Comparative Single-Cell Analysis of Different E. coli Expression Systems during Microfluidic Cultivation

Dennis Binder; Christopher Probst; Alexander Grünberger; Fabienne Hilgers; Anita Loeschcke; Karl-Erich Jaeger; Dietrich Kohlheyer; Thomas Drepper

doi:10.1371/journal.pone.0160711

Comparative Single-Cell Analysis of Different E. coli Expression Systems during Microfluidic Cultivation

PLoS One. 2016 Aug 15;11(8):e0160711. doi: 10.1371/journal.pone.0160711. eCollection 2016.

Authors

Dennis Binder¹, Christopher Probst², Alexander Grünberger², Fabienne Hilgers¹, Anita Loeschcke¹, Karl-Erich Jaeger^{1

2}, Dietrich Kohlheyer², Thomas Drepper¹

Affiliations

¹ Institute of Molecular Enzyme Technology, Heinrich-Heine-University Düsseldorf, Forschungszentrum Jülich, Jülich, Germany.
² Institute of Bio- and Geosciences (IBG-1), Forschungszentrum Jülich, Jülich, Germany.

Abstract

Recombinant protein production is mostly realized with large-scale cultivations and monitored at the level of the entire population. Detailed knowledge of cell-to-cell variations with respect to cellular growth and product formation is limited, even though phenotypic heterogeneity may distinctly hamper overall production yields, especially for toxic or difficult-to-express proteins. Unraveling phenotypic heterogeneity is thus a key aspect in understanding and optimizing recombinant protein production in biotechnology and synthetic biology. Here, microfluidic single-cell analysis serves as the method of choice to investigate and unmask population heterogeneities in a dynamic and spatiotemporal fashion. In this study, we report on comparative microfluidic single-cell analyses of commonly used E. coli expression systems to uncover system-inherent specifications in the synthetic M9CA growth medium. To this end, the PT7lac/LacI, the PBAD/AraC and the Pm/XylS system were systematically analyzed in order to gain detailed insights into variations of growth behavior and expression phenotypes and thus to uncover individual strengths and deficiencies at the single-cell level. Specifically, we evaluated the impact of different system-specific inducers, inducer concentrations as well as genetic modifications that affect inducer-uptake and regulation of target gene expression on responsiveness and phenotypic heterogeneity. Interestingly, the most frequently applied expression system based on E. coli strain BL21(DE3) clearly fell behind with respect to expression homogeneity and robustness of growth. Moreover, both the choice of inducer and the presence of inducer uptake systems proved crucial for phenotypic heterogeneity. Conclusively, microfluidic evaluation of different inducible E. coli expression systems and setups identified the modified lacY-deficient PT7lac/LacI as well as the Pm/XylS system with conventional m-toluic acid induction as key players for precise and robust triggering of bacterial gene expression in E. coli in a homogeneous fashion.

Publication types

Comparative Study

MeSH terms

Cell Culture Techniques / instrumentation*
Cell Proliferation
Escherichia coli / cytology*
Escherichia coli / genetics*
Gene Expression
Genetic Engineering / instrumentation*
Lab-On-A-Chip Devices*
Phenotype
Single-Cell Analysis / instrumentation*

Grants and funding

Supported by grants from the Federal Ministry of Education and Research (OptoSys, FKZ 031A16), Ministry of Innovation, Science and Research of North-Rhine Westphalia and German Research Foundation (INST 208/654-1 FUGG). Moreover, the Helmholtz Association (VH-NG-1029 and PD-311) is gratefully acknowledged for funding. This work was partly performed at the Helmholtz Nanoelectronic Facility (HNF) of Forschungszentrum Jülich. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.