RESUMO
Global interest in sugarcane has increased significantly in recent years due to its economic impact on sustainable energy production. Sugarcane breeding and better agronomic practices have contributed to a huge increase in sugarcane yield in the last 30 years. Additional increases in sugarcane yield are expected to result from the use of biotechnology tools in the near future. Genetically modified (GM) sugarcane that incorporates genes to increase resistance to biotic and abiotic stresses could play a major role in achieving this goal. However, to bring GM sugarcane to the market, it is necessary to follow a regulatory process that will evaluate the environmental and health impacts of this crop. The regulatory review process is usually accomplished through a comparison of the biology and composition of the GM cultivar and a non-GM counterpart. This review intends to provide information on non-GM sugarcane biology, genetics, breeding, agronomic management, processing, products and byproducts, as well as the current technologies used to develop GM sugarcane, with the aim of assisting regulators in the decision-making process regarding the commercial release of GM sugarcane cultivars.
RESUMO
O objetivo deste trabalho foi comparar a eficiência da solubilização de quatro detergentes comercialmente disponíveis, ASB 14, SB 3-10, CHAPS e Triton X100, na extração de proteínas de membrana da bactéria Xylella fastidiosa para estudos proteômicos. Estas proteínas foram solubilizadas em duas etapas em tampões diferenciados pelos detergentes e submetidas à eletroforese bidimensional (2-DE) em uma faixa de pH não linear de 3-10. Os detergentes ASB 14 e SB 3-10 foram os mais efecientes, revelando 221 e 157 proteínas, respectivamente, enquanto que o CHAPS e o Triton X100 resultaram somente 72 e 43 proteínas, respectivamente. A identificação das proteínas foi feita por 'peptide mass fingerprinting' em espectrometria de massa MALDI-TOF, através de peptídeos obtidos por digestão com tripsina in gel. Os 18 spots de proteínas do gel com tratamento com ASB 14 mostrou que 83% eram proteínas de membrana. Este estudo concluiu que o detergente ASB-14 foi o mais eficiente na solubilização de proteínas de membrana de Xylella fastidiosa.
RESUMO
A lectin was purified from Crotalaria paulina seeds by ion-exchange and FPLC molecular exclusion chromatography. CrpL had an apparent molecular mass of 30 kDa, as determined by SDS-PAGE under non-reducing and reducing conditions. CrpL effectively agglutinated human and cow erythrocytes, and this activity was not affected by 20 mM EDTA, showing no dependence of divalent cations. Hemagglutination was inhibited by N-acetyl-D-galactosamine, D-galactose and was also inhibited by glycoproteins, fetuin and asialofetuin. The N-terminal amino acid sequence of CrpL was identical to those of other lectins from the genus Crotalaria, and amino acid composition showed high amounts of Asx and Glx, and was rich in Gly, Ala and Ser, as also reported for lectins from other Crotalaria species. CrpL inhibited the growth of Xanthomonas axonopodis pv. phaseoli and Xanthomonas axonopodis pv. passiflorae, suggesting a role of this lectin in the defense of seeds against bacterial infections.
Assuntos
Crotalaria/química , Lectinas de Plantas/isolamento & purificação , Sementes/química , Sequência de Aminoácidos , Dados de Sequência Molecular , Lectinas de Plantas/análise , Lectinas de Plantas/químicaRESUMO
Four different detergents, ASB 14, SB 3-10, CHAPS and Triton X100, were utilized to determine the optimal detergent for the solubilization of membrane proteins from the phytopathogenic bacterium Xylella fastidiosa. These proteins were differentially solubilized in distinct buffers containing the detergent and subjected to bidimensional electrophoresis within the non-linear pH range of 3-10. The detergents ASB 14 and SB 3-10 were the most effective revealing 221 and 157 spots, respectively. CHAPS and Triton X100 were less effective and revealed only 72 and 43 spots, respectively. MALDI-TOF tryptic peptide mass fingerprinting of 18 excised proteins from the ASB 14 treatment revealed that 83% were membrane proteins and that the theoretical efficiency of solubilization for ASB 14 was estimated to be 87%. This study demonstrates the effectiveness of the detergent ASB 14 for the solubilization of membrane proteins from the bacterium X. fastidiosa.
O objetivo deste trabalho foi comparar a eficiência da solubilização de quatro detergentes comercialmente disponíveis, ASB 14, SB 3-10, CHAPS e Triton X100, na extração de proteínas de membrana da bactéria Xylella fastidiosa para estudos proteômicos. Estas proteínas foram solubilizadas em duas etapas em tampões diferenciados pelos detergentes e submetidas à eletroforese bidimensional (2-DE) em uma faixa de pH não linear de 3-10. Os detergentes ASB 14 e SB 3-10 foram os mais efecientes, revelando 221 e 157 proteínas, respectivamente, enquanto que o CHAPS e o Triton X100 resultaram somente 72 e 43 proteínas, respectivamente. A identificação das proteínas foi feita por 'peptide mass fingerprinting' em espectrometria de massa MALDI-TOF, através de peptídeos obtidos por digestão com tripsina in gel. Os 18 spots de proteínas do gel com tratamento com ASB 14 mostrou que 83% eram proteínas de membrana. Este estudo concluiu que o detergente ASB-14 foi o mais eficiente na solubilização de proteínas de membrana de Xylella fastidiosa.