Towards a targeted therapy for arthritis
Lead Research Organisation:
Queen Mary, University of London
Department Name: William Harvey Research Institute
Abstract
We have developed a new drug delivery technology that allows the drug to be protected from being degraded in the body and targets it to the site of disease. The drug delivery system is composed of a shell derived from a naturally occurring molecule called latency associated peptide (LAP). LAP forms a shell around the drug and is therefore protecting the drug from degradation within the body. The shell is opened through an enzyme-sensitive cleavage site. The enzymes that can open the shell are found at sites of inflammation particularly in joints affected by arthritis. The shell is therefore only opened and it?s contents released at the sites of disease.
This technology has many advantages over current biological drugs as it targets the release of the drug only to sites of disease thus preventing side effects, and the drug can be used in small doses. In this study we will produce and purify sufficient material of different forms of the shell and drug that can be tested, pharmaceutically assessed, and compared in a model of arthritis. In this way, we will obtain data that is essential to allow us bring this novel technology to clinical trials in humans. The success of this project will enable us to expand the use of this technology to other diseases that have a destructive/inflammatory component such as Crohn?s disease, multiple sclerosis and atherosclerosis.
This technology has many advantages over current biological drugs as it targets the release of the drug only to sites of disease thus preventing side effects, and the drug can be used in small doses. In this study we will produce and purify sufficient material of different forms of the shell and drug that can be tested, pharmaceutically assessed, and compared in a model of arthritis. In this way, we will obtain data that is essential to allow us bring this novel technology to clinical trials in humans. The success of this project will enable us to expand the use of this technology to other diseases that have a destructive/inflammatory component such as Crohn?s disease, multiple sclerosis and atherosclerosis.
Technical Summary
To enable targeting of cytokines and other therapeutic molecules to sites of disease, we have developed a novel platform technology that harnesses the pathological process to release the therapeutic moiety in situ and provides for longer half-life. We built a stable ?shell? by fusing the latency associated peptide precursor part of transforming growth factor beta, through a linker with a matrix metalloproteinase- or aggrecanase-sensitive site (thus targeting release/activation to inflammatory sites) to a therapeutic cytokine (IFN beta) for arthritis treatment. In this study we will express and biochemically purify sufficient recombinant protein to provide data on pharmacokinetics, pharmacodynamics, immunogenicity, toxicology and therapeutic efficacy in an arthritis model. This work is essential to produce preclinical data and bring this technology to the level of a phase I/II clinical trial.
Publications
Koutsokeras A
(2014)
Generation of an efficiently secreted, cell penetrating NF-?B inhibitor.
in FASEB journal : official publication of the Federation of American Societies for Experimental Biology
Mullen L
(2014)
Latency can be conferred to a variety of cytokines by fusion with latency-associated peptide from TGF-ß.
in Expert opinion on drug delivery
Mullen L
(2014)
A comparative study of matrix metalloproteinase and aggrecanase mediated release of latent cytokines at arthritic joints
in Annals of the Rheumatic Diseases
Mullen L
(2014)
Latent cytokines for targeted therapy of inflammatory disorders.
in Expert opinion on drug delivery
Mullen LM
(2012)
Increased disulphide dimer formation of latent associated peptide fusions of TGF-ß by addition of L-cystine.
in Journal of biotechnology
| Description | project grant |
| Amount | £103,000 (GBP) |
| Funding ID | PG/09/093 |
| Organisation | British Heart Foundation (BHF) |
| Sector | Charity/Non Profit |
| Country | United Kingdom |
| Start | 06/2010 |
| End | 06/2011 |
| Description | project grant |
| Amount | £213,000 (GBP) |
| Organisation | Breast Cancer Campaign (BCC) |
| Sector | Charity/Non Profit |
| Country | United Kingdom |
| Start | 03/2011 |
| End | 02/2013 |
| Title | mLAP-aggrecanase-IFN beta |
| Description | This material is cleaved specifically by aggreacanase and synovila fluid from osteoarthritic patients |
| Type Of Material | Technology assay or reagent |
| Provided To Others? | No |
| Impact | This material has shown better therapeutic efficacy in a collagen-induced arthritis model than that obtained with a MMP cleavable fusion protein |
| Title | mouse LAP-IFN beta |
| Description | CHO expressed glycosylated material with murine sequences in various isoforms for testing in vivo |
| Type Of Material | Technology assay or reagent |
| Provided To Others? | No |
| Impact | Better PK data expected than originally planned in original application |
| Description | Crystal structure of LAP-IL-10 |
| Organisation | Amgen Inc |
| Country | United States |
| Sector | Private |
| PI Contribution | We are expressing LAp-IL-10 in a baculovirus system with a view to crystalise and define its structure with colleagues at Birbeck College. This study is funded by Amgen Corp. USA |
| Collaborator Contribution | I spend a mini sabbatical at Amgen in Seattle (3 months) that as a result this collaboration was set up |
| Impact | NA |
| Start Year | 2011 |
| Description | In vivo real time pharmacodynamic imaging using a transgenic mouse |
| Organisation | Helmholtz Association of German Research Centres |
| Department | Helmholtz Centre for Infection Research (HZI) |
| Country | Germany |
| Sector | Academic/University |
| PI Contribution | We are starting to image these Mx2-luciferase Tg mice after administration of IFN beta followed by luciferin substrate and imaging the PK/PD |
| Collaborator Contribution | this is allowing us to measure in real time delivery of LAP-IFN constructs to sites of disease |
| Impact | na |
| Start Year | 2011 |
| Title | Latency Associated Protein Construct With Aggrecanase Sensitive Cleavage Site |
| Description | The present provides a fusion protein comprising a latency associated peptide (LAP) and a pharmaceutically active agent in which the LAP and the pharmaceutically active agent are connected by an amino acid sequence comprising an aggrecanase proteolytic cleavage site. |
| IP Reference | US2010310515 |
| Protection | Patent granted |
| Year Protection Granted | 2010 |
| Licensed | No |
| Impact | N/A |
| Title | MODIFIED LATENCY ASSOCIATED PROTEIN CONSTRUCT |
| Description | The present invention provides a fusion protein comprising a latency associated peptide (LAP), a pharmaceutically active agent and an amino acid sequence comprising a dimerisation domain, wherein the LAP and the pharmaceutically active agent are connected by an amino acid sequence comprising a proteolytic cleavage site. Also provided are nucleic acids enclosing such fusion proteins, process for their preparation, pharmaceutical compositions, kits and uses thereof in medicine. |
| IP Reference | WO2015198072 |
| Protection | Patent application published |
| Year Protection Granted | 2015 |
| Licensed | Commercial In Confidence |
| Impact | see above |