicos atuantes no processo de amaciamento da carne, o que pode colaborar para melhor entender e gerar novas estratégias de seleção nos programas de melhoramento genético de bovinos Nelore. / The objective of this study was to evaluate the association of gene expression and proteomics with meat tenderness in Nellore cattle. From population of 90 animals three experimental groups were selected by shear force (SF) and/or myofibrillar fragmentation index (MFI): moderately tender meat, moderately tough meat and very tough meat. Gene expression was evaluated by real-time PCR and proteomics analysis was performed based on protein separation by two-dimensional gel electrophoresis (2D-PAGE) and characterisation by eletrospray ionisation mass spectrometry (ESI-MS/MS). Expression of the calpastatin isoform (CAST2) was up-regulated (P<0.05) in the moderately tough and very tough meat groups. Expression of the HSP90AA1, DNAJA1 and HSPB1 genes, wich represent the heat shock proteins Hsp90, Hsp40 and Hsp27, respectively, were down-regulated (P<0.05) in the moderately tender meat in relation to the very tough group. In the proteomics analysis, the expression of the protein spots of metabolism TPI1 and PGM1, structural protein PFN1, and aminopeptidase LAP3 were up regulated (P<0.05) in the moderately tender meat, while the expression of structural proteins (ACTA1, ACTB, ACTG1 and MLC1), oxidative stress (PRDX6, PRDX2, PRDX1 and PARK7), heat shock protein (HSP90AA1, HSP90AB1, HSPA1A, HSPA1B, HSPA1L, HSPD1 and HSPB1) and co-chaperones and cellular regulatory (CD37, STIP1 and ARHGDIA) were down regulated (P>0.05) in the same experimental group. The present results suggest an important view of possible new biological markers in the meat tenderization process, wich permit to unsderstand and generate new strategies for selection in Nellore cattle breeding programs. / FAPESP: 15/13021-1
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Indução da ovulação com hcg e acetato de deslorelina altera o perfil proteico do líquido folicular de éguasSantos, Gabriel de Oliveira January 2014 (has links)
O líquido folicular é o microambiente do oócito durante sua maturação in vivo que é, em parte constituído por exsudato do soro sanguíneo e por substâncias produzidas localmente, que estão relacionados com a atividade metabólica das células ovarianas. Tais substâncias podem ser essenciais para a proliferação e diferenciação das células somáticas bem como na maturação e posterior fertilização de um oócito competente. A busca por biomarcadores capazes de predizer a saúde de um folículo ou a capacidade do oócito em se tornar um embrião saudável é objeto de estudo na medicina reprodutiva humana e veterinária. Para tanto é essencial o conhecimento a nível molecular dos constituintes do liquido folicular e suas funções. O objetivo do presente estudo foi avaliar o perfil proteico do líquido folicular de éguas submetidas à indução de ovulação, com dois diferentes protocolos usuais na prática clínica, utilizando eletroforese bidimensional em gel de poliacrilamida. Para tanto 19 amostras de liquido folicular de éguas que tiveram sua ovulação induzida por dois diferentes protocolos (1000UI hCG IV, Grupo H, ou 1000UI hCG IV + 1,5mg de acetato de deslorelina IM, Grupo H + G) foram submetidos a eletroforese 2D e posterior análise dos géis no PDQuest. Os valores de proteína total foram significativamente diferente nos Grupo H e Grupo H+G, 63,97 ± 6,97 e 73,07 ± 6,42, respectivamente. O número máximo de spots em um mesmo gel foi de 157 e o mínimo de 34, com média de 90 spots para o Grupo H e 83 spots para o Grupo H+G. Os 19 géis foram avaliados e a porcentagem máxima de spots relacionados foi de 52% e a mínima de 0%. Com média de 37,8% de similaridade entre spots para o Grupo H e 22% para o Grupo H+G. Estes resultados são de grande importância devido à escassez de trabalhos com proteômica de liquido folicular de éguas induzidas a ovulação e demonstram que a associação entre hCG e acetato de deslorelina aumenta a concentração de proteínas no líquido folicular em folículos pré-ovulatórios (>35 mm). / Follicular fluid is the oocyte microenvironment during its in vivo maturation. It is partly composed by blood serum exudate, and also by locally produced substances, related to ovarian cells metabolic activity. These substances may be essential for somatic cells proliferation and differentiation, as well as on the oocyte maturation and fertilization. The search for biomarkers able to predict oocyte ability to grow into a healthy embryo are targets on human and veterinary reproductive medicine. It is essential to know the components of follicular fluid and their functions. The aim of the present study was to evaluate protein profile of the follicular fluid in mares with inducted ovulation, in two different protocols, using 2D electrophoresis in polyacrylamide gel. 19 follicular fluid samples from mares in which ovulation induction was performed with two different protocols (1000UI hCG IV or 1000UI hCG IV + 1,5mg deslorelin acetate IM), submitted to 2D electrophoresis, and gel analysis on PDQuest. Total protein values were significantly different in Group H and Group H+G, 63,97 ± 6,97 and 73,07 ± 6,42, respectively. The highest number of spots on a same gel was 157 and the minimum was 34, with a mean of 90 spots to Group H and 83 spots for Group H+G. All of the19 gels were evaluated according to MasterGel and the highest percent of related spots was 52% and the lowest, 0%, with mean similarity between spots 37,8% to Group H and 22% to Group H+G. These results are of great importance, due to lack of works on follicular fluid proteomics using fluid from mares with induced ovulation, and demonstrate that the association hCG + deslorelin acetate increase proteins concentration on pre-ovulatory follicles fluid.
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Análise fisiológica e proteômica do meristema apical da cana-de-açúcar (Saccharum spp) sob aplicação de cálcioVILELA, Romel Duarte 03 March 2016 (has links)
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Previous issue date: 2016-03-03 / Na cana-de-açúcar, a conversão de meristema vegetativo para reprodutivo é uma etapa importante para o melhoramento genético, no entanto, é indesejável na produção comercial por consumir sacarose para o desenvolvimento da inflorescência. Este estudo teve como objetivo identificar proteínas diferencialmente acumuladas no meristema apical da variedade de cana RB867515 sob aplicação foliar de sulfato de cálcio, através de eletroforese 2D e espectrometria de massas. Foi testado o efeito do cálcio em parâmetros morfofisiológicos, concentração de macronutrientes e anatomia do ápice meristemático por microscopia ótica. Adicionalmente, foi avaliado o efeito do cálcio no proteoma do ápice meristemático durante as fases de pré e pós-indução do florescimento. A aplicação foliar de cálcio aumentou a altura de colmos, e a abertura estomática também foi alterada. A composição dos macronutrientes mostrou maiores níveis de cálcio e menores teores de potássio e magnésio. A aplicação foliar de cálcio reduziu em cerca de 20% o florescimento da cana planta e 35% na cana soca. Na análise proteômica, um total de 60 DEPs foram identificados por PMF a partir de perfis 2D de meristemas em pré ou pós indução floral, dos quais 14 foram observadas exclusivamente em meristemas tratados com cálcio, 11 foram identificadas exclusivamente após a indução floral, e 29 foram comuns em ambas as situações, porém mais abundantes em meristemas sem aplicação de cálcio antes da indução floral. A aplicação foliar de cálcio alterou significativamente o proteoma meristemático da cana-de-açúcar. O cálcio parece também melhorar a sinalização celular e a atividade antioxidante em meristemas. O efeito da aplicação foliar de cálcio no proteoma parece ser atenuado pelo tempo. As proteínas identificadas são fortes candidatas a estudos futuros envolvendo o controle do florescimento da cana, visando sua aplicação como marcador molecular funcional associadas ao cálcio, podendo auxiliar os programas de melhoramento genético desta cultura. / In sugarcane (Saccharum spp.), the conversion of apical meristem to breeding is an important step for the genetic improvement, however, it is undesirable in commercial production due to consuming sucrose to develop inflorescence. This study aimed to identify differentially accumulated proteins in the apical meristem of the RB867515 variety under foliar application of calcium sulfate through 2D electrophoresis and mass spectrometry. It has been tested the calcium effect on morphophysiological parameters, macronutrient contents and anatomy of the shoot apical meristem by optical microscopy. Additionally, we evaluated the effect of calcium on the proteome of sugarcane apical meristem during the phases of pre and post-induction of flowering. Foliar applications of calcium increased the stalk height, and stomatal opening was also measured. The macronutrient composition showed higher calcium levels and lower levels of potassium and magnesium. Leaf applications of calcium reduces flowering by 20% in sugarcane plant, and 35% reduction in the ratoon cane. In the proteome analysis, a total of 60 DEPs have been identified by PMF from 2D meristems profiles in pre and post-floral induction, of which 14 were found exclusively in meristems treated with calcium, 11 were identified only after floral induction, and 29 were common in both cases, but more abundant in meristems without application of calcium before floral induction. Foliar applications of calcium significantly altered the meristematic proteome of sugarcane. Calcium also appears to enhance cell signaling and antioxidant activity in meristems. It was observed that the effect of foliar calcium application in proteome appears to be attenuated by time. The proteins identified are strong candidates for future studies aiming its use as a functional molecular marker involving control of flowering of sugarcane associated with calcium, can help breeding programs of this culture.
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Indução da ovulação com hcg e acetato de deslorelina altera o perfil proteico do líquido folicular de éguasSantos, Gabriel de Oliveira January 2014 (has links)
O líquido folicular é o microambiente do oócito durante sua maturação in vivo que é, em parte constituído por exsudato do soro sanguíneo e por substâncias produzidas localmente, que estão relacionados com a atividade metabólica das células ovarianas. Tais substâncias podem ser essenciais para a proliferação e diferenciação das células somáticas bem como na maturação e posterior fertilização de um oócito competente. A busca por biomarcadores capazes de predizer a saúde de um folículo ou a capacidade do oócito em se tornar um embrião saudável é objeto de estudo na medicina reprodutiva humana e veterinária. Para tanto é essencial o conhecimento a nível molecular dos constituintes do liquido folicular e suas funções. O objetivo do presente estudo foi avaliar o perfil proteico do líquido folicular de éguas submetidas à indução de ovulação, com dois diferentes protocolos usuais na prática clínica, utilizando eletroforese bidimensional em gel de poliacrilamida. Para tanto 19 amostras de liquido folicular de éguas que tiveram sua ovulação induzida por dois diferentes protocolos (1000UI hCG IV, Grupo H, ou 1000UI hCG IV + 1,5mg de acetato de deslorelina IM, Grupo H + G) foram submetidos a eletroforese 2D e posterior análise dos géis no PDQuest. Os valores de proteína total foram significativamente diferente nos Grupo H e Grupo H+G, 63,97 ± 6,97 e 73,07 ± 6,42, respectivamente. O número máximo de spots em um mesmo gel foi de 157 e o mínimo de 34, com média de 90 spots para o Grupo H e 83 spots para o Grupo H+G. Os 19 géis foram avaliados e a porcentagem máxima de spots relacionados foi de 52% e a mínima de 0%. Com média de 37,8% de similaridade entre spots para o Grupo H e 22% para o Grupo H+G. Estes resultados são de grande importância devido à escassez de trabalhos com proteômica de liquido folicular de éguas induzidas a ovulação e demonstram que a associação entre hCG e acetato de deslorelina aumenta a concentração de proteínas no líquido folicular em folículos pré-ovulatórios (>35 mm). / Follicular fluid is the oocyte microenvironment during its in vivo maturation. It is partly composed by blood serum exudate, and also by locally produced substances, related to ovarian cells metabolic activity. These substances may be essential for somatic cells proliferation and differentiation, as well as on the oocyte maturation and fertilization. The search for biomarkers able to predict oocyte ability to grow into a healthy embryo are targets on human and veterinary reproductive medicine. It is essential to know the components of follicular fluid and their functions. The aim of the present study was to evaluate protein profile of the follicular fluid in mares with inducted ovulation, in two different protocols, using 2D electrophoresis in polyacrylamide gel. 19 follicular fluid samples from mares in which ovulation induction was performed with two different protocols (1000UI hCG IV or 1000UI hCG IV + 1,5mg deslorelin acetate IM), submitted to 2D electrophoresis, and gel analysis on PDQuest. Total protein values were significantly different in Group H and Group H+G, 63,97 ± 6,97 and 73,07 ± 6,42, respectively. The highest number of spots on a same gel was 157 and the minimum was 34, with a mean of 90 spots to Group H and 83 spots for Group H+G. All of the19 gels were evaluated according to MasterGel and the highest percent of related spots was 52% and the lowest, 0%, with mean similarity between spots 37,8% to Group H and 22% to Group H+G. These results are of great importance, due to lack of works on follicular fluid proteomics using fluid from mares with induced ovulation, and demonstrate that the association hCG + deslorelin acetate increase proteins concentration on pre-ovulatory follicles fluid.
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Transkriptom- und Proteom-Analysen von Escherichia coli unter hyperosmotischen Stressbedingungen und biochemische Charakterisierung von UspGWeber, Arnim 26 November 2003 (has links)
No description available.
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