The role of RNA Binding Proteins (RBPs) in breast cancer progression and metastasis
Lead Research Organisation:
Queen Mary University of London
Department Name: Barts Cancer Institute
Abstract
Metastasis is the process by which cancer spreads through the body and colonises distant, sometimes vital, organs and tissues. It is estimated that more than 90% of all cancer related mortalities are due to metastasis. In breast cancer in particular, despite great advances in detection and treatment of the disease over the past decades, related mortality rates have remained high due to recurrence of cancer as metastases in secondary organs and tissues, which often happens several years after the initial diagnosis and treatment. Importantly, no therapies are currently available for breast cancer patients to prevent the spread of cancer within the body.
To metastasise, cancer cells must acquire the capacity to invade into their surroundings, move through tissues and vasculature, and colonise distant sites in the body. This requires activation of cellular pathways that promote cell movement. While much has been revealed on molecular machineries that mediate cell movement, little is known about regulators of movement which become abhorrently activated during metastasis. Recent works by me and other have revealed that an unexpected group of cellular proteins, called RNA Binding Proteins (RBPs), can promote cancer cell movement and invasion, ultimately leading to metastasis. However, it is unclear how different RBPs function to promote the movement of cancer cells, and more importantly, whether they could be targeted to tackle metastasis.
My research aims to reveal which RBPs are involved in regulating different aspects of cancer cell movement, cancer invasion, and ultimately metastasis in breast cancer. I will use cutting edge methodologies that I have been developing and using during my previous work, to systematically assess which RBPs are linked to the movement and metastasis of breast cancer cells. I will then assess how these RBPs are promoting movement and metastasis at the molecular level. Ultimately, such molecular level understanding of the processes that control cancer cell movement and metastasis may be useful for designing novel drugs to intervene in the metastatic process.
To metastasise, cancer cells must acquire the capacity to invade into their surroundings, move through tissues and vasculature, and colonise distant sites in the body. This requires activation of cellular pathways that promote cell movement. While much has been revealed on molecular machineries that mediate cell movement, little is known about regulators of movement which become abhorrently activated during metastasis. Recent works by me and other have revealed that an unexpected group of cellular proteins, called RNA Binding Proteins (RBPs), can promote cancer cell movement and invasion, ultimately leading to metastasis. However, it is unclear how different RBPs function to promote the movement of cancer cells, and more importantly, whether they could be targeted to tackle metastasis.
My research aims to reveal which RBPs are involved in regulating different aspects of cancer cell movement, cancer invasion, and ultimately metastasis in breast cancer. I will use cutting edge methodologies that I have been developing and using during my previous work, to systematically assess which RBPs are linked to the movement and metastasis of breast cancer cells. I will then assess how these RBPs are promoting movement and metastasis at the molecular level. Ultimately, such molecular level understanding of the processes that control cancer cell movement and metastasis may be useful for designing novel drugs to intervene in the metastatic process.
Technical Summary
My aim is to assess the mechanisms by which invasiveness and metastatic behaviour is regulated via different RNA Binding Proteins (RBPs) in breast cancer cells. While much has been revealed on molecular machineries that control cell motility, little is known about upstream regulators of motility which are deregulated during metastasis. Recent works by me and others have highlighted a crucial role for regulation of local mRNA translation in controlling cell protrusions and adhesions. Accordingly, various RBPs have been reported to localise to such motility related compartments and control cell-migration, invasion, and metastasis. However, it is unclear how different RBPs function to regulate cell motility, and whether their activity could be targeted to tackle cancer dissemination.
I will use sub-cellular fractionation coupled with proteomics to reveal RBPs that associate with specific motility related compartments in invasive breast cancer cells. Using RNAi in combination with morphology, migration, and invasion assays, I will reveal key RBPs that regulate breast cancer cell motility in-vitro. RBP roles in-vivo, in regulation of local invasion to lymph nodes and distant metastasis will then be assessed using orthotopic mouse models. Using fractionation coupled with RNAseq and pulse-labelling proteomics, I will investigate how loss of RBPs affects RNA localisation and local translation in motility associated cellular compartments where RBPs are localised. Through analysis of UTR sequence elements, along with methods to assess mRNA-protein binding, I will determine the mechanisms of interaction between RBPs and their local target mRNAs. Finally through mutagenesis, I will abrogate mRNA-RBP bindings and assess the impact on invasiveness and metastasis. Showing that specific RBP-mRNA interactions can impact on invasiveness and metastatic potential may lead to devising new therapeutic strategies to tackle cancer dissemination by disrupting such interactions.
I will use sub-cellular fractionation coupled with proteomics to reveal RBPs that associate with specific motility related compartments in invasive breast cancer cells. Using RNAi in combination with morphology, migration, and invasion assays, I will reveal key RBPs that regulate breast cancer cell motility in-vitro. RBP roles in-vivo, in regulation of local invasion to lymph nodes and distant metastasis will then be assessed using orthotopic mouse models. Using fractionation coupled with RNAseq and pulse-labelling proteomics, I will investigate how loss of RBPs affects RNA localisation and local translation in motility associated cellular compartments where RBPs are localised. Through analysis of UTR sequence elements, along with methods to assess mRNA-protein binding, I will determine the mechanisms of interaction between RBPs and their local target mRNAs. Finally through mutagenesis, I will abrogate mRNA-RBP bindings and assess the impact on invasiveness and metastasis. Showing that specific RBP-mRNA interactions can impact on invasiveness and metastatic potential may lead to devising new therapeutic strategies to tackle cancer dissemination by disrupting such interactions.
Planned Impact
Academia:
The findings of this research proposal are likely to be of interest to scientist across various different disciplines, both in basic and applied research fields, within the UK and abroad. In addition to cancer biologists, academics in basic research fields studying RNA biology are likely to benefit from the results of this research. Other target academics include developmental biologists and neurobiologist who study the role of RBPs in various different normal or pathological contexts. Many of the RBPs that seem to be associated with cell-motility are also known have roles in development and maintenance of the nervous system, with a number of them having been implicated in neuronal disorders, such as Fragile-X mental retardation and amyotrophic lateral sclerosis (ALS). Thus, findings of this proposal are likely to be of great interest to these scientists, as well as those within the immediate related fields of my research.
Industry:
Apart from benefiting academics, findings of this proposal may pave the way for pharmaceutical companies to devise novel therapeutic strategies that tackle cancer cell motility through the use of RNA therapeutics. Specifically, my research will reveal the molecular details of interactions between certain RBPs and their target mRNAs that mediate RBP effects on cancer cell motility. Such data can be used to design RNA mimicking compounds that can interfere with the RBP-mRNA interactions, in order to inhibit cancer cell movement. Efforts to target RBP-mRNA interactions through use of our findings may not be limited to cancer therapeutics, and could be also useful for pharmaceutical companies which are active in developing drugs for different neuronal disorders, since as mentioned above, a number of RBPs associated with motility also seem to be important players in certain neuronal disorders. Crucially, latest advances in RNA therapeutics, particularly the recent development of small molecules that sterically interfere with certain protein-RNA interactions, suggests that there is likely to be great potential for clinical targeting of RBPs in the near future.
General Public:
Ultimately, if this study contributes towards development of novel therapies that target breast cancer metastasis, the general public will be the main beneficiary in the long run. Metastasis remains the major cause of death due to breast cancer, and currently no specific therapies that target metastasis exists in the clinic. Also, as mentioned above, knowledge generated from this work may also lead to devising novel treatments for certain neuronal disorders, ultimately benefiting public health.
The findings of this research proposal are likely to be of interest to scientist across various different disciplines, both in basic and applied research fields, within the UK and abroad. In addition to cancer biologists, academics in basic research fields studying RNA biology are likely to benefit from the results of this research. Other target academics include developmental biologists and neurobiologist who study the role of RBPs in various different normal or pathological contexts. Many of the RBPs that seem to be associated with cell-motility are also known have roles in development and maintenance of the nervous system, with a number of them having been implicated in neuronal disorders, such as Fragile-X mental retardation and amyotrophic lateral sclerosis (ALS). Thus, findings of this proposal are likely to be of great interest to these scientists, as well as those within the immediate related fields of my research.
Industry:
Apart from benefiting academics, findings of this proposal may pave the way for pharmaceutical companies to devise novel therapeutic strategies that tackle cancer cell motility through the use of RNA therapeutics. Specifically, my research will reveal the molecular details of interactions between certain RBPs and their target mRNAs that mediate RBP effects on cancer cell motility. Such data can be used to design RNA mimicking compounds that can interfere with the RBP-mRNA interactions, in order to inhibit cancer cell movement. Efforts to target RBP-mRNA interactions through use of our findings may not be limited to cancer therapeutics, and could be also useful for pharmaceutical companies which are active in developing drugs for different neuronal disorders, since as mentioned above, a number of RBPs associated with motility also seem to be important players in certain neuronal disorders. Crucially, latest advances in RNA therapeutics, particularly the recent development of small molecules that sterically interfere with certain protein-RNA interactions, suggests that there is likely to be great potential for clinical targeting of RBPs in the near future.
General Public:
Ultimately, if this study contributes towards development of novel therapies that target breast cancer metastasis, the general public will be the main beneficiary in the long run. Metastasis remains the major cause of death due to breast cancer, and currently no specific therapies that target metastasis exists in the clinic. Also, as mentioned above, knowledge generated from this work may also lead to devising novel treatments for certain neuronal disorders, ultimately benefiting public health.
People |
ORCID iD |
| Faraz Mardakheh (Principal Investigator / Fellow) |
Publications
Adams SD
(2021)
Centrosome amplification mediates small extracellular vesicle secretion via lysosome disruption.
in Current biology : CB
D'Amico G
(2022)
ERG activity is regulated by endothelial FAK coupling with TRIM25/USP9x in vascular patterning.
in Development (Cambridge, England)
Dermit M
(2017)
Methods for monitoring and measurement of protein translation in time and space.
in Molecular bioSystems
Dermit M
(2021)
Purification and quantitative proteomic analysis of cell bodies and protrusions.
in STAR protocols
Dermit M
(2020)
Subcellular mRNA Localization Regulates Ribosome Biogenesis in Migrating Cells.
in Developmental cell
Fish L
(2021)
A prometastatic splicing program regulated by SNRPA1 interactions with structured RNA elements.
in Science (New York, N.Y.)
Hau HTA
(2020)
Maternal Larp6 controls oocyte development, chorion formation and elevation.
in Development (Cambridge, England)
Khoroshkin M
(2023)
Systematic Identification of Post-Transcriptional Regulatory Modules
| Description | BBSRC Lido PhD studentship |
| Amount | £100,000 (GBP) |
| Organisation | Biotechnology and Biological Sciences Research Council (BBSRC) |
| Sector | Public |
| Country | United Kingdom |
| Start | 09/2020 |
| End | 09/2023 |
| Description | Barts Cancer Institute Incentivisation Award |
| Amount | £106,200 (GBP) |
| Organisation | Queen Mary University of London |
| Department | Barts Cancer Institute |
| Sector | Academic/University |
| Country | United Kingdom |
| Start | 10/2018 |
| End | 10/2021 |
| Description | Deciphering a novel interplay between RNA and chromatin |
| Amount | £634,167 (GBP) |
| Funding ID | BB/X007820/1 |
| Organisation | Biotechnology and Biological Sciences Research Council (BBSRC) |
| Sector | Public |
| Country | United Kingdom |
| Start | 04/2023 |
| End | 10/2026 |
| Description | Deciphering the role of RNA localisation in cancer progression |
| Amount | £465,334 (GBP) |
| Funding ID | MR/W001500/1 |
| Organisation | Medical Research Council (MRC) |
| Sector | Public |
| Country | United Kingdom |
| Start | 10/2021 |
| End | 10/2024 |
| Description | Mass spectrometry system for sensitive proteomics |
| Amount | £780,011 (GBP) |
| Funding ID | MR/X013766/1 |
| Organisation | Medical Research Council (MRC) |
| Sector | Public |
| Country | United Kingdom |
| Start | 11/2022 |
| End | 03/2023 |
| Description | Proteomics mass spectrometry for the Barts Post-Genomic Phenotype Unit |
| Amount | £371,265 (GBP) |
| Funding ID | MGU0346 |
| Organisation | Barts Charity |
| Sector | Charity/Non Profit |
| Country | United Kingdom |
| Start | 02/2017 |
| End | 02/2020 |
| Title | Cross-linking and subcellular fractionation-RNA sequencing (CLIF-seq) |
| Description | In collaboration with Professor Jernej Ule at the Crick, we have devised a novel method to assess subcellular RNA Binding Protein (RBPs)-bound RNAs by combining UV-cross-linking of RNA molecules to RBPs, and then performing subcellular fractionation followed by next generation RNA-sequencing in order to identify and quantify the bound RNAs. Our approach allows capturing even transiently associated RNAs in specific subcellular compartments. We have now performed several successful analyses of the the subcellular transcriptome using this method, by performing whole transcriptome sequencing of subcellularly purified RNAs, as well as carrying out proteomics analysis of the same subcellular compartment, from various normal and malignant cell-lines |
| Type Of Material | Technology assay or reagent |
| Year Produced | 2018 |
| Provided To Others? | No |
| Impact | So far, this method has allowed us to comprehensively assess subcellularly localised RBP bound RNAs as part of our project. |
| Title | Quantitative mass spectormetry for subcellular proteome analysis |
| Description | Since the commencing of the award, we have purchased a new mass-spectrometer (Thermo Q-Exactive plus) using funding from Barts Charity (see additional funds section), installed and successfully setup the methodologies needed for sample preparation and mass spectrometry analysis of our samples using two different quantitative proteomics approaches (SILAC and TMT). We have successfully applied our optimised proteomics pipeline to our project using TMT 11-plexing (which allows mixing and quantification of up to 11 samples in a single run). This was done as part of the beta testing of the TMT 11-plex kit from Thermo Fisher, as the 11-plex kit was not yet released to the public at the time we established it in our lab. |
| Type Of Material | Technology assay or reagent |
| Year Produced | 2017 |
| Provided To Others? | No |
| Impact | Using our proteomics pipeline in conjugation with TMT, we have successfully profiled the subcellular proteomes of various breast cancer cell-lines and have been able to match these with the analysis of RNA, in order to identify RBPs that are specifically enriched in protrusions of more invasive cells. |
| Title | Ribopuroycinylation coupled with FISH (RPF) |
| Description | To quantitatively assess how much individual mRNA molecules undergo translation in specific subcellular locations, we have devised a novel method by combining single molecule RNA-FISH with Ribopuromycinylation. Ribopuromycinylation is an established method that utilises puromycin labelling coupled with Emetine (a translation elongation inhibitor) treatment to fix and label nascent polypeptides associated with ribosomes and later detect them by immunofluorescence using an anti puromycin antibody. So far, Ribopuromycinylation has not been compatible with RNA-FISH (in fact the original protocol even recommend degradation of all RNAs by RNase treatment to enhance puromycin signal). We have now modified the protocol such that it can be combined with single molecule RNA-FISH, thus enabling two colour labelling and colocalisation analysis between individual mRNA molecules and ribosome associated nascent polypeptides. This allows estimation of the level of translation for each individual mRNA in fixed samples. We are currently in the process of bench-marking this method using various FISH probes. |
| Type Of Material | Technology assay or reagent |
| Year Produced | 2019 |
| Provided To Others? | No |
| Impact | This method allows user to estimate the translational output of each detected mRNA molecule simply by doing puromycinylation 5 minutes before fixation and RNA-FISH analysis. This powerful method can be applied to any mRNA so we expect it to be useful to many scientists from diverse fields of research. As part of this award, we will utilise this method to systematically assess if various different subcellularly localised mRNAs undergo translation under different conditions. |
| Title | Database of protein and RNA distributions across protrusions and cell-bodies in 6 different cell-lines |
| Description | As part of our recent publication (DOI: https://doi.org/10.1016/j.devcel.2020.10.006), we generated a vast database of spatial RNA-seq and proteomics, quantifying the cellular distribution of proteins and mRNAs between actin-rich protrusions and cell-bodies of 6 different normal and malignant human cell-lines. This data can be accessed through a web portal that we have generated: http://www.mardakhehlab.info/resources/index |
| Type Of Material | Database/Collection of data |
| Year Produced | 2020 |
| Provided To Others? | Yes |
| Impact | This dataset is an invaluable resource for scientist interested in subcellular RNA localisation, allowing them to map distribution of any RNA of interest, along with its encoded protein, across 6 different cell-lines. |
| URL | http://www.mardakhehlab.info/resources/index |
| Title | Global subcellular RNA and protein enrichment database. |
| Description | Using our quantitative proteomics and RNA-seq methodologies, we have been analysing a panel of breast cancer cell-lines, quantifying the subcellular enrichment patterns of all detected mRNAs and proteins in all subcellular compartments (including cell-protrusions). The proteomics dataset is being generated in house while the RNA-seq set is being generated as part of our collaboration with Prof. Jernej Ule. This dataset is being expanded as we profile more cells. |
| Type Of Material | Database/Collection of data |
| Year Produced | 2018 |
| Provided To Others? | No |
| Impact | Although this dataset is still incomplete, it has already provided us with ample valuable information for our project. In particular, we have mapped the localisation of all cellular RBPs, revealing the ones that are enriched in protrusions across multiple cell-lines, which is directly relevant to the aim 1 of our award. We are now in process of functionally assessing some of the conserved RBPs across different cell-lines, and investigating the roles in cell-migration. |
| Description | Collaboration with Dr Hani Goodarzi, UCSF, USA |
| Organisation | University of California, San Francisco |
| Department | Helen Diller Family Comprehensive Cancer Center |
| Country | United States |
| Sector | Academic/University |
| PI Contribution | We have formed a collaboration with Dr Hani Goodarzi's group at UCSF, San Francisco, in our wider efforts of studying RNA Binding Proteins in Cancer. This collaboration involves us providing Dr Goodarzi's team with our expertise in mass spectrometry to study RBP contributions to various cancers. Our collaborations with Dr goodarzi's team has already resulted in two publications in prestigious journals of Cancer Discovery and Science, with a third manuscript currently in revision in Nature Cell Biology. |
| Collaborator Contribution | In return, Dr Goodarzi's team has been providing us with their expertise in analysis of tumour growth and metastasis in mice. In addition, Dr Goodarzi's team has been assisting us in computational analysis of RNA motifs, for which they have established several cutting-edge methodologies. |
| Impact | This collaboration has so far resulted in two publications, in Cancer Discovery (DOI: 10.1158/2159-8290.CD-19-1375) and Science (DOI: 10.1126/science.abc7531), with a third manuscript currently in revision in Nature Cell Biology. |
| Start Year | 2019 |
| Description | Collaboration with Prof. Jernej Ule |
| Organisation | Francis Crick Institute |
| Country | United Kingdom |
| Sector | Academic/University |
| PI Contribution | A Bi-lateral collaboration has been formed with Professor Jernej Ule at the Crick Institute. This was suggested by one of the reviewers of my grant application, as professor Ule is a leading expert in study of RNA-Protein interactions. We have been performing proteomics runs and data analysis for professor Ule's group in return. |
| Collaborator Contribution | In return, professor Ule's lab has been heavily assisting us with the design and optimisation of our ICLIP experiments, as well as cross-linking and fractionation RNA-sequencing analyses. They have also been carrying out our next-generation sequencing runs at the Crick. The crosslinking and fractionation RNA-sequencing analyses directly led to an MRC project grant (The role of RNA localisation in cancer progression), providing the bulk of preliminary data for this application. |
| Impact | 1 - Comprehensive proteomics analysis of subcellular compartments in cells lacking HuR and Staufen (Prof. Ule's project). 2- Optimisation of cross-linking procedure for assessment of subcellular RNA bound by RBPs (our project - ongoing with project further supported by an MRC project grant awarded in 2020). 3- comprehensive RNA-seq analysis of subcellularly localised RBP-bound RNAs by UV cross-linking and RNA-sequencing (our project - ongoing). 4- iCLIP analysis of LARP6 as part of our project, which led to a joint publication in Developmental Cell (doi: 10.1016/j.devcel.2020.10.006). 5- iCLIP analysis of Nucleolin as part of our project, which led to a joint preprint (doi: https://doi.org/10.1101/2021), currently accepted in EMBO Journal. |
| Start Year | 2017 |
| Description | Collaboration with Prof. Sasi Conte, Kings College London |
| Organisation | King's College London |
| Department | Randall Division of Cell & Molecular Biophysics |
| Country | United Kingdom |
| Sector | Academic/University |
| PI Contribution | In collaboration with Prof. Conte at Kings College, we managed to secure a BBSRC Lido studentship on LARP6 RNA Binding properties. Our joint student (Ms Federica Capraro) has started her first year of PhD studies from September 2020, and will work on deciphering the RNA binding properties of the LARP6 protein using a multi-disciplinary approach. From our part, we will train Federica to perform various omics analysis to characterise the global targets of LARP6, its interactome, and its functional impact on cancer cell proliferation and migration. |
| Collaborator Contribution | On Prof. Conte's side, they will train Federica to perform various structural (e.g. NMR, CD) and biophysical analyses (e.g. EMSA, ITC) to reveal the molecular mechanisms involved in LARP6 RNA target recognition. |
| Impact | So far, the project has resulted in mapping all RNA binding regions of LARP6, revealing two novel RNA interacting regions within the N-terminal and C-terminal of the protein. We are currently working to characterise the contribution of each region to RNA substrate recognition of LARP6 using biophysical approaches. |
| Start Year | 2020 |
| Description | Collaboration with Prof. Simon Hughes and Prof. Maria Conte on LARP6 role in Zebrafish development |
| Organisation | King's College London |
| Department | Randall Division of Cell & Molecular Biophysics |
| Country | United Kingdom |
| Sector | Academic/University |
| PI Contribution | In this collaboration, we contributed with our expertise in proteomics and our knowledge from work on mammalian LARP6 proteins towards a research project on characterising the role of LARP6 proteins in zebrafish development. Specifically, we used quantitative proteomics to analyse Chorions of fish from either maternally wt or knockout fish for Larp6a and Larp6b. |
| Collaborator Contribution | The bulk of the study was carried out by members of Hughes and Conte labs, including generation of the knockout fish, and description of the phenotype. |
| Impact | The collaboration led to a publication in the journal of Development: https://dev.biologists.org/content/147/4/dev187385 |
| Start Year | 2019 |
| Description | School science workshop (Dallington School, London) |
| Form Of Engagement Activity | Participation in an activity, workshop or similar |
| Part Of Official Scheme? | No |
| Geographic Reach | Local |
| Primary Audience | Schools |
| Results and Impact | I ran a DNA workshop for ~30 primary school children in which I first gave a presentation about what DNA is, and why it is important for scientists. This was followed by a practical demonstration of purifying DNA from saliva (Ethanol precipitation). The activity really sparked the curiosity of the students and they asked many questions about DNA and genes. I got a very positive feedback from both the teachers as well as many of the parents who had later heard about the demostration from their children. |
| Year(s) Of Engagement Activity | 2019 |
| Description | School visit (Dallington School, London) |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | Regional |
| Primary Audience | Schools |
| Results and Impact | I talked to ~30 primary school children about bacteria, immune cells, and how our bodies fight infection. The presentation included a number of videos (one of bacteria dividing, the other a Neurtrophil chasing a bacterium - taken by the late David Rogers at Vanderbilt University). I then showed the children some agar plates and performed a little experiment in which I touched one plate with a dirty hand and the other with a clean hand. The plates were then left at room temperature for a few days and we then observed colonies of bacteria growing only on the plate touched by the dirty hand. The children were fascinated by the video of neutrophil chasing the bacterium, and also by the experiment we did. The activity sparked many questions about the immune system and micro-organisms. Interestingly, many children were also very interested about the job scientists do and asked many questions about what being a scientists involves. Later on, I got a lot of positive feedback from the teachers as well as many of the parents who let me know that their kids were fascinated about this experience and kept talking about it. |
| Year(s) Of Engagement Activity | 2019 |