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Titlebook: Recombinant Gene Expression; Reviews and Protocol Paulina Balbás,Argelia Lorence Book 2004Latest edition Humana Press 2004

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1064-3745 ng cells impacts directly on a symbolic meaning deeply imbedded in every culture. During the earlier years of gene expression research, te- nological applications were confined mainly to academic and industrial laboratories, and were perceived as highly beneficial since molecules that were previousl
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Host Cell Compatibility in Protein Expressionduction of substantial amounts of protein and nonprotein molecules for commercial and investigational use. In the case of proteins, strategies for determining the most appropriate vector-host combination for the expression of an exogenous gene depend on a diverse range of factors that relate ultimat
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Production of Recombinant Proteinsigh-quality proteins reach the market. Higher production efficiencies and, consequently, lower costs of the final product are needed for obtaining a commercially viable process. In this chapter, common problems in recombinant protein production are reviewed and strategies for their solution are disc
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Folding-Promoting Agents in Recombinant Protein Production. The target proteins are not in every case soluble and/or correctly folded. That is why different production parameters, such as host, cultivation conditions, and co-expression of chaperones and foldases, are applied in order to gain functional recombinant proteins. Furthermore, the addition of fol
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Back to Basicsn of every cloned gene. Although a number of strategies have been implemented to deal with problems associated to gene transcription and translation, protein folding, secretion, location, posttranslational modifications, particularities of different strains, and the like and more integrated processe
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α-Complementation-Enabled T7 Expression Vectors and Their Use for the Expression of Recombinant Polys method is based on the ability of proteins containing protein transduction domains (PTDs), short stretches of 9–16 predominantly basic amino acids, to traverse the cytoplasmic membrane and accumulate inside cells in a time- and dose-dependent fashion. The number of PTDs, both natural and synthetic
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Expression of Recombinant Alkaline Phosphatase Conjugates in ,oteins fused to a highly active bacterial alkaline phosphatase (PhoA) variant as reporter enzyme. Appropriate insertion of the DNA encoding the foreign peptides, proteic domains, or proteins between codons +6 and +7 of the . gene restores the initial frame of the . gene in the vector. Consequently,
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Plasmid Vectors for Marker-Free Chromosomal Insertion of Genetic Material in , the pBRINTs-rAnb. family. These vectors offer the choice of using the antibiotics chloramphenicol, gentamycin, or kanamycin to select for chromosomal integration events. In addition, it is possible to eliminate these chromosomal antibiotic resistance markers, after integration has taken place. The
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