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 inNature protocols Vol. 4; no. 6; pp. 893 - 901
Main Authors Varadarajan, Navin, Cantor, Jason R, Georgiou, George, Iverson, Brent L
Format Journal Article
LanguageEnglish
Published London Nature Publishing Group UK 01.06.2009
Nature Publishing Group
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ISSN1754-2189
1750-2799
DOI10.1038/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.
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
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Snippet Herein, we describe a methodology for the construction of targeted libraries intended to modify the substrate specificity of proteases expressed on the cell...
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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
URI https://link.springer.com/article/10.1038/nprot.2009.60
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