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	Provedor de dados ArchiMer (8) Autor Noel, Joelle (8) Delbarre Ladrat, Christine (4) Fleurence, Joel (4) Verrez-bagnis, Veronique (4) Auger, Dominique (2) Boutier, Bernard (2) Chiffoleau, Jean-francois (2) Gonzalez, Jean-louis (2) Michel, Pierre (2) Averty, Bernard (1) Cossa, Daniel (1) Sanjuan, Jane (1) Truquet, Isabelle (1) Mais... Palavra-chave Proteolysis (3) Calpain (2) Cathepsins (2) Fish muscle (2) Neutral calcium dependent protease (2) ARSENIC MMA (1) Activité phytoplanctonique (1) BAY OF MARENNES-OLERON (1) Baie de Marennes-Oléron (1) Calpastatin (1) DMA TRACE ELEMENTS ENGLISH CHANNEL NORTH SEA (1) Dicentrarchus labrax L (1) Fish muscle proteins (1) HEAVY METALS (1) In vitro proteolysis (1) MES (1) Myofibrillar protein (1) Métaux (1) Métaux lourds (1) PHYTOPLANKTON ACTIVITY (1) Mais... Tipo do documento Text (8) Ano 2004 (2) 2003 (1) 2002 (1) 1993 (1) 1992 (1) 1991 (1) 1990 (1) Mais... País France (8) Idioma Inglês (7) Francês (1)		Registro completo Provedor de dados:  ArchiMer País:  France Título:  Relative contribution of calpain and cathepsins to protein degradation in muscle of sea bass (Dicentrarchus labrax L.) Autores:  Delbarre Ladrat, Christine Verrez-bagnis, Veronique Noel, Joelle Fleurence, Joel Data:  2004-12 Ano:  2004 Palavras-chave:  Postmortem aging Fish muscle Proteolysis Cathepsins Neutral calcium dependent protease Resumo:  The effects of a milli(m)-calpain isolated from the white muscle of sea bass (Dicentrarchus labrax L) and commercial cathepsins B, D and L, used in combination on the myofibrillar and sarcoplasmic proteins were examined. Protein digestion was first performed by the endogenous m-calpain, (luring 2 h before the addition of a mixture of cathepsins B, D and L and a further incubation up to 22 h. Calpain degraded a 27 kDa sarcoplasmic component as well as myosin heavy chain, a-actinin, desmin and a 32 kDa component from the myofibrillar fraction. A 97 kDa component and the assumed creatine kinase-aldolase doublet were degraded during the incubation of sarcoplasmic proteins with the cathepsin mixture while, among the myofibrillar proteins, myosin, actin, tropomyosin, and the 22 kDa component were digested by the same enzymatic preparation. Myofibril-bound a-actinin and tropomyosin were released into the soluble fraction by m-calpain and the cathepsins mixture. Some smaller fragments were also produced. This appears to be the result of the cumulative action of each protease, as already investigated in our previous studies, except for the degradation of the sarcoplasmic 97 kDa component. It was only degraded if the cathepsins were mixed; this indicates that the three cathepsins functioned synergistically on muscle proteins. No difference in the proteolytic effect of cathepsins was observed, whether calpain was acting first or not. This work showed that calpain did not modify any muscle protein prior to later hydrolysis by the catheptic proteinases. (C) 2004 Elsevier Ltd. All rights reserved. Tipo:  Text Idioma:  Inglês Identificador:  http://archimer.ifremer.fr/doc/2004/publication-1682.pdf DOI:10.1016/j.foodchem.2004.01.053 Editor:  Elsevier Relação:  http://archimer.ifremer.fr/doc/00000/1682/ Formato:  application/pdf Fonte:  Food Chemistry (0308-8146) (Elsevier), 2004-12 , Vol. 88 , N. 3 , P. 389-395 Direitos:  2004 Elsevier Ltd. All rights reserved Fechar

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