Your search keyword '"Martin Clynes"' showing total 373 results

1. Detection of host cell microprotein impurities in antibody drug products

Author

Ioanna Tzani, Marina Castro-Rivadeneyra, Paul Kelly, Lisa Strasser, Lin Zhang, Martin Clynes, Barry L. Karger, Niall Barron, Jonathan Bones, and Colin Clarke

Subjects

Science

Abstract

Abstract Chinese hamster ovary (CHO) cells are used to produce almost 90% of therapeutic monoclonal antibodies (mAbs) and antibody fusion proteins (Fc-fusion). The annotation of non-canonical translation events in these cellular factories remains incomplete, limiting our ability to study CHO cell biology and detect host cell protein (HCP) impurities in the final antibody drug product. We utilised ribosome footprint profiling (Ribo-seq) to identify novel open reading frames (ORFs) including N-terminal extensions and thousands of short ORFs (sORFs) predicted to encode microproteins. Mass spectrometry-based HCP analysis of eight commercial antibody drug products (7 mAbs and 1 Fc-fusion protein) using the extended protein sequence database revealed the presence of microprotein impurities. We present evidence that microprotein abundance varies with growth phase and can be affected by the cell culture environment. In addition, our work provides a vital resource to facilitate future studies of non-canonical translation and the regulation of protein synthesis in CHO cell lines.

Published

2024

2. miRNA- and Cell Line-Specific Constraints on Precursor miRNA Processing of Stably Transfected Pancreatic Cancer and Other Mammalian Cells

Author

Taylor J. Allen-Coyle, Berta Capella Roca, Alan Costello, Niall Barron, Joanne Keenan, Martin Clynes, Fiona O’Neill, and Finbarr O’Sullivan

Subjects

vector design, miRNA processing, precursor miRNA, stable transfections, miRNAs, pancreatic cancer, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

MicroRNAs (miRNAs) regulate approximately one-third of all human genes. The dysregulation of miRNAs has been implicated in the development of numerous human diseases, including cancers. In our investigation focusing on altering specific miRNA expression in human pancreatic cancer cells, we encountered an interesting finding. While two expression vector designs effectively enhanced miR-708 levels, they were unable to elevate mature forms of miR-29b, -1290, -2467, and -6831 in pancreatic cancer cell lines. This finding was also observed in a panel of other non-pancreatic cancer cell lines, suggesting that miRNA processing efficiency was cell line specific. Using a step-by-step approach in each step of miRNA processing, we ruled out alternative strand selection by the RISC complex and transcriptional interference at the primary miRNA (pri-miRNA) level. DROSHA processing and pri-miRNA export from the nucleus also appeared to be occurring normally. We observed precursor (pre-miRNA) accumulation only in cell lines where mature miRNA expression was not achieved, suggesting that the block was occurring at the pre-miRNA stage. To further confirm this, synthetic pre-miRNA mimics that bypass DICER processing were processed into mature miRNAs in all cases. This study has demonstrated the distinct behaviours of different miRNAs with the same vector in the same cell line, the same miRNA between the two vector designs, and with the same miRNA across different cell lines. We identified a stable vector pre-miRNA processing block. Our findings on the structural and sequence differences between successful and non-successful vector designs could help to inform future chimeric miRNA design strategies and act as a guide to other researchers on the intricate processing dynamics that can impact vector efficiency. Our research confirms the potential of miRNA mimics to surmount some of these complexities.

Published

2024

3. Correction: PP2A inhibition overcomes acquired resistance to HER2 targeted therapy

Author

Martina S. J. McDermott, Brigid C. Browne, Neil T. Conlon, Neil A. O’Brien, Dennis J. Slamon, Michael Henry, Paula Meleady, Martin Clynes, Paul Dowling, John Crown, and Norma O’Donovan

Subjects

Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Published

2023

4. Mapping the molecular basis for growth related phenotypes in industrial producer CHO cell lines using differential proteomic analysis

Author

Laura Bryan, Michael Henry, Ronan M. Kelly, Christopher C. Frye, Matthew D. Osborne, Martin Clynes, and Paula Meleady

Subjects

Chinese hamster ovary (CHO) cells, Label free quantitative proteomics, Cell specific productivity (Qp), Viable cell density (VCD) biopharmaceuticals, Biotechnology, TP248.13-248.65

Abstract

Abstract Background The ability to achieve high peak viable cell density earlier in CHO cell culture and maintain an extended cell viability throughout the production process is highly desirable to increase recombinant protein yields, reduce host cell impurities for downstream processing and reduce the cost of goods. In this study we implemented label-free LC-MS/MS proteomic profiling of IgG4 producing CHO cell lines throughout the duration of the cell culture to identify differentially expressed (DE) proteins and intracellular pathways associated with the high peak viable cell density (VCD) and extended culture VCD phenotypes. Results We identified key pathways in DNA replication, mitotic cell cycle and evasion of p53 mediated apoptosis in high peak VCD clonally derived cell lines (CDCLs). ER to Golgi vesicle mediated transport was found to be highly expressed in extended culture VCD CDCLs while networks involving endocytosis and oxidative stress response were significantly downregulated. Conclusion This investigation highlights key pathways for targeted engineering to generate desirable CHO cell phenotypes for biotherapeutic production.

Published

2021

5. Global phosphoproteomic study of high/low specific productivity industrially relevant mAb producing recombinant CHO cell lines

Author

Laura Bryan, Michael Henry, Ronan M. Kelly, Michael Lloyd, Christopher C. Frye, Matthew D. Osborne, Martin Clynes, and Paula Meleady

Subjects

Chinese hamster ovary (CHO) cells, Label free quantitative proteomics, Phosphoproteomics, Cell specific productivity (Qp), Biopharmaceuticals, Biotechnology, TP248.13-248.65

Abstract

Understanding the biology of CHO cells at a cellular level is extremely valuable to the pharmaceutical industry, as it presents the opportunity to rationally engineer clonally derived cell lines (CDCLs) with elevated recombinant specific productivity (Qp). To date, relatively little is understood about the intracellular pathways which influence desirable phenotypes in CHO cell lines. In this study we identified phosphoproteins and total proteins which are differentially expressed between high and low Qp IgG4 producing industry CHO cell lines, some of which upon further investigation, could potentially be used as targets to engineer high Qp CDCLs. We highlighted the importance of phosphoproteins and total proteins associated with amino acid sensing in high Qp cell lines. We also identified increased expression of proteins which promote progression through the cell cycle in low Qp cell lines, suggesting that lower Qp CDCLs are focusing their translational machinery on translating cell cycle associated mRNAs.

Published

2021

6. Alteration in Levels of Specific miRNAs and Their Potential Protein Targets between Human Pancreatic Cancer Samples, Adjacent Normal Tissue, and Xenografts Derived from These Tumors

Author

Fiona O’Neill, Taylor-Jade Allen-Coyle, Sandra Roche, Justine Meiller, Neil T. Conlon, Niall Swan, Robert M. Straubinger, Justin Geoghegan, Ninfa L. Straubinger, Kevin Conlon, Ray McDermott, Finbarr O’Sullivan, Michael Henry, Paula Meleady, Gerard McVey, Robert O’Connor, Michael Moriarty, and Martin Clynes

Subjects

pancreatic cancer, miRNA, PDX, tumour, Science

Abstract

Herein, we describe the global comparison of miRNAs in human pancreatic cancer tumors, adjacent normal tissue, and matched patient-derived xenograft models using microarray screening. RNA was extracted from seven tumor, five adjacent normal, and eight FI PDX tumor samples and analyzed by Affymetrix GeneChip miRNA 4.0 array. A transcriptome analysis console (TAC) was used to generate comparative lists of up- and downregulated miRNAs for the comparisons, tumor vs. normal and F1 PDX vs. tumor. Particular attention was paid to miRNAs that were changed in the same direction in both comparisons. We identified the involvement in pancreatic tumor tissue of several miRNAs, including miR4534, miR3154, and miR4742, not previously highlighted as being involved in this type of cancer. Investigation in the parallel mRNA and protein lists from the same samples allowed the elimination of proteins where altered expression correlated with corresponding mRNA levels and was thus less likely to be miRNA regulated. Using the remaining differential expression protein lists for proteins predicted to be targeted for differentially expressed miRNA on our list, we were able to tentatively ascribe specific protein changes to individual miRNA. Particularly interesting target proteins for miRs 615-3p, 2467-3p, 4742-5p, 509-5p, and 605-3p were identified. Prominent among the protein targets are enzymes involved in aldehyde metabolism and membrane transport and trafficking. These results may help to uncover vulnerabilities that could enable novel approaches to treating pancreatic cancer.

Published

2023

7. Yeast Mannan-Rich Fraction Modulates Endogenous Reactive Oxygen Species Generation and Antibiotic Sensitivity in Resistant E. coli

Author

Helen Smith, Sharon Grant, Paula Meleady, Michael Henry, Donal O’Gorman, Martin Clynes, and Richard Murphy

Subjects

antimicrobial resistance, yeast mannan fraction, bacterial metabolism, antibiotic susceptibility, reactive oxygen species, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

Mannan-rich fraction (MRF) isolated from Saccharomyces cerevisiae has been studied for its beneficial impact on animal intestinal health. Herein, we examined how MRF affected the formation of reactive oxygen species (ROS), impacting antibiotic susceptibility in resistant Escherichia coli through the modulation of bacterial metabolism. The role of MRF in effecting proteomic change was examined using a proteomics-based approach. The results showed that MRF, when combined with bactericidal antibiotic treatment, increased ROS production in resistant E. coli by 59.29 ± 4.03% compared to the control (p ≤ 0.05). We further examined the effect of MRF alone and in combination with antibiotic treatment on E. coli growth and explored how MRF potentiates bacterial susceptibility to antibiotics via proteomic changes in key metabolic pathways. Herein we demonstrated that MRF supplementation in the growth media of ampicillin-resistant E. coli had a significant impact on the normal translational control of the central metabolic pathways, including those involved in the glycolysis–TCA cycle (p ≤ 0.05).

Published

2022

8. Label-Free Quantitative Proteomics Analysis of Adriamycin Selected Multidrug Resistant Human Lung Cancer Cells

Author

Esen Efeoglu, Michael Henry, Martin Clynes, and Paula Meleady

Subjects

drug resistance, DLKP, label-free quantitative proteomics, lipid metabolism, ABC transporters, response to drug, Microbiology, QR1-502

Abstract

The development of drug resistance in lung cancer is a major clinical challenge, leading to a 5-year survival rate of only 18%. Therefore, unravelling the mechanisms of drug resistance and developing novel therapeutic strategies is of crucial importance. This study systematically explores the novel biomarkers of drug resistance using a lung cancer model (DLKP) with a series of drug-resistant variants. In-depth label-free quantitative mass spectrometry-based proteomics and gene ontology analysis shows that parental DLKP cells significantly differ from drug-resistant variants, and the cellular proteome changes even among the drug-resistant subpopulations. Overall, ABC transporter proteins and lipid metabolism were determined to play a significant role in the formation of drug resistance in DKLP cells. A series of membrane-related proteins such as HMOX1, TMB1, EPHX2 and NEU1 were identified to be correlated with levels of drug resistance in the DLKP subpopulations. The study also showed enrichment in biological processes and molecular functions such as drug metabolism, cellular response to the drug and drug binding. In gene ontology analysis, 18 proteins were determined to be positively or negatively correlated with resistance levels. Overall, 34 proteins which potentially have a therapeutic and diagnostic value were identified.

Published

2022

9. A proteomic profiling dataset of recombinant Chinese hamster ovary cells showing enhanced cellular growth following miR-378 depletion

Author

Orla Coleman, Alan Costello, Michael Henry, Nga T. Lao, Niall Barron, Martin Clynes, and Paula Meleady

Subjects

Computer applications to medicine. Medical informatics, R858-859.7, Science (General), Q1-390

Abstract

The proteomic data presented in this article provide supporting information to the related research article ''Depletion of endogenous miRNA-378-3p increases peak cell density of CHO DP12 cells and is correlated with elevated levels of Ubiquitin Carboxyl-Terminal Hydrolase 14'' (Costello et al., in press) [1]. Control and microRNA-378 depleted CHO DP12 cells were profiled using label-free quantitative proteomic profiling. CHO DP12 cells were collected on day 4 and 8 of batch culture, subcellular proteomic enrichment was performed, and subsequent fractions were analyzed by liquid chromatography tandem mass spectrometry (LC-MS/MS). Here we provide the complete proteomic dataset of proteins significantly differentially expressed by greater than 1.25-fold change in abundance between control and miR-378 depleted CHO DP12 cells, and the lists of all identified proteins for each condition.

Published

2018

10. Neutrophil Membrane Cholesterol Content is a Key Factor in Cystic Fibrosis Lung Disease

Author

Michelle M. White, Patrick Geraghty, Elaine Hayes, Stephen Cox, William Leitch, Bader Alfawaz, Gillian M. Lavelle, Oliver J. McElvaney, Ryan Flannery, Joanne Keenan, Paula Meleady, Michael Henry, Martin Clynes, Cedric Gunaratnam, Noel G. McElvaney, and Emer P. Reeves

Subjects

Cystic fibrosis, Neutrophils, Cholesterol, Lung transplant therapy, Ivacaftor therapy, Medicine, Medicine (General), R5-920

Abstract

Background: Identification of mechanisms promoting neutrophil trafficking to the lungs of patients with cystic fibrosis (CF) is a challenge for next generation therapeutics. Cholesterol, a structural component of neutrophil plasma membranes influences cell adhesion, a key step in transmigration. The effect of chronic inflammation on neutrophil membrane cholesterol content in patients with CF (PWCF) remains unclear. To address this we examined neutrophils of PWCF to evaluate the cause and consequence of altered membrane cholesterol and identified the effects of lung transplantation and ion channel potentiator therapy on the cellular mechanisms responsible for perturbed membrane cholesterol and increased cell adhesion. Methodology: PWCF homozygous for the ΔF508 mutation or heterozygous for the G551D mutation were recruited (n = 48). Membrane protein expression was investigated by mass spectrometry. The effect of lung transplantation or ivacaftor therapy was assessed by ELISAs, and calcium fluorometric and μ-calpain assays. Findings: Membranes of CF neutrophils contain less cholesterol, yet increased integrin CD11b expression, and respond to inflammatory induced endoplasmic reticulum (ER) stress by activating μ-calpain. In vivo and in vitro, increased μ-calpain activity resulted in proteolysis of the membrane cholesterol trafficking protein caveolin-1. The critical role of caveolin-1 for adequate membrane cholesterol content was confirmed in caveolin-1 knock-out mice. Lung transplant therapy or treatment of PWCF with ivacaftor, reduced levels of circulating inflammatory mediators and actuated increased caveolin-1 and membrane cholesterol, with concurrent normalized neutrophil adhesion. Interpretation: Results demonstrate an auxiliary benefit of lung transplant and potentiator therapy, evident by a reduction in circulating inflammation and controlled neutrophil adhesion.

Published

2017

11. Establishment and Characterisation by Expression Microarray of Patient-Derived Xenograft Panel of Human Pancreatic Adenocarcinoma Patients

Author

Sandra Roche, Fiona O’Neill, Jean Murphy, Niall Swan, Justine Meiller, Neil T. Conlon, Justin Geoghegan, Kevin Conlon, Ray McDermott, Rozana Rahman, Sinead Toomey, Ninfa L. Straubinger, Robert M. Straubinger, Robert O’Connor, Gerard McVey, Michael Moriarty, and Martin Clynes

Subjects

pancreatic cancer, patient-derived xenograft, microarray, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

Pancreatic cancer remains among the most lethal cancers worldwide, with poor early detection rates and poor survival rates. Patient-derived xenograft (PDX) models have increasingly been used in preclinical and clinical research of solid cancers to fulfil unmet need. Fresh tumour samples from human pancreatic adenocarcinoma patients were implanted in severe combined immunodeficiency (SCID) mice. Samples from 78% of treatment-naïve pancreatic ductal adenocarcinoma patients grew as PDX tumours and were confirmed by histopathology. Frozen samples from F1 PDX tumours could be later successfully passaged in SCID mice to F2 PDX tumours. The human origin of the PDX was confirmed using human-specific antibodies; however, the stromal component was replaced by murine cells. Cell lines were successfully developed from three PDX tumours. RNA was extracted from eight PDX tumours and where possible, corresponding primary tumour (T) and adjacent normal tissues (N). mRNA profiles of tumour vs. F1 PDX and normal vs. tumour were compared by Affymetrix microarray analysis. Differential gene expression showed over 5000 genes changed across the N vs. T and T vs. PDX samples. Gene ontology analysis of a subset of genes demonstrated genes upregulated in normal vs. tumour vs. PDX were linked with cell cycle, cycles cell process and mitotic cell cycle. Amongst the mRNA candidates elevated in the PDX and tumour vs. normal were SERPINB5, FERMT1, AGR2, SLC6A14 and TOP2A. These genes have been associated with growth, proliferation, invasion and metastasis in pancreatic cancer previously. Cumulatively, this demonstrates the applicability of PDX models and transcriptomic array to identify genes associated with growth and proliferation of pancreatic cancer.

Published

2020

12. A Comparative Quantitative LC-MS/MS Profiling Analysis of Human Pancreatic Adenocarcinoma, Adjacent-Normal Tissue, and Patient-Derived Tumour Xenografts

Author

Orla Coleman, Michael Henry, Fiona O'Neill, Sandra Roche, Niall Swan, Lorraine Boyle, Jean Murphy, Justine Meiller, Neil T. Conlon, Justin Geoghegan, Kevin C. Conlon, Vincent Lynch, Ninfa L. Straubinger, Robert M. Straubinger, Gerard McVey, Michael Moriarty, Paula Meleady, and Martin Clynes

Subjects

pancreatic cancer, proteomics, ADC therapy, PDX, membrane-enriched, Microbiology, QR1-502

Abstract

Pancreatic ductal adenocarcinoma (PDAC) is one of the deadliest cancers worldwide; it develops in a relatively symptom-free manner, leading to rapid disease progression and metastasis, leading to a 5-year survival rate of less than 5%. A lack of dependable diagnostic markers and rapid development of resistance to conventional therapies are among the problems associated with management of the disease. A better understanding of pancreatic tumour biology and discovery of new potential therapeutic targets are important goals in pancreatic cancer research. This study describes the comparative quantitative LC-MS/MS proteomic analysis of the membrane-enriched proteome of 10 human pancreatic ductal adenocarcinomas, 9 matched adjacent-normal pancreas and patient-derived xenografts (PDXs) in mice (10 at F1 generation and 10 F2). Quantitative label-free LC-MS/MS data analysis identified 129 proteins upregulated, and 109 downregulated, in PDAC, compared to adjacent-normal tissue. In this study, analysing peptide MS/MS data from the xenografts, great care was taken to distinguish species-specific peptides definitively derived from human sequences, or from mice, which could not be distinguished. The human-only peptides from the PDXs are of particular value, since only human tumour cells survive, and stromal cells are replaced during engraftment in the mouse; this list is, therefore, enriched in tumour-associated proteins, some of which might be potential therapeutic or diagnostic targets. Using human-specific sequences, 32 proteins were found to be upregulated, and 113 downregulated in PDX F1 tumours, compared to primary PDAC. Differential expression of CD55 between PDAC and normal pancreas, and expression across PDX generations, was confirmed by Western blotting. These data indicate the value of using PDX models in PDAC research. This study is the first comparative proteomic analysis of PDAC which employs PDX models to identify patient tumour cell-associated proteins, in an effort to find robust targets for therapeutic treatment of PDAC.

Published

2018

13. MiR-7 triggers cell cycle arrest at the G1/S transition by targeting multiple genes including Skp2 and Psme3.

Author

Noelia Sanchez, Mark Gallagher, Nga Lao, Clair Gallagher, Colin Clarke, Padraig Doolan, Sinead Aherne, Alfonso Blanco, Paula Meleady, Martin Clynes, and Niall Barron

Subjects

Medicine, Science

Abstract

MiR-7 acts as a tumour suppressor in many cancers and abrogates proliferation of CHO cells in culture. In this study we demonstrate that miR-7 targets key regulators of the G1 to S phase transition, including Skp2 and Psme3, to promote increased levels of p27(KIP) and temporary growth arrest of CHO cells in the G1 phase. Simultaneously, the down-regulation of DNA repair-specific proteins via miR-7 including Rad54L, and pro-apoptotic regulators such as p53, combined with the up-regulation of anti-apoptotic factors like p-Akt, promoted cell survival while arrested in G1. Thus miR-7 can co-ordinate the levels of multiple genes and proteins to influence G1 to S phase transition and the apoptotic response in order to maintain cellular homeostasis. This work provides further mechanistic insight into the role of miR-7 as a regulator of cell growth in times of cellular stress.

Published

2013

14. Resistance to paclitaxel in a cisplatin-resistant ovarian cancer cell line is mediated by P-glycoprotein.

Author

Britta Stordal, Marion Hamon, Victoria McEneaney, Sandra Roche, Jean-Pierre Gillet, John J O'Leary, Michael Gottesman, and Martin Clynes

Subjects

Medicine, Science

Abstract

The IGROVCDDP cisplatin-resistant ovarian cancer cell line is also resistant to paclitaxel and models the resistance phenotype of relapsed ovarian cancer patients after first-line platinum/taxane chemotherapy. A TaqMan low-density array (TLDA) was used to characterise the expression of 380 genes associated with chemotherapy resistance in IGROVCDDP cells. Paclitaxel resistance in IGROVCDDP is mediated by gene and protein overexpression of P-glycoprotein and the protein is functionally active. Cisplatin resistance was not reversed by elacridar, confirming that cisplatin is not a P-glycoprotein substrate. Cisplatin resistance in IGROVCDDP is multifactorial and is mediated in part by the glutathione pathway and decreased accumulation of drug. Total cellular glutathione was not increased. However, the enzyme activity of GSR and GGT1 were up-regulated. The cellular localisation of copper transporter CTR1 changed from membrane associated in IGROV-1 to cytoplasmic in IGROVCDDP. This may mediate the previously reported accumulation defect. There was decreased expression of the sodium potassium pump (ATP1A), MRP1 and FBP which all have been previously associated with platinum accumulation defects in platinum-resistant cell lines. Cellular localisation of MRP1 was also altered in IGROVCDDP shifting basolaterally, compared to IGROV-1. BRCA1 was also up-regulated at the gene and protein level. The overexpression of P-glycoprotein in a resistant model developed with cisplatin is unusual. This demonstrates that P-glycoprotein can be up-regulated as a generalised stress response rather than as a specific response to a substrate. Mechanisms characterised in IGROVCDDP cells may be applicable to relapsed ovarian cancer patients treated with frontline platinum/taxane chemotherapy.

Published

2012

15. Supplementary Data from Interactions of the Hdm2/p53 and Proteasome Pathways May Enhance the Antitumor Activity of Bortezomib

Author

Nicholas Mitsiades, Kenneth C. Anderson, Constantine S. Mitsiades, Paul G. Richardson, Peter O'Gorman, Martin Clynes, Leutz Buon, Teru Hideshima, Dharminder Chauhan, Nikhil C. Munshi, Noopur S. Raje, Emily Daskalaki, Elpida Charalambous, Douglas W. McMillin, Vassiliki Kotoula, Patrick J. Hayden, and Melissa G. Ooi

Abstract

Supplementary Data from Interactions of the Hdm2/p53 and Proteasome Pathways May Enhance the Antitumor Activity of Bortezomib

Published

2023

16. Data from Interactions of the Hdm2/p53 and Proteasome Pathways May Enhance the Antitumor Activity of Bortezomib

Author

Nicholas Mitsiades, Kenneth C. Anderson, Constantine S. Mitsiades, Paul G. Richardson, Peter O'Gorman, Martin Clynes, Leutz Buon, Teru Hideshima, Dharminder Chauhan, Nikhil C. Munshi, Noopur S. Raje, Emily Daskalaki, Elpida Charalambous, Douglas W. McMillin, Vassiliki Kotoula, Patrick J. Hayden, and Melissa G. Ooi

Abstract

Purpose: p53 is inactivated in many human malignancies through missense mutations or overexpression of the human homologue of Mdm2 (Hdm2), an E3 ubiquitin ligase that ubiquitinates p53, thereby promoting its proteasomal degradation. The cis-imidazoline nutlin-3 can disrupt the p53-Hdm2 interaction and activate p53, inducing apoptosis in vitro in many malignancies, including multiple myeloma (MM).Experimental Design: We hypothesized that suppression of Hdm2-mediated p53 ubiquitination may augment sequelae of p53 accumulation caused by proteasomal inhibition. We compared the response of MM cells versus several epithelial cancer models to the proteasome inhibitor bortezomib in combination with nutlin-3.Results: The combination of sublethal concentrations of bortezomib plus nutlin-3 induced additive cytotoxicity against bortezomib-sensitive MM cell lines. Importantly, however, in breast, prostate, colon, and thyroid (papillary, follicular, anaplastic, and medullary) carcinoma cell lines, this combination triggered synergistic cytotoxicity, and increased expression of p53, p21, Hdm2, Bax, Noxa, PUMA, and cleavage of caspase-3 and poly ADP ribose polymerase. Coculture with bone marrow stromal cells attenuated MM cell sensitivity to nutlin-3 monotherapy and was associated with evidence of suppression of p53 activity in MM cells, whereas combined bortezomib-nutlin-3 treatment maintained cytotoxicity even in the presence of bone marrow stromal cells.Conclusions: This differential response of MM versus epithelial carcinomas to combination of nutlin-3 with bortezomib sheds new light on the role of p53 in bortezomib-induced apoptosis. Concurrent Hdm2 inhibition with bortezomib may extend the spectrum of bortezomib applications to malignancies with currently limited sensitivity to single-agent bortezomib or, in the future, to MM patients with decreased clinical responsiveness to bortezomib-based therapy. (Clin Cancer Res 2009;15(23):7153–60)

Published

2023

17. FOLFIRINOX Pharmacodynamic Interactions in 2D and 3D Pancreatic Cancer Cell Cultures

Author

Taylor J, Allen-Coyle, Jin, Niu, Eva, Welsch, Neil T, Conlon, Weylon, Garner, Martin, Clynes, Finbarr, O'Sullivan, Robert M, Straubinger, Donald E, Mager, and Sandra, Roche

Subjects

Oxaliplatin, Pancreatic Neoplasms, Drug Combinations, Antineoplastic Combined Chemotherapy Protocols, Cell Culture Techniques, Leucovorin, Humans, Antineoplastic Agents, Fluorouracil, Irinotecan

Abstract

The multi-drug combination regime, FOLFIRINOX, is a standard of care chemotherapeutic therapy for pancreatic cancer patients. However, systematic evaluation of potential pharmacodynamic interactions among multi-drug therapy has not been reported previously. Here, pharmacodynamic interactions of the FOLFIRINOX agents (5-fluorouracil (5-FU), oxaliplatin (Oxa) and SN-38, the active metabolite of irinotecan) were assessed across a panel of primary and established pancreatic cancer cells. Inhibition of cell proliferation was quantified for each drug, alone and in combination, to obtain quantitative, drug-specific interaction parameters and assess the nature of drug interactions. The experimental data were analysed assuming Bliss independent interactions, and nonlinear regression model fitting was conducted in SAS. Estimates of the drug interaction term, psi (ψ), revealed that the Oxa/SN-38 combination appeared synergistic in PANC-1 (ψ = 0.6, 95% CI = 0.4, 0.9) and modestly synergistic, close to additive, in MIAPaCa-2 (ψ = 0.8, 95% CI = 0.6, 1.0) in 2D assays. The triple combination was strongly synergistic in MIAPaCa-2 (ψ = 0.2, 95% CI = 0.1, 0.3) and modestly synergistic/borderline additive in PANC-1 2D (ψ = 0.8, 95% CI = 0.6, 1.0). The triple combination showed antagonistic interactions in the primary PIN-127 and 3D PANC-1 model (ψ 1). Quantitative pharmacodynamic interactions have not been described for the FOLFIRINOX regimen; this analysis suggests a complex interplay among the three chemotherapeutic agents. Extension of this pharmacodynamic analysis approach to clinical/translational studies of the FOLFIRINOX combination could reveal additional pharmacodynamic interactions and guide further refinement of this regimen to achieve optimal clinical responses.

Published

2022

18. Global phosphoproteomic study of high/low specific productivity industrially relevant mAb producing recombinant CHO cell lines

Author

Matthew D. Osborne, Ronan M. Kelly, Martin Clynes, Christopher C. Frye, Michael Henry, Michael E. Lloyd, Laura Bryan, and Paula Meleady

Subjects

chemistry.chemical_classification, Phosphoproteomics, medicine.drug_class, Chinese hamster ovary cell, Cell cycle, Monoclonal antibody, Phenotype, Amino acid, Cell biology, law.invention, Biopharmaceuticals, chemistry, Cell culture, law, medicine, Recombinant DNA, Label free quantitative proteomics, Intracellular, TP248.13-248.65, Chinese hamster ovary (CHO) cells, Cell specific productivity (Qp), Biotechnology

Abstract

Understanding the biology of CHO cells at a cellular level is extremely valuable to the pharmaceutical industry, as it presents the opportunity to rationally engineer clonally derived cell lines (CDCLs) with elevated recombinant specific productivity (Qp). To date, relatively little is understood about the intracellular pathways which influence desirable phenotypes in CHO cell lines. In this study we identified phosphoproteins and total proteins which are differentially expressed between high and low Qp IgG4 producing industry CHO cell lines, some of which upon further investigation, could potentially be used as targets to engineer high Qp CDCLs. We highlighted the importance of phosphoproteins and total proteins associated with amino acid sensing in high Qp cell lines. We also identified increased expression of proteins which promote progression through the cell cycle in low Qp cell lines, suggesting that lower Qp CDCLs are focusing their translational machinery on translating cell cycle associated mRNAs.

Published

2021

19. Proteomic Analysis of Cell Lines and Primary Tumors in Pancreatic Cancer Identifies Proteins Expressed Only In Vitro and Only In Vivo

Author

Fiona O'Neill, Orla Coleman, Niall Swan, Michael Moriarty, Martin Clynes, Gerard McVey, Kevin C. Conlon, Michael Henry, Sandra Roche, Justin Geoghegan, and Paula Meleady

Subjects

Proteomics, Pancreatic ductal adenocarcinoma, Proteome, endocrine system diseases, Endocrinology, Diabetes and Metabolism, Normal tissue, Biology, Mass Spectrometry, 03 medical and health sciences, 0302 clinical medicine, Endocrinology, In vivo, Cell Line, Tumor, Pancreatic cancer, Internal Medicine, medicine, Humans, Pancreas, Aged, Aged, 80 and over, Hepatology, Middle Aged, medicine.disease, digestive system diseases, In vitro, Pancreatic Neoplasms, Cell culture, 030220 oncology & carcinogenesis, Cancer research, 030211 gastroenterology & hepatology, Carcinoma, Pancreatic Ductal, Chromatography, Liquid

Abstract

Objectives A limited repertoire of good pancreatic ductal adenocarcinoma (PDAC) models is one of the main barriers in developing effective new PDAC treatments. We aimed to characterize 6 commonly used PDAC cell lines and compare them with PDAC patient tumor samples using proteomics. Methods Proteomic methods were used to generate an extensive catalog of proteins from 10 PDAC surgical specimens, 9 biopsies of adjacent normal tissue, and 6 PDAC cell lines. Protein lists were interrogated to determine what extent the proteome of the cell lines reflects the proteome of primary pancreatic tumors. Results We identified 7973 proteins from the cell lines, 5680 proteins from the tumor tissues, and 4943 proteins from the adjacent normal tissues. We identified 324 proteins unique to the cell lines, some of which may play a role in survival of cells in culture. Conversely, a list of 63 proteins expressed only in the patient samples, whose expression is lost in culture, may place limitations on the degree to which these model systems reflect tumor biology in vivo. Conclusions Our work offers a catalog of proteins detected in each of the PDAC cell lines, providing a useful guide for researchers seeking model systems for PDAC functional studies.

Published

2020

20. Gene expression profiling of copper-resistant Caco-2 clones

Author

Charles O’Doherty, Karina Horgan, Finbarr O'Sullivan, Martin Clynes, Richard Murphy, Joanne Keenan, Fiona O'Neill, and Indre Sinkunaite

Subjects

0301 basic medicine, Copper Sulfate, Biophysics, Clone (cell biology), Biology, Biochemistry, Biomaterials, 03 medical and health sciences, 0302 clinical medicine, Downregulation and upregulation, Gene expression, Humans, Gene, Gene Expression Profiling, Metals and Alloys, Epithelial Cells, Phenotype, Molecular biology, Gene expression profiling, 030104 developmental biology, Chemistry (miscellaneous), Caco-2, Cell culture, 030220 oncology & carcinogenesis, Caco-2 Cells, Transcriptome, Copper

Abstract

The Caco-2 cell line is composed of a heterogeneous mix of cells; isolation of individual clonal populations from this mix allows for specific mechanisms and phenotypes to be further explored. Previously we exposed Caco-2 cells to inorganic copper sulphate or organic copper proteinate to generate resistant variant populations. Here we describe the isolation and characterisation of clonal subpopulations from these resistant variants to organic (clone Or1, Or2, Or3) or inorganic (clone In1 and In2) copper. The clones show considerable homogeneity in response to Cu-induced toxicity and heterogeneity in morphology with variations in level of cross-resistance to other metals and doxorubicin. Population growth was reduced for Cu-resistant clones In2 and Or3 in selective pressure relative to parental Caco-2 cells. Gene expression analysis identified 4026 total (2102 unique and 1924 shared) differentially expressed genes including those involved in the MAP Kinase and Rap1 signalling pathways, and in the focal adhesion and ECM-receptor contact pathways. Gene expression changes common to all clones included upregulation of ANXA13 and GPx2. Our analysis additionally identified differential expression of multiple genes specific to copper proteinate exposure (including overexpressed UPK1B) in isolated clones Or1, Or2 and Or3 and CuSO4 exposure (including decreased AIFM2 expression) in isolated clones In1 and In2. The adaptive transcriptional responses established in this study indicate a cohort of genes, which may be involved in copper resistance regulation and chronic copper exposure.

Published

2020

21. DR5-targeted, chemotherapeutic drug-loaded nanoparticles induce apoptosis and tumor regression in pancreatic cancer in vivo models

Author

Martin Clynes, Michael C. Johnston, Katie Stott, William J. McDaid, Julie A. Nicoll, Michelle K. Greene, Robert M. Straubinger, Darren K.W. Chan, Daniel B. Longley, Christopher J. Scott, Sandra Roche, Ninfa L. Straubinger, Jennifer Fox, Kelly M. Redmond, Nyree Crawford, and Peter Smyth

Subjects

CASP8 and FADD-Like Apoptosis Regulating Protein, Pharmaceutical Science, Apoptosis, 02 engineering and technology, Article, 03 medical and health sciences, SDG 3 - Good Health and Well-being, In vivo, Pancreatic tumor, Cell Line, Tumor, Pancreatic cancer, medicine, Humans, FADD, Viability assay, 030304 developmental biology, Drug Carriers, 0303 health sciences, biology, Chemistry, 021001 nanoscience & nanotechnology, medicine.disease, Pancreatic Neoplasms, Receptors, TNF-Related Apoptosis-Inducing Ligand, Flip, biology.protein, Cancer research, Nanoparticles, 0210 nano-technology, Camptothecin, medicine.drug

Abstract

Pancreatic cancer is usually advanced and drug resistant at diagnosis. A potential therapeutic approach outlined here uses nanoparticle (NP)-based drug carriers, which have unique properties that enhance intra-tumor drug exposure and reduce systemic toxicity of encapsulated drugs. Here we report that patients whose pancreatic cancers express elevated levels of Death Receptor 5 (DR5) and its downstream regulators/effectors FLIP, Caspase-8, and FADD had particularly poor prognoses. To take advantage of elevated expression of this pathway, we designed drug-loaded NPs with a surface-conjugated αDR5 antibody (AMG 655). Binding and clustering of the DR5 is a prerequisite for efficient apoptosis initiation, and the αDR5-NPs were indeed found to activate apoptosis in multiple pancreatic cancer models, whereas the free antibody did not. The extent of apoptosis induced by αDR5-NPs was enhanced by down-regulating FLIP, a key modulator of death receptor- mediated activation of caspase-8. Moreover, the DNA topoisomerase-1 inhibitor camptothecin (CPT) down-regulated FLIP in pancreatic cancer models and enhanced apoptosis induced by αDR5-NPs. CPT-loaded αDR5-NPs significantly increased apoptosis and decreased cell viability in vitro in a caspase-8- and FADD-dependent manner consistent with their expected mechanism-of-action. Importantly, CPT-loaded αDR5-NPs markedly reduced tumor growth rates in vivo in established pan- creatic tumor models, inducing regressions in one model. These proof-of-concept studies indicate that αDR5-NPs loaded with agents that downregulate or inhibit FLIP are promising candidate agents for the treatment of pancreatic cancer.

Published

2020

22. Altered gene expression in CHO cells following polyamine starvation

Author

Martin Clynes, Berta Capella Roca, Fiona O'Neill, Padraig Doolan, and Niall Barron

Subjects

0106 biological sciences, 0301 basic medicine, Cell Survival, DNA repair, Bioengineering, CHO Cells, 01 natural sciences, Applied Microbiology and Biotechnology, Transcriptome, 03 medical and health sciences, chemistry.chemical_compound, Cricetulus, Cricetinae, 010608 biotechnology, Gene expression, Putrescine, Animals, Gene, Chemistry, General Medicine, Culture Media, Cell biology, 030104 developmental biology, Gene Expression Regulation, RNA splicing, Unfolded protein response, Homologous recombination, Polyamine, Biotechnology

Abstract

To investigate the impact of polyamine deprivation on the transcriptome of CHO cells RESULTS: Polyamines play a central but poorly-understood role in cell proliferation. Most studies to date have utilised chemical inhibitors to probe polyamine function. Here we exploit the fact that CHO cells grown in serum-free medium have an absolute requirement for putrescine supplementation due to their deficiency in activity of the enzyme arginase. A gene expression microarray (Affymetrix) analysis of CHO-K1 cells starved of polyamines for 3 days showed that cessation of growth, associated with increased G1/S transition and inhibition of M/G1 transition was accompanied by increased mRNA levels of mitotic complex checkpoint genes (Mad2l1, Tkk, Bub1b) and in the transition of G1- to S-phase (such as Skp2 and Tfdp1). mRNAs associated with DNA homologous recombination and repair (including Fanconi's anaemia-related genes) and with RNA splicing were consistently increased. Alterations in mRNA levels for genes related to protein processing in the ER, to ER stress, and to p53-related and apoptosis pathways were also observed. mRNAs showing highest levels of fold-change included several which code for membrane-localised proteins and receptors (Thbs1, Tfrc1, Ackr3, Extl1).Growth-arrest induced by polyamine deprivation was associated with significant alterations in levels of mRNAs associated with cell cycle progression, DNA repair, RNA splicing, ER trafficking and membrane signalling as well as p53 and apoptosis-related pathways.

Published

2020

23. Annotation of the non-canonical translatome reveals that CHO cell microproteins are a new class of mAb drug product impurity

Author

Marina Castro-Rivadeneyra, Ioanna Tzani, Paul Kelly, Lisa Strasser, Felipe Guapo, Ciara Tierney, Michelle Chain, Lin Zhang, Martin Clynes, Barry L. Karger, Niall Barron, Jonathan Bones, and Colin Clarke

Abstract

Chinese hamster ovary (CHO) cells are used to produce almost 90% of therapeutic monoclonal antibodies (mAbs). The annotation of non-canonical translation events in these cellular factories remains incomplete, limiting not only our ability to study CHO cell biology but also detect host cell protein (HCP) contaminants in the final mAb drug product. We utilised ribosome footprint profiling (Ribo-seq) to identify novel open reading frames (ORFs) including N-terminal extensions and thousands of short ORFs (sORFs) predicted to encode microproteins. Mass spectrometry-based HCP analysis of four commercial mAb drug products using the extended protein sequence database revealed the presence of microprotein impurities for the first time. We also show that microprotein abundance varies with growth phase and can be affected by the cell culture environment. In addition, our work provides a vital resource to facilitate future studies of non-canonical translation as well as the regulation of protein synthesis in CHO cell lines.

Published

2022

24. Mapping the molecular basis for growth related phenotypes in industrial producer CHO cell lines using differential proteomic analysis

Author

Michael Henry, Laura Bryan, Matthew D. Osborne, Ronan M. Kelly, Christopher C. Frye, Paula Meleady, and Martin Clynes

Subjects

Proteomics, 0106 biological sciences, endocrine system, Proteome, CHO Cells, Biology, Endocytosis, 01 natural sciences, 03 medical and health sciences, Cricetulus, Mitotic cell cycle, Tandem Mass Spectrometry, Cricetinae, 010608 biotechnology, Animals, Label free quantitative proteomics, Viability assay, Cell Proliferation, Chinese hamster ovary (CHO) cells, 030304 developmental biology, 0303 health sciences, Research, Chinese hamster ovary cell, Cell Cycle, DNA replication, Proteins, Viable cell density (VCD) biopharmaceuticals, Cell biology, Phenotype, Cell culture, Apoptosis, Immunoglobulin G, TP248.13-248.65, Intracellular, Chromatography, Liquid, Cell specific productivity (Qp), Biotechnology

Abstract

Background The ability to achieve high peak viable cell density earlier in CHO cell culture and maintain an extended cell viability throughout the production process is highly desirable to increase recombinant protein yields, reduce host cell impurities for downstream processing and reduce the cost of goods. In this study we implemented label-free LC-MS/MS proteomic profiling of IgG4 producing CHO cell lines throughout the duration of the cell culture to identify differentially expressed (DE) proteins and intracellular pathways associated with the high peak viable cell density (VCD) and extended culture VCD phenotypes. Results We identified key pathways in DNA replication, mitotic cell cycle and evasion of p53 mediated apoptosis in high peak VCD clonally derived cell lines (CDCLs). ER to Golgi vesicle mediated transport was found to be highly expressed in extended culture VCD CDCLs while networks involving endocytosis and oxidative stress response were significantly downregulated. Conclusion This investigation highlights key pathways for targeted engineering to generate desirable CHO cell phenotypes for biotherapeutic production.

Published

2021

25. Why we need good mentoring

Author

Anita H. Corbett, Martin Clynes, and Julie Overbaugh

Subjects

Research program, Medical education, Applied Mathematics, General Mathematics, media_common.quotation_subject, education, Dana-Farber Cancer Institute, MEDLINE, Creativity, humanities, Grant Review, 03 medical and health sciences, 0302 clinical medicine, Mentorship, 030220 oncology & carcinogenesis, Research environment, Hiv transmission, health care economics and organizations, media_common

Abstract

Cancer research relies on key values such as creativity, collaboration, research integrity and resource sharing. A positive research environment which fosters these key values is becoming a decisive factor for some funders and research institutions. To create a supportive research culture in laboratories, the training and mentoring of young scientists is important. However, the fast-paced and fierce competition for funding and jobs can present a challenge to the younger generation of scientists who depend on the guidance and mentorship of scientific leaders. The annual Nature Awards for Mentoring in Science have been created to bring attention to one of the most essential but least recognized skills in scientific leadership. Thus far, 35 scientists from across the world, who are working in a range of disciplines, have been recognized by this award for their outstanding scientific mentorship. In this Viewpoint, we have asked three recipients of this award who work in fields associated with cancer research about their views on good mentoring, and how a revised approach to mentorship can help to achieve a positive research culture and contribute to scientific discovery. In this Viewpoint, we have asked recipients of the Nature Awards for Mentoring in Science about their views on good mentoring, and how mentorship can help to achieve a positive research culture and contribute to scientific discovery in cancer research. Martin Clynes was founding Director of the National Institute for Cellular Biotechnology at Dublin City University, Dublin, Ireland, and he has an interest in several applications of cell culture. His cancer-related interests, working closely with clinical experts, include research on mechanisms of chemotherapy resistance and investigation of potential therapeutic targets and biomarkers in pancreatic, lung and breast cancer and in cutaneous melanoma. His research has contributed to a number of clinical trials. Anita Corbett received her undergraduate degree in chemistry from Colgate University and her PhD degree in biochemistry from Vanderbilt University. She was a postdoctoral fellow at Dana Farber Cancer Institute/Harvard Medical School before joining the Department of Biochemistry at Emory University School of Medicine in 1997. In 2016, she moved to the Department of Biology at Emory University, where she is a tenured professor of biology and Co-Director of the Emory MD/PhD Program. Julie Overbaugh, PhD, is the Endowed Chair for Graduate Education and Associate Director for Cancer Research Career Enhancement at Fred Hutchinson Cancer Research Center. Her research focuses on HIV transmission and the study of HIV immunity, including how it evolves and its impact on infection risk and pathogenesis. This research has been a long-standing collaboration with the Kenya Research Program. She has served in numerous leadership roles for grant review groups and major meetings in her field.

Published

2019

26. Increased growth rate and productivity following stable depletion of miR-7 in a mAb producing CHO cell line causes an increase in proteins associated with the Akt pathway and ribosome biogenesis

Author

Justine Meiller, Martin Clynes, Paula Meleady, Srinivas Suda, Michael Henry, Markus Riedl, Orla Coleman, and Niall Barron

Subjects

0301 basic medicine, Translational efficiency, Biophysics, Ribosome biogenesis, CHO Cells, Biochemistry, 03 medical and health sciences, Cricetulus, Animals, Humans, PI3K/AKT/mTOR pathway, 030102 biochemistry & molecular biology, Chemistry, Proteomic Profiling, Chinese hamster ovary cell, Antibodies, Monoclonal, Recombinant Proteins, Cell biology, MicroRNAs, 030104 developmental biology, Cell culture, Proteome, Signal transduction, Proto-Oncogene Proteins c-akt, Ribosomes, Signal Transduction

Abstract

Cell line engineering using microRNAs represents a desirable route for improving the efficiency of recombinant protein production by CHO cells. In this study we generated stable CHO DP12 cells expressing a miR-7 sponge transcript which sequesters miR-7 from its endogenous targets. Depletion of miR-7 results in a 65% increase in cell growth and >3-fold increase in yield of secreted IgG protein. Quantitative labelfree LC-MS/MS proteomic profiling was carried out to identify the targets of miR-7 and understand the functional drivers of the improved CHO cell phenotypes. Subcellular enrichment and total proteome analysis identified more than 3000 proteins per fraction resulting in over 5000 unique proteins identified per timepoint analysed. Early stage culture analysis identified 117 proteins overexpressed in miR-7 depleted cells. A subset of these proteins are involved in the Akt pathway which could be the underlying route for cell density improvement and may be exploited more specifically in the future. Late stage culture identified 160 proteins overexpressed in miR-7 depleted cells with some of these involved in ribosome biogenesis which may be causing the increased productivity through improved translational efficiency. This is the first in-depth proteomic profiling of the IgG producing CHO DP12 cell line stably depleted of miR-7. SIGNIFICANCE: Chinese hamster ovary (CHO) cells are the mammalian cell expression system of choice for production of recombinant therapeutic proteins. There is much research ongoing to characterise CHO cell factories through the application of systems biology approaches that will enable a fundamental understanding of CHO cell physiology, and as a result, a better knowledge and understanding of recombinant protein production. This study profiles the proteomic effects of microRNA-7 depletion on the IgG producing CHO DP12 cell line. This is one of the very few studies that attempts to identify the functioning proteins driving improved CHO cell phenotypes resulting from microRNA manipulation. Using subcellular enrichment and total proteome analysis we identified over 5000 unique proteins in miR-7 depleted CHO cells. This work has identified a cohort of proteins involved in the Akt pathway and ribosome biogenesis. These proteins may drive improved CHO cell phenotypes and are of great interest for future work.

Published

2019

27. Copper-induced non-monotonic dose response in Caco-2 cells

Author

Joanne Keenan, Karina Horgan, Richard Murphy, Charles O’Doherty, Martin Clynes, and Finbarr O'Sullivan

Subjects

0301 basic medicine, Copper Sulfate, Cell Survival, chemistry.chemical_element, Cell Biology, General Medicine, Zinc, Micronutrient, Copper, Intestinal absorption, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, chemistry, Caco-2, Cell culture, 030220 oncology & carcinogenesis, Toxicity, Biophysics, Humans, Caco-2 Cells, Copper chloride, Developmental Biology

Abstract

Copper is an essential dietary micronutrient in humans for proper cell function; however, in excess, it is toxic. The human cell line Caco-2 is popular as an in vitro model for intestinal absorption and toxicology. This study investigated the response of exponentially growing Caco-2 cells to prolonged copper exposure (120 h). An unexpected non-monotonic dose-response profile was observed in Caco-2 cells. Exposure to media supplemented with 3.125 μM CuSO4 resulted in decreased cell yield vs. untreated. However, toxicity was progressively reduced from 90% at 3.125 μM to 60% at 25 μM. This effect was documented between 48 and 120 h continuous exposure (p

Published

2019

28. Differential expression of miRNAs and functional role of mir-200a in high and low productivity CHO cells expressing an Fc fusion protein

Author

Michael Henry, Paula Meleady, Niall Barron, Clair Gallagher, Martin Clynes, Laura Bryan, Christopher C. Frye, Matthew D. Osborne, and Ronan M. Kelly

Subjects

0301 basic medicine, Proteomics, Protein Folding, Recombinant Fusion Proteins, Bioengineering, CHO Cells, Applied Microbiology and Biotechnology, law.invention, Biopharmaceuticals, 03 medical and health sciences, 0302 clinical medicine, Cricetulus, law, Cricetinae, microRNA, Animals, Humans, Label free quantitative proteomics, Chinese hamster ovary (CHO) cells, Chemistry, Chinese hamster ovary cell, General Medicine, Phenotype, Cell biology, Immunoglobulin Fc Fragments, Original Research Paper, MicroRNAs, 030104 developmental biology, Cell culture, 030220 oncology & carcinogenesis, Recombinant DNA, Unfolded protein response, Protein folding, MiRNA, Intracellular, Biotechnology, Cell specific productivity (Qp)

Abstract

Objectives We used miRNA and proteomic profiling to understand intracellular pathways that contribute to high and low specific productivity (Qp) phenotypes in CHO clonally derived cell lines (CDCLs) from the same cell line generation project. Results Differentially expressed (DE) miRNAs were identified which are predicted to target several proteins associated with protein folding. MiR-200a was found to have a number of predicted targets associated with the unfolded protein response (UPR) which were shown to have decreased expression in high Qp CDCLs and have no detected change at the mRNA level. MiR-200a overexpression in a CHO CDCL was found to increase recombinant protein titer by 1.2 fold and Qp by 1.8 fold. Conclusion These results may suggest a role for miR-200a in post-transcriptional regulation of the UPR, presenting miR-200a as a potential target for engineering industrially attractive CHO cell phenotypes.

Published

2021

29. The emerging role of cellular post-translational modifications in modulating growth and productivity of recombinant Chinese hamster ovary cells

Author

Martin Clynes, Paula Meleady, and Laura Bryan

Subjects

0106 biological sciences, Glycosylation, Proteome, Bioengineering, CHO Cells, 01 natural sciences, Applied Microbiology and Biotechnology, law.invention, Transcriptome, 03 medical and health sciences, chemistry.chemical_compound, Cricetulus, Ubiquitin, law, 010608 biotechnology, Cricetinae, Metabolome, Animals, Humans, 030304 developmental biology, 0303 health sciences, biology, Chinese hamster ovary cell, Recombinant Proteins, Cell biology, chemistry, biology.protein, Recombinant DNA, Phosphorylation, Protein Processing, Post-Translational, Biotechnology

Abstract

Chinese hamster ovary (CHO) cells are one of the most commonly used host cell lines used for the production human therapeutic proteins. Much research over the past two decades has focussed on improving the growth, titre and cell specific productivity of CHO cells and in turn lowering the costs associated with production of recombinant proteins. CHO cell engineering has become of particular interest in recent years following the publication of the CHO cell genome and the availability of data relating to the proteome, transcriptome and metabolome of CHO cells. However, data relating to the cellular post-translational modification (PTMs) which can affect the functionality of CHO cellular proteins has only begun to be presented in recent years. PTMs are important to many cellular processes and can further alter proteins by increasing the complexity of proteins and their interactions. In this review, we describe the research presented from CHO cells to date related on three of the most important PTMs; glycosylation, phosphorylation and ubiquitination.

Published

2020

30. Transfection of miR-31* boosts oxidative phosphorylation metabolism in the mitochondria and enhances recombinant protein production in Chinese hamster ovary cells

Author

Martin Clynes, Orla Coleman, Jesus E. Martinez-Lopez, and Paula Meleady

Subjects

0106 biological sciences, 0301 basic medicine, Proteomics, Bioengineering, Oxidative phosphorylation, CHO Cells, Mitochondrion, Transfection, 01 natural sciences, Applied Microbiology and Biotechnology, Oxidative Phosphorylation, 03 medical and health sciences, chemistry.chemical_compound, Cricetulus, 010608 biotechnology, Cricetinae, Animals, Fatty acid metabolism, Chinese hamster ovary cell, General Medicine, Cell cycle, Warburg effect, Recombinant Proteins, Cell biology, Mitochondria, Citric acid cycle, MicroRNAs, 030104 developmental biology, chemistry, Biotechnology

Abstract

MicroRNAs are increasingly being used to enhance relevant pathways of interest during CHO cell line development and to optimise biopharmaceutical production processes. Previous studies have demonstrated that genetic manipulation of microRNAs has led to the development of highly productive phenotypes by increasing cell density through modifying the cell cycle, extending the culture lifespan by delaying apoptotic mechanisms, or improving the energetic flux by targeting mitochondrial metabolism. Re-programming mitochondrial metabolism has arisen as a potential area of interest due to the potential to decrease the Warburg effect and increase cell specific productivity with significant impact on the manufacture of recombinant therapeutic proteins. In this study, we have demonstrated a role for miR-31* to enhance specific productivity in CHO cells by boosting oxidative phosphorylation in the mitochondria. A detailed analysis of the mitochondrial metabolism revealed that miR-31* transfection increases basal oxygen consumption and spare respiratory capacity that leads to an increase in ATP production. Additionally, a proteomic analysis unveiled a number of potential targets involved in fatty acid metabolism and the TCA cycle, both implicated in mitochondrial metabolism. This data demonstrates a potential role for miR-31* to reprogramme the mitochondrial energetic metabolism and increase recombinant protein production in CHO cells.

Published

2020

31. Development of whole-cell and cell-free biosensors for the detection and differentiation of organic and inorganic forms of copper

Author

Alan Costello, Richard Murphy, Martin Clynes, and Joanne Parker

Subjects

0301 basic medicine, 030106 microbiology, Biophysics, chemistry.chemical_element, Cell free, Biosensing Techniques, Biochemistry, Biomaterials, Metal, 03 medical and health sciences, Microbial resistance, Organic Chemicals, Cell-Free System, Chemistry, Significant difference, Metals and Alloys, Antimicrobial, Copper, 030104 developmental biology, Chemistry (miscellaneous), visual_art, Environmental chemistry, visual_art.visual_art_medium, Whole cell, Biosensor

Abstract

The modern world has seen exposure of bacterial communities to toxic metals at selective levels. This manifests itself both intentionally, through medicines and un-intentionally through waste streams. There is growing concern that selective exposure to metals may be linked to microbial resistance to antibiotics. For a microbe to become resistant to a specific metal it must first come in contact with it. The transition metal copper has the ability to enter bacterial cells without need for a copper specific uptake mechanism. Copper is commonly used as an antimicrobial in the healthcare industry, consumer products and as a growth promoter of livestock in the agricultural sector. Here we report a study into the uptake of different organic and inorganic sources of copper. A whole-cell bacterial biosensor was developed to quantify the specific uptake of copper from various sources. Furthermore, a cell-free sensor was utilized to investigate the response to copper sources when uptake is eliminated as a factor. The data within suggest inorganic copper to have greatly reduced uptake compared to organic sources and that there is significant difference between copper oxides, Cu2O and CuO.

Published

2020

32. Proteomic analysis of pancreatic ductal adenocarcinoma

Author

Michael Henry, Michael Moriarty, Rozana Abdul Rahman, Paula Meleady, and Martin Clynes

Subjects

0301 basic medicine, Proteomics, Pancreatic ductal adenocarcinoma, endocrine system diseases, 030102 biochemistry & molecular biology, business.industry, Proteins, Adenocarcinoma, Exosomes, Biochemistry, digestive system diseases, Malignant disease, Mass Spectrometry, Gene Expression Regulation, Neoplastic, Pancreatic Neoplasms, 03 medical and health sciences, 030104 developmental biology, Cancer research, Biomarkers, Tumor, Medicine, Humans, business, Molecular Biology

Abstract

Pancreatic ductal adenocarcinoma (PDAC), which represents approximately 80% of all pancreatic cancers, is a highly aggressive malignant disease and one of the most lethal among all cancers. Overall, the 5-year survival rate among all pancreatic cancer patients is less than 9%; these rates have shown little change over the past 30 years. A more comprehensive understanding of the molecular mechanisms underlying this complex disease is crucial to the development of new diagnostic tools for early detection and disease monitoring, as well as to identify new and more effective therapeutics to improve patient outcomes.We summarize recent advances in proteomic strategies and mass spectrometry to identify new biomarkers for early detection and monitoring of disease progression, predict response to therapy, and to identify novel proteins that have the potential to be 'druggable' therapeutic targets. An overview of proteomic studies that have been conducted to further our mechanistic understanding of metastasis and chemotherapy resistance in PDAC disease progression will also be discussed.The results from these PDAC proteomic studies on a variety of PDAC sample types (e.g., blood, tissue, cell lines, exosomes, etc.) provide great promise of having a significant clinical impact and improving patient outcomes.

Published

2020

33. Copper toxicity of inflection point in human intestinal cell line Caco-2 dissected: influence of temporal expression patterns

Author

Richard Murphy, Joanne Keenan, Paula Meleady, Michael Henry, Martin Clynes, Finbarr O'Sullivan, Charles O’Doherty, and Karina Horgan

Subjects

0301 basic medicine, Proteomics, Time Factors, Cell Survival, chemistry.chemical_element, Cell Count, 03 medical and health sciences, 0302 clinical medicine, Heat shock protein, medicine, Humans, Protein Unfolding, Zinc finger, Chemistry, Copper toxicity, Reproducibility of Results, Cell Biology, General Medicine, medicine.disease, Copper, Glutathione, Heme oxygenase, Intestines, Dose–response relationship, 030104 developmental biology, Caco-2, Cell culture, 030220 oncology & carcinogenesis, Biophysics, Caco-2 Cells, Developmental Biology

Abstract

We previously described a non-monotonic dose response curve at low copper concentrations where 3.125 μM CuSO4 (the early inflection point) was more toxic than 25 μM CuSO4 in Caco-2 cells. We employed global proteomics to investigate this observation. The altered expression levels of a small number of proteins displaying a temporal response may provide the best indication of the underlying mechanism; more well-known copper response proteins including the metal binding metallothioneins (MT1X, MT1F, MT2A) and antioxidant response proteins including Heme oxygenase were upregulated to a similar level in both copper concentrations and so are less likely to underpin this phenomenon.The temporal response proteins include Granulins, AN1-type zinc finger protein 2A (ZFAND2A), and the heat shock proteins (HSPA6 and HSPA1B). Granulins were decreased after 4 h only in 25 μM CuSO4 but from 24 h, were decreased in both copper concentrations to a similar level. Induction of ZFAND2A and increases in HSPA6 and HSPA1B were observed at 24 h only in 25 μM CuSO4 but were present at 48 h in both copper conditions. The early expression of ZFAND2A, HSPs, and higher levels of α-crystallin B (CRYAB) correlated with lower levels of misfolded proteins in 25 μM CuSO4 compared to 3.125 μM CuSO4 at 48 h. These results suggest that 3.125 μM CuSO4 at early time points was unable to activate the plethora of stress responses invoked by the higher copper concentration, paradoxically exposing the Caco-2 cells to higher levels of misfolded proteins and greater proteotoxic stress.

Published

2020

34. Polypyridyl-Based Copper Phenanthrene Complexes: Combining Stability with Enhanced DNA Recognition

Author

John Colleran, Nicoló Zuin Fantoni, Sinéad O'Carroll, Chryssostomos Chatgilialoglu, Suainibhe Kelly, Anna Banasiak, Martin Clynes, Georgia Menounou, Andrew Kellett, George Mitrikas, Sandra Roche, Vickie McKee, Marios G. Krokidis, and Zara Molphy

Subjects

DNA damage, DNA repair, Stereochemistry, Intercalation (chemistry), 010402 general chemistry, Crystallography, X-Ray, 01 natural sciences, Catalysis, chemistry.chemical_compound, Coordination Complexes, Cell Line, Tumor, Organometallic Compounds, Humans, A-DNA, 010405 organic chemistry, Chemistry, fungi, Organic Chemistry, Electron Spin Resonance Spectroscopy, General Chemistry, DNA, Phenanthrenes, Ligand (biochemistry), 0104 chemical sciences, Pancreatic Neoplasms, electrochemistry, copper, Hydroxyl radical, Amine gas treating, Copper, EPR spectroscopy, DNA Damage, Phenanthrolines

Abstract

We report a series of copper(II) artificial metallo-nucleases (AMNs) and demonstrate their DNA damaging properties and in-vitro cytotoxicity against human-derived pancreatic cancer cells. The compounds combine a tris-chelating polypyridyl ligand, di-(2-pycolyl)amine (DPA), and a DNA intercalating phenanthrene unit. Their general formula is Cu-DPA-N,N' (where N,N'=1,10-phenanthroline (Phen), dipyridoquinoxaline (DPQ) or dipyridophenazine (DPPZ)). Characterisation was achieved by X-ray crystallography and continuous-wave EPR (cw-EPR), hyperfine sublevel correlation (HYSCORE) and Davies electron-nuclear double resonance (ENDOR) spectroscopies. The presence of the DPA ligand enhances solution stability and facilitates enhanced DNA recognition with apparent binding constants (Kapp) rising from 105 to 107 m−1 with increasing extent of planar phenanthrene. Cu-DPA-DPPZ, the complex with greatest DNA binding and intercalation effects, recognises the minor groove of guanine–cytosine (G-C) rich sequences. Oxidative DNA damage also occurs in the minor groove and can be inhibited by superoxide and hydroxyl radical trapping agents. The complexes, particularly Cu-DPA-DPPZ, display promising anticancer activity against human pancreatic tumour cells with in-vitro results surpassing the clinical platinum(II) drug oxaliplatin.

Published

2020

35. LC-MS proteomic profiling of Caco-2 human intestinal cells exposed to the copper-chelating agent, triethylenetetramine: A preliminary study

Author

Joanne Keenan, Finbarr O'Sullivan, Charles O’Doherty, Karina Horgan, Michael Henry, Richard Murphy, Paula Meleady, and Martin Clynes

Subjects

0301 basic medicine, Cell Survival, Cell, Biophysics, Biochemistry, Trientine, Mixed Function Oxygenases, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Downregulation and upregulation, Peptide Initiation Factors, medicine, Humans, Molecular Biology, Cell Proliferation, Chelating Agents, Dose-Response Relationship, Drug, Proteomic Profiling, Gene Expression Profiling, Computational Biology, RNA-Binding Proteins, Molecular Sequence Annotation, Cell Biology, Deoxyhypusine Hydroxylase, Cell biology, 030104 developmental biology, medicine.anatomical_structure, Gene Ontology, chemistry, Gene Expression Regulation, Caco-2, Triethylenetetramine, 030220 oncology & carcinogenesis, Proteome, Caco-2 Cells, Homeostasis, Copper

Abstract

Homeostasis of metal micronutrients such as copper is tightly regulated to ensure deficiency does not occur while restricting damage resulting from excess accumulation. Using LC-MS the effect on the proteome of intestinal Caco-2 cells of exposure to the chelator triethylenetetramine (TETA) was investigated. Continuous exposure of TETA at 25 μM to Caco-2 cells caused decreased cell yields and morphological changes. These effects were reversed when cells were no longer exposed to TETA. Quantitative proteomic analysis identified 957 mostly low-fold differentially expressed proteins, 41 of these returned towards control Caco-2 expression following recovery. Proteins exhibiting this “reciprocal” behaviour included upregulated deoxyhypusine hydroxylase (DOHH, 15.69- fold), a protein essential for eIF-5A factor hypsuination, a post translational modification responsible for eIF-5A maturation, which in turn is responsible for translation elongation. Exposure to TETA also resulted in 87 proteins, the expression of which was stable and remained differentially expressed following recovery. This study helps to elucidate the stable and transient proteomic effects of TETA exposure in intestinal cells.

Published

2020

36. Establishment and Characterisation by Expression Microarray of Patient-Derived Xenograft Panel of Human Pancreatic Adenocarcinoma Patients

Author

Martin Clynes, Ray McDermott, Niall Swan, Justine Meiller, Neil T Conlon, Justin Geoghegan, Gerard McVey, Sandra Roche, Kevin C. Conlon, Ninfa L. Straubinger, Robert M. Straubinger, Michael Moriarty, Robert O'Connor, Jean Murphy, Rozana Abdul Rahman, Fiona O'Neill, and Sinead Toomey

Subjects

Male, Amino Acid Transport Systems, Microarray, pancreatic cancer, Cell Culture Techniques, Mice, SCID, Metastasis, lcsh:Chemistry, Mice, Mucoproteins, Mitotic cell cycle, Gene Regulatory Networks, Poly-ADP-Ribose Binding Proteins, lcsh:QH301-705.5, Spectroscopy, Oligonucleotide Array Sequence Analysis, Aged, 80 and over, Oncogene Proteins, General Medicine, Middle Aged, Cell cycle, Neoplasm Proteins, Computer Science Applications, Gene Expression Regulation, Neoplastic, Adenocarcinoma, Female, microarray, hormones, hormone substitutes, and hormone antagonists, Carcinoma, Pancreatic Ductal, endocrine system, patient-derived xenograft, AGR2, Biology, digestive system, Article, Catalysis, Inorganic Chemistry, Cell Line, Tumor, Pancreatic cancer, medicine, Animals, Humans, Physical and Theoretical Chemistry, Molecular Biology, Serpins, Aged, Cell Proliferation, Severe combined immunodeficiency, Gene Expression Profiling, Organic Chemistry, Membrane Proteins, medicine.disease, Pancreatic Neoplasms, DNA Topoisomerases, Type II, lcsh:Biology (General), lcsh:QD1-999, Cancer research, Neoplasm Transplantation

Abstract

Pancreatic cancer remains among the most lethal cancers worldwide, with poor early detection rates and poor survival rates. Patient-derived xenograft (PDX) models have increasingly been used in preclinical and clinical research of solid cancers to fulfil unmet need. Fresh tumour samples from human pancreatic adenocarcinoma patients were implanted in severe combined immunodeficiency (SCID) mice. Samples from 78% of treatment-na&iuml, ve pancreatic ductal adenocarcinoma patients grew as PDX tumours and were confirmed by histopathology. Frozen samples from F1 PDX tumours could be later successfully passaged in SCID mice to F2 PDX tumours. The human origin of the PDX was confirmed using human-specific antibodies, however, the stromal component was replaced by murine cells. Cell lines were successfully developed from three PDX tumours. RNA was extracted from eight PDX tumours and where possible, corresponding primary tumour (T) and adjacent normal tissues (N). mRNA profiles of tumour vs. F1 PDX and normal vs. tumour were compared by Affymetrix microarray analysis. Differential gene expression showed over 5000 genes changed across the N vs. T and T vs. PDX samples. Gene ontology analysis of a subset of genes demonstrated genes upregulated in normal vs. tumour vs. PDX were linked with cell cycle, cycles cell process and mitotic cell cycle. Amongst the mRNA candidates elevated in the PDX and tumour vs. normal were SERPINB5, FERMT1, AGR2, SLC6A14 and TOP2A. These genes have been associated with growth, proliferation, invasion and metastasis in pancreatic cancer previously. Cumulatively, this demonstrates the applicability of PDX models and transcriptomic array to identify genes associated with growth and proliferation of pancreatic cancer.

Published

2020

37. Clonal variation in productivity and proteolytic clipping of an Fc-fusion protein in CHO cells: Proteomic analysis suggests a role for defective protein folding and the UPR

Author

Michael Henry, Paula Meleady, Martin Clynes, Christopher C. Frye, Ciaran P. Brady, Niall Barron, Clair Gallagher, Ronan M. Kelly, and Matthew D. Osborne

Subjects

Proteomics, 0301 basic medicine, Protein Folding, Proteases, 030102 biochemistry & molecular biology, Recombinant Fusion Proteins, Chinese hamster ovary cell, Bioengineering, CHO Cells, General Medicine, Biology, Applied Microbiology and Biotechnology, Cell biology, 03 medical and health sciences, Cricetulus, 030104 developmental biology, Cell culture, Unfolded Protein Response, Protein biosynthesis, Unfolded protein response, Animals, Protein folding, Intracellular, Biotechnology

Abstract

Product degradation, such as clipping, is a common quality issue in the production of Fc-fusion proteins from Chinese hamster ovary (CHO) cells. Degradation of proteins is mainly due to the action of either intracellular or extracellular host cell proteases. This study was carried out to understand more fundamentally the intracellular events that may play a role in determining why cell lines from the same cell line development project can vary with regards to the extent of Fc-fusion protein clipping. The cell lines that displayed the highest levels of clipping also produced less product than the cell lines with a lower level of clipping. In this study we applied differential quantitative label-free LC-MS/MS proteomic analysis to group clonally-derived cell lines (CDCLs) based on the level of clipping of the Fc-fusion protein. The analysis was carried out over two times points in culture and clones were designated as either having 'high' or 'low' clipping phenotypes. We have identified 200 differentially expressed proteins using quantitative label-free LC-MS/MS analysis between the two experimental groups. Functional assessment of the resultant proteomic data using Gene Ontology analysis showed a significant enrichment of biological processes and molecular functions related to protein folding, response to unfolded protein and protein translation. The levels of several proteases were also increased. This study identified protein targets that could be modified using cell line engineering approaches to improve the quality of recombinant Fc-fusion protein production in the biopharmaceutical industry.

Published

2018

38. Sub physiological temperature induces pervasive alternative splicing in Chinese hamster ovary cells

Author

Niall Barron, Jonathan Bones, Paul S. Kelly, Ryan Hagan, Craig Monger, Justine Meiller, Patrick Floris, Krishna Motheramgari, Martin Clynes, Lin Zhang, Colin Clarke, Alan Costello, Clair Gallagher, and Ioanna Tzani

Subjects

0303 health sciences, Messenger RNA, Chinese hamster ovary cell, Alternative splicing, Biology, Exon skipping, Cell biology, Transcriptome, 03 medical and health sciences, 0302 clinical medicine, RNA splicing, Gene expression, Gene, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

RNA sequencing (RNASeq) has been widely used to associate alterations in Chinese hamster ovary (CHO) cell gene expression with bioprocess phenotypes, however alternative mRNA splicing, has thus far, received little attention. In this study, we utilised RNASeq for transcriptomic analysis of a monoclonal antibody producing CHOK1 cell line subjected to a temperature shift. More than 2,365 instances of differential splicing were observed 24hrs after the reduction of cell culture temperature. 1,163 of these alternative splicing events were identified in genes where no changes in abundance were detected by standard differential expression analysis. Ten examples of alternative splicing were selected for independent validation using qPCR in the monoclonal antibody producing CHOK1 line used for RNASeq and a further 2 CHOK1 cell lines. This analysis provided evidence that exon skipping and mutually exclusive splicing events occur in genes linked to the cellular response to changes in temperature and mitochondrial function. While further work is required to determine the impact of changes in mRNA sequence on cellular phenotype, this study demonstrates that alternative splicing analysis can be utilised to gain a deeper understanding of post-transcriptional regulation in CHO cells during biopharmaceutical production.

Published

2019

39. Novel panel of protein biomarkers to predict response to bortezomib-containing induction regimens in multiple myeloma patients

Author

Annemarie Larkin, Michael Henry, Paula Meleady, Peter O'Gorman, Despina Bazou, Martin Clynes, Kay Reen Ting, Justine Meiller, and Paul Dowling

Subjects

Proteomics, 0301 basic medicine, Oncology, medicine.medical_specialty, Protein biomarkers, Biomarker panel, Disease, Bioinformatics, Pathology and Forensic Medicine, Bortezomib, 03 medical and health sciences, 0302 clinical medicine, Physiology (medical), Internal medicine, medicine, Multiple myeloma, Mass spectrometry, business.industry, Albumin, Regular Article, Serum samples, medicine.disease, 030104 developmental biology, 030220 oncology & carcinogenesis, Molecular Medicine, business, Biomarkers, Kappa, medicine.drug

Abstract

Background Multiple myeloma (MM) is a complex heterogeneous disease. Various risk stratification models have been recommended including cytogenetic and FISH analysis to identify high-risk patients who may benefit from novel treatments, but such facilities are not widely available. The International Scoring System (ISS) using beta-2-microglobulin and albumin remains a widely used prognostic scoring system in many clinical practices; however it is not useful in predicting response to treatment in MM. The aim of this study is to identify clinically useful biomarkers to predict response to treatment containing bortezomib. Methods 17 MM patient serum samples (9 responders/8 non-responders) were used for the discovery phase (label-free mass spectrometry) and an additional 20 MM patient serum samples were used for the ELISA-based validation phase (14 responders/6 non-responders). Results CLU and ANG mean levels were higher in the responders group, while Complement C1q had lower concentrations. The combination of all standard biomarkers (albumin, beta-2-microglobulin (ß2M), paraprotein and kappa/lambda (K/L) ratio) had an AUC value of 0.71 with 65% correct classification, while an overall combination of new candidate protein biomarkers with standard biomarkers had an AUC value of 0.89 with 85.3% correct classification. Conclusions A combination of new and standard biomarkers consisting of CLU, ANG, C1Q, albumin, ß2M, paraprotein and K/L ratio may have potential as a novel panel of biomarkers to predict MM response to treatment containing bortezomib. General significance Use of this biomarker panel could facilitate a more personalized therapy approach and to minimize unnecessary side effects from ineffective drugs., Highlights • CLU and ANG mean levels were higher in the responders group. • Complement C1q mean levels were lower in the responders group. • Standard biomarker panel had an AUC value of 0.708 with 64.9% correct classification. • New biomarker panel had an AUC value of 0.89 with 85.3% correct classification. • Use of this biomarker panel could facilitate a more personalized therapy approach.

Published

2017

40. Parallel mRNA, proteomics and miRNA expression analysis in cell line models of the intestine

Author

Fiona O'Neill, Martin Clynes, Finbarr O'Sullivan, Karina Horgan, Michael Henry, Joanne Keenan, Padraig Doolan, Paula Meleady, Richard Murphy, Niall Barron, Sinead T Aherne, Laura Breen, and Colin Clarke

Subjects

Proteomics, 0301 basic medicine, Proteome, Microarray, Datasets as Topic, Down-Regulation, Biology, 03 medical and health sciences, 0302 clinical medicine, Tandem Mass Spectrometry, Mirna expression, microRNA, Humans, RNA, Messenger, Intestinal Mucosa, miRNA, Messenger RNA, Gene ontology, Gene Expression Profiling, Gastroenterology, Computational Biology, Caco-2, General Medicine, Basic Study, Targetscan, Microarray Analysis, Up-Regulation, Cell biology, Intestines, MicroRNAs, 030104 developmental biology, HT-29, 030220 oncology & carcinogenesis, Caco-2 Cells, Line (text file), HT29 Cells, Software

Abstract

AIM To identify miRNA-regulated proteins differentially expressed between Caco2 and HT-29: two principal cell line models of the intestine. METHODS Exponentially growing Caco-2 and HT-29 cells were harvested and prepared for mRNA, miRNA and proteomic profiling. mRNA microarray profiling analysis was carried out using the Affymetrix GeneChip Human Gene 1.0 ST array. miRNA microarray profiling analysis was carried out using the Affymetrix Genechip miRNA 3.0 array. Quantitative Label-free LC-MS/MS proteomic analysis was performed using a Dionex Ultimate 3000 RSLCnano system coupled to a hybrid linear ion trap/Orbitrap mass spectrometer. Peptide identities were validated in Proteome Discoverer 2.1 and were subsequently imported into Progenesis QI software for further analysis. Hierarchical cluster analysis for all three parallel datasets (miRNA, proteomics, mRNA) was conducted in the R software environment using the Euclidean distance measure and Ward’s clustering algorithm. The prediction of miRNA and oppositely correlated protein/mRNA interactions was performed using TargetScan 6.1. GO biological process, molecular function and cellular component enrichment analysis was carried out for the DE miRNA, protein and mRNA lists via the Pathway Studio 11.3 Web interface using their Mammalian database. RESULTS Differential expression (DE) profiling comparing the intestinal cell lines HT-29 and Caco-2 identified 1795 Genes, 168 Proteins and 160 miRNAs as DE between the two cell lines. At the gene level, 1084 genes were upregulated and 711 were downregulated in the Caco-2 cell line relative to the HT-29 cell line. At the protein level, 57 proteins were found to be upregulated and 111 downregulated in the Caco-2 cell line relative to the HT-29 cell line. Finally, at the miRNAs level, 104 were upregulated and 56 downregulated in the Caco-2 cell line relative to the HT-29 cell line. Gene ontology (GO) analysis of the DE mRNA identified cell adhesion, migration and ECM organization, cellular lipid and cholesterol metabolic processes, small molecule transport and a range of responses to external stimuli, while similar analysis of the DE protein list identified gene expression/transcription, epigenetic mechanisms, DNA replication, differentiation and translation ontology categories. The DE protein and gene lists were found to share 15 biological processes including for example epithelial cell differentiation [P value ≤ 1.81613E-08 (protein list); P ≤ 0.000434311 (gene list)] and actin filament bundle assembly [P value ≤ 0.001582797 (protein list); P ≤ 0.002733714 (gene list)]. Analysis was conducted on the three data streams acquired in parallel to identify targets undergoing potential miRNA translational repression identified 34 proteins, whose respective mRNAs were detected but no change in expression was observed. Of these 34 proteins, 27 proteins downregulated in the Caco-2 cell line relative to the HT-29 cell line and predicted to be targeted by 19 unique anti-correlated/upregulated microRNAs and 7 proteins upregulated in the Caco-2 cell line relative to the HT-29 cell line and predicted to be targeted by 15 unique anti-correlated/downregulated microRNAs. CONCLUSION This first study providing “tri-omics” analysis of the principal intestinal cell line models Caco-2 and HT-29 has identified 34 proteins potentially undergoing miRNA translational repression.

Published

2017

41. A novel inhibitory anti-invasive MAb isolated using phenotypic screening highlights AnxA6 as a functionally relevant target protein in pancreatic cancer

Author

Paul Dowling, Niall Swan, Brianan McGovern, Paul Barham, Fergal C. Kelleher, Annemarie Larkin, Susan Kennedy, Andrew McCann, Helena Joyce, Jean Murphy, Michael Henry, Michael Moriarty, Martin Clynes, Dermot O’Sullivan, and Edel McAuley

Subjects

0301 basic medicine, Cancer Research, Pathology, medicine.medical_specialty, Lung Neoplasms, medicine.drug_class, Phenotypic screening, Perineural invasion, Breast Neoplasms, Monoclonal antibody, novel target, Mice, 03 medical and health sciences, Pancreatic cancer, pancreatic adenocarcinoma, Biomarkers, Tumor, medicine, Animals, Humans, Neoplasm Staging, biology, business.industry, annexin A6, Antibodies, Monoclonal, Cancer, Prognosis, medicine.disease, Pancreatic Neoplasms, Survival Rate, 030104 developmental biology, Oncology, monoclonal antibody, therapeutic antibody, Cancer cell, Carcinoma, Squamous Cell, Cancer research, biology.protein, Immunohistochemistry, Female, Antibody, Translational Therapeutics, business, cancer invasion, Carcinoma, Pancreatic Ductal

Abstract

Background: Discovery and validation of new antibody tractable targets is critical for the development of new antibody therapeutics to address unmet needs in oncology. Methods: A highly invasive clonal variant of the MDA-MB-435S cell line was used to generate monoclonal antibodies (MAbs), which were screened for anti-invasive activity against aggressive cancer cells in vitro. The molecular target of selected inhibitory MAb 9E1 was identified using immunoprecipitation/liquid chromatography-tandem mass spectrometry. The potential anti-tumour effects of MAb 9E1 were investigated in vitro together with immunohistochemical analysis of the 9E1 target antigen in normal and cancer tissues. Results: MAb 9E1 significantly decreases invasion in pancreatic, lung squamous and breast cancer cells and silencing of its target antigen, which was revealed as AnxA6, leads to markedly reduced invasive capacity of pancreatic and lung squamous cancer in vitro. IHC using MAb 9E1 revealed that AnxA6 exhibits a high prevalence of membrane immunoreactivity across aggressive tumour types with restricted expression observed in the majority of normal tissues. In pancreatic ductal adenocarcinoma, high AnxA6 IHC score correlated with the presence of tumour budding at the invasive front of tumours (P=0.082), the presence of perineural invasion (P=

Published

2017

42. Neutrophil Membrane Cholesterol Content is a Key Factor in Cystic Fibrosis Lung Disease

Author

Elaine Hayes, Ryan Flannery, Cedric Gunaratnam, Michael Henry, Emer P. Reeves, Michelle M. White, Oliver J. McElvaney, William Leitch, Joanne Keenan, Bader Alfawaz, Martin Clynes, Gillian M. Lavelle, Paula Meleady, Noel G. McElvaney, Patrick Geraghty, and Stephen Cox

Subjects

0301 basic medicine, Male, Proteomics, Proteome, CXCL, C-X-C Motif Chemokine Ligand, Neutrophils, Caveolin 1, Cystic Fibrosis Transmembrane Conductance Regulator, lcsh:Medicine, PWCF, patients with CF, Pharmacology, Cystic fibrosis, Ivacaftor, chemistry.chemical_compound, Mice, 0302 clinical medicine, MβCD, methyl-β-cyclodextrin, TNF-α, tumor necrosis factor alpha, Mice, Knockout, lcsh:R5-920, Calpain, General Medicine, Endoplasmic Reticulum Stress, Cav−/−, caveolin-1 knock-out mice, Cystic fibrosis transmembrane conductance regulator, Respiratory Function Tests, Cholesterol, Integrin alpha M, Pseudomonas aeruginosa, Female, Disease Susceptibility, medicine.symptom, Inflammation Mediators, lcsh:Medicine (General), medicine.drug, Research Paper, Adult, Genotype, Inflammation, HL-60 Cells, Biology, General Biochemistry, Genetics and Molecular Biology, sTNFR1, soluble TNF receptor 1, 03 medical and health sciences, Membrane Microdomains, medicine, Cell Adhesion, Animals, Humans, CFTR, cystic fibrosis transmembrane conductance regulator, Cell adhesion, Alleles, Lung transplant therapy, CF, cystic fibrosis, Cell Membrane, lcsh:R, medicine.disease, CD11b, integrin alpha-M, Disease Models, Animal, 030104 developmental biology, Membrane protein, chemistry, Immunology, Chronic Disease, Mutation, biology.protein, Commentary, Ivacaftor therapy, 030215 immunology

Abstract

Background Identification of mechanisms promoting neutrophil trafficking to the lungs of patients with cystic fibrosis (CF) is a challenge for next generation therapeutics. Cholesterol, a structural component of neutrophil plasma membranes influences cell adhesion, a key step in transmigration. The effect of chronic inflammation on neutrophil membrane cholesterol content in patients with CF (PWCF) remains unclear. To address this we examined neutrophils of PWCF to evaluate the cause and consequence of altered membrane cholesterol and identified the effects of lung transplantation and ion channel potentiator therapy on the cellular mechanisms responsible for perturbed membrane cholesterol and increased cell adhesion. Methodology PWCF homozygous for the ΔF508 mutation or heterozygous for the G551D mutation were recruited (n = 48). Membrane protein expression was investigated by mass spectrometry. The effect of lung transplantation or ivacaftor therapy was assessed by ELISAs, and calcium fluorometric and μ-calpain assays. Findings Membranes of CF neutrophils contain less cholesterol, yet increased integrin CD11b expression, and respond to inflammatory induced endoplasmic reticulum (ER) stress by activating μ-calpain. In vivo and in vitro, increased μ-calpain activity resulted in proteolysis of the membrane cholesterol trafficking protein caveolin-1. The critical role of caveolin-1 for adequate membrane cholesterol content was confirmed in caveolin-1 knock-out mice. Lung transplant therapy or treatment of PWCF with ivacaftor, reduced levels of circulating inflammatory mediators and actuated increased caveolin-1 and membrane cholesterol, with concurrent normalized neutrophil adhesion. Interpretation Results demonstrate an auxiliary benefit of lung transplant and potentiator therapy, evident by a reduction in circulating inflammation and controlled neutrophil adhesion., Highlights • This study explored neutrophil adhesion in cystic fibrosis. • Altered membrane cholesterol lead to increased adhesion. • Circulating inflammatory mediators caused increased calpain activity and reduced membrane cholesterol content. In patients with cystic fibrosis (CF), chronic inflammation in the circulation, in part originating from the pulmonary compartment, leads to decreased membrane cholesterol in circulating neutrophils, resulting in increased cell adhesion. The mechanism of action involves proteolytic down-regulation of the cholesterol trafficking protein caveolin-1. The overall effect of lung transplant therapy, or CFTR potentiator treatment, was to significantly diminish the circulating inflammatory burden thereby permitting caveolin-1 expression, with concomitant decreased CF cell adhesion and significant clinical improvement.

Published

2017

43. Proteomic analysis of bronchoalveolar lavage fluid (BALF) from lung cancer patients using label-free mass spectrometry

Author

Ross K. Morgan, Vincent J. Lynch, Martin Clynes, Abduladim Hmmier, Michael Emmet O'Brien, and Paul Dowling

Subjects

Proteomics, 0301 basic medicine, Pathology, medicine.medical_specialty, Pathology and Forensic Medicine, Plasma, 03 medical and health sciences, 0302 clinical medicine, Physiology (medical), medicine, Lung cancer, Mass spectrometry, medicine.diagnostic_test, business.industry, Regular Article, respiratory system, medicine.disease, respiratory tract diseases, 3. Good health, HSPA1A, BALF, 030104 developmental biology, Bronchoalveolar lavage, 030220 oncology & carcinogenesis, Immunoassay, Molecular Medicine, Biomarker (medicine), Adenocarcinoma, ELISA, business, Biomarkers, Lung cancer screening

Abstract

Background Lung cancer is the leading cause of cancer-related mortality in both men and women throughout the world. The need to detect lung cancer at an early, potentially curable stage, is essential and may reduce mortality by 20%. The aim of this study was to identify distinct proteomic profiles in bronchoalveolar fluid (BALF) and plasma that are able to discriminate individuals with benign disease from those with non-small cell lung cancer (NSCLC). Methods Using label-free mass spectrometry analysis of BALF during discovery-phase analysis, a significant number of proteins were found to have different abundance levels when comparing control to adenocarcinoma (AD) or squamous cell lung carcinoma (SqCC). Validation of candidate biomarkers identified in BALF was performed in a larger cohort of plasma samples by detection with enzyme-linked immunoassay. Results Four proteins (Cystatin-C, TIMP-1, Lipocalin-2 and HSP70/HSPA1A) were selected as a representative group from discovery phase mass spectrometry BALF analysis. Plasma levels of TIMP-1, Lipocalin-2 and Cystatin-C were found to be significantly elevated in AD and SqCC compared to control. Conclusion The results presented in this study indicate that BALF is an important proximal biofluid for the discovery and identification of candidate lung cancer biomarkers. General significance There is good correlation between the trend of protein abundance levels in BALF and that of plasma which validates this approach to develop a blood biomarker to aid lung cancer diagnosis, particularly in the era of lung cancer screening. The protein signatures identified also provide insight into the molecular mechanisms associated with lung malignancy., Highlights • BALF proteome harbours significant differences between control and NCSLC. • Significant difference in proteins detected between AD and SqCC in BALF • Good correlation between proteins with altered abundance levels in BALF and plasma • Cystatin-C, TIP-1 and Lipocalin significantly changed in both BALF and plasma.

Published

2017

44. Characterisation and proteomic profiling of continuously exposed Cu-resistant variants of the Caco-2 cell line

Author

Michael Henry, Paula Meleady, Indre Sinkunaite, Finbarr O'Sullivan, Karina Horgan, Charles O’Doherty, Richard Murphy, Joanne Keenan, and Martin Clynes

Subjects

0301 basic medicine, Proteomics, Proteome, Cell Survival, Cell, Toxicology, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, medicine, Metallothionein, Humans, Gene, Proteomic Profiling, Superoxide Dismutase, General Medicine, Glutathione, Drug Tolerance, Molecular biology, 030104 developmental biology, medicine.anatomical_structure, chemistry, Caco-2, Cell culture, 030220 oncology & carcinogenesis, Subculture (biology), Caco-2 Cells, Reactive Oxygen Species, Copper

Abstract

Studies in hepatic systems identify multiple factors involved in the generation of copper resistance. As the intestine is the route of exposure to dietary copper, we wanted to understand how intestinal cells overcome the toxic effects of high copper and what mechanisms of resistance develop. Using the intestinal cell line Caco-2, resistance was developed by serial subculture in 50 μM copper in inorganic (CuSO4) or organic (Cu proteinate) forms. Caco-2 variants exhibited resistance to copper and retained the non-monotonic dose response while displaying stable phenotypes following repeated subculture in the absence of copper. Phenotypic changes on exposure to copper in parental Caco-2 cells included significantly increased total protein yield, ROS, SOD, metallothionein expression, GSH and total glutathione. These phenotypic changes were not replicated in resistant variants on a per cell basis. Quantitative label-free LC-MS/MS proteomic analysis identified 1113 differentially expressed proteins (DEPs) between parental Caco-2 and resistant cells. With some exceptions, most of the DEPs were overexpressed to a low level around 2-fold suggesting resistance was supported by multiple small changes in protein expression. These variants may be a useful tool in studying the toxicity of stress responses in further Cu-related studies.

Published

2019

45. An arginase-based system for selection of transfected CHO cells without the use of toxic chemicals

Author

Padraig Doolan, Nga T. Lao, Berta Capella Roca, Martin Clynes, and Niall Barron

Subjects

0301 basic medicine, Spermine, CHO Cells, Biochemistry, Cell Line, 03 medical and health sciences, chemistry.chemical_compound, Cricetulus, Polyamines, Putrescine, Animals, Molecular Biology, Erythropoietin, 030102 biochemistry & molecular biology, Arginase, Cell growth, Chinese hamster ovary cell, Methods and Resources, Cell Biology, Transfection, Recombinant Proteins, Cell biology, Spermidine, 030104 developmental biology, chemistry, Polyamine

Abstract

Polyamines have essential roles in cell proliferation, DNA replication, transcription, and translation processes, with intracellular depletion of putrescine, spermidine, and spermine resulting in cellular growth arrest and eventual death. Serum-free media for CHO-K1 cells require putrescine supplementation, because these cells lack the first enzyme of the polyamine production pathway, arginase. On the basis of this phenotype, we developed an arginase-based selection system. We transfected CHO-K1 cells with a bicistronic vector co-expressing GFP and arginase and selected cells in media devoid of l-ornithine and putrescine, resulting in mixed populations stably expressing GFP. Moreover, single clones in these selective media stably expressed GFP for a total of 42 generations. Using this polyamine starvation method, we next generated recombinant CHO-K1 cells co-expressing arginase and human erythropoietin (hEPO), which also displayed stable expression and healthy growth. The hEPO-expressing clones grew in commercial media, such as BalanCD and CHO-S serum-free media (SFM)-II, as well as in a defined serum-free, putrescine-containing medium for at least 9 passages (27 generations), with a minimal decrease in hEPO titer by the end of the culture. We observed a lack of arginase activity also in several CHO cell strains (CHO-DP12, CHO-S, and DUXB11) and other mammalian cell lines, including BHK21, suggesting broader utility of this selection system. In conclusion, we have established an easy-to-apply alternative selection system that effectively generates mammalian cell clones expressing biopharmaceutically relevant or other recombinant proteins without the need for any toxic selective agents. We propose that this system is applicable to mammalian cell lines that lack arginase activity.

Published

2019

46. Investigation and circumvention of transfection inhibition by ferric ammonium citrate in serum-free media for Chinese hamster ovary cells

Author

Martin Clynes, Padraig Doolan, Nga T. Lao, and Berta Capella Roca

Subjects

0106 biological sciences, animal structures, Cell Survival, viruses, CHO Cells, Transfection, 01 natural sciences, Ferric Compounds, Culture Media, Serum-Free, Cricetulus, 010608 biotechnology, medicine, Animals, Liposome, Chemistry, Chinese hamster ovary cell, fungi, 010401 analytical chemistry, Ammonium citrate, Molecular biology, 0104 chemical sciences, Quaternary Ammonium Compounds, Lipofectamine, Cell culture, embryonic structures, Liposomes, Ferric, Biotechnology, medicine.drug, Serum free media

Abstract

While reliable transfection methods are essential for Chinese hamster ovary (CHO) cell line engineering, reduced transfection efficiencies have been observed in several commercially prepared media. In this study, we aimed to assess common media additives that impede efficiency mediated by three chemical transfection agents: liposomal-based (Lipofectamine 2000), polymer-based (TransIT-X2), and lipopolyplex-based (TransIT-PRO). An in-house GFP-expressing vector and serum-free medium (BCR-F12: developed for the purposes of this study) were used to analyze transient transfection efficiencies of three CHO cell lines (CHO-K1, DG44, DP12). Compared to a selection of commercially available media, BCR-F12 displayed challenges associated with transfection in vendor-prepared formulations, with no detection when liposomal-based methods were used, reduced (

Published

2019

47. Why we need good mentoring

Author

Martin, Clynes, Anita, Corbett, and Julie, Overbaugh

Subjects

Leadership, Biomedical Research, Career Choice, Interprofessional Relations, Models, Organizational, Mentors, Awards and Prizes, Humans, Mentoring, Medical Oncology

Abstract

Cancer research relies on key values such as creativity, collaboration, research integrity and resource sharing. A positive research environment which fosters these key values is becoming a decisive factor for some funders and research institutions. To create a supportive research culture in laboratories, the training and mentoring of young scientists is important. However, the fast-paced and fierce competition for funding and jobs can present a challenge to the younger generation of scientists who depend on the guidance and mentorship of scientific leaders. The annual Nature Awards for Mentoring in Science have been created to bring attention to one of the most essential but least recognized skills in scientific leadership. Thus far, 35 scientists from across the world, who are working in a range of disciplines, have been recognized by this award for their outstanding scientific mentorship. In this Viewpoint, we have asked three recipients of this award who work in fields associated with cancer research about their views on good mentoring, and how a revised approach to mentorship can help to achieve a positive research culture and contribute to scientific discovery.

Published

2019

48. Zinc supplementation increases protein titer of recombinant CHO cells

Author

Padraig Doolan, Antonio Alarcon Miguez, Joanne Keenan, Srinivas Suda, Martin Clynes, Berta Capella Roca, Niall Barron, and Donal J. O’Gorman

Subjects

0301 basic medicine, Chinese hamster ovary cell, Clinical Biochemistry, Biomedical Engineering, chemistry.chemical_element, Bioengineering, Cell Biology, Zinc, Metabolism, Molecular biology, law.invention, 03 medical and health sciences, Chemically defined medium, chemistry.chemical_compound, Titer, 030104 developmental biology, 0302 clinical medicine, chemistry, law, Cell culture, 030220 oncology & carcinogenesis, Aurintricarboxylic acid, Recombinant DNA, Original Article, Biotechnology

Abstract

In order to study the impact of zinc and copper on the titer levels of mAb and recombinant protein in CHO cells, the IgG-expressing (DP12) and EPO-expressing (SK15) cell lines were cultured in chemically defined media with increasing concentrations of either metal. Supplementation with 25 mg/l in CDM media resulted in a significant increase in EPO (1.7-fold) and IgG (2.6-fold) titers compared to control (no added zinc). Titers at this Zn concentration in CDM containing the insulin replacing agent aurintricarboxylic acid (ATA) (CDM + A) showed a 1.8-fold (EPO) and 1.2-fold (IgG) titers increase compared to control. ATA appeared to also reduce the specific productivity (Qp) enhancement induced by Zn-25, with up to 4.9-fold (DP12) and 1.9-fold (SK15) Qp increase in CDM compared to the 1.6-fold (DP12) and 1.5-fold (SK15) Qp increase observed in CDM + A. A 31% reduced Viable Cell Density (VCD) in DP12 was observed in both Zn-supplemented media (3 × 10(6) cells/ml vs 4.2 × 10(6) cells/ml, day 5), whereas SK15 Zn-25 cultures displayed a 24% lower peak only in CDM + A (2.2 × 10(6) cells/ml vs 3.2 × 10(6) cells/ml, day 5). Supplementation with copper at 13.7–20 mg/l resulted in less significant cell line/product-type dependent effects on titer, VCD and Viability. Analysis of the energetic phenotype of both cell lines in 25 mg/l Zn-supplemented CDM media revealed a twofold increase in the oxygen consumption rate (OCR) compared to non-supplemented cells. Together, these data suggest that high zinc supplementation may induce an increase in oxidative respiration metabolism that results in increased Qp and titers in suspension CHO cultures. ELECTRONIC SUPPLEMENTARY MATERIAL: The online version of this article (10.1007/s10616-019-00334-1) contains supplementary material, which is available to authorized users.

Published

2019

49. Improvements in single-use bioreactor film material composition leads to robust and reliable Chinese hamster ovary cell performance

Author

Christine Ta, Antonio Alarcon Miguez, Jonathan Bones, Paul S. Kelly, Sara Carillo, Emma Harper, Michael Henry, Orla Coleman, Martin Clynes, Paula Meleady, Noemí Dorival-García, Samantha Paré, Niall Barron, Lisa Connolly, Maeve Shannon, and SFI

Subjects

Single‐use bioreactors, Proteomics, Cell Survival, Seahorse XF96, Cell Culture Techniques, Oxidative phosphorylation, CHO Cells, Mitochondrion, Bioreactors, Cricetulus, Tandem Mass Spectrometry, Cricetinae, Bioreactor, Animals, leachables, Bioprocess, Cells, Cultured, Cell Proliferation, endocrine disruptor, Chemistry, Chinese hamster ovary cell, single-use bioreactors, Metabolism, single use technologies, In vitro, Single-use bioreactor, Cell biology, mitochondria, Culture Media, Conditioned, Chinese hamster ovary cells, Biotechnology, bDtBPP, Chromatography, Liquid

Abstract

Single‐use technologies, in particular disposable bioreactor bags, have become integral within the biopharmaceutical community. However, safety concerns arose upon the identification of toxic leachable compounds derived from the plastic materials. Although the leachable bis(2,4‐di‐tert‐butylphenyl)‐phosphate (bDtBPP) has been previously shown to inhibit CHO cell growth, it is critical to determine if other compounds like this are still present in subsequent generations of films for industrial application. This study compares the performance of CHO cells, CHO‐K1, and CHO‐DP12, cultured in media conditioned in an older single‐use bioreactor (SUB) film (F‐1) and a newer generation film (F‐2) from the same vendor. CHO cells cultured in media conditioned for 7 days in the F‐1 film demonstrated significantly reduced growth and antibody productivity profiles when compared to controls and media conditioned for the same time period in the newer F‐2 film. Proteomic profiling of CHO cells cultured in the F‐1 conditioned media identified differentially expressed proteins involved in oxidative stress response as well as compromised ATP synthesis. These potentially metabolically compromised cells exhibited reduced oxidative phosphorylation activity as well as lower glycolytic metabolism, characteristic of slower growing cells. Nonvolatile and metal leachables analysis of film extracts by LC–MS revealed a reduction in the abundance of the analyzed leachates from F‐2 films when compared to F‐1 films including bDtBPP, potentially explaining improved CHO cell growth in F‐2 conditioned media. Furthermore, in vitro endocrine disruptor testing of the known leachable revealed this molecule to possess the potential to act as an androgen antagonist. This study demonstrates an improvement in the materials composition used in modern generations of SUBs for safe application in the bioprocess. Science Foundation Ireland Irish Industry Technical Group (Allergan Pharmaceuticals Ireland, BioMarin Manufacturing Ireland Ltd., Eli Lilly and Company, Genzyme Ireland Ltd. A Sanofi Company, Janssen Biologics, MSD and Pfizer Ireland Pharmaceuticals) Dublin City University

Published

2018

50. Quantitative label-free mass spectrometry analysis of formalin-fixed, paraffin-embedded tissue representing the invasive cutaneous malignant melanoma proteome

Author

Mairin McMenamin, Paul Dowling, Mary Monks, Martin Clynes, Edel McAuley, Annemarie Larkin, Michael Henry, Paula Meleady, Bairbre Wynne, Benvon Moran, Patrick Ormond, and Niamh Leonard

Subjects

0301 basic medicine, Cancer Research, Pathology, medicine.medical_specialty, Biology, FFPE, 14-3-3ε, Tandem mass spectrometry, Proteomics, Biological pathway, 03 medical and health sciences, proteomics, 0302 clinical medicine, melanoma, medicine, mass spectrometry, Tissue microarray, Melanoma, Cancer, Articles, medicine.disease, FASN, 030104 developmental biology, Oncology, 030220 oncology & carcinogenesis, Proteome, Cancer research, Immunohistochemistry

Abstract

Understanding the events at a protein level that govern the progression from melanoma in situ to invasive melanoma are important areas of current research to be developed. Recent advances in the analysis of formalin-fixed, paraffin-embedded tissue by proteomics, particularly using the filter-aided sample preparation protocol, has opened up the possibility of studying vast archives of clinical material and associated medical records. In the present study, quantitative protein profiling was performed using tandem mass spectrometry, and the proteome differences between melanoma in situ and invasive melanoma were compared. Biological pathway analyses revealed several signalling pathways differing between melanoma in situ and invasive melanoma, including metabolic pathways and the phosphoinositide 3-kinase-Akt signalling pathway. Selected proteins of interest (14–3-3ε and fatty acid synthase) were subsequently investigated using immunohistochemical analysis of tissue microarrays. Identifying the key proteins that play significant roles in the establishment of a more invasive phenotype in melanoma may ultimately aid diagnosis and treatment decisions.

Published

2016