A new generation of E. coli expression hosts and tools for recombinant protein production
Lead Research Organisation:
University of Birmingham
Department Name: Sch of Biosciences
Abstract
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Technical Summary
Many biopharmaceuticals are produced in E. coli but current platforms have a number of limitations and cannot produce many potential target products. This project will develop four entirely novel innovations to produce and harvest a wide range of target proteins, delivering new tools and processes that encompass the entire upstream pipeline:
1: Protein synthesis will be driven by a novel set of promoters and inducers that have clear advantages (better inducible control, higher mRNA yield) over currently-used systems. Many of the currently-used inducible promoters for recombinant protein production (RPP) are extremely strong, inherently leaky and present on high-copy number plasmids. RPP often outstrips the ability of the cell to cope, resulting in insoluble aggregates and inclusion body formation.
2: Export to the periplasm will be mediated by an alternative protein export pathway, known as the Tat pathway, that has unique capabilities and clear advantages over the currently-used Sec pathway. A major problem with the Sec pathway is that it transports its substrates in an unfolded state, and cannot handle proteins that fold too quickly or tightly - a significant proportion of potential target molecules. The Tat pathway will instead be exploited to export a wide range of new biotherapeutics in a prefolded form.
3: We will develop and validate a novel method for releasing periplasmic contents which relies on nano-encapsulation of lipids. The method uses a low cost polymer (SMA) which provides a more specific release method than current osmotic shock methods under a wider range of operating conditions.
4: The above innovations will be combined to deliver an integrated platform that is better than the sum of its parts.
The project will be carried out in collaboration with a range of UK companies who will fully validate the new strains and processes.
1: Protein synthesis will be driven by a novel set of promoters and inducers that have clear advantages (better inducible control, higher mRNA yield) over currently-used systems. Many of the currently-used inducible promoters for recombinant protein production (RPP) are extremely strong, inherently leaky and present on high-copy number plasmids. RPP often outstrips the ability of the cell to cope, resulting in insoluble aggregates and inclusion body formation.
2: Export to the periplasm will be mediated by an alternative protein export pathway, known as the Tat pathway, that has unique capabilities and clear advantages over the currently-used Sec pathway. A major problem with the Sec pathway is that it transports its substrates in an unfolded state, and cannot handle proteins that fold too quickly or tightly - a significant proportion of potential target molecules. The Tat pathway will instead be exploited to export a wide range of new biotherapeutics in a prefolded form.
3: We will develop and validate a novel method for releasing periplasmic contents which relies on nano-encapsulation of lipids. The method uses a low cost polymer (SMA) which provides a more specific release method than current osmotic shock methods under a wider range of operating conditions.
4: The above innovations will be combined to deliver an integrated platform that is better than the sum of its parts.
The project will be carried out in collaboration with a range of UK companies who will fully validate the new strains and processes.
Planned Impact
As described in proposal submitted to TSB
Publications
Lee SC
(2016)
A method for detergent-free isolation of membrane proteins in their local lipid environment.
in Nature protocols
Ruanto P
(2020)
Activation by NarL at the Escherichia coli ogt promoter.
in The Biochemical journal
Hall SCL
(2020)
Adsorption of a styrene maleic acid (SMA) copolymer-stabilized phospholipid nanodisc on a solid-supported planar lipid bilayer.
in Journal of colloid and interface science
Lee SC
(2016)
Encapsulated membrane proteins: A simplified system for molecular simulation.
in Biochimica et biophysica acta
Guerrero Montero I
(2019)
Escherichia coli "TatExpress" strains export several g/L human growth hormone to the periplasm by the Tat pathway.
in Biotechnology and bioengineering
Browning DF
(2017)
Escherichia coli "TatExpress" strains super-secrete human growth hormone into the bacterial periplasm by the Tat pathway.
in Biotechnology and bioengineering
Gulamhussein A
(2019)
Examining the stability of membrane proteins within SMALPs
in European Polymer Journal
Browning DF
(2019)
Exploitation of the Escherichia coli lac operon promoter for controlled recombinant protein production.
in Biochemical Society transactions
Depping P
(2022)
Heterologous Expression of Membrane Proteins in E. coli.
in Methods in molecular biology (Clifton, N.J.)
| Description | We have developed a new process to reduce the cost of drug production. This involves new strains of bacteria that are optimised to produce drugs at a higher level in a form that is easier to purify alongside new methods to extract drugs from bacteria. |
| Exploitation Route | A number of the innovations resulting from the work are being tested by the pharmaceutical industry |
| Sectors | Manufacturing, including Industrial Biotechology,Pharmaceuticals and Medical Biotechnology |
| Description | Development of an improved SMALP toolkit to extract active membrane proteins |
| Amount | £563,000 (GBP) |
| Funding ID | BB/S008160/1 |
| Organisation | Biotechnology and Biological Sciences Research Council (BBSRC) |
| Sector | Public |
| Country | United Kingdom |
| Start | 03/2019 |
| End | 02/2022 |
| Description | Investigating GPCR:RAMP interactions using nanobodies |
| Amount | £404,022 (GBP) |
| Funding ID | BB/R016615/1 |
| Organisation | Biotechnology and Biological Sciences Research Council (BBSRC) |
| Sector | Public |
| Country | United Kingdom |
| Start | 05/2019 |
| End | 05/2022 |
| Description | Unshackling Membrane Protein Research : New Amphiphilic Copolymers for Extraction of Stable, Active Membrane Proteins |
| Amount | £492,954 (GBP) |
| Funding ID | 223728/Z/21/Z |
| Organisation | Wellcome Trust |
| Sector | Charity/Non Profit |
| Country | United Kingdom |
| Start | 03/2022 |
| End | 02/2027 |
| Title | Periplasmic Release |
| Description | The Use of Styrene Maleic Acid Polymers for specific release of materials from E coli periplasm |
| Type Of Material | Technology assay or reagent |
| Year Produced | 2018 |
| Provided To Others? | No |
| Impact | NA |
| Title | SOLUBILISATION OF MEMBRANE PROTEINS |
| Description | Development of a new reagent for extraction of membrane proteins in a stabilised form |
| IP Reference | EP2452199 |
| Protection | Patent granted |
| Year Protection Granted | 2012 |
| Licensed | Yes |
| Impact | Establishment of a newco (Orbiscope BV) in the Netherlands based on selling materials detailed in the patent. Reagents currently being sold globally to academia and the pharmaceutical industry |