Functional enrichment by direct plasmid recovery after fluorescence activated cell sorting

Functional enrichment by direct plasmid recovery after fluorescence activated cell sorting

Iterative screening of expressed protein libraries using fluorescence-activated cell sorting (FACS) typically involves culturing the pooled clones after each sort. In these experiments, if cell viability is compromised by the sort conditions and/or expression of the target protein(s), rescue PCR pro...

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Veröffentlicht in:BioTechniques 2015-09, Vol.59 (3), p.157-161
Hauptverfasser: Ramesh, Balakrishnan, Frei, Christopher S, Cirino, Patrick C, Varadarajan, Navin
Format: Artikel
Sprache:eng
Schlagworte:
Biosensing Techniques
Cells, Cultured
Chymotrypsin - genetics
DNA - isolation & purification
Escherichia coli - genetics
Flow Cytometry - methods
Green Fluorescent Proteins - genetics
Green Fluorescent Proteins - metabolism
High-Throughput Screening Assays - methods
library screening
Peptide Library
Peptides - genetics
plasmid recovery
Plasmids - genetics
Pyrones - analysis
toxicity
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Zusammenfassung:Iterative screening of expressed protein libraries using fluorescence-activated cell sorting (FACS) typically involves culturing the pooled clones after each sort. In these experiments, if cell viability is compromised by the sort conditions and/or expression of the target protein(s), rescue PCR provides an alternative to culturing but requires re-cloning and can introduce amplification bias. We have optimized a simple protocol using commercially available reagents to directly recover plasmid DNA from sorted cells for subsequent transformation. We tested our protocol with 2 different screening systems in which 60% of the sorted cell population was recovered.
ISSN:0736-6205
1940-9818
DOI:10.2144/000114329