Construction and flow cytometric screening of targeted enzyme libraries
Herein, we describe a methodology for the construction of targeted libraries intended to modify the substrate specificity of proteases expressed on the cell surface of Escherichia coli . The native outer membrane protease, OmpT, is used as a model system. The protocol relies on gene assembly using o...
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Published in | Nature protocols Vol. 4; no. 6; pp. 893 - 901 |
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Main Authors | , , , |
Format | Journal Article |
Language | English |
Published |
London
Nature Publishing Group UK
01.06.2009
Nature Publishing Group |
Subjects | |
Online Access | Get full text |
ISSN | 1754-2189 1750-2799 |
DOI | 10.1038/nprot.2009.60 |
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Abstract | Herein, we describe a methodology for the construction of targeted libraries intended to modify the substrate specificity of proteases expressed on the cell surface of
Escherichia coli
. The native outer membrane protease, OmpT, is used as a model system. The protocol relies on gene assembly using oligonucleotides and is easily adaptable to any enzyme in which information is available on the putative active site residues. Increasingly complex libraries can be generated in a systematic manner and screened using flow cytometry (fluorescence-activated cell sorting, FACS) for variants displaying altered function. Furthermore, if the substrate-binding pockets have not been elucidated, a protocol for partial multi-site saturation library construction is presented that allows for sampling a large number of residues, while maintaining an appropriate level of protein function. The entire procedure, from start to finish, should take approximately 2–3 weeks. |
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AbstractList | Herein, we describe a methodology for the construction of targeted libraries intended to modify the substrate specificity of proteases expressed on the cell surface of Escherichia coli. The native outer membrane protease, OmpT, is used as a model system. The protocol relies on gene assembly using oligonucleotides and is easily adaptable to any enzyme in which information is available on the putative active site residues. Increasingly complex libraries can be generated in a systematic manner and screened using flow cytometry (fluorescence-activated cell sorting, FACS) for variants displaying altered function. Furthermore, if the substrate-binding pockets have not been elucidated, a protocol for partial multi-site saturation library construction is presented that allows for sampling a large number of residues, while maintaining an appropriate level of protein function. The entire procedure, from start to finish, should take approximately 2-3 weeks. Herein, we describe a methodology for the construction of targeted libraries intended to modify the substrate specificity of proteases expressed on the cell surface of Escherichia coli . The native outer membrane protease, OmpT, is used as a model system. The protocol relies on gene assembly using oligonucleotides and is easily adaptable to any enzyme in which information is available on the putative active site residues. Increasingly complex libraries can be generated in a systematic manner and screened using flow cytometry (fluorescence-activated cell sorting, FACS) for variants displaying altered function. Furthermore, if the substrate-binding pockets have not been elucidated, a protocol for partial multi-site saturation library construction is presented that allows for sampling a large number of residues, while maintaining an appropriate level of protein function. The entire procedure, from start to finish, should take approximately 2–3 weeks. |
Audience | Academic |
Author | Georgiou, George Varadarajan, Navin Iverson, Brent L Cantor, Jason R |
Author_xml | – sequence: 1 givenname: Navin surname: Varadarajan fullname: Varadarajan, Navin organization: Institute for Cell and Molecular Biology, University of Texas, Department of Chemical Engineering, University of Texas – sequence: 2 givenname: Jason R surname: Cantor fullname: Cantor, Jason R organization: Department of Chemical Engineering, University of Texas – sequence: 3 givenname: George surname: Georgiou fullname: Georgiou, George email: gg@che.utexas.edu organization: Institute for Cell and Molecular Biology, University of Texas, Department of Chemical Engineering, University of Texas – sequence: 4 givenname: Brent L surname: Iverson fullname: Iverson, Brent L email: biverson@mail.utexas.edu organization: Institute for Cell and Molecular Biology, University of Texas, Department of Chemistry and Biochemistry, University of Texas |
BackLink | https://www.ncbi.nlm.nih.gov/pubmed/19478805$$D View this record in MEDLINE/PubMed |
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SubjectTerms | Analytical Chemistry Bacterial Outer Membrane Proteins - chemistry Bacterial Outer Membrane Proteins - genetics Bacterial Outer Membrane Proteins - metabolism Biological Techniques Biomedical and Life Sciences Catalytic Domain - genetics Cell Membrane - enzymology Computational Biology/Bioinformatics Construction E coli Enzymes Enzymes - chemistry Enzymes - genetics Enzymes - metabolism Escherichia coli Escherichia coli - enzymology Escherichia coli - genetics Escherichia coli Proteins - chemistry Escherichia coli Proteins - genetics Escherichia coli Proteins - metabolism Flow cytometry Flow Cytometry - methods Fluorescence Genetic aspects Genetic engineering Genomic libraries Life Sciences Methods Microarrays Models, Molecular Mutagenesis Mutation Organic Chemistry Peptide Hydrolases - chemistry Peptide Hydrolases - genetics Peptide Hydrolases - metabolism Physiological aspects Proteases Protein Engineering Proteins Protocol Residues Substrate Specificity Substrates Synthesis Testing |
Title | Construction and flow cytometric screening of targeted enzyme libraries |
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