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Slowing Bacterial Translation Speed Enhances Eukaryotic Protein Folding Efficiency |
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| Authors: | Efraí n Siller,John F. Anderson,José M. Barral |
| Affiliation: | 1 Department of Neuroscience and Cell Biology, The University of Texas Medical Branch, 301 University Boulevard, Galveston, TX 77555-0620, USA 2 Department of Cell and Developmental Biology, University of Illinois, 601 South Goodwin Avenue, Urbana-Champaign, IL 61801, USA |
| Abstract: | The mechanisms for de novo protein folding differ significantly between bacteria and eukaryotes, as evidenced by the often observed poor yields of native eukaryotic proteins upon recombinant production in bacterial systems. Polypeptide synthesis rates are faster in bacteria than in eukaryotes, but the effects of general variations in translation rates on protein folding efficiency have remained largely unexplored. By employing Escherichia coli cells with mutant ribosomes whose translation speed can be modulated, we show here that reducing polypeptide elongation rates leads to enhanced folding of diverse proteins of eukaryotic origin. These results suggest that in eukaryotes, protein folding necessitates slow translation rates. In contrast, folding in bacteria appears to be uncoupled from protein synthesis, explaining our findings that a generalized reduction in translation speed does not adversely impact the folding of the endogenous bacterial proteome. Utilization of this strategy has allowed the production of a native eukaryotic multidomain protein that has been previously unattainable in bacterial systems and may constitute a general alternative to the production of aggregation-prone recombinant proteins. |
| Keywords: | TF, trigger factor aa/s, amino acids per second Sm, streptomycin SmP, streptomycin pseudodependent FL, firefly luciferase GFP, green fluorescent protein MBP, maltose-binding protein EMSA, electromobility shift assay |
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