Your search keyword '"Anthony D. Whetton"' showing total 99 results

1. Generation of a mouse SWATH-MS spectral library to quantify 10148 proteins involved in cell reprogramming

Author

Anthony D. Whetton, Stefano Patassini, Uxue Ulanga, Matthew R. Russell, Robert Graham, Ciaren Graham, and Julie A. Brazzatti

Subjects

Statistics and Probability, Proteomics, Swath ms, Data Descriptor, Proteome, Computer science, Proteotypic peptide, Absolute quantification, Science, Population, Protein Array Analysis, Computational biology, Library and Information Sciences, Proteome informatics, Education, 03 medical and health sciences, Mice, 0302 clinical medicine, Animals, Data-independent acquisition, education, Databases, Protein, 030304 developmental biology, 0303 health sciences, education.field_of_study, Mass spectrometry, Reprogramming, Cellular Reprogramming, Computer Science Applications, Induced pluripotent stem cells, Statistics, Probability and Uncertainty, 030217 neurology & neurosurgery, Information Systems

Abstract

Murine models are amongst the most widely used systems to study biology and pathology. Targeted quantitative proteomic analysis is a relatively new tool to interrogate such systems. Recently the need for relative quantification on hundreds to thousands of samples has driven the development of Data Independent Acquisition methods. One such technique is SWATH-MS, which in the main requires prior acquisition of mass spectra to generate an assay reference library. In stem cell research, it has been shown pluripotency can be induced starting with a fibroblast population. In so doing major changes in expressed proteins is inevitable. Here we have created a reference library to underpin such studies. This is inclusive of an extensively documented script to enable replication of library generation from the raw data. The documented script facilitates reuse of data and adaptation of the library to novel applications. The resulting library provides deep coverage of the mouse proteome. The library covers 29519 proteins (53% of the proteome) of which 7435 (13%) are supported by a proteotypic peptide., Measurement(s) database type spectral library • protein expression data Technology Type(s) liquid chromatography-electrospray ionisation time-of-flight mass spectrometry • SWATH MS protein profiling assay Factor Type(s) treatment • cell development stage Sample Characteristic - Organism Mus musculus Machine-accessible metadata file describing the reported data: 10.6084/m9.figshare.14135576

Published

2021

2. EVI1 carboxy-terminal phosphorylation is ATM-mediated and sustains transcriptional modulation and self-renewal via enhanced CtBP1 association

Author

Roberto Paredes, Anthony D. Whetton, Adam Stevens, Daniel H. Wiseman, Andrew Pierce, Kathleen Connors, Axel Schambach, Harald Löffler, John A. Chadwick, Stella Pearson, James R Kelly, Henri J. van de Vrugt, Andrew J.K. Williamson, Stefan Meyer, Helen Smith, Olga S. Kustikova, Daniel J. White, Simon C. Lovell, Joanne Muter, Hsiang Ying Teng, Marion Schneider, Richard D. Unwin, Tim C. P. Somervaille, and VU University medical center

Subjects

ResearchInstitutes_Networks_Beacons/MICRA, Ataxia Telangiectasia Mutated Proteins, Biology, Self renewal, Cell Line, CTBP1, Cell Line, Tumor, Genetics, Animals, Humans, Cell Self Renewal, Phosphorylation, Manchester Cancer Research Centre, Gene Expression Regulation, Leukemic, ResearchInstitutes_Networks_Beacons/mcrc, Gene Expression Profiling, Gene regulation, Chromatin and Epigenetics, MDS1 and EVI1 Complex Locus Protein, Cell biology, DNA-Binding Proteins, Alcohol Oxidoreductases, HEK293 Cells, Manchester Institute for Collaborative Research on Ageing, Terminal (electronics), Leukemia, Myeloid, Acute Disease, Mutation, Nucleic acid

Abstract

The transcriptional regulator EVI1 has an essential role in early hematopoiesis and development. However, aberrantly high expression of EVI1 has potent oncogenic properties and confers poor prognosis and chemo-resistance in leukemia and solid tumors. To investigate to what extent EVI1 function might be regulated by post-translational modifications we carried out mass spectrometry- and antibody-based analyses and uncovered an ATM-mediated double phosphorylation of EVI1 at the carboxy-terminal S858/S860 SQS motif. In the presence of genotoxic stress EVI1-WT (SQS), but not site mutated EVI1-AQA was able to maintain transcriptional patterns and transformation potency, while under standard conditions carboxy-terminal mutation had no effect. Maintenance of hematopoietic progenitor cell clonogenic potential was profoundly impaired with EVI1-AQA compared with EVI1-WT, in particular in the presence of genotoxic stress. Exploring mechanistic events underlying these observations, we showed that after genotoxic stress EVI1-WT, but not EVI1-AQA increased its level of association with its functionally essential interaction partner CtBP1, implying a role for ATM in regulating EVI1 protein interactions via phosphorylation. This aspect of EVI1 regulation is therapeutically relevant, as chemotherapy-induced genotoxicity might detrimentally sustain EVI1 function via stress response mediated phosphorylation, and ATM-inhibition might be of specific targeted benefit in EVI1-overexpressing malignancies.

Published

2018

3. The Antiproliferative Activity of Kinase Inhibitors in Chronic Myeloid Leukemia Cells Is Mediated by FOXO Transcription Factors

Author

Francesca Pellicano, Mary T. Scott, Tessa L. Holyoake, G. Vignir Helgason, Andrew Pierce, Mhairi Copland, Brian J. P. Huntly, Mark Aspinall-O'Dea, Anthony D. Whetton, Elaine K. Allan, and Lisa E. M. Hopcroft

Subjects

FOXO transcription factors, Dasatinib, Apoptosis, Biology, Quiescence, Transfection, 03 medical and health sciences, Mice, 0302 clinical medicine, hemic and lymphatic diseases, Cancer Stem Cells, Cell Line, Tumor, Leukemia, Myelogenous, Chronic, BCR-ABL Positive, medicine, Animals, Humans, Phosphorylation, Protein kinase B, BCR-ABL, Protein Kinase Inhibitors, PI3K/AKT/mTOR pathway, 030304 developmental biology, Tyrosine kinase inhibitors, 0303 health sciences, Manchester Cancer Research Centre, ResearchInstitutes_Networks_Beacons/mcrc, Gene Expression Profiling, Chronic myeloid leukemia, G1 Phase, Myeloid leukemia, Forkhead Transcription Factors, Cell Biology, Cell Cycle Checkpoints, Cell cycle, respiratory tract diseases, Cell biology, 030220 oncology & carcinogenesis, Cancer research, Neoplastic Stem Cells, Molecular Medicine, CD34+ progenitor cells, Signal transduction, K562 Cells, Tyrosine kinase, Developmental Biology, medicine.drug, K562 cells, Signal Transduction

Abstract

Chronic myeloid leukemia (CML) is initiated and maintained by the tyrosine kinase BCR-ABL which activates a number of signal transduction pathways, including PI3K/AKT signaling and consequently inactivates FOXO transcription factors. ABL-specific tyrosine kinase inhibitors (TKIs) induce minimal apoptosis in CML progenitor cells, yet exert potent antiproliferative effects, through as yet poorly understood mechanisms. Here, we demonstrate that in CD34+ CML cells, FOXO1 and 3a are inactivated and relocalized to the cytoplasm by BCR-ABL activity. TKIs caused a decrease in phosphorylation of FOXOs, leading to their relocalization from cytoplasm (inactive) to nucleus (active), where they modulated the expression of key FOXO target genes, such as Cyclin D1, ATM, CDKN1C, and BCL6 and induced G1 arrest. Activation of FOXO1 and 3a and a decreased expression of their target gene Cyclin D1 were also observed after 6 days of in vivo treatment with dasatinib in a CML transgenic mouse model. The over-expression of FOXO3a in CML cells combined with TKIs to reduce proliferation, with similar results seen for inhibitors of PI3K/AKT/mTOR signaling. While stable expression of an active FOXO3a mutant induced a similar level of quiescence to TKIs alone, shRNA-mediated knockdown of FOXO3a drove CML cells into cell cycle and potentiated TKI-induced apoptosis. These data demonstrate that TKI-induced G1 arrest in CML cells is mediated through inhibition of the PI3K/AKT pathway and reactivation of FOXOs. This enhanced understanding of TKI activity and induced progenitor cell quiescence suggests that new therapeutic strategies for CML should focus on manipulation of this signaling network. Stem Cells 2014;32:2324–2337

Published

2014

4. The role of the tumor-microenvironment in lung cancer-metastasis and its relationship to potential therapeutic targets

Author

Anthony D. Whetton, Maria Pernemalm, Steven L. Wood, and Philip A.J. Crosbie

Subjects

Pathology, medicine.medical_specialty, Lung Neoplasms, Cell Communication, Metastasis, Cancer stem cell, Carcinoma, Non-Small-Cell Lung, Tumor Microenvironment, medicine, Animals, Humans, Radiology, Nuclear Medicine and imaging, Molecular Targeted Therapy, Epithelial–mesenchymal transition, Neoplasm Metastasis, Lung cancer, Tumor microenvironment, business.industry, Intravasation, General Medicine, medicine.disease, Primary tumor, Oncology, Cancer cell, Cancer research, Stromal Cells, business

Abstract

Non-small cell lung cancer (NSCLC) accounts for >80% of lung cancer cases and currently has an overall five-year survival rate of only 15%. Patients presenting with advanced stage NSCLC die within 18-months of diagnosis. Metastatic spread accounts for >70% of these deaths. Thus elucidation of the mechanistic basis of NSCLC-metastasis has potential to impact on patient quality of life and survival. Research on NSCLC metastasis has recently expanded to include non-cancer cell components of tumors-the stromal cellular compartment and extra-cellular matrix components comprising the tumor-microenvironment. Metastasis (from initial primary tumor growth through angiogenesis, intravasation, survival in the bloodstream, extravasation and metastatic growth) is an inefficient process and few released cancer cells complete the entire process. Micro-environmental interactions assist each of these steps and discovery of the mechanisms by which tumor cells co-operate with the micro-environment are uncovering key molecules providing either biomarkers or potential drug targets. The major sites of NSCLC metastasis are brain, bone, adrenal gland and the liver. The mechanistic basis of this tissue-tropism is beginning to be elucidated offering the potential to target stromal components of these tissues thus targeting therapy to the tissues affected. This review covers the principal steps involved in tumor metastasis. The role of cell-cell interactions, ECM remodeling and autocrine/paracrine signaling interactions between tumor cells and the surrounding stroma is discussed. The mechanistic basis of lung cancer metastasis to specific organs is also described. The signaling mechanisms outlined have potential to act as future drug targets minimizing lung cancer metastatic spread and morbidity.

Published

2014

5. Features of lineage-specific hematopoietic metabolism revealed by mitochondrial proteomics

Author

Dietger Niederwieser, Anthony D. Whetton, Nicole Noack, Claudia Billing, Uta Ceglarek, Michael J. Walker, Michael Cross, and Christian Böhme

Subjects

0301 basic medicine, Proteomics, Myeloid, Mouse, Biology, Mitochondrion, Biochemistry, Mitochondrial Proteins, 03 medical and health sciences, Mice, medicine, Animals, Cell Lineage, Erythropoiesis, Molecular Biology, Mitochondrial transport, Cells, Cultured, Hematopoietic system, Myelopoiesis, Manchester Cancer Research Centre, ResearchInstitutes_Networks_Beacons/mcrc, Cell Differentiation, Hematopoietic Stem Cells, Cell biology, Mitochondria, Haematopoiesis, 030104 developmental biology, medicine.anatomical_structure, Metabolism, Differentiation, Signal transduction, Signal Transduction

Abstract

Hematopoietic bone marrow is a regenerative tissue of high clinical relevance, yet relatively little is known about the metabolism of the stem and progenitor populations concerned. We have used a multipotent murine cell line to generate sufficient numbers of cells undergoing self-renewal, erythroid or myeloid differentiation to allow a proteomics analysis of enriched mitochondria. Stringent analysis identified 37 mitochondria-associated proteins changing on differentiation in this system. Those induced during differentiation were commonly associated with mature cell functions, while those inactivated upon differentiation indicate widespread changes in mitochondrial transport, fatty acid catabolism and oxidative phosphorylation. An erythroid specific reduction in glutamate pyruvate amino transferase 2 was confirmed at the protein level by Western blotting and at the functional level by assays of metabolite turnover. In addition to validating the dataset, these findings suggest significant differences in the core-metabolism between erythropoiesis and myelopoiesis. This knowledge is of relevance to the in vitro production of cell therapy products and to studies of the interdependence of metabolic and signaling pathways in regenerative tissues. Data are available via ProteomeXchange with identifier PXD002968.

Published

2017

6. The Use of Proteomics for Systematic Analysis of Normal and Transformed Hematopoietic Stem Cells

Author

Sara Cadeco, Anthony D. Whetton, and Andrew J.K. Williamson

Subjects

Proteomics, Pharmacology, Biology, Hematopoietic Stem Cells, medicine.disease, Hematopoiesis, Cell biology, Blood cell, Leukemia, Haematopoiesis, Cell Transformation, Neoplastic, Myeloproliferative Disorders, medicine.anatomical_structure, Drug Discovery, medicine, Animals, Humans, Phosphorylation, Stem cell, Progenitor cell, Protein Processing, Post-Translational

Abstract

Blood cell production involves the commitment and differentiation of hematopoietic stem cells to committed progenitor cells which undergo a programmed development to form mature cells such as neutrophils, macrophages and lymphocytes. This complex process can be disrupted in diseases such as the leukemias and myeloproliferative disorders by oncogenes such as protein tyrosine kinases. The analysis of expression patterns for specific genes suggests that the regulation of protein expression can be achieved in a posttranslational fashion. Post-translational protein modification, such as phosphorylation and acetylation govern events in blood cell production and yet cannot be measured using conventional molecular biology approaches. For this reason a suite of techniques in mass spectrometry needs to be applied to define regulation and disregulation in normal and abnormal hematopoiesis. These approaches include discovery proteomics with relative quantification of thousands of proteins. Alternatively targeted examination of a single protein to identify its interaction partners or post-translational modifications using mass spectrometry reveals much mechanistic detail. The use of mass spectrometry and proteomics approaches in stem cell and leukemia studies has thus far revealed a good deal of information on hematopoiesis. Further application of the proteomics approach is a necessity to gain true insight into regulatory processes governing the production of billions of blood cells a day, and ways in which that process can be manipulated to therapeutic advantage.

Published

2012

7. An ataxia-telangiectasia-mutated (ATM) kinase mediated response to DNA damage down-regulates the mRNA-binding potential of THOC5

Author

Sheetal Ramachandran, Sabine Klebba-Faerber, Anthony D. Whetton, Teruko Tamura, Doan Duy Hai Tran, and Christian Kardinal

Subjects

HMG-box, DNA damage, DNA repair, Down-Regulation, Cell Cycle Proteins, Eukaryotic DNA replication, Ataxia Telangiectasia Mutated Proteins, Protein Serine-Threonine Kinases, Biology, Mice, Transcription (biology), Report, Animals, RNA, Messenger, CHEK1, Molecular Biology, Cells, Cultured, DNA-PKcs, DNA clamp, Tumor Suppressor Proteins, Nuclear Proteins, RNA-Binding Proteins, Molecular biology, DNA-Binding Proteins, Mutation, DNA Damage

Abstract

In response to DNA damage, transcription is blocked by inhibition of RNA polymerase II activity. The regulation of a preexisting pool of mRNAs, therefore, plays a key role in DNA repair, cell cycle arrest, or inhibition of differentiation. THOC5 is a member of the THO complex and plays a role in the export of a subset of mRNA, which plays an important role in hematopoiesis and maintaining primitive cells. Since three serine residues in the PEST domain of THOC5 have been shown to be directly phosphorylated by ataxia-telangiectasia-mutated (ATM) kinase, we examined the THOC5-dependent mRNA export under DNA damage. We show here that DNA damage drastically decreased the cytoplasmic pool of a set of THOC5-dependent mRNAs and impaired the THOC5/mRNA complex formation. The mRNP complex formed with nonphosphorylation mutant (S307/312/314A) THOC5, but not with a C-terminal deletion mutant after DNA damage, suggesting that the C-terminal domain of THOC5, but not its phosphorylation in the PEST domain, is necessary for the regulation of the mRNA-binding potency of THOC5. The cytoplasmic THOC5-dependent mRNAs were recovered by treatment with ATM kinase-specific or p53-specific siRNA, as well as by treatment with ATM kinase inhibitor, KU55933, under DNA damage conditions, suggesting that the ATM–kinase–p53 pathway is involved in this response to the DNA damage. Furthermore, the treatment with KU55933 blocked DNA damage-induced THOC5mRNP complex dissociation, indicating that activation of ATM kinase suppresses the ability of THOC5 to bind to its target mRNAs.

Published

2011

8. RAC2, AEP, and ICAM1 expression are associated with CNS disease in a mouse model of pre-B childhood acute lymphoblastic leukemia

Author

Duncan L. Smith, Yvonne Connolly, Fernanda Castro, Shekhar Krishnan, Morgan Blaylock, Clare Dempsey, Anthony D. Whetton, Kate Mulryan, Jizhong Liu, Garry Ashton, Ashish Masurekar, John S. Bridgeman, Steven Bagley, Seema Alexander, Mark Holland, Peter L. Stern, Vaskar Saha, Crispin J. Miller, Danny A. Bitton, and Michael J. Walker

Subjects

Proteomics, Immunology, Central nervous system, Population, Mice, SCID, Biochemistry, CD19, Central Nervous System Neoplasms, Pathogenesis, Mice, Mice, Inbred NOD, Cell Line, Tumor, Precursor B-Cell Lymphoblastic Leukemia-Lymphoma, Precursor cell, Cell Adhesion, medicine, Animals, Humans, Neoplasm Invasiveness, Child, education, Childhood Acute Lymphoblastic Leukemia, CD70, education.field_of_study, biology, Gene Expression Regulation, Leukemic, business.industry, Cell Membrane, Cell Biology, Hematology, Precursor Cell Lymphoblastic Leukemia-Lymphoma, Intercellular Adhesion Molecule-1, rac GTP-Binding Proteins, Cysteine Endopeptidases, Disease Models, Animal, medicine.anatomical_structure, biology.protein, Bone marrow, business

Abstract

We developed a murine model of CNS disease to obtain a better understanding of the pathogenesis of CNS involvement in pre-B-cell acute lymphoblastic leukemia (ALL). Semiquantitative proteomic discovery–based approaches identified unique expression of asparaginyl endopeptidase (AEP), intercellular adhesion molecule 1 (ICAM1), and ras-related C3 botulinum toxin substrate 2 (RAC2), among others, in an invasive pre-B-cell line that produced CNS leukemia in NOD-SCID mice. Targeting RAC2 significantly inhibited in vitro invasion and delayed disease onset in mice. Induced expression of RAC2 in cell lines with low/absent expression of AEP and ICAM1 did not result in an invasive phenotype or murine CNS disease. Flow cytometric analysis identified an enriched population of blast cells expressing ICAM1/lymphocyte function associated antigen-1 (LFA-1)/CD70 in the CD10+/CD19+ fraction of bone marrow aspirates obtained from relapsed compared with normal controls and those with primary disease. CD10+/CD19+ fractions obtained from relapsed patients also express RAC2 and give rise to CNS disease in mice. Our data suggest that combinations of processes are involved in the pathogenesis of CNS disease in pre-B-cell ALL, support a model in which CNS disease occurs as a result of external invasion, and suggest that targeting the processes of adhesion and invasion unique to pre-B cells may prevent recurrences within the CNS.

Published

2011

9. Development of approaches for systematic analysis of protein networks in stem cells

Author

Anthony D. Whetton and Andrew J.K. Williamson

Subjects

Proteomics, Cancer Research, Genome, Proteomics methods, HMGA2 Protein, Proteins, Cell Differentiation, Computational biology, Biology, Mice, Proteins metabolism, Genetics, Animals, Molecular Medicine, Stem cell, Molecular Biology, Protein network, Embryonic Stem Cells, Metabolic Networks and Pathways

Published

2010

10. Developmental Fate Determination and Marker Discovery in Hematopoietic Stem Cell Biology Using Proteomic Fingerprinting

Author

Paul J. Simmons, Susie K. Nilsson, Mira C.P. Liu, Nathalie Brouard, Anthony D. Whetton, Ewa Jaworska, Richard D. Unwin, Brenda Williams, Elaine Spooncer, and David Blinco

Subjects

Proteomics, Proteome, Nerve Tissue Proteins, Biology, Biochemistry, Analytical Chemistry, Mice, medicine, Protein biosynthesis, Animals, Cell Lineage, RNA, Messenger, Molecular Biology, Ataxin-1, Regulation of gene expression, Messenger RNA, Gene Expression Profiling, Nuclear Proteins, Hematopoietic stem cell, Hematopoietic Stem Cells, Molecular biology, Cell biology, Mice, Inbred C57BL, Gene expression profiling, Proto-Oncogene Proteins c-kit, Haematopoiesis, Phenotype, medicine.anatomical_structure, Ataxins, Gene Expression Regulation, Biomarkers

Abstract

In hematopoiesis, co-expression of Sca-1 and c-Kit defines cells (LS(+)K) with long term reconstituting potential. In contrast, poorly characterized LS(-)K cells fail to reconstitute lethally irradiated recipients. Relative quantification mass spectrometry and transcriptional profiling were used to characterize LS(+)K and LS(-)K cells. This approach yielded data on >1200 proteins. Only 32% of protein changes correlated to mRNA modulation demonstrating post-translational protein regulation in early hematopoietic development. LS(+)K cells had lower expression of protein synthesis proteins but did express proteins associated with mature cell function. Major increases in erythroid development proteins were observed in LS(-)K cells; based on this assessment of erythroid potential we showed them to be principally erythroid progenitors, demonstrating effective use of discovery proteomics for definition of primitive cells.

Published

2008

11. Quantitative Proteomics Analysis Demonstrates Post-transcriptional Regulation of Embryonic Stem Cell Differentiation to Hematopoiesis

Author

David Blinco, Georges Lacaud, Richard D. Unwin, Valerie Kouskoff, Anthony D. Whetton, Crispin J. Miller, Andrew J.K. Williamson, Lee Lancashire, Claire Wilson, Stella Pearson, and Duncan L. Smith

Subjects

Fetal Proteins, Proteomics, Transcription, Genetic, Cellular differentiation, Green Fluorescent Proteins, Protein Array Analysis, Germ layer, Biology, Biochemistry, Analytical Chemistry, Transcriptome, Mice, SOX2, Tandem Mass Spectrometry, Animals, RNA, Messenger, Molecular Biology, Embryonic Stem Cells, Gene Expression Profiling, Gene Expression Regulation, Developmental, Reproducibility of Results, Cell Differentiation, Vascular Endothelial Growth Factor Receptor-2, Embryonic stem cell, Molecular biology, Hematopoiesis, Cell biology, Gene expression profiling, Epiblast, Hemangioblast, T-Box Domain Proteins, Metabolic Networks and Pathways

Abstract

Embryonic stem (ES) cells can differentiate in vitro to produce the endothelial and hematopoietic precursor, the hemangioblasts, which are derived from the mesoderm germ layer. Differentiation of Bry(GFP/+) ES cell to hemangioblasts can be followed by the expression of the Bry(GFP/+) and Flk1 genes. Proteomic and transcriptomic changes during this differentiation process were analyzed to identify mechanisms for phenotypic change during early differentiation. Three populations of differentiating Bry(GFP) ES cells were obtained by flow cytometric sorting, GFP-Flk1- (epiblast), GFP+Flk1- (mesoderm), and GFP+Flk1+ (hemangioblast). Microarray analyses and relative quantification two-dimensional LCLC-MS/MS on nuclear extracts were performed. We identified and quantified 2389 proteins, 1057 of which were associated to their microarray probe set. These included a variety of low abundance transcription factors, e.g. UTF1, Sox2, Oct4, and E2F4, demonstrating a high level of proteomic penetrance. When paired comparisons of changes in the mRNA and protein expression levels were performed low levels of correlation were found. A strong correlation between isobaric tag-derived relative quantification and Western blot analysis was found for a number of nuclear proteins. Pathway and ontology analysis identified proteins known to be involved in the regulation of stem cell differentiation, and proteins with no described function in early ES cell development were also shown to change markedly at the proteome level only. ES cell development is regulated at the mRNA and protein level.

Published

2008

12. MPL W515L expression induces TGFβ secretion and leads to an increase in chemokinesis via phosphorylation of THOC5

Author

Anthony D, Whetton, Norhaida Che, Azmi, Stella, Pearson, Ewa, Jaworska, Liqun, Zhang, Rognvald, Blance, Alexandra C, Kendall, Anna, Nicolaou, Samuel, Taylor, Andrew J K, Williamson, and Andrew, Pierce

Subjects

Myeloproliferative Disorders, Nuclear Proteins, MYC, THOC5, S1P, Mice, Cell Movement, Transforming Growth Factor beta, Case-Control Studies, Cell Line, Tumor, Animals, Humans, Phosphorylation, MPLW515L, Receptors, Thrombopoietin, chemokinesis, Cells, Cultured, Cell Proliferation, Signal Transduction, Priority Research Paper

Abstract

The thrombopoietin receptor (MPL) has been shown to be mutated (MPL W515L) in myelofibrosis and thrombocytosis yet new approaches to treat this disorder are still required. We have previously shown that transcriptome and proteomic effects do not correlate well in oncogene-mediated leukemogenesis. We therefore investigated the effects of MPL W515L using proteomics. The consequences of MPL W515L expression on over 3300 nuclear and 3500 cytoplasmic proteins were assessed using relative quantification mass spectrometry. We demonstrate that MPL W515L expression markedly modulates the CXCL12/CXCR4/CD45 pathway associated with stem and progenitor cell chemotactic movement. We also demonstrated that MPL W515L expressing cells displayed increased chemokinesis which required the MPL W515L-mediated dysregulation of MYC expression via phosphorylation of the RNA transport protein THOC5 on tyrosine 225. In addition MPL W515L expression induced TGFβ secretion which is linked to sphingosine 1-phosphate production and the increased chemokinesis. These studies identify several pathways which offer potential targets for therapeutic intervention in the treatment of MPL W515L-driven malignancy. We validate our approach by showing that CD34+ cells from MPL W515L positive patients display increased chemokinesis and that treatment with a combination of MYC and sphingosine kinase inhibitors leads to the preferential killing of MPL W515L expressing cells.

Published

2016

13. Glucocorticoid receptor regulates accurate chromosome segregation and is associated with malignancy

Author

David G. Spiller, Anthony D. Whetton, Michael R. H. White, David J. Morgan, David W. Ray, Frederike Kramer, Stuart N. Farrow, Laura Matthews, Karen E. Chapman, Michael R. Norman, Andrew Berry, Toryn Poolman, Jan Tuckermann, Kerstin Bauer, Andrew J.K. Williamson, Rachel V. Richardson, and Stephen S. Taylor

Subjects

Tumor suppressor gene, Mitosis, Biology, medicine.disease_cause, Chromosome segregation, Mice, Glucocorticoid receptor, Receptors, Glucocorticoid, Chromosome Segregation, Neoplasms, medicine, Tumor Cells, Cultured, Animals, Humans, Multidisciplinary, Tumor Suppressor Proteins, Cell cycle, Biological Sciences, Molecular biology, Mice, Mutant Strains, Cell biology, Spindle apparatus, Protein Structure, Tertiary, Gene Expression Regulation, Neoplastic, Cell Transformation, Neoplastic, Nuclear receptor, Carcinogenesis

Abstract

The glucocorticoid receptor (GR) is a member of the nuclear receptor superfamily, which controls programs regulating cell proliferation, differentiation, and apoptosis. We have identified an unexpected role for GR in mitosis. We discovered that specifically modified GR species accumulate at the mitotic spindle during mitosis in a distribution that overlaps with Aurora kinases. We found that Aurora A was required to mediate mitosis-driven GR phosphorylation, but not recruitment of GR to the spindle. GR was necessary for mitotic progression, with increased time to complete mitosis, frequency of mitotic aberrations, and death in mitosis observed following GR knockdown. Complementation studies revealed an essential role for the GR ligand-binding domain, but no clear requirement for ligand binding in regulating chromosome segregation. The GR N-terminal domain, and specifically phosphosites S203 and S211, were not required. Reduced GR expression results in a cell cycle phenotype, with isolated cells from mouse and human subjects showing changes in chromosome content over prolonged passage. Furthermore, GR haploinsufficient mice have an increased incidence of tumor formation, and, strikingly, these tumors are further depleted for GR, implying additional GR loss as a consequence of cell transformation. We identified reduced GR expression in a panel of human liver, lung, prostate, colon, and breast cancers. We therefore reveal an unexpected role for the GR in promoting accurate chromosome segregation during mitosis, which is causally linked to tumorigenesis, making GR an authentic tumor suppressor gene.

Published

2015

14. Differential effect of leukaemogenic tyrosine kinases on cell motility is governed by subcellular localisation

Author

Suzanne Thompson, Hajja G. Hamzah, Andrew Pierce, Anthony D. Whetton, Elaine Spooncer, P. J. Owen-Lynch, and Yuning Lu

Subjects

Oncogene Proteins, Fusion, Fusion Proteins, bcr-abl, Biology, Transfection, Philadelphia chromosome, Cell Line, Mice, Phosphatidylinositol 3-Kinases, Phosphatidylinositol Phosphates, Leukemia, Myelogenous, Chronic, BCR-ABL Positive, hemic and lymphatic diseases, medicine, Animals, Tyrosine, Cytoskeleton, ABL, Dose-Response Relationship, Drug, Chemotaxis, breakpoint cluster region, Hematology, Hematopoietic Stem Cells, medicine.disease, Actins, Chemokine CXCL12, Cell Transformation, Neoplastic, Second messenger system, Cancer research, Signal transduction, Chemokines, CXC, Tyrosine kinase, Signal Transduction

Abstract

The chemokine, stromal cell-derived factor-1 (SDF-1) is a crucial regulator of stem cell homing and tethering, and potentiation of this pathway in leukaemias may contribute to the pathogenesis of the disease. A key second messenger in SDF-1 signal/response coupling is phosphatidylinositol 3,4,5-triphosphate [PtdIns(3,4,5)P3]. SDF-1 elevated PtdIns(3,4,5)P3 levels markedly in the multipotent FDCP-mix stem cell line. Similarly, transfection with BCR/ABL or TEL/PDGFRbeta leukaemogenic tyrosine kinases chronically elevated PtdIns(3,4,5)P3 levels. However, whilst an SDF-1 chemotactic response was observed in TEL/PDGFRbeta-transfected cells, in BCR/ABL cells this was markedly decreased, which was not due to Ras-pathway activation. Thus, multipotent cells can respond to SDF-1, despite chronic increases in this second messenger indicating that a discrete pool of SDF-1-stimulated PtdIns(3,4,5)P3 production drives the chemotactic response. To discern the mechanism for the differential effects of these oncogenes we considered subcellular localisation. As TEL/PDGFRbeta has a cytosolic location whilst BCR/ABL associates with actin, we removed the actin-binding domain from BCR/ABL. We observed relocation of BCR/ABL to the cytosol and increased SDF-1 responses. We conclude that the localisation of BCR/ABL to the cytoskeleton is essential for effects on motility and moderating SDF-1 responses is not essential in tyrosine kinase-mediated leukaemic transformation.

Published

2006

15. Quantitative Proteomic Analysis Using Isobaric Protein Tags Enables Rapid Comparison of Changes in Transcript and Protein Levels in Transformed Cells

Author

Richard D. Unwin, Andrew Pierce, Rod B. Watson, Anthony D. Whetton, and David W. Sternberg

Subjects

Oncogene Proteins, Fusion, Proteome, Transcription, Genetic, Oncogene Proteins, Molecular Sequence Data, Peptide, Protein tag, Biology, Biochemistry, Mass Spectrometry, Cell Line, Analytical Chemistry, Transcriptome, Mice, Animals, Amino Acid Sequence, Molecular Biology, Peptide sequence, chemistry.chemical_classification, Microarray analysis techniques, Lysine, Multipotent Stem Cells, Hematopoietic Stem Cells, Molecular biology, Gene Expression Regulation, Neoplastic, Isobaric labeling, Cell Transformation, Neoplastic, chemistry, Cell culture, Isotope Labeling, Peptides, Chromatography, Liquid

Abstract

Isobaric tags for relative and absolute quantitation, an approach to concurrent, relative quantification of proteins present in four cell preparations, have recently been described. To validate this approach using complex mammalian cell samples that show subtle differences in protein levels, a model stem cell-like cell line (FDCP-mix) in the presence or absence of the leukemogenic oncogene TEL/PDGFRbeta has been studied. Cell lysates were proteolytically digested, and peptides within each sample were labeled with one of four isobaric, isotope-coded tags via their N-terminal and/or lysine side chains. The four labeled samples are mixed and peptides separated by two-dimensional liquid chromatography online to a mass spectrometer (LC-MS). Upon peptide fragmentation, each tag releases a distinct mass reporter ion; the ratio of the four reporters therefore gives relative abundances of the given peptide. Relative quantification of proteins is derived using summed data from a number of peptides. TEL/PDGFRbeta leukemic oncogene-mediated changes in protein levels were compared with those seen in microarray analysis of control and transfected FDCP-mix cells. Changes at the protein level in most cases reflected those seen at the transcriptome level. Nonetheless, novel differences in protein expression were found that indicate potential mechanisms for effects of this oncogene.

Published

2005

16. Comparative proteomics of primitive hematopoietic cell populations reveals differences in expression of proteins regulating motility

Author

Andrew Pierce, Anthony D. Whetton, Elaine Spooncer, C. Peter Downes, Simon J. Gaskell, Alexander Gray, Caroline A. Evans, Robert Tonge, Yuning Lu, David Blinco, Hajja G. Hamzah, and Joanne Shaw

Subjects

Proteomics, Difference gel electrophoresis, Immunology, Cell, Motility, Bone Marrow Cells, Stem cell factor, Biology, Biochemistry, Mice, Phosphatidylinositol 3-Kinases, chemistry.chemical_compound, Phosphatidylinositol Phosphates, medicine, Animals, Phosphatidylinositol, Cells, Cultured, Gelsolin, Actin, Cell Size, Chemotaxis, Microfilament Proteins, Proteins, Acetylation, Cell Biology, Hematology, Hematopoietic Stem Cells, Molecular biology, Chemokine CXCL12, Cell biology, Mice, Inbred C57BL, Proto-Oncogene Proteins c-kit, medicine.anatomical_structure, Gene Expression Regulation, chemistry, Stem cell, Chemokines, CXC

Abstract

Lineage-marker depleted (Lin(-)) murine bone marrow cells expressing stem cell antigen 1 (Sca-1) were sorted on the basis of stem cell factor receptor (c-kit) expression to obtain Lin(-)Sca(+)Kit(+) or Lin(-)Sca(+)Kit(-) cells. Lin(-)Sca(+)Kit(-) cells have a markedly greater chemotactic response to stromal derived factor-1 (SDF-1). Using a novel fluorescent stain, we show that both populations generate similar levels of a key messenger, phosphatidylinositol 3,4,5 trisphosphate (PIP(3)), in response to SDF-1. Differences in motile behavior may therefore lie downstream of phosphatidylinositol 3-kinase (PI3-kinase) activation at the level of cytoskeleton regulation. The 2 cell populations were compared using 2-dimensional difference gel electrophoresis (2D-DIGE), with a maleimide CyDye fluorescent protein labeling technique that has enhanced sensitivity for low abundance samples. Comparative proteomic analysis of Cy3- and Cy5-labeled protein samples allows relative quantification of protein spots present in both cell populations; of these, 73% were common. Key protein differences were adseverin and gelsolin, actin micro-filament splicing proteins, regulated by Rac, downstream of PI3-kinase activation. Adseverin was shown to be acetylated, a novel modification for this protein. Differences in major regulators of cell shape and motility between the 2 populations can explain the differential response to SDF-1.

Published

2004

17. Proteomics techniques and their application to hematology

Author

Simon J. Gaskell, Anthony D. Whetton, and Ileana M. Cristea

Subjects

Proteomics, Absolute quantification, Immunology, Protein Array Analysis, Proteins, Cell Biology, Hematology, Computational biology, Biology, Bioinformatics, Biochemistry, Genome, Mass spectrometric, Mass Spectrometry, DNA sequencing, Proteome, Posttranslational modification, Animals, Humans, Extracellular material, Electrophoresis, Gel, Two-Dimensional, Protein Processing, Post-Translational, Sequence Analysis

Abstract

The recent sequencing of a number of genomes has raised the level of opportunities for studies on proteins. This area of research has been described with the all-embracing term, proteomics. In proteomics, the use of mass spectrometric techniques enables genomic databases to be used to establish the identity of proteins with relatively little data, compared to the era before genome sequencing. The use of related analytical techniques also offers the opportunity to gain information on regulation, via posttranslational modification, and potential new diagnostic and prognostic indicators. Relative quantification of proteins and peptides in cellular and extracellular material remains a challenge for proteomics and mass spectrometry. This review presents an analysis of the present and future impact of these proteomic technologies with emphasis on relative quantification for hematologic research giving an appraisal of their potential benefits.

Published

2004

18. The potential for proteomic definition of stem cell populations

Author

Simon J. Gaskell, Caroline A. Evans, Anthony D. Whetton, and Richard D. Unwin

Subjects

Proteomics, Cancer Research, Gene Expression Profiling, Stem Cells, Proteins, Cell Biology, Hematology, Biology, Embryonic stem cell, Chemistry Techniques, Analytical, Cell biology, Gene expression profiling, Transplantation, Haematopoiesis, Proteome, Genetics, Animals, Humans, Stem cell, Molecular Biology, Adult stem cell

Abstract

Embryonic and adult stem cell populations have great potential value in medicine, and hematopoietic stem cells are already being used in transplantation. Definition of these populations to increase our understanding of the programs that control differentiation, self-renewal, and possibly plasticity would be of great interest. The relative quantitation of transcriptional activity in stem cells and other populations has defined a profile of gene expression activity in stem cells. Confirmation that these differences have an impact on protein levels within stem cells via their complete protein complement and protein interactions will enable further understanding of regulatory processes in these cells. The recent developments in proteomics and their potential application to the definition of the stem cell proteome are discussed, and examples are given. Advances in mass spectrometry, subcellular prefractionation protocols, and electrophoresis that make stem cell proteomics a tractable problem are discussed. Beyond the proteome per se, advances in post-translational modification profiling mean that comparative analysis of phosphorylation patterns between stem cells and other populations can be approached.

Published

2003

19. Quantitative phosphoproteome analysis of embryonic stem cell differentiation toward blood

Author

Manuela Piazzi, Chia-Fang Lee, Anthony D. Whetton, James A. McCubrey, Georges Lacaud, Lucio Cocco, Andrew J.K. Williamson, Valerie Kouskoff, Stella Pearson, Piazzi, Manuela, Williamson, Andrew, Lee, Chia-Fang, Pearson, Stella, Lacaud, George, Kouskoff, Valerie, Mccubrey, James A, Cocco, Lucio, and Whetton, Anthony D

Subjects

Fetal Proteins, Proteomics, Brachyury, Mesoderm, nucleu, Time Factors, Time Factor, Hemangioblasts, Cellular differentiation, Germ layer, Biology, Transfection, Mass Spectrometry, Cell Line, Mice, Embryonic Stem Cell, Genes, Reporter, Fetal Protein, medicine, Animals, Cell Lineage, Databases, Protein, Transcription factor, Embryonic Stem Cells, Animal, nucleus, T-Box Domain Protein, Gene Expression Regulation, Developmental, Cell Differentiation, Phosphoproteins, hemangioblast, Embryonic stem cell, Vascular Endothelial Growth Factor Receptor-2, phosphoproteomic, Cell biology, Haematopoiesis, medicine.anatomical_structure, Oncology, iTRAQ, Phosphoprotein, Immunology, embryonic structures, Hemangioblast, T-Box Domain Proteins, Chromatography, Liquid, Signal Transduction, Research Paper

Abstract

Murine embryonic stem (ES) cells can differentiate in vitro into three germ layers (endodermic, mesodermic, ectodermic). Studies on the differentiation of these cells to specific early differentiation stages has been aided by an ES cell line carrying the Green Fluorescent Protein (GFP) targeted to the Brachyury (Bry) locus which marks mesoderm commitment. Furthermore, expression of the Vascular Endothelial Growth Factor receptor 2 (Flk1) along with Bry defines hemangioblast commitment. Isobaric-tag for relative and absolute quantification (iTRAQ(TM)) and phosphopeptide enrichment coupled to liquid chromatography separation and mass spectrometry allow the study of phosphorylation changes occurring at different stages of ES cell development using Bry and Flk1 expression respectively. We identified and relatively quantified 37 phosphoentities which are modulated during mesoderm-induced ES cells differentiation, comparing epiblast-like, early mesoderm and hemangioblast-enriched cells. Among the proteins differentially phosphorylated toward mesoderm differentiation were: the epigenetic regulator Dnmt3b, the protein kinase GSK3b, the chromatin remodeling factor Smarcc1, the transcription factor Utf1; as well as protein specifically related to stem cell differentiation, as Eomes, Hmga2, Ints1 and Rif1. As most key factors regulating early hematopoietic development have also been implicated in various types of leukemia, understanding the post-translational modifications driving their regulation during normal development could result in a better comprehension of their roles during abnormal hematopoiesis in leukemia.

Published

2015

20. Flt3 ligand can promote survival and macrophage development without proliferation in myeloid progenitor cells

Author

Jaleel A. Miyan, Rachel Mottram, Anthony D. Whetton, S E Nicholls, and Sandra A. Winter

Subjects

Cancer Research, Time Factors, Myeloid, Cell Survival, Apoptosis, Stem cell factor, Receptor tyrosine kinase, Mice, Genetics, medicine, Animals, Macrophage, Progenitor cell, Clonogenic assay, Receptor, Molecular Biology, Stem Cell Factor, biology, Macrophage Colony-Stimulating Factor, Macrophages, Stem Cells, Membrane Proteins, Cell Differentiation, Cell Biology, Hematology, Molecular biology, Clone Cells, Cell biology, Granulocyte macrophage colony-stimulating factor, medicine.anatomical_structure, embryonic structures, biology.protein, Cell Division, Granulocytes, medicine.drug

Abstract

Flt3 ligand elicits a variety of effects on early hemopoietic progenitors by occupying its cognate receptor, Flt3, a member of the type III tyrosine kinase receptor family. The cytokines macrophage colony-stimulating factor (M-CSF) and stem cell factor (SCF) bind to related members of this tyrosine kinase receptors family, c-fms and c-kit, respectively. The relative effects of the cytokines M-CSF, SCF, and Flt3L on the proliferation and development of the late myeloid progenitors granulocyte-macrophage colony-forming cells (GM-CFC) were investigated. Distinct biologic responses were stimulated by ligand binding to these different tyrosine kinase receptors in enriched GM-CFC. M-CSF stimulated GM-CFC to proliferate and develop into macrophages. SCF, on the other hand, stimulated GM-CFC to develop into neutrophils. Flt3 ligand had a relatively small proliferative effect on enriched GM-CFC compared to SCF and M-CSF and had no ability to either stimulate colony formation or synergize with these two cytokines in promoting DNA synthesis, colony formation, or expansion in liquid culture. Flt3 ligand, however, was capable of maintaining the clonogenic potential of GM-CFC and acted as an anti-apoptotic agent as assessed using the Annexin-V apoptosis assay. GM-CFC cultured in Flt3 ligand eventually formed macrophages and neutrophils in liquid culture. Labeling with the membrane-associated cell tracker dye PKH26 indicated that the majority of the enriched GM-CFC responded to Flt3 ligand by undergoing limited proliferation and macrophage development, whereas other cells survived but did not proliferate and differentiate into macrophages. Thus, Flt3 ligand promoted survival and stimulated development without proliferation in primary-enriched myeloid progenitor cells.

Published

1999

21. An Activated Protein Kinase C α Gives a Differentiation Signal for Hematopoietic Progenitor Cells and Mimicks Macrophage Colony-stimulating Factor–stimulated Signaling Events

Author

Andrew Pierce, Gwen Wark, Janet M. Lord, T. Michael Dexter, Anthony D. Whetton, S E Nicholls, Elaine Spooncer, Clare M. Heyworth, and P. Jane Owen-Lynch

Subjects

Macrophage colony-stimulating factor, Protein Kinase C-alpha, Stem cell factor, Biology, Transfection, Article, Mice, Granulocyte macrophage colony-stimulating factor receptor, medicine, Animals, Protein Kinase C, Protein kinase C, Interleukin 3, Microscopy, Confocal, Granulocyte-Macrophage Colony-Stimulating Factor, Cell Biology, Flow Cytometry, Hematopoietic Stem Cells, Molecular biology, Culture Media, Cell biology, Enzyme Activation, Isoenzymes, Haematopoiesis, Granulocyte macrophage colony-stimulating factor, Interleukin-3, Signal transduction, Signal Transduction, medicine.drug

Abstract

Highly enriched, bipotent, hematopoietic granulocyte macrophage colony-forming cells (GM-CFC) require cytokines for their survival, proliferation, and development. GM-CFC will form neutrophils in the presence of the cytokines stem cell factor and granulocyte colony-stimulating factor, whereas macrophage colony-stimulating factor leads to macrophage formation. Previously, we have shown that the commitment to the macrophage lineage is associated with lipid hydrolysis and translocation of protein kinase C alpha (PKCalpha) to the nucleus. Here we have transfected freshly prepared GM-CFC with a constitutively activated form of PKCalpha, namely PKAC, in which the regulatory domain has been truncated. Greater than 95% of the transfected cells showed over a twofold increase in PKCalpha expression with the protein being located primarily within the nucleus. The expression of PKAC caused macrophage development even in the presence of stimuli that normally promote only neutrophilic development. Thus, M-CSF-stimulated translocation of PKCalpha to the nucleus is a signal associated with macrophage development in primary mammalian hematopoietic progenitor cells, and this signal can be mimicked by ectopic PKAC, which is also expressed in the nucleus.

Published

1998

22. A hierarchical statistical modeling approach to analyze proteomic isobaric tag for relative and absolute quantitation data

Author

Anthony D. Whetton, Cong Zhou, Andrew J.K. Williamson, Caroline Dive, Michael J. Walker, Andrew Pierce, and Carlo Berzuini

Subjects

Statistics and Probability, Proteomics, Quantitative proteomics, Robust statistics, Computational biology, Biology, Bioinformatics, Biochemistry, 03 medical and health sciences, Mice, 0302 clinical medicine, Animals, Molecular Biology, Cells, Cultured, 030304 developmental biology, 0303 health sciences, Models, Statistical, Staining and Labeling, Escherichia coli Proteins, Precursor Cells, B-Lymphoid, Proteins, Statistical model, Computer Science Applications, Computational Mathematics, Isobaric labeling, Matrix-assisted laser desorption/ionization, Computational Theory and Mathematics, 030220 oncology & carcinogenesis, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Isobaric process, Biological regulation, Peptides, Algorithms, Isobaric tag for relative and absolute quantitation

Abstract

Motivation: Isobaric tag for relative and absolute quantitation (iTRAQ) is a widely used method in quantitative proteomics. A robust data analysis strategy is required to determine protein quantification reliability, i.e. changes due to biological regulation rather than technical variation, so that proteins that are differentially expressed can be identified. Methods: Samples were created by mixing 5, 10, 15 and 20 μg Escherichia coli cell lysate with 100 μg of cell lysate from mouse, corresponding to expected relative fold changes of one for mouse proteins and from 0.25 to 4 for E.coli proteins. Relative quantification was carried out using eight channel isobaric tagging with iTRAQ reagent, and proteins were identified using a TripleTOF 5600 mass spectrometer. Technical variation inherent in this iTRAQ dataset was systematically investigated. Results: A hierarchical statistical model was developed to use quantitative information at peptide level and protein level simultaneously to estimate variation present in each individual peptide and protein. A novel data analysis strategy for iTRAQ, denoted in short as WHATraq, was subsequently proposed with its performance evaluated by the proportion of E.coli proteins that are successfully identified as differentially expressed. Compared with two benchmark data analysis strategies WHATraq was able to identify at least 62.8% more true positive proteins that are differentially expressed. Further validated using a biological iTRAQ dataset including multiple biological replicates from varied murine cell lines, WHATraq performed consistently and identified 375% more proteins as being differentially expressed among different cell lines than the other data analysis strategies. Contact: cdive@picr.man.ac.uk or tony.whetton@manchester.ac.uk Supplementary information: Supplementary data are available at Bioinformatics online.

Published

2013

23. A Specific PTPRC/CD45 Phosphorylation Event Governed by Stem Cell Chemokine CXCL12 Regulates Primitive Hematopoietic Cell Motility*

Author

Richard D. Unwin, Anthony D. Whetton, Tessa L. Holyoake, Cong Zhou, Elaine Spooncer, Andrew Pierce, Michael J. Walker, Sara Cadecco, Sheela A. Abraham, Ewa Jaworska, Mark Aspinall-O'Dea, Lee Lancashire, and Andrew J.K. Williamson

Subjects

Proteomics, Fusion Proteins, bcr-abl, Protein tyrosine phosphatase, Biology, PTPRC, Biochemistry, Analytical Chemistry, Cell Line, Mice, Cell Movement, Leukemia, Myelogenous, Chronic, BCR-ABL Positive, medicine, Animals, Humans, Progenitor cell, Enzyme Inhibitors, Phosphorylation, Molecular Biology, Mice, Knockout, Research, Phosphoproteomics, Hematopoietic stem cell, Hematopoietic Stem Cells, Chemokine CXCL12, Cell biology, Rac GTP-Binding Proteins, Mice, Inbred C57BL, medicine.anatomical_structure, Pyrimidines, Cancer research, biology.protein, Aminoquinolines, Leukocyte Common Antigens, Stem cell, Signal Transduction

Abstract

CXCL12 governs cellular motility, a process deregulated by hematopoietic stem cell oncogenes such as p210-BCR-ABL. A phosphoproteomics approach to the analysis of a hematopoietic progenitor cell line treated with CXCL12 and the Rac 1 and 2 inhibitor NSC23766 has been employed to objectively discover novel mechanisms for regulation of stem cells in normal and malignant hematopoiesis. The proteomic data sets identified new aspects of CXCL12-mediated signaling and novel features of stem cell regulation. We also identified a novel phosphorylation event in hematopoietic progenitor cells that correlated with motile response and governed by the chemotactic factor CXCL12. The novel phosphorylation site on PTPRC/CD45; a protein tyrosine phosphatase, was validated by raising an antibody to the site and also using a mass spectrometry absolute quantification strategy. Site directed mutagenesis and inhibitor studies demonstrated that this single phosphorylation site governs hematopoietic progenitor cell and lymphoid cell motility, lies downstream from Rac proteins and potentiates Src signaling. We have also demonstrated that PTPRC/CD45 is down-regulated in leukemogenic tyrosine kinase expressing cells. The use of discovery proteomics has enabled further understanding of the regulation of PTPRC/CD45 and its important role in cellular motility in progenitor cells.

Published

2013

24. A caspase-3 'death-switch' in colorectal cancer cells for induced and synchronous tumor apoptosis in vitro and in vivo facilitates the development of minimally invasive cell death biomarkers

Author

Gavin Brown, Kaye J. Williams, Anthony D. Whetton, Michael J. Walker, Christopher Cawthorne, Caroline Dive, Cassandra L Hodgkinson, Marion MacFarlane, Manikandan Kadirvel, Francesca Trapani, Cong Zhou, Kathryn Simpson, and Martin J Dawson

Subjects

Proteomics, death-switch, Cancer Research, Programmed cell death, Colorectal cancer, Immunology, Transplantation, Heterologous, Caspase 3, Antineoplastic Agents, Apoptosis, Mice, SCID, Cellular and Molecular Neuroscience, Mice, In vivo, medicine, Animals, Humans, HMGB1 Protein, Gelsolin, biology, Keratin-18, CD44, Midkine, Cancer, biomarkers, imaging, Cell Biology, medicine.disease, Molecular biology, Transplantation, Radiography, Doxorubicin, Positron-Emission Tomography, Cancer research, biology.protein, Cytokines, Original Article, Radiopharmaceuticals, Colorectal Neoplasms, HT29 Cells, capase-3

Abstract

Novel anticancer drugs targeting key apoptosis regulators have been developed and are undergoing clinical trials. Pharmacodynamic biomarkers to define the optimum dose of drug that provokes tumor apoptosis are in demand; acquisition of longitudinal tumor biopsies is a significant challenge and minimally invasive biomarkers are required. Considering this, we have developed and validated a preclinical 'death-switch' model for the discovery of secreted biomarkers of tumour apoptosis using in vitro proteomics and in vivo evaluation of the novel imaging probe [(18)F]ML-10 for non-invasive detection of apoptosis using positron emission tomography (PET). The 'death-switch' is a constitutively active mutant caspase-3 that is robustly induced by doxycycline to drive synchronous apoptosis in human colorectal cancer cells in vitro or grown as tumor xenografts. Death-switch induction caused caspase-dependent apoptosis between 3 and 24 hours in vitro and regression of 'death-switched' xenografts occurred within 24 h correlating with the percentage of apoptotic cells in tumor and levels of an established cell death biomarker (cleaved cytokeratin-18) in the blood. We sought to define secreted biomarkers of tumor apoptosis from cultured cells using Discovery Isobaric Tag proteomics, which may provide candidates to validate in blood. Early after caspase-3 activation, levels of normally secreted proteins were decreased (e.g. Gelsolin and Midkine) and proteins including CD44 and High Mobility Group protein B1 (HMGB1) that were released into cell culture media in vitro were also identified in the bloodstream of mice bearing death-switched tumors. We also exemplify the utility of the death-switch model for the validation of apoptotic imaging probes using [(18)F]ML-10, a PET tracer currently in clinical trials. Results showed increased tracer uptake of [(18)F]ML-10 in tumours undergoing apoptosis, compared with matched tumour controls imaged in the same animal. Overall, the death-switch model represents a robust and versatile tool for the discovery and validation of apoptosis biomarkers.

Published

2013

25. Application of the MIDAS approach for analysis of lysine acetylation sites

Author

Caroline A, Evans, John R, Griffiths, Richard D, Unwin, Anthony D, Whetton, and Bernard M, Corfe

Subjects

Tandem Mass Spectrometry, Lysine, Animals, Humans, Proteins, Acetylation, Protein Processing, Post-Translational, Mass Spectrometry, Peptide Fragments

Abstract

Multiple Reaction Monitoring Initiated Detection and Sequencing (MIDAS™) is a mass spectrometry-based technique for the detection and characterization of specific post-translational modifications (Unwin et al. 4:1134-1144, 2005), for example acetylated lysine residues (Griffiths et al. 18:1423-1428, 2007). The MIDAS™ technique has application for discovery and analysis of acetylation sites. It is a hypothesis-driven approach that requires a priori knowledge of the primary sequence of the target protein and a proteolytic digest of this protein. MIDAS essentially performs a targeted search for the presence of modified, for example acetylated, peptides. The detection is based on the combination of the predicted molecular weight (measured as mass-charge ratio) of the acetylated proteolytic peptide and a diagnostic fragment (product ion of m/z 126.1), which is generated by specific fragmentation of acetylated peptides during collision induced dissociation performed in tandem mass spectrometry (MS) analysis. Sequence information is subsequently obtained which enables acetylation site assignment. The technique of MIDAS was later trademarked by ABSciex for targeted protein analysis where an MRM scan is combined with full MS/MS product ion scan to enable sequence confirmation.

Published

2013

26. Drosophila F-BAR protein Syndapin contributes to coupling the plasma membrane and contractile ring in cytokinesis

Author

Harvey T. McMahon, Tetsuya Takeda, Matthew M. Savoian, Anthony D. Whetton, David M. Glover, Iain M. Robinson, and John R. Griffiths

Subjects

Phosphatidylinositol 4,5-Diphosphate, Immunology, cytokinesis, Biology, Microtubules, General Biochemistry, Genetics and Molecular Biology, Cell Line, Cell membrane, 03 medical and health sciences, Contractile Proteins, 0302 clinical medicine, Microtubule, medicine, Animals, Drosophila Proteins, Cleavage furrow, Central spindle, membrane, lcsh:QH301-705.5, 030304 developmental biology, 0303 health sciences, f-bar, phosphorylation, Research, General Neuroscience, Cell Membrane, Microfilament Proteins, Microfilament Protein, Actin cytoskeleton, actomyosin contractile ring, Cell biology, Actin Cytoskeleton, Drosophila melanogaster, medicine.anatomical_structure, lcsh:Biology (General), Membrane curvature, Carrier Proteins, Protein Processing, Post-Translational, 030217 neurology & neurosurgery, Cytokinesis, Research Article

Abstract

Cytokinesis is a highly ordered cellular process driven by interactions between central spindle microtubules and the actomyosin contractile ring linked to the dynamic remodelling of the plasma membrane. The mechanisms responsible for reorganizing the plasma membrane at the cell equator and its coupling to the contractile ring in cytokinesis are poorly understood. We report here that Syndapin, a protein containing an F-BAR domain required for membrane curvature, contributes to the remodelling of the plasma membrane around the contractile ring for cytokinesis. Syndapin colocalizes with phosphatidylinositol 4,5-bisphosphate (PI(4,5)P2) at the cleavage furrow, where it directly interacts with a contractile ring component, Anillin. Accordingly, Anillin is mislocalized during cytokinesis in Syndapin mutants. Elevated or diminished expression of Syndapin leads to cytokinesis defects with abnormal cortical dynamics. The minimal segment of Syndapin, which is able to localize to the cleavage furrow and induce cytokinesis defects, is the F-BAR domain and its immediate C-terminal sequences. Phosphorylation of this region prevents this functional interaction, resulting in reduced ability of Syndapin to bind to and deform membranes. Thus, the dephosphorylated form of Syndapin mediates both remodelling of the plasma membrane and its proper coupling to the cytokinetic machinery.

Published

2013

27. v-Abl-mediated Apoptotic Suppression Is Associated with SHC Phosphorylation without Concomitant Mitogen-activated Protein Kinase Activation

Author

Anthony D. Whetton, P. J. Owen-Lynch, and A. K.Y. Wong

Subjects

Cell Survival, Apoptosis, Genes, abl, Mitogen-activated protein kinase kinase, Transfection, Biochemistry, Cell Line, MAP2K7, Glycogen Synthase Kinase 3, Animals, Humans, ASK1, c-Raf, Phosphorylation, Oncogene Proteins v-abl, Phosphotyrosine, Molecular Biology, MAPK14, Mitogen-Activated Protein Kinase Kinases, biology, MAP kinase kinase kinase, Chemistry, GTPase-Activating Proteins, Cyclin-dependent kinase 2, Temperature, Proteins, Cell Biology, Clone Cells, Cell biology, Enzyme Activation, Kinetics, Mutagenesis, Type C Phospholipases, Calcium-Calmodulin-Dependent Protein Kinases, biology.protein, Tyrosine, Interleukin-3, Cyclin-dependent kinase 9, Protein Kinases, Cell Division

Abstract

A temperature-sensitive mutant of the v-Abl protein has previously been shown to exhibit tyrosine protein kinase activity in Interleukin 3 (IL-3)-dependent IC.DP cells grown at the permissive temperature (32 degrees C) but not at the restrictive temperature (39 degrees C). These IC.DP cells are dependent on IL-3 for suppression of apoptosis at 39 degrees C, but at 32 degrees C cells will survive without added growth factor. Both IL-3 and v-Abl stimulated the tyrosine phosphorylation of SHC and GTPase-activating protein. However, while IL-3 stimulated similar levels of tyrosine phosphorylation in p46shc and p52shc, v-Abl preferentially phosphorylated p52shc, an event that occurred within 1 h of temperature switch. v-Abl also differentially associated with p46shc in a temperature-independent manner. In contrast, only IL-3 stimulated detectable increases in both myelin basic protein kinase and mitogen-activated protein (MAP) kinase kinase in in vitro assays, although in more specific MAP kinase activity assays a very slight increase in the activity of this enzyme was observed after 6 h at the permissive temperature. Time course studies suggest that phosphorylation and association of SHC with v-Abl is insufficient to lead to significant activation of MAP kinase and that activation of the MAP kinase kinase/MAP kinase pathway is not required for apoptotic suppression.

Published

1995

28. Identification of Nuclear Protein Targets for Six Leukemogenic Tyrosine Kinases Governed by Post-Translational Regulation

Author

Andrew J.K. Williamson, Richard D. Unwin, Michael J. Walker, Elaine Spooncer, Ewa Jaworska, Anthony D. Whetton, Samuel J. Taylor, David W. Ray, Toryn Poolman, Mark Aspinall O’Dea, John R. Griffiths, and Andrew Pierce

Subjects

Proteomics, Proteome, Hematopoietic Progenitor Cells, Science, Biology, Biochemistry, Mass Spectrometry, Cell Line, Hematologic Cancers and Related Disorders, Mice, Glucocorticoid receptor, Receptors, Glucocorticoid, Molecular Cell Biology, Tyrosine Kinase Signaling Cascade, Leukemias, Animals, Post-translational regulation, Nuclear protein, Transcription factor, Multidisciplinary, Myeloproliferative Disorders, Kinase, Systems Biology, Proteins, Nuclear Proteins, Hematology, Protein-Tyrosine Kinases, Molecular biology, Signaling Cascades, Cell biology, Phosphorylation, Medicine, Signal transduction, Cellular Types, Tyrosine kinase, Protein Processing, Post-Translational, Research Article, Signal Transduction

Abstract

Mutated tyrosine kinases are associated with a number of different haematological malignancies including myeloproliferative disorders, lymphoma and acute myeloid leukaemia. The potential commonalities in the action of six of these leukemogenic proteins on nuclear proteins were investigated using systematic proteomic analysis. The effects on over 3600 nuclear proteins and 1500 phosphopeptide sites were relatively quantified in seven isogenic cell lines. The effects of the kinases were diverse although some commonalities were found. Comparison of the nuclear proteomic data with transcriptome data and cytoplasmic proteomic data indicated that the major changes are due to post-translational mechanisms rather than changes in mRNA or protein distribution. Analysis of the promoter regions of genes whose protein levels changed in response to the kinases showed the most common binding site found was that for NFκB whilst other sites such as those for the glucocorticoid receptor were also found. Glucocorticoid receptor levels and phosphorylation were decreased by all 6 PTKs. Whilst Glucocorticoid receptor action can potentiate NFκB action those proteins where genes have NFκB binding sites were in often regulated post-translationally. However all 6 PTKs showed evidence of NFkB pathway modulation via activation via altered IkB and NFKB levels. Validation of a common change was also undertaken with PMS2, a DNA mismatch repair protein. PMS2 nuclear levels were decreased in response to the expression of all 6 kinases, with no concomitant change in mRNA level or cytosolic protein level. Response to thioguanine, that requires the mismatch repair pathway, was modulated by all 6 oncogenic kinases. In summary common targets for 6 oncogenic PTKs have been found that are regulated by post-translational mechanisms. They represent potential new avenues for therapies but also demonstrate the post-translational regulation is a key target of leukaemogenic kinases.

Published

2012

29. BCR/ABL modulates protein phosphorylation associated with the etoposide-induced DNA damage response

Author

Anthony D. Whetton, Andrew Pierce, Andrew J.K. Williamson, David N. Potier, Samuel J. Taylor, François Griaud, and Elaine Spooncer

Subjects

Genome instability, Phosphosite, DNA repair, DNA damage, Biophysics, Fusion Proteins, bcr-abl, Apoptosis, Biology, Biochemistry, Mice, hemic and lymphatic diseases, Cell Line, Tumor, Leukemia, Myelogenous, Chronic, BCR-ABL Positive, Animals, Phosphorylation, Transcription factor, BCR/ABL, Etoposide, ABL, Gene Expression Regulation, Leukemic, Phosphoproteomics, breakpoint cluster region, Hemogen, Nuclear Proteins, Protein-Tyrosine Kinases, Antineoplastic Agents, Phytogenic, MDC1, Cancer research, NFκB, DNA Damage

Abstract

BCR/ABL expression is the key characteristic of chronic myeloid leukaemia (CML). The progression of CML is associated with genomic instability. Systematic analysis of DNA damage signalling in the presence of BCR/ABL thus offers opportunities to identify mechanisms of leukaemic progression. We therefore undertook a quantitative phosphoproteomics study to test whether BCR/ABL expression could globally affect the response to genotoxic stress signalling. Etoposide-induced DNA damage was chosen and the concentration and time of exposure determined such that apoptosis was not associated with the study. More than 1100 phosphoentities were identified. BCR/ABL was shown to significantly alter the response to etoposide in many cases. These include sites on MDC1, a key component of DNA repair, and Hemogen. Hemogen is a transcriptional target of HOXB4 and GATA1, two transcription factors involved in haemopoietic development, and is overexpressed in acute myeloid leukaemia. To validate Hemogen phosphorylation, absolute quantification using an isotopomeric standard and selected reaction monitoring was performed. This revealed a strong correlation with isobaric tagging data and offering quantification at about 10 fmol per million cells. Furthermore we found that multiple protein phosphorylation changes mediated by BCR/ABL were connected to the increased activation of NFκB, a key survival transcription factor, after etoposide exposure. © 2012 Elsevier B.V.

Published

2012

30. The requirement for proteomics to unravel stem cell regulatory mechanisms

Author

Andrew J.K. Williamson and Anthony D. Whetton

Subjects

Pluripotent Stem Cells, Proteomics, Physiology, Systems biology, Clinical Biochemistry, Cell Differentiation, Cell Biology, Biology, Cell biology, Protein–protein interaction, Cancer stem cell, Tandem Mass Spectrometry, Phosphorylation, Animals, Humans, Stem cell, Reprogramming, Transcription factor, Protein Processing, Post-Translational, Cell Division, Chromatography, Liquid

Abstract

Stem cells are defined by their ability to self-renew and to differentiate, the processes whereby these events are achieved is the subject of much investigation. These studies include cancer stem cell populations, where eradication of this specific population is the ultimate goal of treatment. Whilst cellular signalling events and transcription factor complex-mediated changes in gene expression have been analysed in some detail within stem cells, full systematic understanding of the events promoting self-renewal or the commitment process leading to formation of a specific cell type require a systems biology approach. This in turn demands a need for proteomic analysis of post-translational regulation of protein levels, protein interactions, protein post-translational modification (e.g. ubiquitination, methylation, acetylation, phosphorylation) to identify networks for stem cell regulation. Furthermore, the phenomenon of induced pluripotency via cellular reprogramming also can be understood optimally using combined molecular biology and proteomics approaches; here we describe current research employing proteomics and mass spectrometry to dissect stem cell regulatory mechanisms.

Published

2011

31. The application of quantification techniques in proteomics for biomedical research

Author

Eva, Rodríguez-Suárez and Anthony D, Whetton

Subjects

Proteomics, Biomedical Research, Proteome, Isotope Labeling, Animals, Humans, Biomarkers, Mass Spectrometry

Abstract

The systematic analysis of biological processes requires an understanding of the quantitative expression patterns of proteins, their interacting partners and their subcellular localization. This information was formerly difficult to accrue as the relative quantification of proteins relied on antibody-based methods and other approaches with low throughput. The advent of soft ionization techniques in mass spectrometry plus advances in separation technologies has aligned protein systems biology with messenger RNA, DNA, and microarray technologies to provide data on systems as opposed to singular protein entities. Another aspect of quantitative proteomics that increases its importance for the coming few years is the significant technical developments underway both for high pressure liquid chromatography and mass spectrum devices. Hence, robustness, reproducibility and mass accuracy are still improving with every new generation of instruments. Nonetheless, the methods employed require validation and comparison to design fit for purpose experiments in advanced protein analyses. This review considers the newly developed systematic protein investigation methods and their value from the standpoint that relative or absolute protein quantification is required de rigueur in biomedical research.

Published

2011

32. Influence of growth factors and substrates on differentiation of haemopoietic stem cells

Author

T. Michael Dexter and Anthony D. Whetton

Subjects

Stromal cell, Apoptosis, Bone Marrow Cells, Receptors, Cell Surface, Biology, Hematopoietic Cell Growth Factors, Mice, Growth factor receptor, medicine, Animals, Progenitor cell, Transcription factor, Cells, Cultured, Connective Tissue Cells, Gene Transfer Techniques, Cell Differentiation, Cell Biology, Hematopoietic Stem Cells, Growth Inhibitors, Culture Media, Hematopoiesis, Cell biology, Haematopoiesis, medicine.anatomical_structure, Immunology, Bone marrow, Stem cell, Transforming growth factor

Abstract

During the last few years there has been major progress in our understanding of the mechanisms underlying the regulation of haemopoietic stem cell proliferation and development. In the past 12 months, advances have been made in identifying how growth factor receptor expression is regulated in primitive haemopoietic cells, in determining the transcription factors that are associated with development, and in recognizing some of the specific molecular interactions that occur between the bone marrow stromal cells and the haemopoietic progenitor cells. These and previous studies clearly demonstrate that the environment can influence the survival, the proliferation and the differentiation of haemopoietic cells at every stage of development.

Published

1993

33. Haemopoietic stem cell development to neutrophils is associated with subcellular redistribution and differential expression of protein kinase C subspecies

Author

Anthony D. Whetton, M.S. Shearman, B. Haefner, C.M. Heyworth, P.J. Owen, and T M Dexter

Subjects

DNA Replication, medicine.medical_specialty, Neutrophils, Cellular differentiation, Biology, Hematopoietic Cell Growth Factors, Cytosol, Internal medicine, medicine, Animals, Cells, Cultured, Protein Kinase C, Protein kinase C, Respiratory Burst, Interleukin 3, Cell growth, Membrane Proteins, Cell Differentiation, Cell Biology, Hematopoietic Stem Cells, Molecular biology, Respiratory burst, Enzyme Activation, Isoenzymes, N-Formylmethionine Leucyl-Phenylalanine, Haematopoiesis, Granulocyte macrophage colony-stimulating factor, Endocrinology, Tetradecanoylphorbol Acetate, Interleukin-3, Stem cell, medicine.drug

Abstract

Multipotential FDCP-Mix A4 (A4) cells can be induced either to self-renew or to differentiate and develop into mature neutrophils in liquid culture, depending on the haemopoietic growth factors with which they are cultured. When cultured in low concentrations of interleukin 3 (IL-3, 1 unit/ml)) plus Granulocyte Macrophage Colony Stimulating Factor (GM-CSF) and Granulocyte-CSF (G-CSF), A4 cells proliferate with accompanying development to form cells which resemble mature, postmitotic neutrophils. The presence of high concentrations of IL-3 (100 units/ml) blocks the development of A4 cells even in the presence of GM-CSF plus G-CSF. A4 cell development to neutrophils is accompanied by major changes in the expression of protein kinase C (PKC) subspecies in these cells. The predominant subspecies present in multipotent A4 cells, as judged by direct chromatographic analysis, was the type III enzyme (alpha) subspecies, whereas in mature A4 cell neutrophils, the type II (beta I + beta II) enzymes were predominant. Phorbol esters added to immature A4 cells resulted in a proliferative response, but when added to postmitotic A4 cells resembling neutrophils they elicited a large increase in reactive oxygen intermediate production. This suggests that the type III (alpha) subspecies may mediate proliferative responses in stem cells, whilst the type II (beta I + beta II) enzymes are more important for the mature cell functions of postmitotic neutrophils. In cultures containing IL-3 (100 units/ml) both the type III, and also the type II subspecies were predominantly membrane-associated for prolonged periods (> 24 hours).(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1993

34. Simultaneous analysis of relative protein expression levels across multiple samples using iTRAQ isobaric tags with 2D nano LC-MS/MS

Author

Richard D. Unwin, Anthony D. Whetton, and John R. Griffiths

Subjects

chemistry.chemical_classification, Analyte, Chromatography, Chemistry, Gene Expression Profiling, Proteins, Peptide, Tandem mass spectrometry, Bioinformatics, Tandem mass tag, Mass spectrometry, General Biochemistry, Genetics and Molecular Biology, Isobaric labeling, Tandem Mass Spectrometry, Isobaric process, Animals, Humans, Isobaric tag for relative and absolute quantitation, Chromatography, Liquid

Abstract

In this paper, we describe the use of iTRAQ (isobaric Tags for Relative and Absolute Quantitation) tags for comparison of protein expression levels between multiple samples. These tags label all peptides in a protein digest before labeled samples are pooled, fractionated and analyzed using mass spectrometry (MS). As the tags are isobaric, the intensity of each peak is the sum of the intensity of this peptide from all samples, providing a moderate enhancement in sensitivity. On peptide fragmentation, amino-acid sequence ions also show this summed intensity, providing a sensitivity enhancement. However, the distinct distribution of isotopes in the tags is such that, on further fragmentation, a tag-specific reporter ion is released. The relative intensities of these ions represent the relative amount of peptide in the analytes. Integration of the relative quantification data for the peptides allows relative quantification of the protein. This protocol discusses the rationale behind design, optimization and performance of experiments, comparing protein samples using iTRAQ chemistries combined with strong cation exchange chromatographic fractionation and MS.

Published

2010

35. Assessment of downstream effectors of BCR/ABL protein tyrosine kinase using combined proteomic approaches

Author

Eva Rodríguez-Suárez, Chia Fang Lee, Richard D. Unwin, Anthony D. Whetton, Ewa Jaworska, Andrew Pierce, Caroline A. Evans, Simon J. Gaskell, and Stephen D. Griffiths

Subjects

Proteomics, animal structures, Molecular Sequence Data, Fusion Proteins, bcr-abl, Biochemistry, Cell Line, Mice, hemic and lymphatic diseases, Animals, Amino Acid Sequence, HSP90 Heat-Shock Proteins, Phosphorylation, Molecular Biology, ABL, biology, breakpoint cluster region, Phosphoproteins, Fusion protein, Hsp90, Ubiquitin ligase, biology.protein, Cancer research, Signal transduction, Tyrosine kinase, Protein Binding, Signal Transduction

Abstract

Leukaemic transformation is frequently associated with the aberrant activity of a protein tyrosine kinase (PTK). As such it is of clinical relevance to be able to map the effects of these leukaemogenic PTKs on haemopoietic cells at the level of phosphorylation modulation. In this paradigm study we have employed a range of proteomic approaches to analyse the effects of one such PTK, BCR/ABL. We have employed phosphoproteome enrichment techniques allied to peptide and protein quantification to identify proteins and pathways involved in cellular transformation. Amongst the proteins shown to be regulated at the post-translational level were cofilin, an actin-severing protein thus linked to altered motility and Cbl an E3 ubiquitin ligase integrally linked to the control of tyrosine kinase signalling (regulated by 5 and 6 PTKs respectively). The major class of proteins identified however were molecular chaperones. We also showed that HSP90 phosphorylation is altered by BCR/ABL action and that HSP90 plays a crucial role in oncogene stability. Further investigation with another six leukaemogenic PTKs demonstrates that this HSP90 role in oncogene stability appears to be a common phenomenon in a range of leukaemias. This opens up the potential opportunity to treat different leukaemias with HSP90 inhibitors.

Published

2010

36. Systems-level dynamic analyses of fate change in murine embryonic stem cells

Author

Avi Ma'ayan, Ben D. MacArthur, Olga G. Troyanskaya, Laurie A. Boyer, Alexander Lachmann, Anthony D. Whetton, Ihor R. Lemischka, Edoardo M. Airoldi, Rong Lu, Florian Markowetz, Richard D. Unwin, Jeffrey T. Leek, Roye Rozov, Massachusetts Institute of Technology. Department of Biology, Boyer, Laurie Ann, and Boyer, Laurie

Subjects

Genetics, Regulation of gene expression, Homeobox protein NANOG, Multidisciplinary, Time Factors, Proteome, Cellular differentiation, Gene Expression Profiling, Gene regulatory network, Gene Expression Regulation, Developmental, Cell Differentiation, Epigenome, Cell fate determination, Biology, Article, Chromatin, Cell biology, Epigenesis, Genetic, Mice, Animals, Transcription factor, Embryonic Stem Cells

Abstract

Molecular regulation of embryonic stem cell (ESC) fate involves a coordinated interaction between epigenetic[superscript 1, 2, 3, 4], transcriptional[superscript 5, 6, 7, 8, 9, 10] and translational[superscript 11, 12] mechanisms. It is unclear how these different molecular regulatory mechanisms interact to regulate changes in stem cell fate. Here we present a dynamic systems-level study of cell fate change in murine ESCs following a well-defined perturbation. Global changes in histone acetylation, chromatin-bound RNA polymerase II, messenger RNA (mRNA), and nuclear protein levels were measured over 5 days after downregulation of Nanog, a key pluripotency regulator[superscript 13, 14, 15]. Our data demonstrate how a single genetic perturbation leads to progressive widespread changes in several molecular regulatory layers, and provide a dynamic view of information flow in the epigenome, transcriptome and proteome. We observe that a large proportion of changes in nuclear protein levels are not accompanied by concordant changes in the expression of corresponding mRNAs, indicating important roles for translational and post-translational regulation of ESC fate. Gene-ontology analysis across different molecular layers indicates that although chromatin reconfiguration is important for altering cell fate, it is preceded by transcription-factor-mediated regulatory events. The temporal order of gene expression alterations shows the order of the regulatory network reconfiguration and offers further insight into the gene regulatory network. Our studies extend the conventional systems biology approach to include many molecular species, regulatory layers and temporal series, and underscore the complexity of the multilayer regulatory mechanisms responsible for changes in protein expression that determine stem cell fate.

Published

2009

37. THOC5/FMIP, an mRNA export TREX complex protein, is essential for hematopoietic primitive cell survival in vivo

Author

Rüdiger Pankow, Sabine Klebba-Färber, Elaine Spooncer, Anthony D. Whetton, Susanne C Niemann-Seyde, Annalisa Mancini, Alexandra Koch, Achim D. Gruber, Omar El Bounkari, Ewa Jaworska, and Teruko Tamura

Subjects

Physiology, THO complex, Cell Survival, RNA-binding protein, Apoptosis, Bone Marrow Cells, Plant Science, Biology, General Biochemistry, Genetics and Molecular Biology, Mice, Structural Biology, Transcription (biology), Interferon, Research article, medicine, Leukocytes, Animals, RNA, Messenger, Nuclear export signal, lcsh:QH301-705.5, Ecology, Evolution, Behavior and Systematics, Bone Marrow Transplantation, Mice, Knockout, Messenger RNA, Blood Cells, Agricultural and Biological Sciences(all), Biochemistry, Genetics and Molecular Biology(all), Intracellular Signaling Peptides and Proteins, RNA-Binding Proteins, Anemia, Cell Biology, Leukopenia, Hematopoietic Stem Cells, Molecular biology, Hematopoiesis, DNA-Binding Proteins, Mice, Inbred C57BL, Haematopoiesis, medicine.anatomical_structure, lcsh:Biology (General), Hepatocytes, Bone marrow, General Agricultural and Biological Sciences, Developmental Biology, Biotechnology, medicine.drug

Abstract

Background The transcription/export complex is evolutionarily conserved from yeast to man and is required for coupled transcription elongation and nuclear export of mRNAs. FMIP(Fms interacting protein) is a member of the THO (suppressors of the transcriptional defects of hpr1delta by overexpression) complex which is a subcomplex of the transcription/export complex. THO complex (THOC) components are not essential for bulk poly (A)+ RNA export in higher eukaryotes, but for the nuclear export of subset of mRNAs, however, their exact role is still unclear. Results To study the role of THOC5/Fms interacting protein in vivo, we generated THOC5/Fms interacting protein knockout mice. Since these mice are embryonic lethal, we then generated interferon inducible conditional THOC5/Fms interacting protein knockout mice. After three poly injections all of the mice died within 14 days. No pathological alterations, however, were observed in liver, kidney or heart. Thus we considered the hematopoietic system and found that seven days after poly injection, the number of blood cells in peripheral blood decreased drastically. Investigation of bone marrow cells showed that these became apoptotic within seven days after poly injection. Committed myeloid progenitor cells and cells with long term reconstituting potential were lost from bone marrow within four days after poly injection. Furthermore, infusion of normal bone marrow cells rescued mice from death induced by loss of THOC5/Fms interacting protein. Conclusion THOC5/Fms interacting protein is an essential element in the maintenance of hematopoiesis. Furthermore, mechanistically depletion of THOC5/Fms interacting protein causes the down-regulation of its direct interacting partner, THOC1 which may contribute to altered THO complex function and cell death.

Published

2009

38. Control of proliferation by myeloid growth factors

Author

Anthony D. Whetton and Susan J. Vallance

Subjects

Myeloid, Macrophage Colony-Stimulating Factor, Granulocyte-Macrophage Colony-Stimulating Factor, Bone Marrow Cells, Cell Differentiation, Biology, Molecular cloning, Hematopoietic Stem Cells, Biochemistry, Cell biology, Haemopoietic cell, Transformation (genetics), medicine.anatomical_structure, Bone Marrow, Granulocyte Colony-Stimulating Factor, medicine, Animals, Humans, Interleukin-3, Receptor, Cell Division

Abstract

At present the molecular events which regulate the proliferation and developmental fates of haemopoietic cells are poorly understood. Until recently, the only receptor for the myeloid growth factors which had been characterized extensively was that for M-CSF (c-fms). The molecular cloning of receptors for IL-3, GM-CSF and G-CSF should now permit rapid progress in the analysis of receptor-mediated haemopoietic cell differentiation and development, and should also reveal how the process of leukaemic transformation effects these events.

Published

1991

39. Regulation of neutrophil and macrophage production by growth factors

Author

Anthony D. Whetton and S. J. Vallance

Subjects

Neutrophils, Cell growth, Macrophages, Neutrophile, Cellular differentiation, medicine.medical_treatment, Cell Differentiation, Biology, Hematopoietic Cell Growth Factors, Colony-stimulating factor, Biochemistry, Haematopoiesis, Cytokine, Granulocyte macrophage colony-stimulating factor receptor, Immunology, medicine, Animals, Humans, Macrophage

Published

1991

40. Nuclear localization of the pre-mRNA associating protein THOC7 depends upon its direct interaction with Fms tyrosine kinase interacting protein (FMIP)

Author

Maike Claußen, Anthony D. Whetton, Anuja Guria, Tomas Pieler, Teruko Tamura, John R. Griffiths, Sabine Klebba-Faerber, Omar El Bounkari, and Alexandra Koch

Subjects

THO complex, Xenopus, Amino Acid Motifs, Nuclear Localization Signals, Biophysics, RNA-binding protein, Biology, Xenopus Proteins, Biochemistry, 03 medical and health sciences, Mice, 0302 clinical medicine, Structural Biology, Protein Interaction Mapping, Genetics, medicine, RNA Precursors, NLS, Animals, Humans, Nuclear protein, Molecular Biology, 030304 developmental biology, Nucleocytoplasmic shuttling protein, Cell Nucleus, 0303 health sciences, THOC7/fSAP24, mRNA processing complex, Nuclear Proteins, RNA-Binding Proteins, Cell Biology, Cell biology, Cell nucleus, medicine.anatomical_structure, Cytoplasm, 030220 oncology & carcinogenesis, Mutation, FMIP/THOC5/fSAP79, Precursor mRNA, Nuclear localization sequence

Abstract

THOC7 and Fms-interacting protein (FMIP) are members of the THO complex that associate with the mRNA export apparatus. FMIP is a nucleocytoplasmic shuttling protein with a nuclear localization signal (NLS), whereas THOC7 does not contain a typical NLS motif. We show here that THOC7 (50–137, amino acid numbers) binds to the N-terminal portion (1–199) of FMIP directly. FMIP is detected mainly in the nucleus. In the absence of exogenous FMIP, THOC7 resides mainly in the cytoplasm, while in the presence of FMIP, THOC7 is transported into the nucleus with FMIP. Furthermore, THOC7 lacking the FMIP binding site does not co-localize with FMIP, indicating that THOC7/FMIP interaction is required for nuclear localization of THOC7.Structured summaryMINT-6799962, MINT-6799973, MINT-6800005: THOC7 (uniprotkb:Q6I9Y2) physically interacts (MI:0218) with THOC5 (uniprotkb:Q13769) by pull down (MI:0096)MINT-6800108: FMIP (uniprotkb:Q13769) and THOC7 (uniprotkb: Q6I9Y2) co-localize (MI:0403) by fluorescence microscopy (MI:0416)MINT-6800052: FMIP (uniprotkb:Q13769) physically interacts (MI:0218) with THOC1 (uniprotkb: Q96FV9) by anti tag coimmunoprecipitation (MI:0007)MINT-6800022: THOC7 (uniprotkb:Q6I9Y2) physically interacts (MI:0218) with FMIP (uniprotkb:Q6DFL5) by pull down (MI:0096)MINT-6799989: THOC7 (uniprotkb:Q6I9Y2) binds (MI:0407) to FMIP (uniprotkb:Q13769) by pull down (MI:0096)MINT-6800071, MINT-6800089: FMIP (uniprotkb:Q13769) physically interacts (MI:0218) with THOC7 (uniprotkb:Q6I9Y2) and THOC1 (uniprotkb:Q96FV9) by anti tag coimmunoprecipitation (MI:0007)

Published

2008

41. THOC5 couples M-CSF receptor signaling to transcription factor expression

Author

Marco Rijnen, Louise Carney, Liqun Zhang, Hajja G. Hamzah, Andrew Pierce, M. Belen Gonzalez Sanchez, Anthony D. Whetton, and Teruko Tamura

Subjects

Cell signaling, GAB2, Receptor, Macrophage Colony-Stimulating Factor, Biology, Transfection, Monocytes, Cell Line, Mice, Phosphatidylinositol 3-Kinases, Animals, Humans, Phosphorylation, Transcription factor, Ccaat-enhancer-binding proteins, CCAAT-Enhancer-Binding Protein-beta, Macrophage Colony-Stimulating Factor, Nuclear Proteins, Cell Biology, Molecular biology, Cell biology, Monocyte differentiation, Second messenger system, biology.protein, Ectopic expression, Signal transduction, Signal Transduction, Transcription Factors

Abstract

THOC5 is a nuclear/cytoplasmic protein member of the spliceosome complex which potentiates C/EBP expression in adipocyte differentiation. As C/EBP family members are important regulators of myelopoiesis and THOC5 is highly expressed in neutrophil/macrophage progenitor cells we assessed the role of THOC5 in cytokine-stimulated monocytic development. M-CSF stimulated maturation of the NFS60 cell line was associated with enhanced THOC5 expression and phosphorylation. THOC5 was also shown to form a complex with C/EBPbeta. Ectopic expression of THOC5 mimicked M-CSF mediated cell maturation and enhanced protein expression of the myeloid transcription factors C/EBPbeta, C/EBPalpha, Pu-1 and also GAB2 (a PI-3 Kinase and macrophage development regulator). Increased THOC5 expression also mimicked M-CSF stimulated increases in the lipid second messenger PtdInsP(3). Inhibition of THOC5-induced increases in PtdInsP(3) levels abrogated the elevated levels of C/EBPbeta. Thus THOC5 expression can potentiate receptor signalling to transcription factor expression and monocyte differentiation.

Published

2008

42. Proteome biology of stem cells: a new joint HUPO and ISSCR initiative

Author

Jeroen, Krijgsveld, Anthony D, Whetton, Bonghee, Lee, Ihor, Lemischka, Steve, Oh, Martin, Pera, Christine, Mummery, and Albert J R, Heck

Subjects

Proteomics, Proteome, International Cooperation, Stem Cells, Animals, Humans

Published

2008

43. The biology and clinical potential of growth factors that regulate myeloid cell production

Author

Anthony D. Whetton

Subjects

Pharmacology, Myeloid, Cell, Bone Marrow Cells, Disease, Biology, Molecular cloning, Toxicology, In vitro, Haematopoiesis, medicine.anatomical_structure, Colony-Stimulating Factors, Bone Marrow, In vivo, Immunology, Cancer research, medicine, Animals, Humans, Gene, Cell Division

Abstract

The colony-stimulating factors are a group of growth factors important in regulating the production of myeloid cells. The past 25 years have seen the identification and characterization of many of these growth factors and, more recently, the molecular cloning of their genes. This has enabled the production of sufficient quantities to assess their biological activity in vivo and in vitro . Some of these recombinant growth factors have also been employed in clinical trials, which have indicated potential uses in the treatment of a variety of disease. Here, Anthony Whetton considers the biology of haematopoietic growth factors, and the evidence that they may be of value in the treatment of haematopoietic, infectious and malignant disease.

Published

1990

44. Eight-channel iTRAQ enables comparison of the activity of six leukemogenic tyrosine kinases

Author

Danny A. Bitton, Elaine Spooncer, Chia-Fang Lee, Michal J. Okoniewski, Anthony D. Whetton, Liqun Zhang, Louise Carney, Caroline A. Evans, Ewa Jaworska, Richard D. Unwin, David Blinco, Crispin J. Miller, Stephen D. Griffiths, and Andrew Pierce

Subjects

Proteomics, Proteome, Biology, Protein Serine-Threonine Kinases, Biochemistry, Leukemogenic, Mass Spectrometry, Analytical Chemistry, Cell Line, Transcriptome, Mice, Animals, Molecular Biology, Oligonucleotide Array Sequence Analysis, Genetics, Oncogene Proteins, ABL, Leukemia, Chemotaxis, Gene Expression Profiling, breakpoint cluster region, Exons, Cell biology, Gene expression profiling, Protein Biosynthesis, Tyrosine kinase

Abstract

There are a number of leukemogenic protein-tyrosine kinases (PTKs) associated with leukemic transformation. Although each is linked with a specific disease their functional activity poses the question whether they have a degree of commonality in their effects upon target cells. Exon array analysis of the effects of six leukemogenic PTKs (BCR/ABL, TEL/PDGFRbeta, FIP1/PDGFRalpha, D816V KIT, NPM/ALK, and FLT3ITD) revealed few common effects on the transcriptome. It is apparent, however, that proteome changes are not directly governed by transcriptome changes. Therefore, we assessed and used a new generation of iTRAQ tagging, enabling eight-channel relative quantification discovery proteomics, to analyze the effects of these six leukemogenic PTKs. Again these were found to have disparate effects on the proteome with few common targets. BCR/ABL had the greatest effect on the proteome and had more effects in common with FIP1/PDGFRalpha. The proteomic effects of the four type III receptor kinases were relatively remotely related. The only protein commonly affected was eosinophil-associated ribonuclease 7. Five of six PTKs affected the motility-related proteins CAPG and vimentin, although this did not correspond to changes in motility. However, correlation of the proteomics data with that from the exon microarray not only showed poor levels of correlation between transcript and protein levels but also revealed alternative patterns of regulation of the CAPG protein by different oncogenes, illustrating the utility of such a combined approach.

Published

2007

45. FMIP controls the adipocyte lineage commitment of C2C12 cells by downmodulation of C/EBP alpha

Author

Alison H. Banham, Michaela Scherr, Annalisa Mancini, Anthony D. Whetton, Karen Pulford, O. El Bounkari, Teruko Tamura, A. F. Norrenbrock, D. Schaefer, Linden Lyne, and Matthias Eder

Subjects

Cancer Research, Small interfering RNA, Cellular differentiation, Down-Regulation, Receptor tyrosine kinase, Cell Line, Mice, Enhancer binding, Genetics, Adipocytes, CCAAT-Enhancer-Binding Protein-alpha, RNA Precursors, Animals, Humans, Cell Lineage, RNA, Small Interfering, Molecular Biology, Gene knockdown, Muscle Cells, biology, Intracellular Signaling Peptides and Proteins, Cell Differentiation, Molecular biology, Insulin receptor, Phenotype, biology.protein, Ectopic expression, C2C12

Abstract

Fms interacting protein (FMIP) is a substrate for Fms tyrosine kinase, and a nuclear/cytoplasm shuttling protein with a leucine zipper. As the phosphorylation of FMIP is observed in insulin-stimulated preadipocytes, we examined the role of FMIP in adipocyte differentiation, using the mesenchymal multipotent stem cells, C2C12 cells, that can differentiate into adipocytes, muscle cells and osteoblasts. Ectopic expression of FMIP in C2C12 impairs the adipocyte differentiation induced by treatment with insulin, dexamethasone and 3-isobutyl-1-methylxanthine. These cells exhibit muscle phenotype with multinuclear morphology. Furthermore, knockdown of endogenous FMIP expression by small interfering RNA improves adipocytic lineage commitment of C2C12 cells, while impairing muscle differentiation. Upon stimulation with insulin, CCAAT/enhancer binding protein (C/EBP)beta, but not C/EBPalpha, is upregulated in cells expressing ectopic FMIP, whereas in FMIP knockdown cells, C/EBPalpha is constitutively expressed. Ectopic expression of C/EBPalpha counteracts the effects of FMIP, whereas C/EBPalpha knockdown partially mimics the effects of FMIP in this system. Northern blot analysis and reverse transcriptase-polymerase chain reaction study reveal that ectopic FMIP-expressing cells do not contain the polyadenylated C/EBPalpha mRNA, but contain the C/EBPalpha pre-mRNA, suggesting that FMIP plays a role in RNA processing and/or export. Indeed, a member of the THO complex that plays a role in mRNA export, THOC1, is co-precipitated with FMIP. The data we have acquired on FMIP suggest that it is a target for tyrosine kinase receptors that potentiate mRNA export.

Published

2007

46. Systematic proteome and transcriptome analysis of stem cell populations

Author

Anthony D. Whetton and Richard D. Unwin

Subjects

Proteomics, Messenger RNA, Proteome, Transcription, Genetic, Stem Cells, Cell, Cell Biology, Biology, Cell biology, Transcriptome, Haematopoiesis, medicine.anatomical_structure, medicine, Protein biosynthesis, Animals, Humans, Stem cell, Molecular Biology, Developmental Biology

Abstract

Methods for relative assessment of the transcriptional activity of the cell are now routinely employed and obtain large amounts of information regarding process such as transformation or development. These approaches have great impact and are of significant value. Nonetheless, mRNA is an intermediate in the process of protein synthesis and changes in mRNA expression do not reflect absolute or relative changes in protein levels. The mechanisms which translate mRNA to protein are highly regulated, and it remains unclear how the transcriptome reflects the functional state of the cell, as defined by its protein output. Large scale analyses of the proteome are now becoming a reality due to technical advances in protein arrays and mass spectrometry. Thus for the first time data on large numbers of mRNA transcripts and the levels of expression of their associated proteins is available in dynamic systems. Analysis of one such comparison, the transcriptome and proteome of primary haematopoietic stem cells, reveals post-translational regulation of the proteome in stem cell populations. The factors which must be considered when comparing two systematically acquired 'omics' datasets are reviewed and the relative merits of transcriptome and proteome approaches are discussed.

Published

2006

47. The survival of differentiating embryonic stem cells is dependent on the SCF-KIT pathway

Author

Anu Bashamboo, Anthony D. Whetton, Kay Samuel, A. Helen Taylor, Jean Jacque Panthier, and Lesley M. Forrester

Subjects

Mice, Knockout, Stem Cell Factor, Cell Survival, Cellular differentiation, Stem cell factor, Apoptosis, Cell Differentiation, Cell Biology, Biology, Embryonic stem cell, Molecular biology, Null allele, Tacrolimus, Cell biology, Endothelial stem cell, Mice, Proto-Oncogene Proteins c-kit, Phenotype, Mutation, Inner cell mass, Animals, Progenitor cell, Signal transduction, Embryonic Stem Cells, Signal Transduction

Abstract

The stem cell factor (SCF)-KIT signal transduction pathway plays a role in the proliferation, differentiation and survival of a range of stem and progenitor cell types but little is known about its function in embryonic stem (ES) cells. We generated ES cells carrying a null allele of Kit as well as a knock-in allele that encodes an SCF-independent hybrid KIT receptor that can be activated by the FKBP binding drug, AP20187. KIT null ES cells die when induced to differentiate upon withdrawal of leukaemia inhibitory factor in monolayer culture. This phenotype is recapitulated in wild-type ES cells treated with a KIT-neutralising antibody and reversed in mutant cells by activation of the hybrid KIT receptor. Differentiating KIT null ES cells exhibit elevated levels of DNA laddering and reduced BCL2 expression, indicative of apoptosis. We conclude that mouse ES cell differentiation in vitro is dependent on the SCF-KIT pathway contrasting with the apparently normal differentiation of KIT null inner cell mass or epiblast cells in vivo. This discrepancy could be explained by the presence of compensatory signals in the embryo or it could lend support to the idea of a phenotypic relationship between ES cells and early germ cells.

Published

2006

48. Quantitative proteomics reveals posttranslational control as a regulatory factor in primary hematopoietic stem cells

Author

Anthony D. Whetton, Crispin J. Miller, Duncan L. Smith, Kay Barnes, Richard D. Unwin, Stephen A. Baldwin, Andrew Pierce, Claire Wilson, David Blinco, Ewa Jaworska, Elaine Spooncer, and Caroline A. Evans

Subjects

Proteomics, Proteome, Immunology, Quantitative proteomics, Cell Biology, Hematology, Biology, Hematopoietic Stem Cells, Biochemistry, Molecular biology, Cell Hypoxia, Mass Spectrometry, Cell biology, Transcriptome, Haematopoiesis, Mice, Protein biosynthesis, Animals, Progenitor cell, Stem cell, Oxidation-Reduction, Protein Processing, Post-Translational, Chromatography, Liquid

Abstract

The proteome is determined by rates of transcription, translation, and protein turnover. Definition of stem cell populations therefore requires a stem cell proteome signature. However, the limit to the number of primary cells available has restricted extensive proteomic analysis. We present a mass spectrometric method using an isobaric covalent modification of peptides for relative quantification (iTRAQ), which was employed to compare the proteomes of approximately 1 million long-term reconstituting hematopoietic stem cells (Lin–Sca+Kit+; LSK+) and non–long-term reconstituting progenitor cells (Lin–Sca+Kit–; LSK–), respectively. Extensive 2-dimensional liquid chromatography (LC) peptide separation prior to mass spectrometry (MS) enabled enhanced proteome coverage with relative quantification of 948 proteins. Of the 145 changes in the proteome, 54% were not seen in the transcriptome. Hypoxia-related changes in proteins controlling metabolism and oxidative protection were observed, indicating that LSK+ cells are adapted for anaerobic environments. This approach can define proteomic changes in primary samples, thereby characterizing the molecular signature of stem cells and their progeny.

Published

2006

49. Global effects of BCR/ABL and TEL/PDGFRbeta expression on the proteome and phosphoproteome: identification of the Rho pathway as a target of BCR/ABL

Author

Richard D, Unwin, David W, Sternberg, Yuning, Lu, Andrew, Pierce, D Gary, Gilliland, and Anthony D, Whetton

Subjects

Oncogene Proteins, Fusion, Proteome, Gene Expression Profiling, Fusion Proteins, bcr-abl, Phosphoproteins, Transfection, Piperazines, Cell Line, Gene Expression Regulation, Neoplastic, Mice, Cell Transformation, Neoplastic, Pyrimidines, Benzamides, Imatinib Mesylate, Animals, Electrophoresis, Gel, Two-Dimensional

Abstract

Many leukemic oncogenes form as a consequence of gene fusions or mutation that result in the activation or overexpression of a tyrosine kinase. To identify commonalities and differences in the action of two such kinases, breakpoint cluster region (BCR)/ABL and TEL/PDGFRbeta, two-dimensional gel electrophoresis was employed to characterize their effects on the proteome. While both oncogenes affected expression of specific proteins, few common effects were observed. A number of proteins whose expression is altered by BCR/ABL, including gelsolin and stathmin, are related to cytoskeletal function whereas no such changes were seen in TEL/PDGFRbeta-transfected cells. Treatment of cells with the kinase inhibitor STI571 for 4-h reversed changes in expression of some of these cytoskeletal proteins. Correspondingly, BCR/ABL-transfected cells were less responsive to chemotactic and chemokinetic stimuli than non-transfected cells and TEL/PDGFRbeta-transfected Ba/F3 cells. Decreased motile response was reversed by a 16-h treatment with STI571. A phosphoprotein-specific gel stain was used to identify TEL/PDGFRbeta and BCR/ABL-mediated changes in the phosphoproteome. These included changes on Crkl, Ras-GAP-binding protein 1, and for BCR/ABL, cytoskeletal proteins such as tubulin, and Nedd5. Decreased phosphorylation of Rho-GTPase dissociation inhibitor (Rho GDI) was also observed in BCR/ABL-transfected cells. This results in the activation of the Rho pathway, and treatment of cells with Y27632, an inhibitor of Rho kinase, inhibited DNA synthesis in BCR/ABL-transfected Ba/F3 cells but not TEL/PDGFRbeta-expressing cells. Expression of a dominant-negative RhoA inhibited both DNA synthesis and transwell migration, demonstrating the significance of this pathway in BCR/ABL-mediated transformation.

Published

2004

50. PEDRo: A database for storing, searching and disseminating experimental proteomics data

Author

Simon J. Gaskell, Zhikang Yin, Kathleen M. Carroll, Julie Howard, Keith F. Chater, Chris F. Taylor, Sarah R. Hart, Alistair J. P. Brown, Caroline A. Evans, Norman Morrison, Lena Hansson, Norman W. Paton, Stephen G. Oliver, David Stead, Kathryn S. Lilley, Andy Brass, Muriel Mewissen, Thomas McLaughlin, Peter Ghazal, Kevin Garwood, Andrew Hesketh, Anthony D. Whetton, Chris Garwood, Scott Joens, Simon J. Hubbard, Lilley, Kathryn [0000-0003-0594-6543], Oliver, Stephen [0000-0001-6330-7526], and Apollo - University of Cambridge Repository

Subjects

Proteomics, Saccharomyces cerevisiae Proteins, lcsh:QH426-470, GeneralLiterature_INTRODUCTORYANDSURVEY, lcsh:Biotechnology, Data management, Candida glabrata, Streptomyces coelicolor, Biology, computer.software_genre, Database, Fungal Proteins, Mice, 03 medical and health sciences, Upload, 0302 clinical medicine, Bacterial Proteins, Software Design, lcsh:TP248.13-248.65, Candida albicans, Genetics, Human proteome project, Animals, Databases, Protein, Trichinella spiralis, 030304 developmental biology, 0303 health sciences, Fungal protein, Arabidopsis Proteins, business.industry, QH, Computational Biology, Proteins, Experimental data, Trichinellosis, Helminth Proteins, Jejunal Diseases, lcsh:Genetics, ComputingMethodologies_PATTERNRECOGNITION, Data model, 030220 oncology & carcinogenesis, Proteome, Database Management Systems, business, computer, Biotechnology

Abstract

Background Proteomics is rapidly evolving into a high-throughput technology, in which substantial and systematic studies are conducted on samples from a wide range of physiological, developmental, or pathological conditions. Reference maps from 2D gels are widely circulated. However, there is, as yet, no formally accepted standard representation to support the sharing of proteomics data, and little systematic dissemination of comprehensive proteomic data sets. Results This paper describes the design, implementation and use of a Proteome Experimental Data Repository (PEDRo), which makes comprehensive proteomics data sets available for browsing, searching and downloading. It is also serves to extend the debate on the level of detail at which proteomics data should be captured, the sorts of facilities that should be provided by proteome data management systems, and the techniques by which such facilities can be made available. Conclusions The PEDRo database provides access to a collection of comprehensive descriptions of experimental data sets in proteomics. Not only are these data sets interesting in and of themselves, they also provide a useful early validation of the PEDRo data model, which has served as a starting point for the ongoing standardisation activity through the Proteome Standards Initiative of the Human Proteome Organisation.

Published

2004