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Titlebook: In Vitro Mutagenesis Protocols; Jeff Braman Book 20022nd edition Humana Press 2002

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In Vitro Scanning-Saturation Mutagenesis,). However, a stumbling block to the wider application of these techniques is that each desired mutation must be introduced into a gene, cloned into bacteria, and the protein produced then purified (.). This is a resource and time intensive process that precludes routine use.
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1064-3745 r biologists in establishing the functions of components of the proteome. In this second edition of In Vitro Mutagenesis Protocols, active researchers with proven track records describe in stepwise fashion their advanced mutagenesis techniques. Each contributor focuses on improvements to conventiona
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High-Throughput Scanning Mutagenesis by Recombination Polymerase Chain Reaction,ng mutagenesis (.) are popular means for investigating the structure and function of proteins and the interactions between proteins. Cys-scanning mutagenesis is particularly useful, since the introduction of Cys allows targeted chemical modification with a wide variety of sulfhydryl-reactive reagents (.,.).
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Book 20022nd editiontechnique includes detailed step-by-step instructions, tips on pitfalls to avoid, and notes on reagents and suppliers...Time-tested and highly practical, the techniques in In Vitro Mutagenesis Protocols, Second Edition offer today‘s molecular biologists a rich compendium of reliable and powerful tec
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Site-Directed Mutagenesis Using Altered /gb-Lactamase Specificity,of Kunkel (.), Eckstein (.), and Deng (.,.) employ negative selection against the wild-type DNA strand, in which the parental DNA is selectively degraded, either by growth in an alternate host strain, or by digestion with a nuclease or restriction enzyme. The methods of Lewis and Thompson (.) and Bo
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Efficient and Accurate Site-Directed Mutagenesis of Large Plasmids,d by recombination in vivo following cotransformation of the two fragments into competent recA.. cells. Since both DNA strands carry the desired mutation as directed by the mutagenic primers, the recovery of mutant clones should, in theory, approach 100%, although, in practice, mutant yields, rangin
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