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Literature DB >> 26345509

Functional enrichment by direct plasmid recovery after fluorescence activated cell sorting.

Balakrishnan Ramesh¹, Christopher S Frei¹, Patrick C Cirino¹, Navin Varadarajan¹.

Abstract

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 <10% of sorted cells survive culturing and demonstrate that >60% of the sorted cell population was recovered.

Entities: CellLine Chemical Disease Gene Mutation Species

Keywords: library screening; plasmid recovery; toxicity

Mesh：

Substances：

Year: 2015 PMID： 26345509 PMCID： PMC5173293 DOI： 10.2144/000114329

Source DB: PubMed Journal: Biotechniques ISSN： 0736-6205 Impact factor: 1.993

19 in total

1. High copy number plasmids compatible with commonly used cloning vectors.

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4. Single-cell characterization of autotransporter-mediated Escherichia coli surface display of disulfide bond-containing proteins.

Authors: Balakrishnan Ramesh; Victor G Sendra; Patrick C Cirino; Navin Varadarajan
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5. A flow cytometry-based screening system for directed evolution of proteases.

Authors: Ran Tu; Ronny Martinez; Radivoje Prodanovic; Mathias Klein; Ulrich Schwaneberg
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6. The toxicity of recombinant proteins in Escherichia coli: a comparison of overexpression in BL21(DE3), C41(DE3), and C43(DE3).

Authors: Laurence Dumon-Seignovert; Guillaume Cariot; Laurent Vuillard
Journal: Protein Expr Purif Date: 2004-09 Impact factor: 1.650

Functional enrichment by direct plasmid recovery after fluorescence activated cell sorting.

1. High copy number plasmids compatible with commonly used cloning vectors.

2. High-throughput screening for industrial enzyme production hosts by droplet microfluidics.

3. The crystal structure of a trypsin-like mutant chymotrypsin: the role of position 226 in the activity and specificity of S189D chymotrypsin.

4. Single-cell characterization of autotransporter-mediated Escherichia coli surface display of disulfide bond-containing proteins.

5. A flow cytometry-based screening system for directed evolution of proteases.

6. The toxicity of recombinant proteins in Escherichia coli: a comparison of overexpression in BL21(DE3), C41(DE3), and C43(DE3).

7. Conflict between noise and plasticity in yeast.

8. AraC regulatory protein mutants with altered effector specificity.

9. Determination of cell fate selection during phage lambda infection.

10. Directed evolution of cell size in Escherichia coli.

1. Analysis of amino acid substitutions in AraC variants that respond to triacetic acid lactone.

2. Directed Evolution Using Stabilized Bacterial Peptide Display.