Analysis of 11,430 recombinant protein production experiments reveals that protein yield is tunable by synonymous codon changes of translation initiation sites |
| |
| Authors: | Bikash K. Bhandari Chun Shen Lim Daniela M. Remus Augustine Chen Craig van Dolleweerd Paul P. Gardner |
| |
| Affiliation: | 1. Department of Biochemistry, School of Biomedical Sciences, University of Otago, Dunedin, New Zealand ; 2. Callaghan Innovation Protein Science and Engineering, University of Canterbury, Christchurch, New Zealand ; 3. Biomolecular Interaction Center, University of Canterbury, Christchurch, New Zealand ; Harvard University, UNITED STATES |
| |
| Abstract: | Recombinant protein production is a key process in generating proteins of interest in the pharmaceutical industry and biomedical research. However, about 50% of recombinant proteins fail to be expressed in a variety of host cells. Here we show that the accessibility of translation initiation sites modelled using the mRNA base-unpairing across the Boltzmann’s ensemble significantly outperforms alternative features. This approach accurately predicts the successes or failures of expression experiments, which utilised Escherichia coli cells to express 11,430 recombinant proteins from over 189 diverse species. On this basis, we develop TIsigner that uses simulated annealing to modify up to the first nine codons of mRNAs with synonymous substitutions. We show that accessibility captures the key propensity beyond the target region (initiation sites in this case), as a modest number of synonymous changes is sufficient to tune the recombinant protein expression levels. We build a stochastic simulation model and show that higher accessibility leads to higher protein production and slower cell growth, supporting the idea of protein cost, where cell growth is constrained by protein circuits during overexpression. |
| |
| Keywords: | |
|
|
