55 results on '"Irina Nazarenko"'
Search Results
2. Wnt5A modulates integrin expression in a receptor-dependent manner in ovarian cancer cells
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Vajihe Azimian-Zavareh, Zeinab Dehghani-Ghobadi, Marzieh Ebrahimi, Kian Mirzazadeh, Irina Nazarenko, and Ghamartaj Hossein
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Medicine ,Science - Abstract
Abstract Wnt5A signals through various receptors that confer versatile biological functions. Here, we used Wnt5A overexpressing human ovarian SKOV-3 and OVCAR-3 stable clones for assessing integrin expression, cell proliferation, migration, invasion, and the ability of multicellular aggregates (MCAs) formation. We found here, that Wnt5A regulates differently the expression of its receptors in the stable Wnt5A overexpressing clones. The expression levels of Frizzled (FZD)-2 and -5, were increased in different clones. However ROR-1, -2 expression levels were differently regulated in clones. Wnt5A overexpressing clones showed increased cell proliferation, migration, and clonogenicity. Moreover, Wnt5A overexpressing SKOV-3 clone showed increased MCAs formation ability. Cell invasion had been increased in OVCAR-3-derived clones, while this was decreased in SKOV-3-derived clone. Importantly, αv integrin expression levels were increased in all assessed clones, accompanied by increased cell attachment to fibronectin and focal adhesion kinase activity. Moreover, the treatment of clones with Box5 as a Wnt5A/FZD5 antagonist abrogates ITGAV increase, cell proliferation, migration, and their attachment to fibronectin. Accordingly, we observed significantly higher expression levels of ITGAV and ITGB3 in human high-grade serous ovarian cancer specimens and ITGAV correlated positively with Wnt5A in metastatic serous type ovarian cancer. In summary, we hypothesize here, that Wnt5A/FZD-5 signaling modulate αv integrin expression levels that could be associated with ovarian cancer cell proliferation, migration, and fibronectin attachment.
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- 2021
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3. Tspan8 is expressed in breast cancer and regulates E‐cadherin/catenin signalling and metastasis accompanied by increased circulating extracellular vesicles
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Marie Follo, Andreas R. Thomsen, Andreas Hippe, Richa Khanduri, Marina Veil, Christine Sers, Ghamartaj Hossein, Irina Nazarenko, Gerhard Puetz, Elena Grueso Navarro, Celine Greco, Wilko Thiele, Tanja Gainey‐Schleicher, Florian Rossner, Bernhard Homey, Cornelius F. Waller, Paul Jank, Thalia Erbes, Jonathan P. Sleeman, Claude Boucheix, Maren Voglstaetter, Arend Koch, Jochen Dindorf, Clemens M. Franz, Carina Blaue, Andrea Groß, Andreas Baur, Jubin Kashef, and Jerome Nouvel
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Life sciences ,biology ,0301 basic medicine ,endocrine system ,Tetraspanins ,three‐dimensional cell culture ,Motility ,Breast Neoplasms ,Pathology and Forensic Medicine ,Metastasis ,Extracellular Vesicles ,03 medical and health sciences ,breast cancer ,0302 clinical medicine ,Breast cancer ,Tspan8 ,Cell Line, Tumor ,ddc:570 ,Biomarkers, Tumor ,medicine ,Carcinoma ,Animals ,Humans ,Neoplasm Metastasis ,metastases ,Original Paper ,Cadherin ,business.industry ,Melanoma ,Carcinoma, Ductal, Breast ,Cancer ,beta‐catenin signalling pathway ,Cadherins ,medicine.disease ,Original Papers ,mesenchymal–epithelial transition ,Rats ,3. Good health ,Carcinoma, Lobular ,Carcinoma, Intraductal, Noninfiltrating ,030104 developmental biology ,030220 oncology & carcinogenesis ,Catenin ,Cancer research ,Female ,business ,Signal Transduction - Abstract
Tspan8 exhibits a functional role in many cancer types including pancreatic, colorectal, oesophagus carcinoma, and melanoma. We present a first study on the expression and function of Tspan8 in breast cancer. Tspan8 protein was present in the majority of human primary breast cancer lesions and metastases in the brain, bone, lung, and liver. In a syngeneic rat breast cancer model, Tspan8+ tumours formed multiple liver and spleen metastases, while Tspan8− tumours exhibited a significantly diminished ability to metastasise, indicating a role of Tspan8 in metastases. Addressing the underlying molecular mechanisms, we discovered that Tspan8 can mediate up‐regulation of E‐cadherin and down‐regulation of Twist, p120‐catenin, and β‐catenin target genes accompanied by the change of cell phenotype, resembling the mesenchymal–epithelial transition. Furthermore, Tspan8+ cells exhibited enhanced cell–cell adhesion, diminished motility, and decreased sensitivity to irradiation. As a regulator of the content and function of extracellular vesicles (EVs), Tspan8 mediated a several‐fold increase in EV number in cell culture and the circulation of tumour‐bearing animals. We observed increased protein levels of E‐cadherin and p120‐catenin in these EVs; furthermore, Tspan8 and p120‐catenin were co‐immunoprecipitated, indicating that they may interact with each other. Altogether, our findings show the presence of Tspan8 in breast cancer primary lesion and metastases and indicate its role as a regulator of cell behaviour and EV release in breast cancer. © 2019 The Authors. The Journal of Pathology published by John Wiley & Sons Ltd on behalf of Pathological Society of Great Britain and Ireland.
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- 2019
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4. Identification and characterization of 40 novel hydroxymethylbilane synthase mutations that cause acute intermittent porphyria
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Constanza Solis-Villa, Brenden Chen, Robert J. Desnick, Makiko Yasuda, Irina Nazarenko, Manisha Balwani, Angelika Erwin, and John D. Phillips
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Male ,0301 basic medicine ,030213 general clinical medicine ,Hydroxymethylbilane Synthase ,Mutant ,Mutation, Missense ,Biology ,medicine.disease_cause ,Article ,03 medical and health sciences ,Exon ,0302 clinical medicine ,Genetics ,medicine ,Humans ,Missense mutation ,Thermolabile ,Genetics (clinical) ,Sequence Deletion ,Acute intermittent porphyria ,Mutation ,Wild type ,medicine.disease ,Molecular biology ,Mutagenesis, Insertional ,030104 developmental biology ,Porphyria, Acute Intermittent ,Female - Abstract
Acute intermittent porphyria (AIP), an autosomal dominant disorder due to the half-normal activity of hydroxymethylbilane synthase (HMBS), is characterized by acute neurovisceral attacks that are precipitated by factors that induce heme biosynthesis. Molecular diagnosis is the most sensitive and specific diagnostic test for AIP, and importantly, it permits the identification of asymptomatic family members for genetic counseling and avoidance of precipitating factors. Here, we report the identification of 40 novel HMBS mutations, including 11 missense, four nonsense, 16 small insertions or deletions, eight consensus splice site mutations, and a complex insertion-deletion mutation in unrelated individuals with AIP. Prokaryotic expression of the missense mutations demonstrated that all mutants had ≤5% of expressed wildtype activity, except for c.1039G>C (p.A347P), which had 51% residual HMBS activity but was markedly thermolabile. Of note, the mutation c.612G>T (p.Q204H) altered the last nucleotide of exon 10, which resulted in an alternative HMBS transcript with an in-frame nine base-pair deletion at the 3'-terminus of exon 10 (encoding protein Q204HΔ3). When expressed, Q204HΔ3 and an in-frame three base-pair deletion (c.639_641delTGC) had no detectable HMBS activity. Western blot analyses and mapping of the missense mutations on the human HMBS crystal structure revealed that mutations near the active site or at the dimerization interface resulted in stably expressed proteins, while most that altered surface residues resulted in unstable proteins, presumably due to improper protein folding. These studies identified novel pathogenic HMBS mutations and expanded the molecular heterogeneity of AIP.
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- 2019
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5. Wnt5A modulates integrin expression in a receptor-dependent manner in ovarian cancer cells
- Author
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Marzieh Ebrahimi, Ghamartaj Hossein, Kian Mirzazadeh, Vajihe Azimian-Zavareh, Irina Nazarenko, and Zeinab Dehghani-Ghobadi
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0301 basic medicine ,Frizzled ,Integrins ,endocrine system diseases ,Cell ,Clone (cell biology) ,Mesoderm ,0302 clinical medicine ,Cell Movement ,Gene Regulatory Networks ,Receptor ,Cell Aggregation ,Ovarian Neoplasms ,Multidisciplinary ,biology ,Cadherins ,female genital diseases and pregnancy complications ,Cell biology ,medicine.anatomical_structure ,030220 oncology & carcinogenesis ,embryonic structures ,Medicine ,Female ,Protein Binding ,Science ,Receptors, Cell Surface ,Article ,Morphogen signalling ,Wnt-5a Protein ,03 medical and health sciences ,Cell Line, Tumor ,medicine ,Biomarkers, Tumor ,Cell Adhesion ,Humans ,Neoplasm Invasiveness ,ITGAV ,Cell Proliferation ,Cell growth ,Epithelial Cells ,medicine.disease ,Clone Cells ,Cystadenocarcinoma, Serous ,Fibronectins ,Fibronectin ,body regions ,030104 developmental biology ,Gene Ontology ,biology.protein ,sense organs ,Laminin ,Ovarian cancer - Abstract
Wnt5A signals through various receptors that confer versatile biological functions. Here, we used Wnt5A overexpressing human ovarian SKOV-3 and OVCAR-3 stable clones for assessing integrin expression, cell proliferation, migration, invasion, and the ability of multicellular aggregates (MCAs) formation. We found here, that Wnt5A regulates differently the expression of its receptors in the stable Wnt5A overexpressing clones. The expression levels of Frizzled (FZD)-2 and -5, were increased in different clones. However ROR-1, -2 expression levels were differently regulated in clones. Wnt5A overexpressing clones showed increased cell proliferation, migration, and clonogenicity. Moreover, Wnt5A overexpressing SKOV-3 clone showed increased MCAs formation ability. Cell invasion had been increased in OVCAR-3-derived clones, while this was decreased in SKOV-3-derived clone. Importantly, αv integrin expression levels were increased in all assessed clones, accompanied by increased cell attachment to fibronectin and focal adhesion kinase activity. Moreover, the treatment of clones with Box5 as a Wnt5A/FZD5 antagonist abrogates ITGAV increase, cell proliferation, migration, and their attachment to fibronectin. Accordingly, we observed significantly higher expression levels of ITGAV and ITGB3 in human high-grade serous ovarian cancer specimens and ITGAV correlated positively with Wnt5A in metastatic serous type ovarian cancer. In summary, we hypothesize here, that Wnt5A/FZD-5 signaling modulate αv integrin expression levels that could be associated with ovarian cancer cell proliferation, migration, and fibronectin attachment.
- Published
- 2021
6. Airway Basal Cells show a dedifferentiated KRT17highPhenotype and promote Fibrosis in Idiopathic Pulmonary Fibrosis
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Malgorzata Wygrecka, Gian Kayser, Taylor Adams, Axel Schambach, Benedikt Jaeger, Oliver Terwolbeck, Robert Zweigerdt, Danny Jonigk, Naftali Kaminski, Stefan Lienenklaus, Wiebke Garrels, Antje Prasse, Henning Kempf, Denise Klatt, Peggy Engelhard, Jonas C. Schupp, Irina Nazarenko, and Linda Plappert
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Cell type ,Lung ,business.industry ,Cell ,respiratory system ,medicine.disease ,respiratory tract diseases ,Extracellular matrix ,Idiopathic pulmonary fibrosis ,medicine.anatomical_structure ,Fibrosis ,medicine ,Cancer research ,Fibroblast ,business ,Proto-oncogene tyrosine-protein kinase Src - Abstract
Idiopathic pulmonary fibrosis (IPF) is a fatal disease with limited treatment options. In this study we focus on the profibrotic properties of airway basal cells (ABC) obtained from patients with IPF (IPF-ABC). Single cell RNA sequencing of bronchial brushes revealed extensive reprogramming of IPF-ABC towards a KRT17high PTENlow dedifferentiated cell type. In the 3D organoid model, compared to ABC obtained from healthy volunteers, IPF-ABC give rise to more bronchospheres, de novo bronchial structures resembling lung developmental processes, induce fibroblast proliferation and extracellular matrix deposition in co-culture. Intratracheal application of IPF-ABC into minimally injured lungs of Rag2-/- or NRG mice causes severe fibrosis, remodeling of the alveolar compartment, and formation of honeycomb cyst-like structures. Connectivity MAP analysis of scRNA seq of bronchial brushings suggested that gene expression changes in IPF-ABC can be reversed by SRC inhibition. After demonstrating enhanced SRC expression and activity in these cells, and in IPF lungs, we tested the effects of saracatinib, a potent SRC inhibitor previously studied in humans. We demonstrated that saracatinib modified in-vitro and in-vivo the profibrotic changes observed in our 3D culture system and novel mouse xenograft model.
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- 2020
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7. The CD151-midkine pathway regulates the immune microenvironment in inflammatory breast cancer
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Fedor Berditchevski, Daniel Rea, Mariam Gachehiladze, Steven Van Laere, Steven Hayward, Nahla M Badr, Guerman Molostvov, Naoto T. Ueno, Heather M. Long, Fiona Hoar, Nisha Sharma, Barbora Sopikova, Irina Nazarenko, Dominic Burg, Andrew M. Hanby, Yoshiya Horimoto, Bedrich L. Eckhardt, Liliia Paniushkina, Abeer M Shaaban, Regina Andrijes, Giorgi Mgebrishvili, Zuzana Slobodova, and Graham R. Robertson
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0301 basic medicine ,Chemokine ,medicine.medical_treatment ,Integrin ,Tetraspanin 24 ,Pathology and Forensic Medicine ,03 medical and health sciences ,0302 clinical medicine ,Immune system ,Tetraspanin ,Cell Line, Tumor ,medicine ,Tumor Microenvironment ,Humans ,skin and connective tissue diseases ,CD151 ,Midkine ,biology ,Growth factor ,Macrophages ,030104 developmental biology ,030220 oncology & carcinogenesis ,biology.protein ,Cancer research ,Inflammatory Breast Neoplasms ,Human medicine ,Antibody ,Chemokines - Abstract
The immune microenvironment in inflammatory breast cancer (IBC) is poorly characterised, and molecular and cellular pathways that control accumulation of various immune cells in IBC tissues remain largely unknown. Here, we discovered a novel pathway linking the expression of the tetraspanin protein CD151 in tumour cells with increased accumulation of macrophages in cancerous tissues. It is notable that elevated expression of CD151 and a higher number of tumour-infiltrating macrophages correlated with better patient responses to chemotherapy. Accordingly, CD151-expressing IBC xenografts were characterised by the increased infiltration of macrophages. In vitro migration experiments demonstrated that CD151 stimulates the chemoattractive potential of IBC cells for monocytes via mechanisms involving midkine (a heparin-binding growth factor), integrin alpha 6 beta 1, and production of extracellular vesicles (EVs). Profiling of chemokines secreted by IBC cells demonstrated that CD151 increases production of midkine. Purified midkine specifically stimulated migration of monocytes, but not other immune cells. Further experiments demonstrated that the chemoattractive potential of IBC-derived EVs is blocked by anti-midkine antibodies. These results demonstrate for the first time that changes in the expression of a tetraspanin protein by tumour cells can affect the formation of the immune microenvironment by modulating recruitment of effector cells to cancerous tissues. Therefore, a CD151-midkine pathway can be considered as a novel target for controlled changes of the immune landscape in IBC. (c) 2020 Pathological Society of Great Britain and Ireland. Published by John Wiley & Sons, Ltd.
- Published
- 2020
8. Considerations towards a roadmap for collection, handling and storage of blood extracellular vesicles
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Dakota Gustafson, Andrew M. Hoffman, Aled Clayton, Cecilia Lässer, Joshua A. Welsh, Pia Siljander, Carolina Soekmadji, Juan Manual Falcón-Perez, Charlotte Lawson, Chris Gardiner, Lorraine O'Driscoll, Edit I. Buzás, Ryan C. Pink, Jennifer Jones, Eric Boilard, Kenneth W. Witwer, Marca H. M. Wauben, Rienk Nieuwland, Lei Zheng, Alice Gualerzi, Irina Nazarenko, An Hendrix, Lesley Cheng, Metka Lenassi, Extracellular Vesicles, Molecular and Integrative Biosciences Research Programme, Drug Research Program, Division of Pharmaceutical Biosciences, LS Celbiologie-Algemeen, dB&C I&I, Laboratory Specialized Diagnostics & Research, ACS - Microcirculation, and CCA - Imaging and biomarkers
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0301 basic medicine ,medicine.medical_specialty ,Histology ,SOCIETY ,exosomes ,Meeting Report ,Exosomes ,Extracellular vesicles ,03 medical and health sciences ,0302 clinical medicine ,pre-analytical ,blood ,Medicine and Health Sciences ,medicine ,lcsh:QH573-671 ,Intensive care medicine ,plasma ,Body fluid ,High concentration ,lcsh:Cytology ,Pre analytical ,business.industry ,Cell Biology ,Extracellular vesicle ,STANDARDIZATION ,Microvesicles ,3. Good health ,Biomarker (cell) ,030104 developmental biology ,030220 oncology & carcinogenesis ,pre-analytical variables ,biomarker ,1182 Biochemistry, cell and molecular biology ,extracellular vesicle ,business ,Relevant information ,microvesicles ,serum - Abstract
There is an increasing interest in exploring clinically relevant information that is present in body fluids, and extracellular vesicles (EVs) are intrinsic components of body fluids (?liquid biopsies?). In this report, we will focus on blood. Blood contains not only EVs but also cells, and non-EV particles including lipoproteins. Due to the high concentration of soluble proteins and lipoproteins, blood, plasma and serum have a high viscosity and density, which hampers the concentration, isolation and detection of EVs. Because most if not all studies on EVs are single-centre studies, their clinical relevance remains limited. Therefore, there is an urgent need to improve standardization and reproducibility of EV research. As a first step, the International Society on Extracellular Vesicles organized a biomarker workshop in Birmingham (UK) in November 2017, and during that workshop several working groups were created to focus on a particular body fluid. This report is the first output of the blood EV work group and is based on responses by work group members to a questionnaire in order to discover the contours of a roadmap. From the answers it is clear that most respondents are in favour of evidence-based research, education, quality control procedures, and physical models to improve our understanding and comparison of concentration, isolation and detection methods. Since blood is such a complex body fluid, we assume that the outcome of the survey may also be valuable for exploring body fluids other than blood. Non
- Published
- 2019
9. Biodegradable Nanocarriers Resembling Extracellular Vesicles Deliver Genetic Material with the Highest Efficiency to Various Cell Types
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Gleb B. Sukhorukov, Seppo Vainio, Ilya Skovorodkin, Maria N. Antipina, Boris Kochergin, Igor Meglinski, Jamal Alzubi, Marie Follo, Alexey Popov, Toni Cathomen, Albert R. Muslimov, Vsevolod S. Atkin, Valentina Pennucci, Tatjana I. Cornu, Irina Nazarenko, Yana V. Tarakanchikova, and Dmitry A. Gorin
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Cell type ,Cell ,02 engineering and technology ,Gene delivery ,010402 general chemistry ,Transfection ,01 natural sciences ,Nanocapsules ,Biomaterials ,Extracellular Vesicles ,In vivo ,Cell Line, Tumor ,medicine ,Humans ,General Materials Science ,biomimetics ,Primary cell ,gene delivery ,Drug Carriers ,Chemistry ,nanocapsules ,General Chemistry ,021001 nanoscience & nanotechnology ,0104 chemical sciences ,microcapsules ,Kinetics ,medicine.anatomical_structure ,Drug delivery ,drug delivery ,Biophysics ,Nanoparticles ,Nanocarriers ,0210 nano-technology ,extracellular vesicles ,Biotechnology - Abstract
Efficient delivery of genetic material to primary cells remains challenging. Here, efficient transfer of genetic material is presented using synthetic biodegradable nanocarriers, resembling extracellular vesicles in their biomechanical properties. This is based on two main technological achievements: generation of soft biodegradable polyelectrolyte capsules in nanosize and efficient application of the nanocapsules for co-transfer of different RNAs to tumor cell lines and primary cells, including hematopoietic progenitor cells and primary T cells. Near to 100% efficiency is reached using only 2.5 × 10−4 pmol of siRNA, and 1 × 10−3 nmol of mRNA per cell, which is several magnitude orders below the amounts reported for any of methods published so far. The data show that biodegradable nanocapsules represent a universal and highly efficient biomimetic platform for the transfer of genetic material with the utmost potential to revolutionize gene transfer technology in vitro and in vivo.
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- 2019
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10. STRUCTURE OF TRAINING ACTIVITY OF SWIMMERS BASED ON THE FUNCTIONAL STATUS OF SKELETAL MUSCLES
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Irina Nazarenko, Konstantin Bondarenko, Mariya Palashenko, and Olga Zaharchenko
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medicine.medical_specialty ,Physical medicine and rehabilitation ,Training Activity ,General Engineering ,medicine ,Functional status ,Biology - Published
- 2016
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11. Synovial Sarcoma Microvesicles Harbor the SYT-SSX Fusion Gene Transcript: Comparison of Different Methods of Detection and Implications in Biomarker Research
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P. V. Ullrich, Steffen U. Eisenhardt, A. F. V. Cimniak, Holger Bannasch, Sigrun Nestel, Alba Fricke, Marie Follo, Irina Nazarenko, David Braig, Bernd Heimrich, and G. B. Stark
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0301 basic medicine ,lcsh:Internal medicine ,Pathology ,medicine.medical_specialty ,Article Subject ,Peripheral blood mononuclear cell ,Fusion gene ,03 medical and health sciences ,0302 clinical medicine ,Medicine ,lcsh:RC31-1245 ,Molecular Biology ,Messenger RNA ,business.industry ,Microvesicle ,Cell Biology ,medicine.disease ,Molecular biology ,Synovial sarcoma ,Microvesicles ,030104 developmental biology ,Fusion transcript ,030220 oncology & carcinogenesis ,business ,Nested polymerase chain reaction ,Research Article - Abstract
Background. Synovial sarcoma is an aggressive soft-tissue malignancy. This study examines the presence of the SYT-SSX fusion transcript in synovial sarcoma microvesicles as well as its potential role as a biomarker for synovial sarcoma.Patients and Methods. Microvesicle release of synovial sarcoma cells was examined by transmission electron microscopy. RNA-content was analyzed by qPCR, nested PCR, nested qPCR, and droplet digital PCR to compare their sensitivity for detection of the SYT-SSX fusion gene transcript. Whole blood RNA, RNA of mononuclear cells, and microvesicle RNA of synovial sarcoma patients were analyzed for the presence of the fusion gene transcripts.Results. Electron microscopic analysis revealed synovial sarcoma cells releasing membrane-enclosed microvesicles.In vitro, the SYT-SSX fusion gene transcript was detected in both synovial sarcoma cells and microvesicles. Nested qPCR proved to be the most sensitive in detecting the SYT-SSX fusion gene mRNA. In contrast, the fusion gene transcript was not detected in peripheral blood cells and microvesicles of synovial sarcoma patients.Conclusion. Synovial sarcoma cells release microvesicles harboring the SYT-SSX fusion transcript. Nested qPCR proved to be the most sensitive in detecting the SYT-SSX fusion gene mRNA; however, more sensitive assays are needed to detect cancer-specific microvesicles in the peripheral blood of cancer patients.
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- 2016
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12. Cytotoxic and genotoxic responses of human lung cells to combustion smoke particles of Miscanthus straw, softwood and beech wood chips
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Volker Mersch-Sundermann, Christoph Maschowski, Ali Arif, Tatiana Petithory, Gwenaëlle Trouvé, Polla Azad Khanaqa, Patxi Garra, Alain Dieterlen, Irina Nazarenko, Reto Gieré, Richard Gminski, and Manuel Garcia-Käufer
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Smoke ,Atmospheric Science ,Softwood ,010504 meteorology & atmospheric sciences ,biology ,Waste management ,Chemistry ,Miscanthus ,010501 environmental sciences ,Particulates ,Straw ,biology.organism_classification ,Combustion ,medicine.disease_cause ,01 natural sciences ,Article ,Fly ash ,Environmental chemistry ,medicine ,Genotoxicity ,0105 earth and related environmental sciences ,General Environmental Science - Abstract
Inhalation of particulate matter (PM) from residential biomass combustion is epidemiologically associated with cardiovascular and pulmonary diseases. This study investigates PM0.4-1 emissions from combustion of commercial Miscanthus straw (MS), softwood chips (SWC) and beech wood chips (BWC) in a domestic-scale boiler (40 kW). The PM0.4-1 emitted during combustion of the MS, SWC and BWC were characterized by ICP-MS/OES, XRD, SEM, TEM, and DLS. Cytotoxicity and genotoxicity in human alveolar epithelial A549 and human bronchial epithelial BEAS-2B cells were assessed by the WST-1 assay and the DNA-Alkaline Unwinding Assay (DAUA). PM0.4-1 uptake/translocation in cells was investigated with a new method developed using a confocal reflection microscope. SWC and BWC had a inherently higher residual water content than MS. The PM0.4-1 emitted during combustion of SWC and BWC exhibited higher levels of Polycyclic Aromatic Hydrocarbons (PAHs), a greater variety of mineral species and a higher heavy metal content than PM0.4-1 from MS combustion. Exposure to PM0.4-1 from combustion of SWC and BWC induced cytotoxic and genotoxic effects in human alveolar and bronchial cells, whereby the strongest effect was observed for BWC and was comparable to that caused by diesel PM (SRM 2 975), In contrast, PM0.4-1 from MS combustion did not induce cellular responses in the studied lung cells. A high PAH content in PM emissions seems to be a reliable chemical marker of both combustion efficiency and particle toxicity. Residual biomass water content strongly affects particulate emissions and their toxic potential. Therefore, to minimize the harmful effects of fine PM on health, improvement of combustion efficiency (aiming to reduce the presence of incomplete combustion products bound to PM) and application of fly ash capture technology, as well as use of novel biomass fuels like Miscanthus straw is recommended.
- Published
- 2018
13. Porphyria Cutanea Tarda and Hepatoerythropoietic Porphyria: Identification of 19 Novel Uroporphyrinogen III Decarboxylase Mutations
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Brenden Chen, Karl E. Anderson, Robert J. Desnick, Irina Nazarenko, Makiko Yasuda, and Yedidyah Weiss
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0301 basic medicine ,Male ,Porphyria Cutanea Tarda ,congenital, hereditary, and neonatal diseases and abnormalities ,Endocrinology, Diabetes and Metabolism ,Uroporphyrinogen III decarboxylase ,Heme ,030105 genetics & heredity ,Compound heterozygosity ,Biochemistry ,Article ,03 medical and health sciences ,Genetic Heterogeneity ,0302 clinical medicine ,Endocrinology ,Genetics ,medicine ,Genetic predisposition ,Missense mutation ,Humans ,Uroporphyrinogen Decarboxylase ,Porphyria cutanea tarda ,Family ,Genetic Predisposition to Disease ,Child ,Molecular Biology ,Hemochromatosis ,business.industry ,Hepatoerythropoietic porphyria ,Genetic Carrier Screening ,Porphyria, Hepatoerythropoietic ,medicine.disease ,Porphyria ,Molecular Diagnostic Techniques ,Immunology ,Mutation ,business ,030217 neurology & neurosurgery - Abstract
Porphyria Cutanea Tarda (PCT) is a cutaneous porphyria that results from the hepatic inhibition of the heme biosynthetic enzyme uroporphyrinogen decarboxylase (UROD), and can occur either in the absence or presence of an inherited heterozygous UROD mutation (PCT subtypes 1 and 2, respectively). A heterozygous UROD mutation causes half-normal levels of UROD activity systemically, which is a susceptibility factor but is not sufficient alone to cause type 2 PCT. In both Types 1 and 2 PCT, the cutaneous manifestations are precipitated by additional factors that lead to generation of an inhibitor that more profoundly reduces hepatic UROD activity. PCT is an iron-related disorder, and many of its known susceptibility factors, which include infections (e.g. hepatitis C virus, HIV), high alcohol consumption, smoking, estrogens, and genetic traits (e.g. hemochromatosis mutations) can increase hepatic iron accumulation. Hepatoerythropoietic Porphyria (HEP) is a rare autosomal recessive disease that results from homozygosity or compound heterozygosity for UROD mutations and often causes infantile or childhood onset of both erythropoietic and cutaneous manifestations. During the 11-year period from 01/01/2007 through 12/31/2017, the Mount Sinai Porphyrias Diagnostic Laboratory provided molecular diagnostic testing for 387 unrelated patients with PCT and four unrelated patients with HEP. Of the 387 unrelated individuals tested for Type 2 PCT, 79 (20%) were heterozygous for UROD mutations. Among 26 family members of mutation-positive PCT patients, eight (31%) had the respective family mutation. Additionally, of the four unrelated HEP patients referred for UROD mutation analyses, all had homozygosity or compound heterozygosity for UROD mutations, and all eight asymptomatic family members were heterozygotes for UROD mutations. Of the UROD mutations identified, 19 were novel, including nine missense, two nonsense, one consensus splice-site, and seven insertions and deletions. These results expand the molecular heterogeneity of PCT and HEP by adding a total of 19 novel UROD mutations. Moreover, the results document the usefulness of molecular testing to confirm a genetic susceptibility trait in Type 2 PCT, confirm a diagnosis in HEP, and identify heterozygous family members.
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- 2018
14. Congenital erythropoietic porphyria and erythropoietic protoporphyria: Identification of 7 uroporphyrinogen III synthase and 20 ferrochelatase novel mutations
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Yedidyah Weiss, Manisha Balwani, Irina Nazarenko, Makiko Yasuda, Robert J. Desnick, and Brenden Chen
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0301 basic medicine ,Male ,Protoporphyria, Erythropoietic ,Endocrinology, Diabetes and Metabolism ,Uroporphyrinogen III synthase ,Porphyria, Erythropoietic ,Congenital erythropoietic porphyria ,Heme ,030105 genetics & heredity ,medicine.disease_cause ,Biochemistry ,03 medical and health sciences ,Genetic Heterogeneity ,0302 clinical medicine ,Endocrinology ,Genetics ,medicine ,Humans ,Family ,Photosensitivity Disorders ,Molecular Biology ,Mutation ,biology ,business.industry ,Genetic Carrier Screening ,Ferrochelatase ,medicine.disease ,ALAS2 ,Uroporphyrinogen III Synthetase ,Molecular Diagnostic Techniques ,Erythropoietic porphyria ,Aminolevulinic acid synthase ,biology.protein ,Female ,Erythropoietic protoporphyria ,business ,030217 neurology & neurosurgery - Abstract
The erythropoietic porphyrias are inborn errors of heme biosynthesis with prominent cutaneous manifestations. They include autosomal recessive Congenital Erythropoietic Porphyria (CEP) due to loss-of-function (LOF) mutations in the Uroporphyrinogen III Synthase (UROS) gene, Erythropoietic Protoporphyria (EPP) due to LOF mutations in the ferrochelatase (FECH) gene, and X-Linked Protoporphyria (XLP) due to gain-of-function mutations in the terminal exon of the Aminolevulinic Acid Synthase 2 (ALAS2) gene. During the 11-year period from 01/01/2007 through 12/31/2017, the Mount Sinai Porphyrias Diagnostic Laboratory provided molecular diagnostic testing for one or more of these disorders in 628 individuals, including 413 unrelated individuals. Of these 628, 120 patients were tested for CEP, 483 for EPP, and 331 for XLP, for a total of 934 tests. For CEP, 24 of 78 (31%) unrelated individuals tested had UROS mutations, including seven novel mutations. For EPP, 239 of 362 (66%) unrelated individuals tested had pathogenic FECH mutations, including twenty novel mutations. The IVS3-48 T > C low-expression allele was present in 231 (97%) of 239 mutation-positive EPP probands with a pathogenic FECH mutation. In the remaining 3%, three patients with two different FECH mutations in trans were identified. For XLP, 24 of 250 (10%) unrelated individuals tested had ALAS2 exon 11 mutations. No novel ALAS2 mutations were identified. Among family members referred for testing, 33 of 42 (79%) CEP, 62 of 121 (51%) EPP, and 31 of 81 (38%) XLP family members had the respective family mutation. Mutation-positive CEP, EPP, and XLP patients who had been biochemically tested had marked elevations of the disease-appropriate porphyrin intermediates. These results expand the molecular heterogeneity of the erythropoietic porphyrias by adding a total of 27 novel mutations. The results document the usefulness of molecular testing to confirm the positive biochemical findings in these patients and to identify heterozygous family members.
- Published
- 2018
15. Acute hepatic porphyrias: Identification of 46 hydroxymethylbilane synthase, 11 coproporphyrinogen oxidase, and 20 protoporphyrinogen oxidase novel mutations
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Brenden Chen, Yonina Loskove, Robert J. Desnick, Irina Nazarenko, Neal Cody, and Makiko Yasuda
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0301 basic medicine ,Endocrinology, Diabetes and Metabolism ,Variegate porphyria ,Hydroxymethylbilane Synthase ,Heme ,030105 genetics & heredity ,medicine.disease_cause ,Biochemistry ,03 medical and health sciences ,Coproporphyrinogen Oxidase ,Genetic Heterogeneity ,0302 clinical medicine ,Endocrinology ,Genetics ,medicine ,Humans ,Family ,Protoporphyrinogen Oxidase ,Molecular Biology ,Acute intermittent porphyria ,Mutation ,business.industry ,medicine.disease ,Hereditary coproporphyria ,Porphyria ,Molecular Diagnostic Techniques ,Porphyria, Acute Intermittent ,Asymptomatic Diseases ,Protoporphyrinogen oxidase ,business ,030217 neurology & neurosurgery - Abstract
The acute hepatic porphyrias (AHPs) are inborn errors of heme biosynthesis, which include three autosomal dominant porphyrias, Acute Intermittent Porphyria (AIP), Hereditary Coproporphyria (HCP), and Variegate Porphyria (VP), and the ultra-rare autosomal recessive porphyria, δ-Aminolevulinic Acid Dehydratase Deficiency Porphyria (ADP). AIP, HCP, VP, and ADP each results from loss-of-function (LOF) mutations in their disease-causing genes: hydroxymethylbilane synthase (HMBS); coproporphyrinogen oxidase (CPOX); protoporphyrinogen oxidase (PPOX), and δ-aminolevulinic acid dehydratase (ALAD), respectively. During the 11-year period from January 1, 2007 through December 31, 2017, the Mount Sinai Porphyrias Diagnostic Laboratory diagnosed 315 unrelated AIP individuals with HMBS mutations, including 46 previously unreported mutations, 29 unrelated HCP individuals with CPOX mutations, including 11 previously unreported mutations, and 54 unrelated VP individuals with PPOX mutations, including 20 previously unreported mutations. Overall, of the 1692 unrelated individuals referred for AHP molecular diagnostic testing, 398 (23.5%) had an AHP mutation. Of the 650 family members of mutation-positive individuals tested for an autosomal dominant AHP, 304 (46.8%) had their respective family mutation. These data expand the molecular genetic heterogeneity of the AHPs and document the usefulness of molecular testing to confirm the positive biochemical findings in symptomatic patients and identify at-risk asymptomatic family members.
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- 2018
16. Micro-ribonucleic acids and extracellular vesicles repertoire in the spent culture media is altered in women undergoing In Vitro Fertilization
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Masood Abu-Halima, Sigrun Nestel, Claudia Staib, Andreas Keller, Irina Nazarenko, Tobias Fehlmann, Eckart Meese, Sebastian Häusler, and Christina Backes
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Adult ,0301 basic medicine ,medicine.medical_treatment ,lcsh:Medicine ,Fertilization in Vitro ,Biology ,Real-Time Polymerase Chain Reaction ,Article ,Andrology ,Extracellular Vesicles ,03 medical and health sciences ,Pregnancy ,microRNA ,medicine ,Humans ,Gene Regulatory Networks ,ddc:610 ,lcsh:Science ,Oligonucleotide Array Sequence Analysis ,Regulation of gene expression ,Multidisciplinary ,In vitro fertilisation ,Microarray analysis techniques ,lcsh:R ,fungi ,Embryo ,Embryo Transfer ,Embryo, Mammalian ,medicine.disease ,Embryo transfer ,Culture Media ,MicroRNAs ,030104 developmental biology ,Real-time polymerase chain reaction ,Immunology ,Female ,lcsh:Q - Abstract
MicroRNAs (miRNAs) are class of small RNA molecules with major impact on gene regulation. We analyzed the potential of miRNAs secreted from pre-implantation embryos into the embryonic culture media as biomarkers to predict successful pregnancy. Using microarray analysis, we profiled the miRNome of the 56 spent culture media (SCM) after embryos transfer and found a total of 621 miRNAs in the SCM. On average, we detected 163 miRNAs in SCM of samples with failed pregnancies, but only 149 SCM miRNAs of embryos leading to pregnancies. MiR-634 predicted an embryo transfer leading to a positive pregnancy with an accuracy of 71% and a sensitivity of 85%. Among the 621 miRNAs, 102 (16.4%) showed a differential expression between positive and negative outcome of pregnancy with miR-29c-3p as the most significantly differentially expressed miRNA. The number of extracellular vehicles was lower in SCM with positive outcomes (3.8 × 109/mL EVs), as compared to a negative outcome (7.35 × 109/mL EVs) possibly explaining the reduced number of miRNAs in the SCM associated with failed pregnancies. The analysis of the miRNome in the SCM of couples undergoing fertility treatment lays the ground towards development of biomarkers to predict successful pregnancy and towards understanding the role of embryonic miRNAs found in the SCM.
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- 2017
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17. Extracellular vesicles or free circulating DNA: where to search for BRAF and cKIT mutations?
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Jennifer Klump, Ulrike Phillipp, Hannes Lehmann, Irina Nazarenko, Sigrun Nestel, Marie Follo, Anna Eremin, and Nikolas von Bubnoff
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0301 basic medicine ,Proto-Oncogene Proteins B-raf ,DNA Copy Number Variations ,Mutant ,Biomedical Engineering ,Pharmaceutical Science ,Medicine (miscellaneous) ,Bioengineering ,medicine.disease_cause ,03 medical and health sciences ,chemistry.chemical_compound ,Extracellular Vesicles ,0302 clinical medicine ,Mastocytosis, Systemic ,medicine ,Biomarkers, Tumor ,Humans ,General Materials Science ,Liquid biopsy ,Vemurafenib ,Melanoma ,Mutation ,Wild type ,Imatinib ,medicine.disease ,Molecular biology ,Proto-Oncogene Proteins c-kit ,030104 developmental biology ,chemistry ,030220 oncology & carcinogenesis ,Molecular Medicine ,Cell-Free Nucleic Acids ,DNA ,medicine.drug - Abstract
Clinical evidence in oncology argues for the advantages of performing molecular analysis of blood biomarkers to provide information about systemic changes and tumor heterogeneity. Whereas the diagnostic value of cell-free circulating DNA (fcDNA) has successfully been demonstrated in several studies, DNA enclosed in extracellular vesicles (EV) has only recently been described, and its potential diagnostic value is unclear. We established a protocol for separation of EV and fc fractions and tested for presence of mutant BRAFV600E mediating resistance to Vemurafenib and cKITD816V mediating resistance to Imatinib in blood of patients with melanoma and mastocytosis. Our results show that EV contain significantly higher amounts of total DNA as compared to the fc fraction. However, about ten-fold higher copy numbers of the wild type and mutant BRAF and cKIT were detected in the fcDNA fraction supporting its diagnostic value and pointing to differences in fc and EV DNA content.
- Published
- 2017
18. Frequency of the cholesteryl ester storage disease commonLIPAE8SJM mutation (c.894G>A) in various racial and ethnic groups
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Robert J. Desnick, Suparna Martis, Yao Yang, Irina Nazarenko, Stuart A. Scott, Yumi Kasai, Tommy Hyatt, Benny Liu, Julia Kozlitina, Charina M. Ramirez, and Inga Peter
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Adult ,Heterozygote ,medicine.medical_specialty ,Adolescent ,New York ,Lysosomal acid lipase deficiency ,Gastroenterology ,Article ,White People ,Young Adult ,Internal medicine ,Ethnicity ,Prevalence ,Humans ,Medicine ,Allele ,Allele frequency ,Aged ,Retrospective Studies ,Aged, 80 and over ,Genetics ,Asian ,Cholesterol Ester Storage Disease ,Hepatology ,business.industry ,Exons ,Hispanic or Latino ,Cholesterol ester storage disease ,Enzyme replacement therapy ,Middle Aged ,Sterol Esterase ,medicine.disease ,Confidence interval ,Black or African American ,Sebelipase alfa ,Jews ,Mutation ,business - Abstract
Cholesteryl ester storage disease (CESD) and Wolman disease are autosomal recessive later-onset and severe infantile disorders, respectively, which result from the deficient activity of lysosomal acid lipase (LAL). LAL is encoded by LIPA (10q23.31) and the most common mutation associated with CESD is an exon 8 splice junction mutation (c.894G>A; E8SJM), which expresses only ∼3%-5% of normally spliced LAL. However, the frequency of c.894G>A is unknown in most populations. To estimate the prevalence of CESD in different populations, the frequencies of the c.894G>A mutation were determined in 10,000 LIPA alleles from healthy African-American, Asian, Caucasian, Hispanic, and Ashkenazi Jewish individuals from the greater New York metropolitan area and 6,578 LIPA alleles from African-American, Caucasian, and Hispanic subjects enrolled in the Dallas Heart Study. The combined c.894G>A allele frequencies from the two cohorts ranged from 0.0005 (Asian) to 0.0017 (Caucasian and Hispanic), which translated to carrier frequencies of 1 in 1,000 to ∼1 in 300, respectively. No African-American heterozygotes were detected. Additionally, by surveying the available literature, c.894G>A was estimated to account for 60% (95% confidence interval [CI]: 51%-69%) of reported mutations among multiethnic CESD patients. Using this estimate, the predicted prevalence of CESD in the Caucasian and Hispanic populations is ∼0.8 per 100,000 (∼1 in 130,000; 95% CI: ∼1 in 90,000 to 1 in 170,000). Conclusion: These data indicate that CESD may be underdiagnosed in the general Caucasian and Hispanic populations, which is important since clinical trials of enzyme replacement therapy for LAL deficiency are currently being developed. Moreover, future studies on CESD prevalence in African and Asian populations may require full-gene LIPA sequencing to determine heterozygote frequencies, since c.894G>A is not common in these racial groups. (HEPATOLOGY 2013;53:958–965)
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- 2013
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19. Molecular Expression and Characterization of Erythroid-Specific 5-Aminolevulinate Synthase Gain-of-Function Mutations Causing X-Linked Protoporphyria
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Robert J. Desnick, David F. Bishop, Irina Nazarenko, and Vassili Tchaikovskii
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Male ,Erythrocytes ,Protoporphyria, Erythropoietic ,Mutant ,Biology ,medicine.disease_cause ,chemistry.chemical_compound ,Enzyme Stability ,Genetics ,medicine ,Humans ,Molecular Biology ,Genetics (clinical) ,chemistry.chemical_classification ,Gel electrophoresis ,Mutation ,Temperature ,Genetic Diseases, X-Linked ,Articles ,medicine.disease ,ALAS2 ,Molecular biology ,Amino acid ,Kinetics ,Enzyme ,Biochemistry ,chemistry ,Erythropoietic porphyria ,Molecular Medicine ,Female ,Protoporphyrin ,5-Aminolevulinate Synthetase - Abstract
X-linked protoporphyria (XLP) (MIM 300752) is a recently recognized erythropoietic porphyria due to gain-of-function mutations in the erythroid-specific aminolevulinate synthase gene (ALAS2). Previously, two exon 11 small deletions, c.1699_1670ΔAT (ΔAT) and c.1706_1709ΔAGTG (ΔAGTG), that prematurely truncated or elongated the ALAS2 polypeptide, were reported to increase enzymatic activity 20- to 40-fold, causing the erythroid accumulation of protoporphyrins, cutaneous photosensitivity and liver disease. The mutant ΔAT and ΔAGTG ALAS2 enzymes, two novel mutations, c.1734ΔG (ΔG) and c.1642C>T (p.Q548X), and an engineered deletion c.1670-1671TC>GA p.F557X were expressed, and their purified enzymes were characterized. Wild-type and ΔAGTG enzymes exhibited similar amounts of 54- and 52-kDa polypeptides on sodium dodecyl sulfate–polyacrylamide gel electrophoresis (SDS-PAGE), whereas the ΔAT and p.F557X had only 52-kDa polypeptides. Compared to the purified wild-type enzyme, ΔAT, ΔAGTG and Q548X enzymes had increased specific activities that were only 1.8-, 3.1- and 1.6-fold, respectively. Interestingly, binding studies demonstrated that the increased activity Q548X enzyme did not bind to succinyl-CoA synthetase. The elongated ΔG enzyme had wild-type specific activity, kinetics and thermostability; twice the wild-type purification yield (56 versus 25%); and was primarily a 54-kDa form, suggesting greater stability in vivo. On the basis of studies of mutant enzymes, the maximal gain-of function region spanned 57 amino acids between 533 and 580. Thus, these ALAS2 gain-of-function mutations increased the specific activity (ΔAT, ΔAGTG and p.Q548X) or stability (ΔG) of the enzyme, thereby leading to the increased erythroid protoporphyrin accumulation causing XLP.
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- 2013
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20. Expression of the tetraspanin family members Tspan3, Tspan4, Tspan5 and Tspan7 during Xenopus laevis embryonic development
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Tanja Diana, Irina Nazarenko, Michael Oelgeschläger, and Jubin Kashef
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Transcription, Genetic ,Tetraspanins ,Notochord ,Xenopus ,Embryonic Development ,Ectoderm ,Xenopus Proteins ,Biology ,Evolution, Molecular ,Neural crest ,Xenopus laevis ,Cellular and Molecular Neuroscience ,Cranial neural crest ,Developmental Neuroscience ,Tetraspanin ,Genetics ,medicine ,Animals ,Cell migration ,RNA, Messenger ,Molecular Biology ,Phylogeny ,Cancer ,TSPAN4 ,Tm4sf ,TSPAN7 ,Gene Expression Regulation, Developmental ,Tspans ,Blastula ,biology.organism_classification ,medicine.anatomical_structure ,Somites ,embryonic structures ,Developmental Biology - Abstract
Tetraspanins comprise a large family of integral membrane proteins involved in the regulation of cell adhesion, migration and fusion. In humans it consists of 33 members divided in four subfamilies. Here, we examined the spatial and temporal gene expression of four related tetraspanins during the embryonic development of Xenopus laevis by quantitative real-time PCR and in situ hybridization: Tspan3 (encoded by the gene Tm4sf8 gene) Tspan4 (encoded by the gene Tm4sf7), Tspan5 (encoded by the gene Tm4sf9) and Tspan7 (encoded by the gene Tm4sf2). These genes appeared first in the vertebrates during the evolution and are conserved across different species. In humans, they were associated with several diseases such as sclerosis, mental retardation and cancer; however their physiological role remained unclear. This work provides a comprehensive comparative analysis of the expression of these tetraspanins during the development of X. laevis. The more closely related tetraspanins Tspan3, Tspan4 and Tspan7 exhibited very similar spatial expression patterns, albeit differing in their temporal occurrence. The corresponding transcripts were found in the dorsal animal ectoderm at blastula stage. At early tailbud stages (stage 26) the genes were expressed in the migrating cranial neural crest located in the somites, developing eye, brain, and in otic vesicles. In contrast, Tspan5 appeared first at later stages of development and was detected prominently in the notochord. These data support close relatedness of Tspan3, Tspan4 and Tspan7. The expression of these tetraspanins in the cells with a high migratory potential, e.g. neural crest cells, suggests their role in the regulation of migration processes, characteristic for tetraspanin family members, during development. Similarity of the expression profiles might indicate at least partial functional redundancy, which is in concordance with earlier findings of tissue-limited or absent phenotypes in the knock-down studies of tetraspanins family members performed.
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- 2013
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21. A specific spectral signature of serum and plasma-derived extracellular vesicles for cancer screening
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Wolfgang Schultze-Seemann, Anna Eremin, Sigrun Nestel, Konrad Wilhelm, Juergen Popp, Nikolas von Bubnoff, Christoph Krafft, and Irina Nazarenko
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0301 basic medicine ,Male ,Pathology ,medicine.medical_specialty ,Spectrophotometry, Infrared ,Biomedical Engineering ,Prostatic Hyperplasia ,Pharmaceutical Science ,Medicine (miscellaneous) ,Bioengineering ,Pilot Projects ,Spectrum Analysis, Raman ,Extracellular vesicles ,03 medical and health sciences ,Prostate cancer ,Extracellular Vesicles ,0302 clinical medicine ,Cell-Derived Microparticles ,Cancer screening ,medicine ,Humans ,General Materials Science ,Differential centrifugation ,Plasma derived ,Chemistry ,Prostate ,Cancer ,Prostatic Neoplasms ,medicine.disease ,Microvesicles ,030104 developmental biology ,Tumor progression ,030220 oncology & carcinogenesis ,Cancer research ,Molecular Medicine - Abstract
In cancer, extracellular vesicles (EV) contribute to tumor progression by regulating local and systemic effects. Being released into body fluids, EV may be used in nanomedicine as a valuable source for diagnostic biomarkers. In this work, infrared and Raman spectroscopy were used for comprehensive comparative analysis of cancer versus non-cancer EV and patient screening. Two different EV fractions enriched in exosomes and microvesicles were isolated by differential centrifugation from serum and plasma of cancer and non-cancer patients and from serum and plasma of a healthy donor. The EV fractions were then subjected to drop-coating deposition and drying on calcium fluoride substrates. Reduction of alpha-helix-rich proteins and enhancement of beta-sheet-rich proteins as a cancer-specific blood EV signature was determined, and subsequently this feature was applied for a pilot study aiming to detect prostate cancer in a test cohort of patients with high-grade prostate carcinoma and benign hypoplasia.
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- 2016
22. Extracellular vesicles in ovarian cancer: applications to tumor biology, immunotherapy and biomarker discovery
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Thomas Kislinger, Aneesa Sultan, Giovanni Camussi, Karin M. Ekström, Hadi Valadi, Farah Fatima, Muhammad Nawaz, Mariam Anees, Irina Nazarenko, Luciano Neder, Jeremy A. Squire, and Iram Murtaza
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0301 basic medicine ,Proteomics ,medicine.medical_treatment ,Computational biology ,Biology ,Biochemistry ,03 medical and health sciences ,Extracellular Vesicles ,0302 clinical medicine ,Pancreatic cancer ,medicine ,Biomarkers, Tumor ,Animals ,Humans ,Biomarker discovery ,Molecular Biology ,Ovarian Neoplasms ,Cancer ,Immunotherapy ,medicine.disease ,Microvesicles ,Cell biology ,MicroRNAs ,030104 developmental biology ,030220 oncology & carcinogenesis ,IMUNOTERAPIA ,Biomarker (medicine) ,Female ,Ovarian cancer - Abstract
In recent years there has been tremendous interest in both the basic biology and applications of extracellular vesicles (EVs) in translational cancer research. This includes a better understanding of their biogenesis and mechanisms of selective cargo packaging, their precise roles in horizontal communication, and their application as non-invasive biomarkers. The rapid advances in next-generation omics technologies are the driving forces for these discoveries. In this review, the authors focus on recent results of EV research in ovarian cancer. A deeper understanding of ovarian cancer-derived EVs, the types of cargo molecules and their biological roles in cancer growth, metastases and drug resistance, could have significant impact on the discovery of novel biomarkers and innovative therapeutics. Insights into the role of EVs in immune regulation could lead to novel approaches built on EV-based immunotherapy.
- Published
- 2016
23. Revealing non-genetic adhesive variations in clonal populations by comparative single-cell force spectroscopy
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Heinz Kalt, Ulrich Weiland, Lu Dao, Martin Bastmeyer, Irina Nazarenko, Clemens M. Franz, and Mario Hauser
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Receptor expression ,Cell ,Population ,CHO Cells ,Integrin alpha6 ,Biology ,Microscopy, Atomic Force ,Cricetulus ,Laminin ,Cricetinae ,Cell Adhesion ,medicine ,Animals ,Cell adhesion ,education ,Cells, Cultured ,education.field_of_study ,Cell adhesion molecule ,Cell Cycle ,Force spectroscopy ,Cell Biology ,Adhesion ,Flow Cytometry ,Extracellular Matrix ,Cell biology ,medicine.anatomical_structure ,biology.protein ,Collagen ,Protein Binding - Abstract
Cell populations often display heterogeneous behavior, including cell-to-cell variations in morphology, adhesion and spreading. However, better understanding the significance of such cell variations for the function of the population as a whole requires quantitative single-cell assays. To investigate adhesion variability in a CHO cell population in detail, we measured integrin-mediated adhesion to laminin and collagen, two ubiquitous ECM components, by AFM-based single-cell force spectroscopy (SCFS). CHO cells generally adhered more strongly to laminin than collagen but population adhesion force distributions to both ECM components were broad and partially overlapped. To determine the levels of laminin and collagen binding in individual cells directly, we alternatingly measured single cells on adjacent microstripes of collagen and laminin arrayed on the same adhesion substrate. In repeated measurements (≥60) individual cells showed a stable and ECM type-specific adhesion response. All tested cells bound laminin more strongly, but the scale of laminin over collagen binding varied between cells. Together, this demonstrates that adhesion levels to different ECM components are tightly yet differently set in each cell of the population. Adhesion variability to laminin was non-genetic and cell cycle-independent but scaled with the range of α6 integrin expression on the cell surface. Adhesive cell-to-cell variations due to varying receptor expression levels thus appear to be an inherent feature of cell populations and should to be considered when fully characterizing population adhesion. In this approach, SCFS performed on multifunctional adhesion substrates can provide quantitative single-cell information not obtainable from population-averaging measurements on homogeneous adhesion substrates.
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- 2012
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24. Detection of Human Papillomavirus in Anal Specimens Using the Hybrid Capture 2 Assay
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Szymon Rus, Guorong Chen, Irina Nazarenko, Hiam Salim, Thomas Rothmann, Stephen E. Goldstone, and Brian Lowe
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Adult ,Male ,Pathology ,medicine.medical_specialty ,Anal Canal ,Sensitivity and Specificity ,Specimen Handling ,Pathology and Forensic Medicine ,law.invention ,law ,Cytology ,medicine ,Humans ,DNA Probes, HPV ,Human papillomavirus ,Human Papillomavirus DNA Test ,Prospective cohort study ,Papillomaviridae ,Molecular Biology ,Aged ,business.industry ,Papillomavirus Infections ,Hybrid capture ,Nucleic Acid Hybridization ,Brush ,Anal dysplasia ,Cell Biology ,Middle Aged ,Anus Neoplasms ,medicine.disease ,Dysplasia ,Female ,business ,Precancerous Conditions - Abstract
The hc2 human papillomavirus DNA test (HC2) is effective when screening women for cervical dysplasia, and it might be effective in the screening for anal dysplasia. Differences between the anal and the cervical canals could affect the test performance. This prospective study (n = 292) measured the HC2 signal and in agreement with a histologic endpoint of high- grade dysplasia for anal specimens collected in various ways. Sensitivities were 91%, 85%, and 62% for specimens collected in a sample transport medium and a liquid-based cytology medium processed by Gyn or Non-Gyn protocol, respectively. HC2 sensitivity and specificity to predict high-grade anal dysplasia were similar for brush or swab specimen collections, but HC2 signal was 6 times higher with the brush. Specificity and sensi- tivity were similar whether the sample was collected first or after a cytology sample for brush or swab, but swab specimens at the second collection had an HC2 signal (mean) 48% lower than that of the first collection, and the swab cellularity was lower. The presence of maximum stool decreased the HC2 signal in anal swab specimens. Consensus polymerase chain reaction (PCR) confirmed that the 13 human papillomavirus probe types in HC2 were optimal for performance. HC2 could potentially be further investigated for use in screening anal dysplasia. A larger prospective study is indicated.
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- 2012
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25. A hybrid-capture assay to detect HPV mRNA ratios in cervical specimens
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Anna Fulbright, Irina Nazarenko, and Brian Lowe
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Virulence Factors ,Cervix Uteri ,Cross Reactions ,Biology ,Sensitivity and Specificity ,Cell Line ,HeLa ,Virology ,Gene expression ,medicine ,Humans ,RNA, Messenger ,Papillomaviridae ,Early Detection of Cancer ,Cervical cancer ,Messenger RNA ,virus diseases ,RNA ,Cancer ,medicine.disease ,biology.organism_classification ,Molecular biology ,female genital diseases and pregnancy complications ,In vitro ,Body Fluids ,Molecular Diagnostic Techniques ,Cancer cell ,RNA, Viral ,Female - Abstract
Human papillomavirus (HPV) DNA screening benefits cervical cancer diagnosis, but a few HPV infections result in cancer. Assays that predict cancer are desirable. A potential biomarker is the ratio of HPV E6–7 over E2 transcripts, which may increase during early cancer progression. Modified hybrid-capture technology detected, in separate wells, HPV E6–7 or E2 mRNA of HPV 16 or HPV 18 in samples. The limit of detection was approximately 1000 copies of in vitro transcribed RNA with linear dynamic range approximately four logs. No cross-reactivity between HPV 16 and HPV 18 mRNAs was detected. RNA of SiHa cells was stable in clinical specimen pools for 67 days, as determined by RT-PCR. The ratio of HPV E6–7:E2 mRNAs was relatively high for cancer cells lines, SiHa, Caski and HeLa cells preserved in clinical specimen pools. A broad distribution of HPV 16 E6–7:E2 mRNA ratio was detected in a small set of clinical specimens with various histological diagnoses. Some specimen ratios were so high for cancer cell lines, but the significance of the results needs to be determined. This method may help determine the pattern of gene expression in HPV-related disease or in other systems.
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- 2012
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26. Do all roads lead to Rome? Routes to metastasis development
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Jonathan P. Sleeman, Wilko Thiele, and Irina Nazarenko
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Cancer Research ,Disease ,Biology ,Metastasis ,03 medical and health sciences ,0302 clinical medicine ,Circulating tumor cell ,medicine ,Animals ,Humans ,Neoplasm Metastasis ,Lymph node ,030304 developmental biology ,0303 health sciences ,Metastasis formation ,Cancer ,medicine.disease ,Primary tumor ,3. Good health ,Lymphatic system ,medicine.anatomical_structure ,Oncology ,030220 oncology & carcinogenesis ,Immunology ,Disease Progression ,Cancer research - Abstract
Metastasis, the life-threatening aspect of cancer, is a systemic disease process. Considerable progress has been made in recent years regarding how tumor cells circulating in the blood and lymphatic systems interact with and extravasate into secondary sites, and what determines whether these disseminated tumors cells survive, remain dormant or go on to form macrometastases. New insights into the routes that tumor cells take once leaving the primary tumor have emerged. Novel concepts regarding early seeding of metastases coupled to parallel progression, self-seeding of primary tumors by circulating tumor cells and the induction of premetastatic niches in distant organs by primary tumors have come to the fore. The perceived role of the lymphatic system in determining patterns of metastasis formation in distant organs has been reassessed. Together these new insights have the potential to offer new therapeutic options. In particular, the regulation of tumor cell dormancy emerges as a key event in metastasis formation, and therapeutic control of dormancy holds the promise of rendering cancer a chronic rather than life-threatening disease.
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- 2011
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27. Harderoporphyria due to homozygosity for coproporphyrinogen oxidase missense mutation H327R
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David F. Bishop, Sonia Clavero, Leyla Tümer, Robert J. Desnick, İlyas Okur, Çiğdem Seher Kasapkara, Alev Hasanoglu, Fatih Süheyl Ezgü, Manisha Balwani, Chunli Yu, Alpay Cakmak, and Irina Nazarenko
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Male ,Mutation, Missense ,Biology ,Coproporphyrinogen III ,Article ,Consanguinity ,Coproporphyrinogen Oxidase ,chemistry.chemical_compound ,Coproporphyrins ,Genetics ,medicine ,Humans ,Missense mutation ,Porphyria cutanea tarda ,Genetics (clinical) ,Infant ,Harderoporphyria ,Coproporphyria, Hereditary ,medicine.disease ,Porphyrinogens ,Molecular biology ,Hereditary coproporphyria ,Porphyria ,Amino Acid Substitution ,chemistry - Abstract
Hereditary coproporphyria (HCP) is an autosomal dominant acute hepatic porphyria due to the half-normal activity of the heme biosynthetic enzyme, coproporphyrinogen oxidase (CPOX). The enzyme catalyzes the step-wise oxidative decarboxylation of the heme precursor, coproporphyrinogen III, to protoporphyrinogen IX via a tricarboxylic intermediate, harderoporphyrinogen. In autosomal dominant HCP, the deficient enzymatic activity results primarily in the accumulation of coproporphyrin III. To date, only a few homozygous HCP patients have been described, most having Harderoporphyria, a rare variant due to specific CPOX mutations that alter enzyme residues D400-K404, most patients described to date having at least one K404E allele. Here, we describe a Turkish male infant, the product of a consanguineous union, who presented with the Harderoporphyria phenotype including neonatal hyperbilirubinemia, hemolytic anemia, hepatosplenomegaly, and skin lesions when exposed to UV light. He was homoallelic for the CPOX missense mutation, c.980A > G (p.H327R), and had massively increased urinary uroporphyrins I and III (9,250 and 2,910 mu M, respectively) and coproporphyrins I and III (895 and 19,400 mu M, respectively). The patient expired at 5 months of age from an apparent acute neurologic porphyric attack. Structural studies predicted that p.H327R interacts with residue W399 in the CPOX active site, thereby accounting for the Harderoporphyria phenotype.
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- 2010
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28. An HPV 16, 18, and 45 genotyping test based on Hybrid Capture® technology
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Ha Thai, Sameera Rangwala, Tanya Gay, Kimberly Keating, Sarah McLeod, Irina Nazarenko, Dominic O'Neil, Dana Pfister, and Dirk Loeffert
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Genotype ,Cervix Uteri ,Cross Reactions ,Biology ,Cervical intraepithelial neoplasia ,Sensitivity and Specificity ,Virology ,medicine ,Humans ,Typing ,Papillomaviridae ,Genotyping ,Cervix ,Cervical cancer ,Human papillomavirus 16 ,Human papillomavirus 18 ,Papillomavirus Infections ,Hybrid capture ,Nucleic Acid Hybridization ,medicine.disease ,Infectious Diseases ,medicine.anatomical_structure ,Molecular Diagnostic Techniques ,Specimen transport medium ,DNA, Viral ,Female - Abstract
Background It has been shown that women positive for HPV 16 and HPV 18 have an increased risk of high-grade cervical intraepithelial neoplasia (CIN) compared with women positive for other high-risk (HR) HPV types. In addition, HPV 18 and HPV 45 have been closely linked to aggressive and difficult to detect adenocarcinomas. Objectives To develop a test based on the Hybrid Capture® technology capable of specifically detecting the most important carcinogenic HPV types; 16, 18, and 45. Study design The assay is based on Hybrid Capture technology utilizing a mixture of short type-specific oligoribonucleotides to detect HPV types 16, 18, or 45. The assay utilizes no target amplification and shares workflow and critical reagents with the Digene HC2 HPV screening assay. Studies to evaluate specificity, performance of the test in comparison to HC2, and capability to detect a single genotype in the presence of multiple infections are described. Specificity was evaluated analytically using a panel of HR- and LR-HPV types to illustrate cross-reactivity. Performance in comparison to the HC2 test was evaluated by testing aliquots of the same prepared samples by the genotyping test and HC2. Ability to detect a single genotype during multiple infections was modeled by detecting HPV 16 plasmid in the presence of HPV 6 or HPV 31 at high copy numbers. Results The proposed genotyping assay specifically detects HPV 16, 18, and 45 with an analytical sensitivity of 5,000 copies per assay. The assay is highly specific and does not detect other tested high-risk or low-risk types at 10 8 copies per reaction. Utility of the genotyping test was demonstrated using clinical samples collected in Digene Specimen Transport Medium (STM) and results were confirmed by PCR. Conclusions The target-amplification free assay provides a genotyping method for highly specific detection of HPV 16, 18, and 45 without the complexity of PCR technology.
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- 2009
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29. Tumorigenicity of IL-1α– and IL-1β–Deficient Fibrosarcoma Cells
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Mohini Rajasagi, Elena Voronov, Elena Elter, Eli Reich, Dagmar Hildebrand, Ron N. Apte, Margot Zöller, Mario Vitacolonna, Rachid Marhaba, and Irina Nazarenko
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Cancer Research ,Chemokine ,Matrigel ,Cell growth ,Angiogenesis ,Inflammation ,Biology ,medicine.disease ,lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens ,lcsh:RC254-282 ,Immune system ,Immunology ,medicine ,biology.protein ,Cancer research ,Myeloid-derived Suppressor Cell ,medicine.symptom ,Fibrosarcoma - Abstract
Analyzing the growth of fibrosarcoma lines derived from IL-1alpha-, IL-1beta- , or IL-1alphabeta-knockout (-/-) mice in the immunocompetent host revealed that tumor-derived IL-1alpha and IL-1beta exert strong and opposing effects on immune response induction, which prohibited the evaluation of a potential impact on tumorigenicity. Therefore, in vivo growth of IL-1-deficient tumor lines was evaluated in nu/nu mice and was compared with in vitro growth characteristics. All IL-1-deficient fibrosarcoma lines grow in immunocompromised mice. However, IL-1alpha(-/-)beta-competent (comp) lines grow more aggressively, efficiently induce angiogenesis, and recruit inflammatory cells. Despite stronger tumorigenicity of IL-1beta(comp) lines, IL-1alpha strengthens anchorage-independent growth, but both IL-1alpha and IL-1beta support drug resistance. Corresponding to the aggressive growth, IL-1beta(comp) cells display increased matrix adhesion, motility, and cable formation on matrigel, likely supported by elevated alpha(v)/beta3 and matrix metalloroteinase expression. Recruitment of myeloid cells requires IL-1beta but is regulated by IL-1alpha, because inflammatory chemokine and cytokine expression is stronger in IL-1alpha(-/-)beta(comp) than in IL-1(wt) lines. This regulatory effect of tumor-derived IL-1alpha is restricted to the tumor environment and does not affect systemic inflammatory response induction by tumor-derived IL-1beta. Both sarcoma cell-derived IL-1alpha and IL-1beta promote tumor growth. However, IL-1alpha exerts regulatory activity on the tumor cell-matrix cross-talk, and only IL-1beta initiates systemic inflammation.
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- 2008
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30. Opposing effects of fibrosarcoma cell-derived IL-1α and IL-1β on immune response induction
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Daniela Knöfler, Irina Nazarenko, Elena Elter, Eli Reich, Ron N. Apte, Mario Vitacolonna, Rachid Marhaba, Margot Zöller, Elena Voronov, and Dagmar Hildebrand
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Cancer Research ,Regulatory T cell ,Fibrosarcoma ,Interleukin-1beta ,Mice, Nude ,Alpha (ethology) ,Biology ,Immune tolerance ,Mice ,Immune system ,Interleukin-1alpha ,Immune Tolerance ,Tumor Cells, Cultured ,medicine ,Animals ,T helper cell ,Flow Cytometry ,medicine.disease ,Specific Pathogen-Free Organisms ,Mice, Inbred C57BL ,CTL ,medicine.anatomical_structure ,Oncology ,Immunology ,Myeloid-derived Suppressor Cell ,Cancer research ,Methylcholanthrene ,T-Lymphocytes, Cytotoxic - Abstract
There is evidence that cell-associated IL-1 alpha supports immune response induction. Here we explored the impact of malignant cell-derived IL-1 on immunogenicity, immune response induction and tumor-induced immunosuppression using 3-methylcholanthrene-induced fibrosarcoma lines derived from wild-type (wt), IL-1 alpha-, IL-1 beta- or IL-1a beta-knockout (IL-1 alpha(-/-), IL-1 beta(-/-), IL-1 alphabeta(-/-)) C57BL6 mice. The wt, IL-1 alpha(-/-), IL-1 beta(-/-) and IL-1 alphabeta(-/-) fibrosarcoma lines express MHC class I molecules at a high level. The lines do not differ in their susceptibility toward NK cells, macrophages, and allogeneic CTL, or in their capacity as stimulators of an allogeneic response. However, IL-1 beta(-/-) tumors rarely grow in the syngeneic host, which is the consequence of a strong T helper and CTL response induction by IL-1 alpha-competent, IL-1 beta(-/-) tumors. On the other hand, IL-1 beta-competent, IL-1 alpha(-/-) tumors strongly assist CD11b(+)Gr-1(+) myeloid-derived suppressor cell and regulatory T cell expansion, which both suppress with high efficacy activated T helper cell proliferation and CTL lysis. In IL-1 alphabeta(-/-) tumors, the absence of IL-1 alpha becomes decisive, i.e. despite reduced suppressor cell recruitment, tumor growth was unimpaired due to inefficient immune response induction. Thus, sarcoma cell-derived IL-1 alpha and IL-1 beta do not act in concert. Induction of a strong immune response by IL-1 alpha demands therapeutic exploitation, which may become more efficient if systemic induction of immunosuppression by IL-1 beta can also be circumvented.
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- 2008
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31. Impact of α1-adrenoceptor expression on contractile properties of vascular smooth muscle cells
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Irina Nazarenko, Peter Martinka, Adrian Gericke, Pontus B. Persson, and Andreas Patzak
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Male ,medicine.medical_specialty ,Sympathetic nervous system ,Vascular smooth muscle ,Physiology ,Genetic Vectors ,Hemodynamics ,Cell Separation ,In Vitro Techniques ,Transfection ,Muscle, Smooth, Vascular ,Rats, Sprague-Dawley ,Phenylephrine ,Receptors, Adrenergic, alpha-1 ,Physiology (medical) ,Internal medicine ,medicine ,Animals ,Antibodies, Blocking ,Adrenergic alpha-Antagonists ,Microscopy, Confocal ,Chemistry ,Immunohistochemistry ,Rats ,Mayer waves ,medicine.anatomical_structure ,Endocrinology ,Circulatory system ,medicine.symptom ,Adrenergic alpha-Agonists ,Muscle Contraction ,Muscle contraction ,Blood vessel ,Artery - Abstract
Low-frequency blood pressure oscillations (Mayer waves) are discussed as a marker for sympathetic modulation of vascular tone. However, the factors that determine the frequency response of the vasculature to sympathetic stimuli are not fully understood. Possible mechanisms include functions related to α1-adrenergic receptors (α1-AR) and postreceptor processes involved in the vascular contractile response. The purpose of the present study was to examine the hypothesis that expression levels of α1-AR and their subtype distribution determine velocity and magnitude of α1-AR-mediated vascular smooth muscle cell (VSMC) contraction. α1A-, α1B-, and α1D-AR subtypes were transfected into VSMCs from rat aorta and characterized immunocytochemically via confocal microscopy. Functional studies in isolated cells were performed using video microscopy. The α1-AR agonist phenylephrine produced dose-dependent contractions of VSMCs. All transfected groups were more sensitive to phenylephrine compared with controls. Maximal contraction velocity almost doubled in transfected cells. However, no differences in observed parameters were found between the three transfected groups. Contractile properties in response to membrane depolarization with KCl were similar in all groups. In conclusion, α1-AR density determines velocity and sensitivity of α1-AR-mediated contraction in VSMCs. α1-AR subtype distribution does not appear to influence vasoconstriction to sympathetic stimuli.
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- 2007
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32. H-REV107-1 Stimulates Growth in Non-Small Cell Lung Carcinomas via the Activation of Mitogenic Signaling
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Christine Sers, Glen Kristiansen, Cornelia Gieseler, Wolfgang Kemmner, Irina Nazarenko, Sabine Fonfara, Raphaela Guenther, Iver Petersen, and Reinhold Schäfer
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Transcriptional Activation ,Pathology ,medicine.medical_specialty ,Lung Neoplasms ,Tumor suppressor gene ,Cell ,Biology ,Pathology and Forensic Medicine ,Carcinoma, Non-Small-Cell Lung ,Tumor Cells, Cultured ,medicine ,Humans ,RNA, Small Interfering ,Lung cancer ,Mitogen-Activated Protein Kinase 3 ,Tumor Suppressor Proteins ,Intracellular Signaling Peptides and Proteins ,Intracellular Membranes ,Prognosis ,medicine.disease ,Immunohistochemistry ,Enzyme Activation ,medicine.anatomical_structure ,Cytoplasm ,Tumor progression ,Cell culture ,Phospholipases A2, Calcium-Independent ,ras Proteins ,Cancer research ,Phosphorylation ,Signal transduction ,Signal Transduction ,Regular Articles - Abstract
H-REV107-1, a known member of the class II tumor suppressor gene family, is involved in the regulation of differentiation and survival. We analyzed H-REV107-1 in non-small cell lung carcinomas, in normal lung, and in immortalized and tumor-derived cell lines. Sixty-eight percent of lung tumors revealed positive H-REV107-1-specific staining. Furthermore, survival analysis demonstrated a significant association of cytoplasmic H-REV107-1 with decreased patient survival. This suggested that H-REV107-1, known as a tumor suppressor, plays a different role in non-small cell lung carcinomas. Knock-down of H-REV107-1 expression in lung carcinoma cells inhibited anchorage-dependent and anchorage-independent growth whereas overexpression of H-REV107-1 induced tumor cell proliferation. Consistent with results of the survival analysis, cytoplasmic localization of the protein was essential for this growth-inducing function. Analysis of signaling pathways potentially involved in this process demonstrated that overexpression of H-REV107-1 stimulated RAS-GTPase activity, ERK1,2 phosphorylation, and caveolin-1 expression in the cell lines analyzed. These results indicate that H-REV107-1 is deficient in its function as a tumor suppressor in non-small cell lung carcinomas and is required for proliferation and anchorage-independent growth in cells expressing high levels of the protein, thus contributing to tumor progression in a subset of non-small cell lung carcinomas.
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- 2006
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33. The class II tumour suppressor gene H-REV107-1 is a target of interferon-regulatory factor-1 and is involved in IFNγ-induced cell death in human ovarian carcinoma cells
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Knut Husmann, Christine Sers, Irina Nazarenko, Artur Gontarewicz, Kai Wiechen, Steffen Reich, Punam Adhikari, Katharina Schröder, Bakhyt Zhumabayeva, and Reinhold Schäfer
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Cancer Research ,Programmed cell death ,medicine.medical_specialty ,Down-Regulation ,Ovary ,Biology ,3T3 cells ,Interferon-gamma ,Mice ,Interferon ,Ovarian carcinoma ,Internal medicine ,Tumor Cells, Cultured ,Genetics ,medicine ,Animals ,Humans ,Genes, Tumor Suppressor ,Interferon gamma ,Molecular Biology ,Ovarian Neoplasms ,Cell Death ,Tumor Suppressor Proteins ,Intracellular Signaling Peptides and Proteins ,Proteins ,3T3 Cells ,Phosphoproteins ,Epithelium ,Rats ,DNA-Binding Proteins ,Gene Expression Regulation, Neoplastic ,medicine.anatomical_structure ,Endocrinology ,Cell culture ,Phospholipases A2, Calcium-Independent ,Cancer research ,Female ,Interferon Regulatory Factor-1 ,medicine.drug - Abstract
H-rev107-1 is a growth inhibitory RAS target gene capable of suppressing anchorage independent growth in vitro and in vivo. Using a tumour tissue array with 241 matched tumour and normal tissue cDNA pools, we found down-regulation of H-REV107-1 in 7 out of 14 ovary-derived cDNAs. RT-PCR analysis and immunohistochemical investigation confirmed expression of H-REV107-1 in normal ovarian epithelial cells but down-regulation in high grade ovarian carcinomas. H-REV107-1 is also strongly expressed in immortalized rat and human ovarian epithelial cells in vitro, but suppressed in transformed cells by two different mechanisms. KRAS-transformed rat ovarian cells and PA1 teratocarcinoma cells, reversibly repress H-REV107-1 via MAP/ERK signaling. In contrast, treatment of A27/80 and OVCAR-3 epithelial ovarian cancer cells with IFNgamma stimulated H-REV107-1 expression. In NIH3T3 cells harbouring an estrogen-inducible IRF-1, H-rev107-1 is directly induced after activation of IRF-1, indicating that H-rev107-1 is a target of IRF-1. Stimulation of H-REV107-1 expression was also observed in ovarian epithelial cells suggesting that IRF-1 is involved in H-REV107-1 regulation in human ovarian epithelium. In the IFNgamma-sensitive cell line A27/80, H-REV107-1 suppresses colony formation. A27/80 and OVCAR-3 cells overexpressing H-REV107-1 protein underwent apoptosis. These results demonstrate down-regulation of the class II tumour suppressor H-REV107-1 in human ovarian carcinomas and suggest an involvement of H-REV107-1 in interferon-dependent cell death.
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- 2002
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34. Distribution of Human papillomavirus load in clinical specimens
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Dominic O'neil, Dirk Loeffert, Brian Lowe, and Irina Nazarenko
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Pathology ,medicine.medical_specialty ,Clinical tests ,Serial dilution ,Papillomavirus Infections ,Statistics as Topic ,Viral Load ,Biology ,Severity of Illness Index ,Virology ,Virus ,Molecular Diagnostic Techniques ,Disease severity ,Cytology ,medicine ,Humans ,Distribution (pharmacology) ,Reagent Kits, Diagnostic ,Human papillomavirus ,Papillomaviridae ,Viral load ,Biomarkers - Abstract
The information about the range and distribution of Human papillomavirus load in clinical specimens is important for the design of accurate clinical tests. The amount of Human papillomavirus in cervical specimens was estimated using the digene HC2 HPV DNA Test® (QIAGEN). This semi-quantitative assay is based on linear signal amplification with an analytical limit-of-detection of approximately 2500 virus copies per assay and 3–4 log dynamic range. The dynamic range of the assay was extended by a serial dilution strategy. Two large sets of positive specimens (n = 501 and 569) were analyzed and 9–11% of specimens was estimated to contain more than 7 × 107 copies of virus. The viral load was also assessed for an assortment of specimens with known cytology diagnoses (n = 9435) and histological diagnoses (n = 2056). The percentage of specimens with more than 7 × 107 copies of virus was estimated to be 0.89 for normal cells, 4.2 for atypical cells (unknown significance), 14.31 for cells of low-grade lesions and 22.24 for cells of high-grade lesions. The viral load increased with disease severity, but its broad distribution may not support its use as a disease biomarker. This information is important for assay design and automation, where cross-reactivity and sample-to-sample contamination must be addressed rigorously.
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- 2011
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35. The emerging role of extracellular vesicles as biomarkers for urogenital cancers
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Giovanni Camussi, Naeem Mahmood Ashraf, Luciano Neder, Farah Fatima, Simona Principe, Hadi Valadi, Xiaoqin Wang, Muhammad Nawaz, Neelam Shah, Thomas Kislinger, Irina Nazarenko, and Karin M. Ekström
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Male ,Proteomics ,Pathology ,medicine.medical_specialty ,Urology ,APOPTOSE ,Exosomes ,Extracellular vesicles ,Prostate ,Cell-Derived Microparticles ,Semen ,Urological cancer ,Biomarkers, Tumor ,Medicine ,Humans ,Carcinoma, Renal Cell ,Kidney ,business.industry ,Secretory Vesicles ,Urogenital Cancers ,Prostatic Neoplasms ,Genomics ,Kidney Neoplasms ,medicine.anatomical_structure ,Urinary Bladder Neoplasms ,Cancer research ,Cancer biomarkers ,business ,Intracellular ,Biogenesis - Abstract
The knowledge gained from comprehensive profiling projects that aim to define the complex genomic alterations present within cancers will undoubtedly improve our ability to detect and treat those diseases, but the influence of these resources on our understanding of basic cancer biology is still to be demonstrated. Extracellular vesicles have gained considerable attention in past years, both as mediators of intercellular signalling and as potential sources for the discovery of novel cancer biomarkers. In general, research on extracellular vesicles investigates either the basic mechanism of vesicle formation and cargo incorporation, or the isolation of vesicles from available body fluids for biomarker discovery. A deeper understanding of the cargo molecules present in extracellular vesicles obtained from patients with urogenital cancers, through high-throughput proteomics or genomics approaches, will aid in the identification of novel diagnostic and prognostic biomarkers, and can potentially lead to the discovery of new therapeutic targets.
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- 2014
36. Focal facial dermal dysplasia, type IV, is caused by mutations in CYP26C1
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Pavni Mehrotra, Richard Lao, Trine Prescott, Robert J. Desnick, Ben Li, Ann L. Marqueling, Thomas M Glaser, Don Cameron, Catherine Chu, Chris Chou, Anne Slavotinek, Irina Nazarenko, Marie Anne Morren, Martin Petkovich, Kelly M. Cordoro, Pui-Yan Kwok, Paul Ling-Fung Tang, Ilona J. Frieden, Mani Yahyavi, and Koen Devriendt
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Ectodermal dysplasia ,Focal facial dermal dysplasia ,DNA Mutational Analysis ,Mutation, Missense ,Biology ,medicine.disease_cause ,Medical and Health Sciences ,Frameshift mutation ,Mice ,Congenital ,Cytochrome P-450 Enzyme System ,Ectodermal Dysplasia ,Clinical Research ,Gene duplication ,Chlorocebus aethiops ,medicine ,Genetics ,Missense mutation ,Animals ,Humans ,2.1 Biological and endogenous factors ,Aetiology ,Frameshift Mutation ,Molecular Biology ,Gene ,Genetics (clinical) ,Exome sequencing ,Genetic Association Studies ,Cytochrome P450 Family 26 ,Pediatric ,Genetics & Heredity ,Mutation ,Focal Facial Dermal Dysplasias ,General Medicine ,Articles ,Biological Sciences ,medicine.disease ,COS Cells ,Congenital Structural Anomalies ,Missense ,Microsatellite Repeats ,Biotechnology - Abstract
Focal facial dermal dysplasia (FFDD) Type IV is a rare syndrome characterized by facial lesions resembling aplasia cutis in a preauricular distribution along the line of fusion of the maxillary and mandibular prominences. To identify the causative gene(s), exome sequencing was performed in a family with two affected siblings. Assuming autosomal recessive inheritance, two novel sequence variants were identified in both siblings in CYP26C1-a duplication of seven base pairs, which was maternally inherited, c.844_851dupCCATGCA, predicting p.Glu284fsX128 and a missense mutation, c.1433G>A, predicting p.Arg478His, that was paternally inherited. The duplication predicted a frameshift mutation that led to a premature stop codon and premature chain termination, whereas the missense mutation was not functional based on its in vitro expression in mammalian cells. The FFDD skin lesions arise along the sites of fusion of the maxillary and mandibular prominences early in facial development, and Cyp26c1 was expressed exactly along the fusion line for these facial prominences in the first branchial arch in mice. Sequencing of four additional, unrelated Type IV FFDD patients and eight Type II or III TWIST2-negative FFDD patients revealed that three of the Type IV patients were homozygous for the duplication, whereas none of the Type II or III patients had CYP26C1 mutations. The seven base pairs duplication was present in 0.3% of healthy controls and 0.3% of patients with other birth defects. These findings suggest that the phenotypic manifestations of FFDD Type IV can be non-penetrant or underascertained. Thus, FFDD Type IV results from the loss of function mutations in CYP26C1.
- Published
- 2013
37. Loss-of-Function Ferrochelatase and Gain-of-Function Erythroid-Specific 5-Aminolevulinate Synthase Mutations Causing Erythropoietic Protoporphyria and X-Linked Protoporphyria in North American Patients Reveal Novel Mutations and a High Prevalence of X-Linked Protoporphyria
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D. Montgomery Bissell, Robert J. Desnick, Manisha Balwani, Makiko Yasuda, Lawrence Liu, Herbert L. Bonkovsky, Irina Nazarenko, John D. Phillips, Joseph R. Bloomer, David F. Bishop, Harry A. Dailey, Karl E. Anderson, and Dana Doheny
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Male ,Genotype ,Biology ,medicine.disease_cause ,Genetics ,medicine ,Prevalence ,Humans ,Allele ,Molecular Biology ,Genetics (clinical) ,Mutation ,Heterozygote advantage ,Genetic Diseases, X-Linked ,Articles ,Ferrochelatase ,medicine.disease ,Molecular biology ,ALAS2 ,Phenotype ,Porphyrias, Hepatic ,North America ,biology.protein ,Molecular Medicine ,Female ,Erythropoietic protoporphyria ,5-Aminolevulinate Synthetase - Abstract
Erythropoietic protoporphyria (EPP) and X-linked protoporphyria (XLP) are inborn errors of heme biosynthesis with the same phenotype but resulting from autosomal recessive loss-of-function mutations in the ferrochelatase (FECH) gene and gain-of-function mutations in the X-linked erythroid-specific 5-aminolevulinate synthase (ALAS2) gene, respectively. The EPP phenotype is characterized by acute, painful, cutaneous photosensitivity and elevated erythrocyte protoporphyrin levels. We report the FECH and ALAS2 mutations in 155 unrelated North American patients with the EPP phenotype. FECH sequencing and dosage analyses identified 140 patients with EPP: 134 with one loss-of-function allele and the common IVS3-48T>C low expression allele, three with two loss-of-function mutations and three with one loss-of-function mutation and two low expression alleles. There were 48 previously reported and 23 novel FECH mutations. The remaining 15 probands had ALAS2 gain-of-function mutations causing XLP: 13 with the previously reported deletion, c.1706_1709delAGTG, and two with novel mutations, c.1734delG and c.1642C>T(p.Q548X). Notably, XLP represented ~10% of EPP phenotype patients in North America, two to five times more than in Western Europe. XLP males had twofold higher erythrocyte protoporphyrin levels than EPP patients, predisposing to more severe photosensitivity and liver disease. Identification of XLP patients permits accurate diagnosis and counseling of at-risk relatives and asymptomatic heterozygotes.
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- 2013
38. Exosomes as a Potential Tool for a Specific Delivery of Functional Molecules
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Irina Nazarenko, Peter Altevogt, and Anne-Kathleen Rupp
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Cell membrane ,medicine.anatomical_structure ,Cell culture ,Endosome ,Chemistry ,Vesicle ,Cancer cell ,Extracellular ,medicine ,Molecular biology ,In vitro ,Microvesicles - Abstract
Extracellular membrane vesicles derived from the endosomal compartments and released by the fusion of the multivesicular bodies with the cell membrane are referred as exosomes (Exo) [Van Niel et al., J Biochem 140:13-21, 2006]. They function as mediators of intercellular communication and are employed by the organism in the regulation of systemic and local processes. Meantime, Exo are recognized as an indispensable entity of physiological fluids [Caby et al., Int Immunol 17:879-887, 2005; Lasser et al., J Transl Med 9:9, 2011; Lasser et al., Am J Rhinol Allergy 25:89-93, 2011]. Exo and other types of extracellular vesicles, e.g., exosome-like vesicles [van Niel et al., Gastroenterology 121:337-349, 2001] and microvesicles (MV) [Daveloose et al., Thromb Res 22:195-201, 1981], contain multiple functional molecules including lipids [Vidal et al., J Cell Physiol 140:455-462, 1989]; proteins [Simpson et al., Expert Rev Proteomics 6:267-283, 2009]; mRNA [Valadi et al., Nat Cell Biol 9:654-659, 2007]; DNA [Waldenstrom et al., PLoS One 7:e34653, 2012]; noncoding RNA, e.g., miRNA [Simpson et al., Expert Rev Proteomics 6:267-283, 2009]; and retrotransposon elements [Balaj et al., Nat Commun 2:180, 2011]. Assessment of the biological functions of Exo showed that they deliver specifically their cargo from the donor to recipient cells. Albeit the molecular mechanisms of this process are not fully understood, approaches for the application of Exo and MV as a tool for a cell-specific delivery of signalling molecules were successfully tested in in vitro and in vivo models [Maguire et al., Mol Ther 20:960-971, 2012]. Ovarian cancer cells release Exo, which bind stroma cells as well as donor cancer cells [Escrevente et al., BMC Cancer 11:108, 2011]. Here we describe an experimental approach for the assessment of Exo interaction and uptake by target cells. Methods for the isolation and purification of Exo from cell culture supernatants are included. To allow visualization of vesicle uptake, labelling of Exo with different fluorescent dyes, such as CFSE, PKH, DHPE, and DiOC18, is presented. Finally, we explain qualitative and quantitative analysis of Exo uptake by immunofluorescence and flow cytometry, respectively.
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- 2013
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39. Apoptosis Pathways in Ovarian Cancer
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Irina Nazarenko, Christine Sers, and Reinhold Schäfer
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MAPK/ERK pathway ,Oncology ,Life sciences ,biology ,medicine.medical_specialty ,Kinase ,Cell ,Biology ,medicine.disease ,medicine.anatomical_structure ,Internal medicine ,ddc:570 ,Cancer research ,medicine ,Protein kinase A ,Ovarian cancer ,Protein kinase B ,Protein kinase C ,PI3K/AKT/mTOR pathway - Abstract
Tumour initiation and progression are driven by constitutively activated oncogenes mediating deregulation of the balance between cell deathand survival pathways. Among the most relevant signalling cascades activated in the majority of tumour types, the RAS/mitogen-activated protein kinase (Ras/MAPK), the phosphatidyl inositol-3kinase/protein kinase B (PI3K/PKB) and the protein kinases C (PKC) signalling cascades were postulated (Weinstein, 1987; Nicosia et al., 2003; Roberts and Der, 2007; McCubrey et al., 2007; Breitkreutz et al., 2007). These cascades define individual characteristics of particular tumours and consequently their individual responsiveness to cancer therapy. In this chapter, we will address the characteristics of the apoptotic signalling pathways in ovarian carcinomas. Particular attention will be given to the HRS family of tumour suppressor genes encoding proteins with phospholipase activity and suppressed in the majority of ovarian malignancies. We will describe signalling cascades down regulating two well-characterized members of this family H-REV107-1/HRLS3/PLA2G16 and TIG3/RARRES/RIG1 in tumour cells. Furthermore, potential therapeutic consequences of the re-expression of these genes defined as a class II tumour suppressors will be discussed.
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- 2012
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40. Evaluation of Chlamydia trachomatis and Neisseria gonorrhoeae Detection in Urine, Endocervical, and Vaginal Specimens by a Multiplexed Isothermal Thermophilic Helicase-Dependent Amplification (tHDA) Assay ▿
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Thomas Rothmann, Dominic O'neil, Irina Nazarenko, John Wolff, and Victoria Doseeva
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Microbiology (medical) ,DNA, Bacterial ,Male ,Loop-mediated isothermal amplification ,Chlamydia trachomatis ,Urine ,Cervix Uteri ,Biology ,medicine.disease_cause ,Microbiology ,Gonorrhea ,Plasmid ,medicine ,Humans ,Sample preparation ,Helicase-dependent amplification ,Bacteriological Techniques ,Thermophile ,Bacteriology ,Neisseria gonorrhoeae ,Molecular Diagnostic Techniques ,Lymphogranuloma Venereum ,Vagina ,Female ,Nucleic Acid Amplification Techniques ,Bacterial Outer Membrane Proteins ,Plasmids - Abstract
We have developed a new research assay that combines sequence-specific sample preparation and isothermal amplification for the detection of Chlamydia trachomatis and Neisseria gonorrhoeae infections. The assay targets both the omp gene and the cryptic plasmid of C. trachomatis and the multicopy opa gene of N. gonorrhoeae , which are amplified and detected in a single reaction. We evaluated the ability of the assay to detect C. trachomatis and N. gonorrhoeae infections in first-catch urine, swab, and liquid-based cytology samples. Total agreement between the new assay and APTIMA Combo 2 varied between 95.3% and 100%, depending on the sample type and target detected. Total agreement between the new assay and BD ProbeTec varied between 96.7% and 100%, depending on the sample type and target detected. The assay has a simple work flow, and endpoint results can be achieved in 3 h, including sample preparation. The assay described here was evaluated for research use and was compared to commercially available assays.
- Published
- 2011
41. Setleis syndrome in Mexican-Nahua sibs due to a homozygous TWIST2 frameshift mutation and partial expression in heterozygotes: review of the focal facial dermal dysplasias and subtype reclassification
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Carola Durán-McKinster, Camilo E. Villarroel, Irina Nazarenko, Robert J. Desnick, Vanessa Bosch-Canto, Victoria del-Castillo, David E. Cervantes-Barragán, Amy Yang, and Alma Medrano-Hernández
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Male ,Heterozygote ,Distichiasis ,Nonsense mutation ,Biology ,Skin Diseases ,Frameshift mutation ,Ectodermal Dysplasia ,Genetics ,medicine ,Humans ,Facial development ,Child ,Frameshift Mutation ,Mexico ,Genetics (clinical) ,Eyelashes ,Setleis syndrome ,Autosomal recessive inheritance ,Siblings ,Twist-Related Protein 1 ,Focal Facial Dermal Dysplasias ,Infant ,Heterozygote advantage ,medicine.disease ,Phenotype ,Pedigree ,Focal Dermal Hypoplasia ,Repressor Proteins ,Face ,Indians, North American ,Female - Abstract
Background The focal facial dermal dysplasias (FFDDs) are a group of inherited disorders of facial development, characterised by bitemporal or preauricular scar-like defects, the former resembling ‘forceps marks’. Recently, different homozygous TWIST2 nonsense mutations were reported in unrelated Setleis syndrome (FFDD Type III) patients from consanguineous families, consistent with autosomal recessive inheritance. Mexican-Nahua sibs with facial and ophthalmologic features of FFDD type III were evaluated. Methods Genomic DNAs were isolated for sequencing of the TWIST2 gene. The clinical features and inheritance of all previously reported FFDD patients were reviewed. Results The affected sibs were homozygous for a novel TWIST2 frameshift mutation, c.168delC (p.S57AfsX45). Notably, both parents and two heterozygous sibs had distichiasis and partial absence of lower eyelashes. The FFDD subtypes were reclassified: the ‘Brauer-Setleis’ phenotype (autosomal dominant with variable expressivity) as FFDD type II; and patients with preauricular lesions as a new subtype, FFDD type IV. Conclusions FFDD type III heterozygotes with TWIST2 mutations may have syndromic manifestations. Review of previous FFDD patients resulted in reclassification of the subtypes.
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- 2011
42. Evaluation of the hybrid capture 2 assay for detecting anal high-grade dysplasia
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Thomas Rothmann, Stephen E. Goldstone, Brian Lowe, and Irina Nazarenko
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Adult ,Male ,Cancer Research ,Pathology ,medicine.medical_specialty ,Sensitivity and Specificity ,Young Adult ,Cytology ,Biopsy ,HIV Seropositivity ,Medicine ,Anal cancer ,Humans ,Cervix ,Aged ,Anus Diseases ,medicine.diagnostic_test ,business.industry ,Papillomavirus Infections ,Anoscopy ,Anal dysplasia ,Middle Aged ,medicine.disease ,Squamous intraepithelial lesion ,medicine.anatomical_structure ,Oncology ,Dysplasia ,Female ,Reagent Kits, Diagnostic ,business - Abstract
Hybrid Capture 2 (HC2) Human Papillomavirus (HPV) DNA Test® is FDA approved and is a proven aid in detecting HPV infections of the cervix and as an aid in diagnosing, with cytology, cervical disease. A prospective feasibility study was conducted to determine if HC2 testing has utility when screening for high-grade anal dysplasia (AIN2+). We enrolled 298 patients (45% HIV+) who had AIN2+ screening with cytology, histology and HC2 testing for two specimens: a swab into liquid-based cytology medium and either a swab or a brush collection in specimen transport medium (STM). High-resolution anoscopy was performed on all patients with biopsy of AIN2+ suspicious lesions. Cytology was benign (42%), atypical squamous cells of undetermined significance (30%), low-grade squamous intraepithelial lesion (18%), high-grade squamous intraepithelial lesion (1%), ASCUS possibly high-grade dysplasia (1.7%) and nondiagnostic (7%) and 36% had AIN2+ histology. Sensitivity and specificity for predicting AIN2+ histology for any abnormal cytology were 77 and 52%, whereas HC2 sensitivity and specificity were 91 and 40% (p = 0.005 for sensitivity), respectively. There was no significant difference in HC2 sensitivity or specificity between brush and swab or STM and residual cells from cytology. AIN2+ was found in 20% of patients with benign cytology. Only nine AIN2+ specimens were HC2−. This prospective study indicates that HC2 may be useful when screening for anal dysplasia; however, a larger study is recommended.
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- 2011
43. Multiplex isothermal helicase-dependent amplification assay for detection of Chlamydia trachomatis and Neisseria gonorrhoeae
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Dominic O'neil, Thomas Rothmann, Thomas Forbes, Irina Nazarenko, John Wolff, Yuri Khripin, and Victoria Doseeva
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Microbiology (medical) ,Point-of-Care Systems ,Chlamydia trachomatis ,medicine.disease_cause ,Sensitivity and Specificity ,chemistry.chemical_compound ,Gonorrhea ,medicine ,Humans ,Multiplex ,Sample preparation ,Helicase-dependent amplification ,Bacteriological Techniques ,biology ,DNA Helicases ,Helicase ,General Medicine ,Chlamydia Infections ,Molecular biology ,Microspheres ,Neisseria gonorrhoeae ,Infectious Diseases ,chemistry ,Molecular Diagnostic Techniques ,biology.protein ,Nucleic acid ,Oligonucleotide Probes ,Nucleic Acid Amplification Techniques ,DNA - Abstract
Thermophilic helicase dependent amplification (tHDA), which employs helicase to unwind double-stranded DNA at constant temperature, is a relatively new isothermal nucleic acid amplification technology. In this study, the development and optimization of a 4-plex tHDA assay for detection of Chlamydia trachomatis (CT) and Neisseria gonorrhoeae (NG) are described. tHDA is combined with sequence-specific sample preparation on magnetic beads and homogeneous endpoint fluorescence detection using dual-labeled probes. This 4-plex tHDA assay was applied to the detection of 2 genes on CT and a multicopy gene on NG in the presence of an internal control. The assay showed high analytical sensitivity and specificity of simultaneous CT/NG detection and is compatible with a wide variety of sample types and media. The isothermal reaction conditions and homogeneous endpoint detection utilized in this assay are well suited for laboratory automation and high-throughput screening applications as well as for point-of-care testing.
- Published
- 2011
44. Diagnostic dilemma: a young woman with Fabry disease symptoms, no family history, and a 'sequencing cryptic' α-galactosidase a large deletion
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Lis Hasholt, Åse Krogh Rasmussen, Robert J. Desnick, Ulla Feldt-Rasmussen, Martin Ballegaard, Irina Nazarenko, Erik Christensen, Robert Dobrovolny, Søren Schwartz Sørensen, and Flemming Wibrand
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Pathology ,medicine.medical_specialty ,Adolescent ,Endocrinology, Diabetes and Metabolism ,Biopsy ,Gene Dosage ,Biology ,medicine.disease_cause ,Kidney ,Biochemistry ,Gene dosage ,Polymerase Chain Reaction ,Loss of heterozygosity ,Endocrinology ,Genetics ,medicine ,Lysosomal storage disease ,Humans ,Enzyme Replacement Therapy ,Multiplex ligation-dependent probe amplification ,Family history ,Molecular Biology ,Sequence Deletion ,Mutation ,Genetic Carrier Screening ,Enzyme replacement therapy ,Sequence Analysis, DNA ,medicine.disease ,Fabry disease ,Gene Components ,alpha-Galactosidase ,Fabry Disease ,Female - Abstract
Fabry disease, an X-linked lysosomal storage disorder, results from the deficient activity of α-galactosidase A (α-Gal A). In affected males, the clinical diagnosis is confirmed by the markedly decreased α-Gal A activity. However, in female heterozygotes, the α-Gal A activity can range from low to normal due to random X-chromosomal inactivation, and diagnostic confirmation requires identification of the family's α-Gal A gene mutation. In a young female who had occasional acroparesthesias, corneal opacities, and 15 to 50% of the lower limit of normal leukocyte α-Gal A activity, α-Gal A sequencing in two expert laboratories did not identify a confirmatory mutation, presenting a diagnostic dilemma. A renal biopsy proved diagnostic and renewed efforts to detect an α-Gal A mutation. Subsequent gene dosage analyses identified a large α-Gal A deletion confirming her heterozygosity, and she was started on enzyme replacement therapy. Thus, gene dosage analyses can detect large deletions (>50bp) in suspect heterozygotes for X-linked and autosomal dominant diseases that are "sequencing cryptic," resolving molecular diagnostic dilemmas.
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- 2011
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- View/download PDF
45. LiCl induces TNF-α and FasL production, thereby stimulating apoptosis in cancer cells
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Irina Nazarenko, Wilko Thiele, Christine Blattner, Gabriela Marinescu, Jonathan P. Sleeman, Larissa Kaufmann, and Carolin Oberle
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Life sciences ,biology ,inorganic chemicals ,Programmed cell death ,Poly ADP ribose polymerase ,lcsh:Medicine ,Biochemistry ,Fas ligand ,ddc:570 ,medicine ,lcsh:QH573-671 ,Receptor ,Glycogen synthase ,Molecular Biology ,lcsh:Cytology ,Chemistry ,Research ,lcsh:R ,Cancer ,food and beverages ,Cell Biology ,medicine.disease ,equipment and supplies ,Apoptosis ,Immunology ,Cancer cell ,biology.protein ,Cancer research - Abstract
BackgroundThe incidence of cancer in patients with neurological diseases, who have been treated with LiCl, is below average. LiCl is a well-established inhibitor of Glycogen synthase kinase-3, a kinase that controls several cellular processes, among which is the degradation of the tumour suppressor protein p53. We therefore wondered whether LiCl induces p53-dependent cell death in cancer cell lines and experimental tumours.ResultsHere we show that LiCl induces apoptosis of tumour cells bothin vitroandin vivo. Cell death was accompanied by cleavage of PARP and Caspases-3, -8 and -10. LiCl-induced cell death was not dependent on p53, but was augmented by its presence. Treatment of tumour cells with LiCl strongly increased TNF-α and FasL expression. Inhibition of TNF-α induction using siRNA or inhibition of FasL binding to its receptor by the Nok-1 antibody potently reduced LiCl-dependent cleavage of Caspase-3 and increased cell survival. Treatment of xenografted rats with LiCl strongly reduced tumour growth.ConclusionsInduction of cell death by LiCl supports the notion that GSK-3 may represent a promising target for cancer therapy. LiCl-induced cell death is largely independent of p53 and mediated by the release of TNF-α and FasL.Key words: LiCl, TNF-α, FasL, apoptosis, GSK-3, FasL
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- 2011
- Full Text
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46. HPV genotype detection using hybrid capture sample preparation combined with whole genome amplification and multiplex detection with Luminex XMAP
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Brian Lowe, Ha Thai, Attila T. Lorincz, Richard L. Mallonee, Irina Nazarenko, Lori Kobayashi, and Dominic O'neil
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Genotype ,Uterine Cervical Neoplasms ,Cervix Uteri ,Genome, Viral ,Sensitivity and Specificity ,Pathology and Forensic Medicine ,Limit of Detection ,medicine ,Humans ,Multiplex ,Papillomaviridae ,Genotyping ,Cervical cancer ,Detection limit ,Whole Genome Amplification ,biology ,Papillomavirus Infections ,Nucleic acid amplification technique ,medicine.disease ,biology.organism_classification ,Virology ,Molecular biology ,DNA, Viral ,Molecular Medicine ,Female ,Nucleic Acid Amplification Techniques ,Regular Articles - Abstract
Infection with a high-risk carcinogenic type of human papillomavirus (HPV) is necessary for the development of cervical cancer. The digene HC2 HPV Test (HC2) is an important screening tool but lacks genotyping capability. To address this issue, we developed an assay for the rapid genotyping of HPV in cervical specimens. The three steps of this assay include Hybrid Capture target enrichment, whole-genome amplification, and Luminex XMAP detection. The assay includes the simultaneous detection of two genomic regions from each of 17 high-risk and two low-risk HPV types most associated with disease. The assay performance was tested on HPV plasmids as well as clinical specimens. An analytical limit of detection of 100 copies or less was demonstrated for linear, circular, and integrated HPV DNA. This finding is at least 1 log lower than the HC2 assay limit of detection. There was no cross-reactivity among the HPV types up to 1,000,000 copies. There was also no substantial assay interference from substances in cervical specimens. Although the clinical performance of the assay was not formally tested, the assay had good agreement (Cohen's kappa equal to 0.72) with both a PCR-based HPV genotyping assay (n = 131) and the HC2 assay (n = 502) using representative cervical specimens. This assay may be easy to automate and could be applied for the detection of other targets in future studies.
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- 2010
47. Activation-induced internalization differs for the tetraspanins CD9 and Tspan8: Impact on tumor cell motility
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Christoph Claas, Margot Zoeller, Sanyukta Rana, Irina Nazarenko, and Cosima C. Kretz
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endocrine system ,Endosome ,Tetraspanins ,media_common.quotation_subject ,education ,Fluorescent Antibody Technique ,Biology ,Exosomes ,Biochemistry ,Exosome ,Tetraspanin 29 ,Cell membrane ,Antigens, CD ,Cell Movement ,Cell Line, Tumor ,medicine ,Cell Adhesion ,Animals ,Internalization ,Cell adhesion ,media_common ,Membrane Glycoproteins ,Neovascularization, Pathologic ,Cell Membrane ,Endothelial Cells ,Cell migration ,Cell Biology ,Microvesicles ,Endocytosis ,Cell biology ,Rats ,medicine.anatomical_structure ,Multiprotein Complexes ,embryonic structures ,Intercellular Signaling Peptides and Proteins ,Tetradecanoylphorbol Acetate ,Intersectin 2 - Abstract
Exosomes are most important intercellular communicators and tetraspanins/tetraspanin-complexes have been suggested to play an important role in exosomal target cell selection. We have shown that only exosomes expressing a Tspan8–CD49d complex preferentially bind endothelial cells, which initiates angiogenesis. This finding was unexpected as in the exosome donor cell Tspan8 is associated with CD49c and the tetraspanins CD9 and CD151. In view of the discussed therapeutic power of exosomes as message/drug transporter, it became important to clarify the mechanisms accounting for the distinct Tspan8-web in the cell membrane versus exosomes. We therefore compared the route of Tspan8 and Tspan8-chimera internalization, where the N- and/or C-terminal regions were exchanged with the corresponding regions of CD9 or CD151. Activation-induced Tspan8-internalization proceeds more rapidly than CD9 internalization and is accompanied by disassembly of the Tspan8–CD9–CD151 membrane complex in resting cells. Tspan8-internalization relies on the association of the Tspan8 N-terminal region with intersectin-2, a multimodular complex involved in clathrin-coated pit internalization. Internalization and recovery of Tspan8 in early endosomes is further promoted by the recruitment of CD49d such that only in PMA-activated cells a Tspan8–INS2–CD49d–clathrin complex is recovered in cholesterol-depletion-resistant membrane microdomains. PMA-induced Tspan8-internalization promotes cell migration, but reduces matrix and cell adhesion. Thus, stimulation initiates tetraspanin-web rearrangements, which have strong functional consequences for the cell, exosome-delivery and exosome target selection. This knowledge will be essential for generating tailored therapeutic exosomes.
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- 2010
48. Frequency of unrecognized Fabry disease among young European-American and African-American men with first ischemic stroke
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Stanley Tuhrim, Barney J. Stern, Steven J. Kittner, Robert J. Desnick, Eric McDade, Robert Dobrovolny, Mark T Dobbins, Marie E. Grace, John W. Cole, Irina Nazarenko, and Marcella A. Wozniak
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Adult ,Male ,Washington ,medicine.medical_specialty ,Pediatrics ,Adolescent ,White People ,Article ,Brain Ischemia ,Central nervous system disease ,Brain ischemia ,Young Adult ,Risk Factors ,medicine ,Prevalence ,Humans ,Young adult ,Stroke ,Advanced and Specialized Nursing ,Polymorphism, Genetic ,business.industry ,Vascular disease ,Cerebral infarction ,Case-control study ,Middle Aged ,medicine.disease ,Fabry disease ,Surgery ,Black or African American ,Case-Control Studies ,alpha-Galactosidase ,Baltimore ,Fabry Disease ,Neurology (clinical) ,Cardiology and Cardiovascular Medicine ,business - Abstract
Background and Purpose— The cause of initial ischemic stroke in up to 30% of young patients remains unclear. Fabry disease, due to deficient α-galactosidase A (α-Gal A) activity, is a vascular endothelial glycosphingolipid storage disease typically presenting in childhood. With advancing age, patients develop renal, cardiac, and cerebrovascular disease and die prematurely. A European study suggested an increased prevalence of unrecognized Fabry disease in patients with cryptogenic stroke. We hypothesized that α-Gal A deficiency is a rare cause of initial early-onset ischemic stroke in men. Methods— The Stroke Prevention in Young Men Study enrolled >550 men (15 to 49 years) with first ischemic stroke in the Baltimore–Washington area in 2004 to 2007. Frozen plasma samples were assayed for α-Gal A activity, and DNA from patients with consistently low plasma α-Gal A activities were sequenced. Results— The study sample consisted of 558 men (42% African-American; median age 44 years). Stroke was cryptogenic in 154 men (40% African-American). In 10 patients with low plasma α-Gal A activities, DNA sequencing identified alterations in the α-Gal A gene in 2 patients. The polymorphism, D313Y, which results in low plasma enzyme activity, but near normal levels of cellular activity was seen in one European-American male. The Fabry disease-causing A143T mutation was seen in an African-American male with cryptogenic stroke (0.18% of all strokes: upper 95% CI=0.53%; 0.65% of cryptogenic strokes: upper 95% CI=1.92%). Conclusions— In this biracial population, unrecognized Fabry disease is a rare but treatable cause of initial ischemic stroke in young men.
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- 2009
49. CD44 and EpCAM: cancer-initiating cell markers
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Tobias Nuebel, Rachid Marhaba, Margot Zoeller, Markus W. Buechler, Irina Nazarenko, and Pamela Klingbeil
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Pathology ,medicine.medical_specialty ,Exosomes ,Biochemistry ,Exosome ,Models, Biological ,chemistry.chemical_compound ,Cancer stem cell ,Antigens, Neoplasm ,Neoplasms ,medicine ,Biomarkers, Tumor ,Animals ,Humans ,Molecular Biology ,biology ,CD44 ,Membrane Proteins ,Epithelial cell adhesion molecule ,General Medicine ,Epithelial Cell Adhesion Molecule ,Embryonic stem cell ,Neoplasm Proteins ,Adult Stem Cells ,Hyaluronan Receptors ,chemistry ,Cancer cell ,biology.protein ,Cancer research ,Neoplastic Stem Cells ,Molecular Medicine ,Stem cell ,Cell Adhesion Molecules ,Adult stem cell ,Signal Transduction - Abstract
Embryonic stem cells are immortal, can self renew, and differentiate into all cells of the body. The adult organism maintains adult stem cells in regenerative organs that can differentiate into all cells of the respective organ. Virchow's hypothesis that cancer may arise from embryonic-like cells has received strong support, as it was demonstrated that tumors contain few cells, known as cancer stem or cancer-initiating cells (CIC), that account for primary and metastatic tumor growth. CIC are mostly defined by expression of CIC-markers that are associated and correlated with the potential of CIC to grow in xenogeneic mice. CIC marker profiles have been elaborated for many tumors, with several markers as CD24, CD44, CD133, CD166, EpCAM, and some integrins, being expressed by tumors of different histological type. Their function in promoting CIC maintenance and activity is largely unknown. The fate of stem cells, determined by their position, is minutely regulated by few adjacent cells creating a niche. CIC also require a niche, mostly for settlement and growth in distant organs. This so called pre-metastatic niche is initiated by the primary tumor before metastasizing cell arrival. How do CIC prepare the pre-metastatic niche? Cancer cells secrete a matrix that serves a cross-talk with surrounding tissues. Additionally, cancer cells can abundantly deliver exosomes, which function as long-distance intercellular communicators. Studies on a rat pancreatic adenocarcinoma support our hypothesis that tumor-derived matrix and exosomes are the main actors in forming the pre-metastatic niche with CIC markers being engaged in matrix preparation and/or exosome delivery.
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- 2008
50. CEBPbeta, JunD and c-Jun contribute to the transcriptional activation of the metastasis-associated C4.4A gene
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Andreas Claas, Frank Fries, Irina Nazarenko, Margot Zöller, Peter Angel, and Jochen Hess
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Transcriptional Activation ,Cancer Research ,Transcription, Genetic ,Proto-Oncogene Proteins c-jun ,Response element ,Molecular Sequence Data ,Biology ,medicine.disease_cause ,Transfection ,Genes, jun ,Transcription (biology) ,Cell Line, Tumor ,Gene expression ,medicine ,Animals ,Neoplasm Metastasis ,Promoter Regions, Genetic ,Gene ,Base Sequence ,CCAAT-Enhancer-Binding Protein-beta ,c-jun ,Antibodies, Monoclonal ,Promoter ,Neoplasms, Experimental ,Molecular biology ,Rats ,Sp3 Transcription Factor ,Oncology ,Tumor progression ,Carcinogenesis - Abstract
The glycosylphosphatidylinositol-anchored molecule C4.4A, which shares structural features with uPAR, is frequently expressed on carcinomas with upregulated expression during tumor progression. Moreover, rare expression on nontransformed epithelial cells is strongly increased during tissue remodeling, e.g., during wound healing. This strictly regulated expression prompted us to define transcriptional activation of the C4.4A gene. C4.4A transcription was analyzed in 2 syngenic rat tumor cell lines with low or high metastatic potential, respectively. Though genomic C4.4A DNA was present in both lines, C4.4A mRNA and transcription of a reporter construct containing the C4.4A promoter was only observed in the metastasizing subline. Deletions and point mutations in the C4.4A promoter-driven reporter construct revealed that activation of the TATA-less, GC-rich core promoter (-1 to -50 bp) does not suffice to initiate transcription that requires coactivation of a proximal response element (-71 to -88 bp) and can be further increased by more distal response elements (-89 to -133 bp). Mobility-shift and cotransfection studies showed that Sp3 binding enhances C4.4A transcription, whereas potential Sp1 binding sites were ineffective. C4.4A transcription essentially requires C/EBPbeta binding to a TRE/CCAAT composite element (-71 to -88 bp) as measured by ChIP assay. C4.4A transcription is strikingly enhanced by cotransfection with JunD or c-Jun, such that C4.4A is most strongly transcribed even in the C4.4A-negative tumor cell line after cotransfection with C/EBPbeta plus JunD or c-Jun. Thus, upregulation of C/EBPbeta during tumor progression and wound repair may well provide a sufficient trigger for transcription of the C4.4A gene.
- Published
- 2007
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