A novel method to recover inclusion body protein from recombinant E. coli fed-batch processes based on phage ΦX174-derived lysis protein E

Daniela Ehgartner; Patrick Sagmeister; Timo Langemann; Andrea Meitz; Werner Lubitz; Christoph Herwig

doi:10.1007/s00253-017-8281-x

A novel method to recover inclusion body protein from recombinant E. coli fed-batch processes based on phage ΦX174-derived lysis protein E

Appl Microbiol Biotechnol. 2017 Jul;101(14):5603-5614. doi: 10.1007/s00253-017-8281-x. Epub 2017 Apr 20.

Authors

Daniela Ehgartner^{1

2}, Patrick Sagmeister^{1

3}, Timo Langemann^{4

5}, Andrea Meitz⁴, Werner Lubitz⁵, Christoph Herwig^{6

7}

Affiliations

¹ Institute for Chemical, Environmental and Biological Engineering, TU Wien, Gumpendorferstrasse 1a/166, 1060, Vienna, Austria.
² CD Laboratory on Mechanistic and Physiological Methods for Improved Bioprocesses, TU Wien, Gumpendorferstrasse 1a/166, 1060, Vienna, Austria.
³ Exputec GmbH, Pfeilgasse 32/20, 1080, Vienna, Austria.
⁴ RCPE-Research Center of Pharmaceutical Engineering GmbH, Inffeldgasse 13, 8010, Graz, Austria.
⁵ BIRD-C GmbH, Dr.-Bohr-Gasse 2-8, 1030, Vienna, Austria.
⁶ Institute for Chemical, Environmental and Biological Engineering, TU Wien, Gumpendorferstrasse 1a/166, 1060, Vienna, Austria. christoph.herwig@tuwien.ac.at.
⁷ CD Laboratory on Mechanistic and Physiological Methods for Improved Bioprocesses, TU Wien, Gumpendorferstrasse 1a/166, 1060, Vienna, Austria. christoph.herwig@tuwien.ac.at.

Abstract

Production of recombinant proteins as inclusion bodies is an important strategy in the production of technical enzymes and biopharmaceutical products. So far, protein from inclusion bodies has been recovered from the cell factory through mechanical or chemical disruption methods, requiring additional cost-intensive unit operations. We describe a novel method that is using a bacteriophage-derived lysis protein to directly recover inclusion body protein from Escherichia coli from high cell density fermentation process: The recombinant inclusion body product is expressed by using a mixed feed fed-batch process which allows expression tuning via adjusting the specific uptake rate of the inducing substrate. Then, bacteriophage ΦX174-derived lysis protein E is expressed to induce cell lysis. Inclusion bodies in empty cell envelopes are harvested via centrifugation of the fermentation broth. A subsequent solubilization step reveals the recombinant protein. The process was investigated by analyzing the impact of fermentation conditions on protein E-mediated cell lysis as well as cell lysis kinetics. Optimal cell lysis efficiencies of 99% were obtained with inclusion body titers of >2.0 g/l at specific growth rates higher 0.12 h^-1 and inducer uptake rates below 0.125 g/(g × h). Protein E-mediated cell disruption showed a first-order kinetics with a kinetic constant of -0.8 ± 0.3 h^-1. This alternative inclusion body protein isolation technique was compared to the one via high-pressure homogenization. SDS gel analysis showed 10% less protein impurities when cells had been disrupted via high-pressure homogenization, than when empty cell envelopes including inclusion bodies were investigated. Within this contribution, an innovative technology, tuning recombinant protein production and substituting cost-intensive mechanical cell disruption, is presented. We anticipate that the presented method will simplify and reduce the production costs of inclusion body processes to produce technical enzymes and biopharmaceutical products.

Keywords: Bacterial Ghost; Bioprocess technology; Escherichia coli; Mixed feed bioprocesses; Recombinant protein release; pBAD expression system.

MeSH terms

Bacteriological Techniques*
Bacteriolysis
Batch Cell Culture Techniques / economics
Escherichia coli / chemistry
Escherichia coli / cytology
Escherichia coli / genetics*
Escherichia coli / metabolism
Fermentation
Inclusion Bodies / chemistry*
Inclusion Bodies / genetics
Kinetics
Recombinant Proteins / genetics
Recombinant Proteins / isolation & purification*
Recombinant Proteins / metabolism
Viral Proteins / genetics
Viral Proteins / isolation & purification
Viral Proteins / metabolism*

Substances

E protein, bacteriophage X174
Recombinant Proteins
Viral Proteins