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Site-saturation mutagenesis: a powerful tool for structure-based design of combinatorial mutation libraries.

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dc.contributor.author Chronopoulou, EG en
dc.contributor.author Labrou, NE en
dc.date.accessioned 2014-06-06T06:51:02Z
dc.date.available 2014-06-06T06:51:02Z
dc.date.issued 2011 en
dc.identifier.issn 19343663 en
dc.identifier.uri http://62.217.125.90/xmlui/handle/123456789/5285
dc.relation.uri http://www.scopus.com/inward/record.url?eid=2-s2.0-79958246432&partnerID=40&md5=092828f26aa83870ea66cb5c8aa6ecb6 en
dc.subject.other article en
dc.subject.other combinatorial chemistry en
dc.subject.other gene library en
dc.subject.other methodology en
dc.subject.other mutation en
dc.subject.other polymerase chain reaction en
dc.subject.other protein engineering en
dc.subject.other site directed mutagenesis en
dc.subject.other Combinatorial Chemistry Techniques en
dc.subject.other Gene Library en
dc.subject.other Mutagenesis, Site-Directed en
dc.subject.other Mutation en
dc.subject.other Polymerase Chain Reaction en
dc.subject.other Protein Engineering en
dc.title Site-saturation mutagenesis: a powerful tool for structure-based design of combinatorial mutation libraries. en
heal.type journalArticle en
heal.publicationDate 2011 en
heal.abstract This unit describes a method for site-saturation mutagenesis (SSM) using PCR amplification with degenerate synthetic oligonucleotides as primers. SSM allows the substitution of predetermined protein sites against all twenty possible amino acids at once. Therefore, SSM is a powerful approach in protein engineering to characterize structure-function relationships, as well as to create improved protein variants. The procedure accepts double-stranded plasmid isolated from the dam(+) E. coli strain. The procedure is simple, fast, efficient, and eliminates time-consuming subcloning and ligation steps. © 2011 by John Wiley & Sons, Inc. en
heal.journalName Current protocols in protein science / editorial board, John E. Coligan ... [et al.] en
dc.identifier.volume Chapter 26 en


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