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	Provedor de dados Colegio de Postgraduados (3) AgEcon (2) Electron. J. Biotechnol. (1) Autor Vázquez Hernández, Lorena (2) Brorsen, B. Wade (1) Chan,Hsin-Hua (1) Chen,Yeh (1) Fofana, N'Zue F. (1) Hernández Ortiz, Juan (1) Hsiao,Nai-Wan (1) Huang, Chung L. (1) Kao,Chao-Hung (1) Kuan,Yi-Chia (1) Lee,Shuo-Kang (1) Lee,Yen-Chung (1) Lin, Biing-Hwan (1) Luo, Haobo (1) Mais... Palavra-chave Homogeneity (6) Homogeneidad (3) Café (2) Chemometrics (2) Coffee (2) Maestría (2) NIRS (2) PCA (2) Producción Agroalimentaria en el Trópico (2) Quimiometría (2) SIMCA (2) Symmetry (2) Active cash market (1) Buyer concentration (1) Chromatography (1) Delphi approach (1) Demand and Price Analysis (1) Differential-form demand system (1) Doctorado (1) Domestic price (1) Mais... Tipo do documento Conference Paper or Presentation (1) Journal Article (1) Journal article (1) Tesis (1) Ano 2014 (1) 2011 (3) 2007 (1) 2001 (1) País Mexico (3) United States (2) Chile (1) Idioma Espanhol (3) Inglês (3)		Registro completo Provedor de dados:  Electron. J. Biotechnol. País:  Chile Título:  Purification and characterization of an aspartic protease from the Rhizopus oryzae protease extract, Peptidase R Autores:  Hsiao,Nai-Wan Chen,Yeh Kuan,Yi-Chia Lee,Yen-Chung Lee,Shuo-Kang Chan,Hsin-Hua Kao,Chao-Hung Data:  2014-03-01 Ano:  2014 Palavras-chave:  Chromatography Endopeptidase Food processing industry Homogeneity Rhizopuspepsin Resumo:  Background Aspartic proteases are a subfamily of endopeptidases that are useful in a variety of applications, especially in the food processing industry. Here we describe a novel aspartic protease that was purified from Peptidase R, a commercial protease preparation derived from Rhizopus oryzae. Results An aspartic protease sourced from Peptidase R was purified to homogeneity by anion exchange chromatography followed by polishing with a hydrophobic interaction chromatography column, resulting in a 3.4-fold increase in specific activity (57.5 × 10³ U/mg) and 58.8% recovery. The estimated molecular weight of the purified enzyme was 39 kDa. The N-terminal sequence of the purified protein exhibited 63-75% identity to rhizopuspepsins from various Rhizopus species. The enzyme exhibited maximal activity at 75°C in glycine-HCl buffer, pH 3.4 with casein as the substrate. The protease was stable at 35°C for 60 min and had an observed half-life of approximately 30 min at 45°C. Enzyme activity was not significantly inhibited by chelation with ethylenediamine tetraacetic acid (EDTA), and the addition of metal ions to EDTA-treated protease did not significantly change enzyme activity, indicating that proteolysis is not metal ion-dependent. The purified enzyme was completely inactivated by the aspartic protease inhibitor Pepstatin A. Conclusion Based on the observed enzyme activity, inhibition profile with Pepstatin A, and sequence similarity to other rhizopuspepsins, we have classified this enzyme as an aspartic protease. Tipo:  Journal article Idioma:  Inglês Identificador:  http://www.scielo.cl/scielo.php?script=sci_arttext&pid=S0717-34582014000200006 Editor:  Pontificia Universidad Católica de Valparaíso Formato:  text/html Fonte:  Electronic Journal of Biotechnology v.17 n.2 2014 Fechar

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