An innovative approach to 'printing' functional protein microarrays from RNA microarrays.
Lead Research Organisation:
University of Portsmouth
Department Name: Inst of Biomedical and Biomolecular Sc
Abstract
Proteins are the fundamental building blocks of all living cells and are essential for the proper functioning of an organism. Understanding how proteins interact with each other, and with other biological molecules, lies at the heart of all biological research and has clear implications for scientific progress within both health and environmental fields. For example, new therapeutics and more efficient bioenergy generation both rely on understanding and exploiting protein interactions. It is therefore unsurprising that developing tools to study protein interactions is a key priority within the BBSRC strategic plan.
One of the most efficient ways of investigating protein interactions is to generate a single surface containing hundreds-to-thousands of proteins, which can all be tested for interactions in one step. A surface of this type is known as a functional protein microarray and can be used to conduct high throughput interaction studies. Considering the real world applications of functional protein microarrays, within the medical arena alone, they have the potential to underpin better health through their use in drug discovery, disease diagnosis and medical screening. Unfortunately, to date, the successful creation of functional protein microarrays has been particularly challenging and they have therefore failed to deliver the impact anticipated.
This application seeks funding for pilot research to demonstrate a novel concept for generating functional protein microarrays that overcomes the limitations of the current approaches. The concept involves using an array of protein precursors (RNA molecules) on a surface, known as an RNA microarray, to generate a corresponding protein microarray on a specially prepared facing surface. The experimental setup involves placing the two surfaces opposite each other in a sandwich arrangement, with a specific biological solution in-between that converts the RNA molecules into protein molecules. Using a novel chemistry step, the newly formed protein molecules in solution attach themselves to the specially prepared facing surface, forming the functional protein microarray. To prove the novel concept, this project will involve demonstrating each stage of the process in turn, before bringing it all together to create a functional protein microarray by effectively 'printing' it from the precursor RNA microarray.
This work is innovative, timely and multi-disciplinary, employing the latest advances in chemistry, to facilitate the attachment of the proteins to the microarray slide surface, as well as our recent, state-of-the-art, patented technology for generating the precursor RNA microarray. Importantly, this application is not about incremental further development of this RNA microarray technology, but is instead about exploiting it and proving a novel concept for a new tool in a completely separate field; specifically, for the generation of functional protein microarrays. The potential of this research is considerable, offering a step change in capability by creating functional protein microarrays with greater robustness, smaller spot sizes and unrestricted protein sizes, in a simple and efficient manner. This overcomes the key limitations of existing functional protein microarray technologies and unlocks the vast benefits originally forecast.
One of the most efficient ways of investigating protein interactions is to generate a single surface containing hundreds-to-thousands of proteins, which can all be tested for interactions in one step. A surface of this type is known as a functional protein microarray and can be used to conduct high throughput interaction studies. Considering the real world applications of functional protein microarrays, within the medical arena alone, they have the potential to underpin better health through their use in drug discovery, disease diagnosis and medical screening. Unfortunately, to date, the successful creation of functional protein microarrays has been particularly challenging and they have therefore failed to deliver the impact anticipated.
This application seeks funding for pilot research to demonstrate a novel concept for generating functional protein microarrays that overcomes the limitations of the current approaches. The concept involves using an array of protein precursors (RNA molecules) on a surface, known as an RNA microarray, to generate a corresponding protein microarray on a specially prepared facing surface. The experimental setup involves placing the two surfaces opposite each other in a sandwich arrangement, with a specific biological solution in-between that converts the RNA molecules into protein molecules. Using a novel chemistry step, the newly formed protein molecules in solution attach themselves to the specially prepared facing surface, forming the functional protein microarray. To prove the novel concept, this project will involve demonstrating each stage of the process in turn, before bringing it all together to create a functional protein microarray by effectively 'printing' it from the precursor RNA microarray.
This work is innovative, timely and multi-disciplinary, employing the latest advances in chemistry, to facilitate the attachment of the proteins to the microarray slide surface, as well as our recent, state-of-the-art, patented technology for generating the precursor RNA microarray. Importantly, this application is not about incremental further development of this RNA microarray technology, but is instead about exploiting it and proving a novel concept for a new tool in a completely separate field; specifically, for the generation of functional protein microarrays. The potential of this research is considerable, offering a step change in capability by creating functional protein microarrays with greater robustness, smaller spot sizes and unrestricted protein sizes, in a simple and efficient manner. This overcomes the key limitations of existing functional protein microarray technologies and unlocks the vast benefits originally forecast.
Technical Summary
Proteomic research spans the biosciences; hence, the BBSRC strategic plan highlights the development of new tools to study proteomics as a key priority underpinning future research advancements. Functional protein microarrays have the potential to significantly benefit proteomic research, but have failed to deliver the anticipated impact due to well recognised limitations. To overcome these limitations, this application requests funding for pilot research to prove the novel concept of generating covalently-bound functional multi-protein microarrays from multi-RNA microarrays.
To demonstrate the concept it is proposed to combine our state-of-the-art, patented, multi-RNA microarray technology with a novel label that can covalently couple a protein to a microarray slide surface upon light activation. Specifically, the novel label is an azide which is incorporated into the protein via an amber suppressor tRNA containing an azide-modified amino acid. The azide can then couple, via 'click' chemistry, to a surface-immobilised dibenzocyclooctyne, generated from a light activated cyclopropenone-masked cyclooctyne. Experimentally, the multi-RNA microarray slide will be set up in a sandwich arrangement facing a second slide, onto which the proteins become immobilised, with an in vitro translation mix in between the two slides. The end result is that the multi-RNA slide 'prints' a functional protein microarray, with each protein covalently immobilised on the surface via its incorporated azide. This work will involve demonstrating each stage of the process in turn, before testing the overall concept. The potential of this research is considerable, offering a step change in capability by creating functional protein microarrays with greater robustness, smaller spot sizes and unrestricted protein sizes, in a simple and efficient manner. This overcomes the key limitations of existing functional protein microarray technologies and unlocks the vast benefits originally predicted.
To demonstrate the concept it is proposed to combine our state-of-the-art, patented, multi-RNA microarray technology with a novel label that can covalently couple a protein to a microarray slide surface upon light activation. Specifically, the novel label is an azide which is incorporated into the protein via an amber suppressor tRNA containing an azide-modified amino acid. The azide can then couple, via 'click' chemistry, to a surface-immobilised dibenzocyclooctyne, generated from a light activated cyclopropenone-masked cyclooctyne. Experimentally, the multi-RNA microarray slide will be set up in a sandwich arrangement facing a second slide, onto which the proteins become immobilised, with an in vitro translation mix in between the two slides. The end result is that the multi-RNA slide 'prints' a functional protein microarray, with each protein covalently immobilised on the surface via its incorporated azide. This work will involve demonstrating each stage of the process in turn, before testing the overall concept. The potential of this research is considerable, offering a step change in capability by creating functional protein microarrays with greater robustness, smaller spot sizes and unrestricted protein sizes, in a simple and efficient manner. This overcomes the key limitations of existing functional protein microarray technologies and unlocks the vast benefits originally predicted.
Planned Impact
This work seeks to prove the novel concept of generating covalently-bound functional multi-protein microarrays from multi-RNA microarrays. Creating functional protein microarrays via this approach would have the potential to significantly benefit proteomic research, a field that spans the breadth of the biosciences domain. Discussions with Portsmouth University Research and Innovation Services indicate that the potential impact of this work falls into four broad categories:
1) Commercialisation
Early steps towards commercialisation will be explored during this project, but a promising proof of concept will require some further investment to mature and strengthen the commercial position. It is anticipated that the primary beneficiaries from successful commercialisation and exploitation will be companies that already manufacture products and supply services for the biosciences array market within the UK and worldwide (e.g. Agilent). Adding this tool to their product line has the potential to create wealth and economic prosperity through increased turn-over, profit and exports, and creating and safeguarding jobs. More broadly, secondary beneficiaries will include those companies that support the biosciences array manufacturers, whether that is in supplying or servicing equipment or providing the specific consumables required.
2) Further development of the tool
Towards the end of this work, once encouraging proof of concept data has been obtained and commercialisation is being explored, it is likely that further development of the tool would be required. This could be completed independently, but would benefit from collaborative research with specific proteomics users. In this manner, the collaborators would also gain early access to the tool, allowing them to conduct research that would not previously have been practicable. Once robust data is generated and the commercial/IP position is secure, then it would be possible to freely publish and release information and data generated using this technology. Such publications would further support commercialisation by generating broad interest and consequently demand for its use. Collaborators are likely to be drawn from across the proteomics field, including academia (e.g. Cambridge Centre for Proteomics) as well as from industry, public sector organisations and the third sector. This not only provides immediate benefits to the knowledge economy by generating research outputs (e.g. publications, patents, further income generation), but these outputs also have the potential to be successfully exploited, generating further impact. This activity will also strengthen collaborative links and encourage placements between institutions, as well as resulting in a host of highly skilled individuals gaining a broader appreciation of the applications of the tool and a detailed understanding of its use.
3) Longer term broader employment of the tool across the research community
Once the tool has been commercialised (see 1) and used to publish exemplary research (see 2) the intent is that it would see broad use across the research community. The beneficiaries at this stage are all those operating within biosciences R&D, including academia, industry, public sector organisations and the third sector. Bringing together the benefits from (1) and (2), the widespread use of the tool will create wealth and economic prosperity for suppliers within the biosciences array market, support research outputs, the knowledge economy and the exploitation of research findings.
4) Public dissemination
Throughout this project it will be possible to engage with the general public and local schools to raise the profile of this project. This will encourage interest in biosciences research and UK innovation and provide a context to local bioscience education.
1) Commercialisation
Early steps towards commercialisation will be explored during this project, but a promising proof of concept will require some further investment to mature and strengthen the commercial position. It is anticipated that the primary beneficiaries from successful commercialisation and exploitation will be companies that already manufacture products and supply services for the biosciences array market within the UK and worldwide (e.g. Agilent). Adding this tool to their product line has the potential to create wealth and economic prosperity through increased turn-over, profit and exports, and creating and safeguarding jobs. More broadly, secondary beneficiaries will include those companies that support the biosciences array manufacturers, whether that is in supplying or servicing equipment or providing the specific consumables required.
2) Further development of the tool
Towards the end of this work, once encouraging proof of concept data has been obtained and commercialisation is being explored, it is likely that further development of the tool would be required. This could be completed independently, but would benefit from collaborative research with specific proteomics users. In this manner, the collaborators would also gain early access to the tool, allowing them to conduct research that would not previously have been practicable. Once robust data is generated and the commercial/IP position is secure, then it would be possible to freely publish and release information and data generated using this technology. Such publications would further support commercialisation by generating broad interest and consequently demand for its use. Collaborators are likely to be drawn from across the proteomics field, including academia (e.g. Cambridge Centre for Proteomics) as well as from industry, public sector organisations and the third sector. This not only provides immediate benefits to the knowledge economy by generating research outputs (e.g. publications, patents, further income generation), but these outputs also have the potential to be successfully exploited, generating further impact. This activity will also strengthen collaborative links and encourage placements between institutions, as well as resulting in a host of highly skilled individuals gaining a broader appreciation of the applications of the tool and a detailed understanding of its use.
3) Longer term broader employment of the tool across the research community
Once the tool has been commercialised (see 1) and used to publish exemplary research (see 2) the intent is that it would see broad use across the research community. The beneficiaries at this stage are all those operating within biosciences R&D, including academia, industry, public sector organisations and the third sector. Bringing together the benefits from (1) and (2), the widespread use of the tool will create wealth and economic prosperity for suppliers within the biosciences array market, support research outputs, the knowledge economy and the exploitation of research findings.
4) Public dissemination
Throughout this project it will be possible to engage with the general public and local schools to raise the profile of this project. This will encourage interest in biosciences research and UK innovation and provide a context to local bioscience education.
People |
ORCID iD |
| Anastasia Callaghan (Principal Investigator) |
Publications
Henderson CA
(2019)
Generation of small molecule-binding RNA arrays and their application to fluorogen-binding RNA aptamers.
in Methods (San Diego, Calif.)
Norouzi M
(2019)
Application of mRNA Arrays for the Production of mCherry Reporter-Protein Arrays for Quantitative Gene Expression Analysis
in ACS Synthetic Biology
Vincent H
(2023)
DNA Manipulation and Analysis
| Description | Proteins are the fundamental building blocks of all living cells and are essential for the proper functioning of an organism. Understanding how proteins interact with each other, and with other biological molecules, lies at the heart of all biological research and has clear implications for scientific progress within both health and environmental fields. One of the most efficient ways of investigating protein interactions is to generate a single surface containing hundreds-to-thousands of proteins, which can all be tested for interactions in one step. This project has demonstrated a novel approach for generating protein microarrays. Specifically, it involves using an array of protein precursors (RNA molecules) on a surface, known as an RNA microarray (created using our recent, state-of-the-art, patented technology), to generate a corresponding protein microarray on a specially prepared facing surface. The experimental setup involves placing the two surfaces opposite each other in a sandwich arrangement, with a specific biological solution in-between that converts the RNA molecules into protein molecules. Using a novel molecular coupling step, the newly formed protein molecules in solution attach themselves to the specially prepared facing surface, forming the protein microarray. This grant has not only demonstrated an efficient and effective means of generating protein microarrays, it has also exemplified a further utility of our novel RNA array technology (discovered and developed following earlier BBSRC investment). |
| Exploitation Route | Creating protein microarrays from RNA microarrays has the potential to significantly benefit proteomic research, a field that spans the breadth of the biosciences domain. However, some further development of the method and demonstration of the broad utility of the approach would be required before being taking forward for commercialisation by industry. Ultimately, the method would be anticipated to be of use to others for studying protein interactions in a high throughput format. |
| Sectors | Manufacturing, including Industrial Biotechology,Pharmaceuticals and Medical Biotechnology |
| Description | The findings of this research project strengthen the exemplification of patent applications which have now been granted in the US (US 9,777,268) and Europe (EP 2732047). The research also leveraged further investment to explore wider applications of the technology. Additionally, the work within this grant provided the basis for recent activities in the translation and commercialisation space. Specifically, securing Innovate UK ICURe funding to explore commercialisation routes, which led to securing a BBSRC Enterprise Fellowship for the PostDoc involved on the project, and a place on the Cambridge-based Start Codon Investment Accelerator programme. This supported steps to create a spin-out venture, RevoNA Bio, which was incorporated in 2022. RevoNA Bio secured an Innovate UK ICURe Follow-on Fund grant and Start Codon investment, and is focused on securing further impact from the RNA technology. |
| First Year Of Impact | 2022 |
| Sector | Pharmaceuticals and Medical Biotechnology |
| Impact Types | Economic |
| Description | Brazil Partnering Award: Imperial-Portsmouth-Vicosa A. pleuropneumoniae collaboration |
| Amount | £50,000 (GBP) |
| Funding ID | BB/S020543/1 |
| Organisation | Biotechnology and Biological Sciences Research Council (BBSRC) |
| Sector | Public |
| Country | United Kingdom |
| Start | 06/2019 |
| End | 05/2023 |
| Description | DigiLab Global Equipment Provision |
| Amount | £30,000 (GBP) |
| Organisation | DigiLab Global |
| Sector | Private |
| Country | United States |
| Start | 11/2015 |
| Description | E3 - Co-Applicant |
| Amount | £5,800,000 (GBP) |
| Organisation | United Kingdom Research and Innovation |
| Department | Research England |
| Sector | Public |
| Country | United Kingdom |
| Start | 08/2019 |
| End | 07/2022 |
| Description | ICURe (Innovation to Commercialise University Research) |
| Amount | £30,000 (GBP) |
| Organisation | Innovation to Commercialisation of University Research |
| Sector | Charity/Non Profit |
| Country | United Kingdom |
| Start | 12/2015 |
| End | 04/2016 |
| Description | Innovation to Commercialise University Research (ICURe) Award |
| Amount | £35,000 (GBP) |
| Organisation | Innovate UK |
| Sector | Public |
| Country | United Kingdom |
| Start | 10/2020 |
| End | 04/2021 |
| Description | Provision of gapmer reagents |
| Amount | £10,000 (GBP) |
| Organisation | Ionis Pharmaceuticals |
| Sector | Private |
| Country | United States |
| Start | 09/2019 |
| End | 08/2022 |
| Description | Provision of test materials and staff time |
| Amount | £2,000 (GBP) |
| Organisation | BioCopy |
| Sector | Private |
| Country | Germany |
| Start | 11/2019 |
| End | 01/2020 |
| Title | Protein Array from RNA Array |
| Description | As part of this research, a novel method has been developed which allows protein arrays to be generated from RNA arrays. Example utilities include: - generating bespoke functional protein arrays for proteomic studies - supporting high throughput approaches for exploring translation and mechanisms to specifically inhibit translation of potential targets, for example, for therapeutic purposes. |
| Type Of Material | Technology assay or reagent |
| Year Produced | 2019 |
| Provided To Others? | Yes |
| Impact | A manuscript has been published describing this method so that it an be used more widely by those in the field. |
| Description | Collaboration with BioCopy |
| Organisation | BioCopy |
| Country | Germany |
| Sector | Private |
| PI Contribution | BioCopy make DNA and protein arrays, as well as using them for commercial research projects. Discussions around possible alignment of their array technologies with Portsmouth's RNA array technology is ongoing. Myself and my team hosted a research scientist from BioCopy to work with us on experiments to explore the potential compatibility of the two different technologies. |
| Collaborator Contribution | BioCopy make DNA and protein arrays, as well as using them for commercial research projects. Discussions around possible alignment of their array technologies with Portsmouth's RNA array technology is ongoing. BioCopy provided array slides with novel surfaces and a research scientist to visit and work with the Portsmouth team to explore potential compatibility between the different technologies. |
| Impact | On-going |
| Start Year | 2019 |
| Description | Collaboration with DigiLab Global |
| Organisation | DigiLab Global |
| Country | United States |
| Sector | Private |
| PI Contribution | Collaboration with DigiLab Global is allowing researchers on the project to access specific instrumentation. This is allowing them to explore and develop automated approaches within the context of our patented novel surface technology. |
| Collaborator Contribution | DigiLab Global provided specific instrumentation to support the research as well as their unique expertise in relation to instrumentation support. |
| Impact | This research is on-going. The disciplines involved include biochemistry and molecular biology coupled with instrumentation engineering expertise. |
| Start Year | 2015 |
| Description | Collaboration with Ionis Pharmaceuticals |
| Organisation | Ionis Pharmaceuticals |
| Country | United States |
| Sector | Private |
| PI Contribution | Ionis Pharmaceuticals are a leading RNA Therapeutics company. They approached us to explore the potential of using the RNA array for screening gapmers binding to RNA targets and the efficiency of subsequent target degradation by RNaseH. A range of gapmers and test RNA sequences were provided and experiments are ongoing. |
| Collaborator Contribution | Ionis Pharmaceuticals are a leading RNA Therapeutics company. They approached us to explore the potential of using the RNA array for screening gapmers binding to RNA targets and the efficiency of subsequent target degradation by RNaseH. Ionis Pharmaceuticals provided gapmers and test RNA sequences for the associated experimental work to be undertaken at Portsmouth. |
| Impact | Experiments and discussions are on-going. |
| Start Year | 2019 |
| Description | Collaboration with Prof. Denise Bazzolli at the Universidade Federal de Viçosa |
| Organisation | Federal University of Viçosa |
| Country | Brazil |
| Sector | Academic/University |
| PI Contribution | My research team are undertaking molecular interaction studies guided by microbiology data provided by Prof. Bazzolli's team. |
| Collaborator Contribution | Prof. Bazzolli's team are providing microbiology data and expertise. |
| Impact | One of Prof. Bazzolli's team has secured funding to undertake a year-long placement in my research group to support this collaboration. |
| Start Year | 2015 |
| Description | Collaboration with Prof. Paul Langford at Imperial College London |
| Organisation | Imperial College London |
| Country | United Kingdom |
| Sector | Academic/University |
| PI Contribution | My research team are conducting in vitro molecular interaction studies, and exploring the applicability of utilising our patented novel array technology, to explore cellular mechanisms within bacteria. |
| Collaborator Contribution | Prof. Langford's team provide microbiology expertise and access to in vivo testing studies. |
| Impact | A joint BBSRC grant was secured to support this collaborative research. |
| Start Year | 2015 |
| Title | METHOD OF IMMOBILISING RNA ONTO A SURFACE |
| Description | The invention relates to a method of immobilising at least one RNA molecule onto a surface of a support comprising: i) providing a first support having a surface on which at least one DNA molecule is immobilised, wherein the DNA molecule encodes an RNA molecule and the encoded RNA molecule comprises a binding molecule; ii) providing a second support having a surface on which at least one binding partner for interacting with the binding molecule is immobilised; iii) arranging the first and second supports such that the surfaces displaying the immobilised molecules are in close proximity and substantially face each other, and contacting the DNA molecule immobilised on the surface of the first support with transcription reagents; and iv) carrying out a transcription reaction to generate the encoded RNA molecule, wherein the RNA molecule is directly immobilised onto the surface of the second support via an interaction between the binding molecule of the RNA molecule and the binding partner on the surface of the second support. |
| IP Reference | WO2012156718 |
| Protection | Patent application published |
| Year Protection Granted | 2012 |
| Licensed | No |
| Impact | - Discussions, under NDA, are on-going with interested companies. - Academic collaborations are supporting the further development of the technology. |
| Title | METHOD OF IMMOBILISING RNA ONTO A SURFACE |
| Description | The invention relates to a method of immobilising at least one RNA molecule onto a surface of a support comprising: i) providing a first support having a surface on which at least one DNA molecule is immobilised, wherein the DNA molecule encodes an RNA molecule and the encoded RNA molecule comprises a binding molecule; ii) providing a second support having a surface on which at least one binding partner for interacting with the binding molecule is immobilised; iii) arranging the first and second supports such that the surfaces displaying the immobilised molecules are in close proximity and substantially face each other, and contacting the DNA molecule immobilised on the surface of the first support with transcription reagents; and iv) carrying out a transcription reaction to generate the encoded RNA molecule, wherein the RNA molecule is directly immobilised onto the surface of the second support via an interaction between the binding molecule of the RNA molecule and the binding partner on the surface of the second support. |
| IP Reference | US2014087972 |
| Protection | Patent granted |
| Year Protection Granted | 2014 |
| Licensed | No |
| Impact | Discussions around licensing/commercialisation with industry partners are presently ongoing. |
| Title | METHOD OF IMMOBILISING RNA ONTO A SURFACE |
| Description | Understanding, manipulating and controlling the flow of genetic information, essential to life, lies at the heart of basic and applied research within the biosciences community. An ability to rapidly analyse the RNA and protein outputs of gene expression, in a high throughput manner, would therefore be of significant value to researchers in the field. Supporting discoveries as diverse as RNA translation inhibitor identification for therapeutic effect, to developing artificial switches for synthe |
| IP Reference | EP2732047 |
| Protection | Patent granted |
| Year Protection Granted | 2014 |
| Licensed | No |
| Impact | Discussions around licensing/commercialisation with industry partners are presently ongoing. |
| Description | Commercialisation discussions with BioCopy |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Industry/Business |
| Results and Impact | Commercialisation discussions to explore potential utilities/applications of the array technology. |
| Year(s) Of Engagement Activity | 2019,2020 |
| Description | Commercialisation discussions with Cambridge Protein Arrays |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | Local |
| Primary Audience | Industry/Business |
| Results and Impact | Presentation and discussions on 'Novel RNA Array Technology' to Cambridge Protein Arrays, December 2013. Effective networking. |
| Year(s) Of Engagement Activity | 2013 |
| Description | Commercialisation discussions with DigiLab Global. |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Industry/Business |
| Results and Impact | Presentation and discussions on the 'Novel RNA Array Technology' to DigiLab Global, January 2014. This lead to them visiting our labs and observing the RNA Array Technology process. DigiLab Global subsequently supported further research in this area by supplying equipment to explore automation approaches. Effective networking. |
| Year(s) Of Engagement Activity | 2014,2015,2016 |
| Description | Commercialisation discussions with Horiba Scientific |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Industry/Business |
| Results and Impact | Presentation and discussions on the 'Novel RNA Array Technology' to Horiba Scientific. The company funding our attendance at their site in France to undertake some collaborative experiments to explore possible opportunities. Effective networking. |
| Year(s) Of Engagement Activity | 2012 |
| Description | Commercialisation discussions with Ionis Pharmaceuticals |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Industry/Business |
| Results and Impact | Commercialisation discussions to explore potential utilities/applications of the array technology. |
| Year(s) Of Engagement Activity | 2019,2020 |
| Description | Commercialisation discussions with Scienion |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Industry/Business |
| Results and Impact | Commercialisation discussions to explore potential utilities/applications of the array technology. |
| Year(s) Of Engagement Activity | 2020 |
| Description | Commercialisation discussions with TTPLabtech |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Industry/Business |
| Results and Impact | Commercialisation discussions with TTPLabtech. |
| Year(s) Of Engagement Activity | 2016 |
| Description | Commercialisation discussions with Twist Bioscience |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Industry/Business |
| Results and Impact | Commercialisation discussions to explore potential utilities/applications of the array technology. |
| Year(s) Of Engagement Activity | 2019 |
| Description | Maintaining an Active Online Presence |
| Form Of Engagement Activity | Engagement focused website, blog or social media channel |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Public/other audiences |
| Results and Impact | My group has an active Twitter account with around 200 followers. We publish highlights from our research, outreach and engagement activities. |
| Year(s) Of Engagement Activity | 2011,2012,2013,2014,2015,2016 |
| Description | Patented Array Technology Website |
| Form Of Engagement Activity | Engagement focused website, blog or social media channel |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Industry/Business |
| Results and Impact | My group has a specific website highlighting our innovative patented array technology to potential commercial partners/business users. |
| Year(s) Of Engagement Activity | 2016 |
| Description | Promoting PG study |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | Local |
| Primary Audience | Undergraduate students |
| Results and Impact | Presentation by members of my research team at various departmental events for undergraduates to promote engagement in postgraduate study. this involved the individuals highlighting their research work, including their day to day work, opportunities for collaboration and engagement as well as their outputs and impact. |
| Year(s) Of Engagement Activity | 2013,2014,2015,2016 |
| Description | Science Fairs |
| Form Of Engagement Activity | Participation in an open day or visit at my research institution |
| Part Of Official Scheme? | No |
| Geographic Reach | Regional |
| Primary Audience | Public/other audiences |
| Results and Impact | Myself and my team have participated in supporting a number of Science Fairs in the region, engaging with attendees to promote science and the research we undertake. |
| Year(s) Of Engagement Activity | 2013,2014,2015,2016 |
| Description | Translation and commercialisation journey included as a feature in BBSRC's Impact Showcase 2022 |
| Form Of Engagement Activity | Engagement focused website, blog or social media channel |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Media (as a channel to the public) |
| Results and Impact | At the request of BBSRC, myself and the BBSRC Enterprise Fellow working with me on the translation and commercialisation of the RNA technology, were asked to generate a video for the 2022 Impact Showcase. We produced a short video, explaining the journey we had been on, and the role that BBSRC and Innovate UK played in supporting this. The intention was that in sharing our experiences, we would encourage others to explore commercialisation routes for securing impact from their research. |
| Year(s) Of Engagement Activity | 2022 |
| URL | https://www.discover.ukri.org/bbsrc-impact-showcase-2022/ |
| Description | University Open Days |
| Form Of Engagement Activity | Participation in an open day or visit at my research institution |
| Part Of Official Scheme? | No |
| Geographic Reach | National |
| Primary Audience | Schools |
| Results and Impact | Myself and my team regularly support University Open days. Activities can be many and varied, including giving talks, presenting posters, running hands-on laboratory demonstrations and engaging in question and answer sessions. There are usually a number of these events per year, with over 100 participants (schools and college students, sometimes accompanied by a parent/guardian) attending each event. Feedback from such events has highlighted our success in inspiring the next generation of scientists and has been specifically linked to an increase in the number of students applying to study Biochemistry over the last few years. |
| Year(s) Of Engagement Activity | 2009,2010,2011,2012,2013,2014,2015,2016 |