Abstract
BackgroundInducible expression systems are frequently used for the production of heterologous proteins. Achieving maximum product concentrations requires induction profiling, namely the optimization of induction time and inducer concentration. However, the respective experiments can be very laborious and time-consuming. In this work, a new approach for induction profiling is presented where induction in a microtiter plate based cultivation system (BioLector) is achieved by light using photocaged isopropyl β-d-1-thiogalactopyranoside (cIPTG).ResultsA flavin mononucleotide-based fluorescent reporter protein (FbFP) was expressed using a T7-RNA-polymerase dependent E. coli expression system which required IPTG as inducer. High power UV-A irradiation was directed into a microtiter plate by light-emitting diodes placed above each well of a 48-well plate. Upon UV irradiation, IPTG is released (uncaged) and induces product formation. IPTG uncaging, formation of the fluorescent reporter protein and biomass growth were monitored simultaneously in up to four 48-well microtiter plates in parallel with an in-house constructed BioLector screening system. The amount of released IPTG can be gradually and individually controlled for each well by duration of UV-A exposure, irradiance and concentration of photocaged IPTG added at the start of the cultivation. A comparison of experiments with either optical or conventional IPTG induction shows that product formation and growth are equivalent. Detailed induction profiles revealed that for the strain and conditions used maximum product formation is reached for very early induction times and with just 6–8 s of UV-A irradiation or 60–80 µM IPTG.ConclusionsOptical induction and online monitoring were successfully combined in a high-throughput screening system and the effect of optical induction with photocaged IPTG was shown to be equivalent to conventional induction with IPTG. In contrast to conventional induction, optical induction is less costly to parallelize, easy to automate, non-invasive and without risk of contamination. Therefore, light-induced gene expression with photocaged IPTG is a highly advantageous method for the efficient optimization of heterologous protein production and has the potential to replace conventional induction with IPTG.Electronic supplementary materialThe online version of this article (doi:10.1186/s12934-016-0461-3) contains supplementary material, which is available to authorized users.
Highlights
Inducible expression systems are frequently used for the production of heterologous proteins
light-emitting diode (LED) array for optical induction To achieve optical induction, UV-A irradiation has to be introduced into the culture broth containing 6-nitropiperonal-photocaged isopropyl β-d-1thiogalactopyranoside (cIPTG) to release uncaged isopropyl β-d-1thiogalactopyranoside (IPTG) from its photocage
The LED array can quickly be mounted on top of the microtiter plate where it is positioned by a notch and fixed by two screws
Summary
Inducible expression systems are frequently used for the production of heterologous proteins. Achiev‐ ing maximum product concentrations requires induction profiling, namely the optimization of induction time and inducer concentration. High productivity in heterologous protein production is achieved by optimization of strains, culture conditions and process related parameters. Inducible expression systems are applied to separate the cultivation into an initial growth phase for unimpeded biomass formation and a subsequent production phase where growth is impeded while metabolic resources are shifted towards product formation. The switch from growth to production phase (induction of target gene expression) can be achieved by addition of small chemical inducer molecules among which isopropyl β-d-1thiogalactopyranoside (IPTG) is the most popular choice and widely applied, especially in lab scale. If IPTG concentration is not sufficiently high, cells may not reach their full expression potential; if IPTG concentration exceeds a critical limit, a balanced metabolism cannot be maintained and toxic effects might be observed [3,4,5]
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