389 results on '"V Moses"'
Search Results
2. Elevating Neuro-Linguistic Decoding: Deepening Neural-Device Interaction with RNN-GRU for Non-Invasive Language Decoding
- Author
-
Jayakumar, V Moses, primary, Rajakumari, R., additional, Padmini, Kuppala, additional, Godla, Sanjiv Rao, additional, El-Ebiary, Yousef A.Baker, additional, and Ponnuswamy, Vijayalakshmi, additional
- Published
- 2024
- Full Text
- View/download PDF
3. Zika virus infection in pregnant rhesus macaques causes placental dysfunction and immunopathology
- Author
-
Alec J. Hirsch, Victoria H. J. Roberts, Peta L. Grigsby, Nicole Haese, Matthias C. Schabel, Xiaojie Wang, Jamie O. Lo, Zheng Liu, Christopher D. Kroenke, Jessica L. Smith, Meredith Kelleher, Rebecca Broeckel, Craig N. Kreklywich, Christopher J. Parkins, Michael Denton, Patricia Smith, Victor DeFilippis, William Messer, Jay A. Nelson, Jon D. Hennebold, Marjorie Grafe, Lois Colgin, Anne Lewis, Rebecca Ducore, Tonya Swanson, Alfred W. Legasse, Michael K. Axthelm, Rhonda MacAllister, Ashlee V. Moses, Terry K. Morgan, Antonio E. Frias, and Daniel N. Streblow
- Subjects
Science - Abstract
Zika virus infection during pregnancy can result in birth defects, but underlying pathogenesis at the maternal-fetal interface is unclear. Here, the authors use non-invasive in vivo imaging of Zika-infected rhesus macaques and show that infection results in abnormal oxygen transport across the placenta.
- Published
- 2018
- Full Text
- View/download PDF
4. Cervical Vertebral Bone Biopsy: Challenges and Tricks
- Author
-
PK Chinniah, B Gopal, V Moses, and SN Keshava
- Subjects
Radiology, Nuclear Medicine and imaging - Published
- 2022
- Full Text
- View/download PDF
5. Data from Novel Cellular Genes Essential for Transformation of Endothelial Cells by Kaposi's Sarcoma–Associated Herpesvirus
- Author
-
Ashlee V. Moses, Klaus Früh, Bruce J. Dezube, Henry Koon, Shane McAllister, Rebecca Ruhl, and Camilo Raggo
- Abstract
Kaposi's sarcoma–associated herpesvirus (KSHV) is involved in the development of lymphoproliferative diseases and Kaposi's sarcoma. The oncogenicity of this virus is reflected in vitro by its ability to transform B cells and endothelial cells. Infection of dermal microvascular endothelial cells (DMVEC) transforms the cells from a cobblestone-like monolayer to foci-forming spindle cells. This transformation is accompanied by dramatic changes in the cellular transcriptome. Known oncogenes, such as c-Kit, are among the KSHV-induced host genes. We previously showed that c-Kit is an essential cellular component of the KSHV-mediated transformation of DMVEC. Here, we test the hypothesis that the transformation process can be used to discover novel oncogenes. When expression of a panel of KSHV-induced cellular transcripts was inhibited with antisense oligomers, we observed inhibition of DMVEC proliferation and foci formation using antisense molecules to RDC1 and Neuritin. We further showed that transformation of KSHV-infected DMVEC was inhibited by small interfering RNA directed at RDC1 or Neuritin. Ectopic expression of Neuritin in NIH 3T3 cells resulted in changes in cell morphology and anchorage-independent growth, whereas RDC1 ectopic expression significantly increased cell proliferation. In addition, both RDC1- and Neuritin-expressing cells formed tumors in nude mice. RDC1 is an orphan G protein–coupled receptor, whereas Neuritin is a growth-promoting protein known to mediate neurite outgrowth. Neither gene has been previously implicated in tumorigenesis. Our data suggest that KSHV-mediated transformation involves exploitation of the hitherto unrealized oncogenic properties of RDC1 and Neuritin.
- Published
- 2023
- Full Text
- View/download PDF
6. Supplementary Table 1 from Novel Cellular Genes Essential for Transformation of Endothelial Cells by Kaposi's Sarcoma–Associated Herpesvirus
- Author
-
Ashlee V. Moses, Klaus Früh, Bruce J. Dezube, Henry Koon, Shane McAllister, Rebecca Ruhl, and Camilo Raggo
- Abstract
Supplementary Table 1 from Novel Cellular Genes Essential for Transformation of Endothelial Cells by Kaposi's Sarcoma–Associated Herpesvirus
- Published
- 2023
- Full Text
- View/download PDF
7. Part Three: Conducting Three Viennese Classical Masterworks
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
8. 10. Franz Joseph Haydn: Missa inangustiis (Nelsonmesse)
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
9. Foreword to the First Edition
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
10. 11. Franz Schubert: Mass in G Major, D.167
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
11. 12. Ludwig van Beethoven: (Choral) Fantasia, op. 80
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
12. Glossary
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
13. Bibliography
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
14. Cover
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
15. Index
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
16. 1. The Nature of the Orchestra
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
17. Title Page, Copyright
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
18. 6. Studying the Scores
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
19. Preface to the Second, Expanded Edition
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
20. 3. Preparing for Rehearsals
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
21. Part One: Working with an Orchestra
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
22. 4. Adjusting Your Baton Technique
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
23. 5. Rehearsing the Orchestra
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
24. 2. The Orchestral Instruments
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
25. 8. J. S. Bach: Magnificat in D Major, BWV 243
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
26. Part Two: Conducting Three Baroque Masterworks
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
27. 7. G. F. Handel: Messiah
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
28. 9. Antonio Vivaldi: Gloria (in D)
- Author
-
Don V Moses, Robert W. Demaree, Jr., and Allen F. Ohmes
- Published
- 2004
29. Kaposi Sarcoma Herpesvirus Induces HO-1 during De Novo Infection of Endothelial Cells via Viral miRNA-Dependent and -Independent Mechanisms
- Author
-
Sara Botto, Jennifer E. Totonchy, Jean K. Gustin, and Ashlee V. Moses
- Subjects
Microbiology ,QR1-502 - Abstract
ABSTRACT Kaposi sarcoma (KS) herpesvirus (KSHV) infection of endothelial cells (EC) is associated with strong induction of heme oxygenase-1 (HO-1), a stress-inducible host gene that encodes the rate-limiting enzyme responsible for heme catabolism. KS is an angioproliferative tumor characterized by the proliferation of KSHV-infected spindle cells, and HO-1 is highly expressed in such cells. HO-1 converts the pro-oxidant, proinflammatory heme molecule into metabolites with antioxidant, anti-inflammatory, and proliferative activities. Previously published work has shown that KSHV-infected EC in vitro proliferate in response to free heme in a HO-1-dependent manner, thus implicating virus-enhanced HO-1 activity in KS tumorigenesis. The present study investigated the molecular mechanisms underlying KSHV induction of HO-1 in lymphatic EC (LEC), which are the likely spindle cell precursors. In a time course analysis of KSHV-infected cells, HO-1 expression displays biphasic kinetics characterized by an early transient induction that is followed by a more sustained upregulation coincident with the establishment of viral latency. A viral microRNA miR-K12-11 deletion mutant of KSHV was found to be defective for induction of HO-1 during latency. A potential mechanism for this phenotype was provided by BACH1, a cellular HO-1 transcriptional repressor targeted by miR-K12-11. In fact, in KSHV-infected LEC, the BACH1 message level is reduced, BACH1 subcellular localization is altered, and miR-K12-11 mediates the inverse regulation of HO-1 and BACH1 during viral latency. Interestingly, the data indicate that neither miR-K12-11 nor de novo KSHV gene expression is required for the burst of HO-1 expression observed at early times postinfection, which suggests that additional virion components promote this phenotype. IMPORTANCE While the mechanisms underlying KSHV induction of HO-1 remain unknown, the cellular mechanisms that regulate HO-1 expression have been extensively investigated in the context of basal and pathophysiological states. The detoxifying action of HO-1 is critical for the protection of cells exposed to high heme levels. KS spindle cells are erythrophagocytic and contain erythrocyte ghosts. Erythrocyte degeneration leads to the localized release of heme, creating oxidative stress that may be further exacerbated by environmental or other cofactors. Our previous work showed that KSHV-infected cells proliferate in response to heme and that this occurs in a HO-1-dependent manner. We therefore hypothesize that KSHV induction of HO-1 contributes to KS tumor development via heme metabolism and propose that HO-1 be evaluated as a therapeutic target for KS. Our present work, which aimed to understand the mechanisms whereby KSHV induces HO-1, will be important for the design and implementation of such a strategy.
- Published
- 2015
- Full Text
- View/download PDF
30. Correction: IRF-3, IRF-5, and IRF-7 Coordinately Regulate the Type I IFN Response in Myeloid Dendritic Cells Downstream of MAVS Signaling.
- Author
-
Helen M. Lazear, Alissa Lancaster, Courtney Wilkins, Mehul S. Suthar, Albert Huang, Sarah C. Vick, Lisa Clepper, Larissa Thackray, Margaret M. Brassil, Herbert W. Virgin, Janko Nikolich-Zugich, Ashlee V. Moses, Michael Gale, Klaus Früh, and Michael S. Diamond
- Subjects
Immunologic diseases. Allergy ,RC581-607 ,Biology (General) ,QH301-705.5 - Published
- 2013
- Full Text
- View/download PDF
31. IRF-3, IRF-5, and IRF-7 coordinately regulate the type I IFN response in myeloid dendritic cells downstream of MAVS signaling.
- Author
-
Helen M Lazear, Alissa Lancaster, Courtney Wilkins, Mehul S Suthar, Albert Huang, Sarah C Vick, Lisa Clepper, Larissa Thackray, Margaret M Brassil, Herbert W Virgin, Janko Nikolich-Zugich, Ashlee V Moses, Michael Gale, Klaus Früh, and Michael S Diamond
- Subjects
Immunologic diseases. Allergy ,RC581-607 ,Biology (General) ,QH301-705.5 - Abstract
Although the transcription factors IRF-3 and IRF-7 are considered master regulators of type I interferon (IFN) induction and IFN stimulated gene (ISG) expression, Irf3(-/-)×Irf7(-/-) double knockout (DKO) myeloid dendritic cells (mDC) produce relatively normal levels of IFN-β after viral infection. We generated Irf3(-/-)×Irf5(-/-)×Irf7(-/-) triple knockout (TKO) mice to test whether IRF-5 was the source of the residual induction of IFN-β and ISGs in mDCs. In pathogenesis studies with two unrelated positive-sense RNA viruses (West Nile virus (WNV) and murine norovirus), TKO mice succumbed at rates greater than DKO mice and equal to or approaching those of mice lacking the type I IFN receptor (Ifnar(-/-)). In ex vivo studies, after WNV infection or exposure to Toll-like receptor agonists, TKO mDCs failed to produce IFN-β or express ISGs. In contrast, this response was sustained in TKO macrophages following WNV infection. To define IRF-regulated gene signatures, we performed microarray analysis on WNV-infected mDC from wild type (WT), DKO, TKO, or Ifnar(-/-) mice, as well as from mice lacking the RIG-I like receptor adaptor protein MAVS. Whereas the gene induction pattern in DKO mDC was similar to WT cells, remarkably, almost no ISG induction was detected in TKO or Mavs(-/-) mDC. The relative equivalence of TKO and Mavs(-/-) responses suggested that MAVS dominantly regulates ISG induction in mDC. Moreover, we showed that MAVS-dependent induction of ISGs can occur through an IRF-5-dependent yet IRF-3 and IRF-7-independent pathway. Our results establish IRF-3, -5, and -7 as the key transcription factors responsible for mediating the type I IFN and ISG response in mDC during WNV infection and suggest a novel signaling link between MAVS and IRF-5.
- Published
- 2013
- Full Text
- View/download PDF
32. Aberrant proliferation in CXCR7+ endothelial cells via degradation of the retinoblastoma protein.
- Author
-
Jennifer E Totonchy, Jessica M Osborn, Sara Botto, Lisa Clepper, and Ashlee V Moses
- Subjects
Medicine ,Science - Abstract
Angiogenesis is a critical factor in the growth and dissemination of solid tumors. Indeed, tumor vasculature is abnormal and contributes to the development and spread of malignancies by creating a hostile microenvironment. The alternative SDF-1/CXCL12 receptor, CXCR7, is frequently and specifically expressed in tumor-associated vessels. In this study, we examine the role of endothelium-expressed CXCR7 in tumor vascular dysfunction by specifically examining the contribution of CXCR7 to endothelial cell (EC) proliferation. We demonstrate that CXCR7 expression is sufficient to drive post-confluent growth in EC cultures. Further, we provide a novel mechanism for CXCR7-mediated proliferation via proteasomal degradation of the tumor suppressor protein Rb. These findings identify a heretofore unappreciated role for CXCR7 in vascular dysfunction and confirm this receptor as a plausible target for anti-tumor therapy.
- Published
- 2013
- Full Text
- View/download PDF
33. Zika virus infection in pregnant rhesus macaques causes placental dysfunction and immunopathology
- Author
-
Rebecca M. Ducore, Peta L. Grigsby, Rhonda MacAllister, Lois M. A. Colgin, Tonya Swanson, Jamie O. Lo, Daniel N. Streblow, Alfred W. Legasse, Xiaojie Wang, Victoria H. J. Roberts, Antonio E. Frias, Alec J. Hirsch, Meredith A. Kelleher, Jon D. Hennebold, Terry K. Morgan, Ashlee V. Moses, Nicole N. Haese, Victor R. DeFilippis, Craig N. Kreklywich, Jessica L. Smith, Matthias C. Schabel, William B. Messer, Zheng Liu, Patricia P. Smith, Michael K. Axthelm, Marjorie R. Grafe, Anne D. Lewis, Christopher J. Parkins, Christopher D. Kroenke, Rebecca Broeckel, Michael Denton, and Jay A. Nelson
- Subjects
0301 basic medicine ,Placenta ,Viral pathogenesis ,General Physics and Astronomy ,Physiology ,Adaptive Immunity ,Zika virus ,Fetal Development ,0302 clinical medicine ,Pregnancy ,Immunopathology ,Pregnancy Complications, Infectious ,lcsh:Science ,Multidisciplinary ,biology ,Zika Virus Infection ,Brain ,Viral Load ,Magnetic Resonance Imaging ,3. Good health ,medicine.anatomical_structure ,embryonic structures ,Cytokines ,Female ,Science ,Permeability ,Article ,General Biochemistry, Genetics and Molecular Biology ,03 medical and health sciences ,Fetus ,medicine ,Animals ,Placental Circulation ,business.industry ,Oxygen transport ,General Chemistry ,biology.organism_classification ,medicine.disease ,Macaca mulatta ,Immunity, Innate ,Oxygen ,Disease Models, Animal ,030104 developmental biology ,lcsh:Q ,business ,030217 neurology & neurosurgery - Abstract
Zika virus (ZIKV) infection during pregnancy leads to an increased risk of fetal growth restriction and fetal central nervous system malformations, which are outcomes broadly referred to as the Congenital Zika Syndrome (CZS). Here we infect pregnant rhesus macaques and investigate the impact of persistent ZIKV infection on uteroplacental pathology, blood flow, and fetal growth and development. Despite seemingly normal fetal growth and persistent fetal-placenta-maternal infection, advanced non-invasive in vivo imaging studies reveal dramatic effects on placental oxygen reserve accompanied by significantly decreased oxygen permeability of the placental villi. The observation of abnormal oxygen transport within the placenta appears to be a consequence of uterine vasculitis and placental villous damage in ZIKV cases. In addition, we demonstrate a robust maternal-placental-fetal inflammatory response following ZIKV infection. This animal model reveals a potential relationship between ZIKV infection and uteroplacental pathology that appears to affect oxygen delivery to the fetus during development., Zika virus infection during pregnancy can result in birth defects, but underlying pathogenesis at the maternal-fetal interface is unclear. Here, the authors use non-invasive in vivo imaging of Zika-infected rhesus macaques and show that infection results in abnormal oxygen transport across the placenta.
- Published
- 2018
34. Viral Takeover of the Host Ubiquitin System
- Author
-
Jean K Gustin, Ashlee V Moses, Klaus eFrüh, and Janet L Douglas
- Subjects
Ubiquitin ,virus ,Proteasome ,ubiquitin proteasome system ,Ubiquitin ligase complex ,Viral lifecycle ,Microbiology ,QR1-502 - Abstract
Like the other more well-characterized post-translational modifications (phosphorylation, methylation, acetylation, acylation, etc.), the attachment of the 76 amino acid ubiquitin (Ub) protein to substrates has been shown to govern countless cellular processes. As obligate intracellular parasites, viruses have evolved the capability to commandeer many host processes in order to maximize their own survival, whether it be to increase viral production or to ensure the long-term survival of latently infected host cells. The first evidence that viruses could usurp the Ub system came from the DNA tumor viruses and Adenoviruses, each of which use Ub to dysregulate the host cell cycle. Today, the list of viruses that utilize Ub includes members from almost every viral class, including both RNA and DNA viruses. Among these, there are examples of Ub usage at every stage of the viral life cycle, and these entail both ubiquitination and de-ubiquitination. In addition to viruses that merely modify the host Ub system, many of the large DNA viruses encode their own Ub modifying machinery. In this review, we highlight the latest discoveries regarding the myriad ways that viruses utilize Ub to their advantage.
- Published
- 2011
- Full Text
- View/download PDF
35. The great escape: viral strategies to counter BST-2/tetherin.
- Author
-
Janet L Douglas, Jean K Gustin, Kasinath Viswanathan, Mandana Mansouri, Ashlee V Moses, and Klaus Früh
- Subjects
Immunologic diseases. Allergy ,RC581-607 ,Biology (General) ,QH301-705.5 - Abstract
The interferon-induced BST-2 protein has the unique ability to restrict the egress of HIV-1, Kaposi's sarcoma-associated herpesvirus (KSHV), Ebola virus, and other enveloped viruses. The observation that virions remain attached to the surface of BST-2-expressing cells led to the renaming of BST-2 as "tetherin". However, viral proteins such as HIV-1 Vpu, simian immunodeficiency virus Nef, and KSHV K5 counteract BST-2, thereby allowing mature virions to readily escape from infected cells. Since the anti-viral function of BST-2 was discovered, there has been an explosion of research into several aspects of this intriguing interplay between host and virus. This review focuses on recent work addressing the molecular mechanisms involved in BST-2 restriction of viral egress and the species-specific countermeasures employed by various viruses.
- Published
- 2010
- Full Text
- View/download PDF
36. Hepatic Subcapsular Haemorrhage: Watering-can Appearance
- Author
-
Shyamkumar N. Keshava, Munawwar Ahmed, P Joseph, S Jain, V Moses, and Shaileshkumar Garge
- Subjects
medicine.medical_specialty ,Subcapsular haemorrhage ,business.industry ,medicine ,Radiology, Nuclear Medicine and imaging ,business ,Surgery - Published
- 2016
- Full Text
- View/download PDF
37. Full-Length Isoforms of Kaposi's Sarcoma-Associated Herpesvirus Latency-Associated Nuclear Antigen Accumulate in the Cytoplasm of Cells Undergoing the Lytic Cycle of Replication
- Author
-
Keiji Ueda, Minako Ikoma, Serge Barcy, Ashlee V. Moses, Gail H. Deutsch, David Wu, Kellie Howard, Timothy M. Rose, and H. Jacques Garrigues
- Subjects
0301 basic medicine ,Cytoplasm ,viruses ,Cellular differentiation ,Immunology ,Cell ,Biology ,Virus Replication ,medicine.disease_cause ,Microbiology ,Mass Spectrometry ,Cell Line ,Immediate-Early Proteins ,03 medical and health sciences ,Virology ,Chlorocebus aethiops ,medicine ,Animals ,Humans ,Protein Isoforms ,Kaposi's sarcoma-associated herpesvirus ,Antigens, Viral ,Sarcoma, Kaposi ,Vero Cells ,Nuclear Proteins ,virus diseases ,biochemical phenomena, metabolism, and nutrition ,Genome Replication and Regulation of Viral Gene Expression ,Virus Latency ,Chromatin ,Cell biology ,030104 developmental biology ,medicine.anatomical_structure ,Viral replication ,Lytic cycle ,Insect Science ,Herpesvirus 8, Human ,Nuclear localization sequence - Abstract
The latency-associated nuclear antigen (LANA) of the Kaposi's sarcoma-associated herpesvirus (KSHV) performs a variety of functions to establish and maintain KSHV latency. During latency, LANA localizes to discrete punctate spots in the nucleus, where it tethers viral episomes to cellular chromatin and interacts with nuclear components to regulate cellular and viral gene expression. Using highly sensitive tyramide signal amplification, we determined that LANA localizes to the cytoplasm in different cell types undergoing the lytic cycle of replication after de novo primary infection and after spontaneous, tetradecanoyl phorbol acetate-, or open reading frame 50 (ORF50)/replication transactivator (RTA)-induced activation. We confirmed the presence of cytoplasmic LANA in a subset of cells in lytically active multicentric Castleman disease lesions. The induction of cellular migration by scratch-wounding confluent cell cultures, culturing under subconfluent conditions, or induction of cell differentiation in primary cultures upregulated the number of cells permissive for primary lytic KSHV infection. The induction of lytic replication was characterized by high-level expression of cytoplasmic LANA and nuclear ORF59, a marker of lytic replication. Subcellular fractionation studies revealed the presence of multiple isoforms of LANA in the cytoplasm of ORF50/RTA-activated Vero cells undergoing primary infection. Mass spectrometry analysis demonstrated that cytoplasmic LANA isoforms were full length, containing the N-terminal nuclear localization signal. These results suggest that trafficking of LANA to different subcellular locations is a regulated phenomenon, which allows LANA to interact with cellular components in different compartments during both the latent and the replicative stages of the KSHV life cycle. IMPORTANCE Kaposi's sarcoma-associated herpesvirus (KSHV) causes AIDS-related malignancies, including lymphomas and Kaposi's sarcoma. KSHV establishes lifelong infections using its latency-associated nuclear antigen (LANA). During latency, LANA localizes to the nucleus, where it connects viral and cellular DNA complexes and regulates gene expression, allowing the virus to maintain long-term infections. Our research shows that intact LANA traffics to the cytoplasm of cells undergoing permissive lytic infections and latently infected cells in which the virus is induced to replicate. This suggests that LANA plays important roles in the cytoplasm and nuclear compartments of the cell during different stages of the KSHV life cycle. Determining cytoplasmic function and mechanism for regulation of the nuclear localization of LANA will enhance our understanding of the biology of this virus, leading to therapeutic approaches to eliminate infection and block its pathological effects.
- Published
- 2017
- Full Text
- View/download PDF
38. An In Vitro Model for Studying Cellular Transformation by Kaposi Sarcoma Herpesvirus
- Author
-
Shane C, McAllister, Ryan L, Hanson, Kyleen N, Grissom, Sara, Botto, and Ashlee V, Moses
- Subjects
Carcinogenesis ,Herpesvirus 8, Human ,Endothelial Cells ,Humans ,Cell Transformation, Viral ,Sarcoma, Kaposi ,Cancer Biology - Abstract
Kaposi sarcoma (KS) is an unusual tumor composed of proliferating spindle cells that is initiated by infection of endothelial cells (EC) with KSHV, and develops most often in the setting of immunosuppression. Despite decades of research, optimal treatment of KS remains poorly defined and clinical outcomes are especially unfavorable in resource-limited settings. KS lesions are driven by pathological angiogenesis, chronic inflammation, and oncogenesis, and various in vitro cell culture models have been developed to study these processes. KS arises from KSHV-infected cells of endothelial origin, so EC-lineage cells provide the most appropriate in vitro surrogates of the spindle cell precursor. However, because EC have a limited in vitro lifespan, and as the oncogenic mechanisms employed by KSHV are less efficient than those of other tumorigenic viruses, it has been difficult to assess the processes of transformation in primary or telomerase-immortalized EC. Therefore, a novel EC-based culture model was developed that readily supports transformation following infection with KSHV. Ectopic expression of the E6 and E7 genes of human papillomavirus type 16 allows for extended culture of age- and passage-matched mock- and KSHV-infected EC and supports the development of a truly transformed (i.e., tumorigenic) phenotype in infected cell cultures. This tractable and highly reproducible model of KS has facilitated the discovery of several essential signaling pathways with high potential for translation into clinical settings.
- Published
- 2017
39. An In Vitro Model for Studying Cellular Transformation by Kaposi Sarcoma Herpesvirus
- Author
-
Ryan S. Hanson, Sara Botto, Kyleen N. Grissom, Shane C McAllister, and Ashlee V. Moses
- Subjects
General Immunology and Microbiology ,General Chemical Engineering ,General Neuroscience ,Cell ,Biology ,medicine.disease ,medicine.disease_cause ,Virology ,Phenotype ,General Biochemistry, Genetics and Molecular Biology ,In vitro ,Endothelial stem cell ,medicine.anatomical_structure ,Cancer research ,medicine ,Ectopic expression ,Sarcoma ,Primary effusion lymphoma ,Carcinogenesis - Abstract
Kaposi sarcoma (KS) is an unusual tumor composed of proliferating spindle cells that is initiated by infection of endothelial cells (EC) with KSHV, and develops most often in the setting of immunosuppression. Despite decades of research, optimal treatment of KS remains poorly defined and clinical outcomes are especially unfavorable in resource-limited settings. KS lesions are driven by pathological angiogenesis, chronic inflammation, and oncogenesis, and various in vitro cell culture models have been developed to study these processes. KS arises from KSHV-infected cells of endothelial origin, so EC-lineage cells provide the most appropriate in vitro surrogates of the spindle cell precursor. However, because EC have a limited in vitro lifespan, and as the oncogenic mechanisms employed by KSHV are less efficient than those of other tumorigenic viruses, it has been difficult to assess the processes of transformation in primary or telomerase-immortalized EC. Therefore, a novel EC-based culture model was developed that readily supports transformation following infection with KSHV. Ectopic expression of the E6 and E7 genes of human papillomavirus type 16 allows for extended culture of age- and passage-matched mock- and KSHV-infected EC and supports the development of a truly transformed (i.e., tumorigenic) phenotype in infected cell cultures. This tractable and highly reproducible model of KS has facilitated the discovery of several essential signaling pathways with high potential for translation into clinical settings.
- Published
- 2017
- Full Text
- View/download PDF
40. The Heme Metabolite Carbon Monoxide Facilitates KSHV Infection by Inhibiting TLR4 Signaling in Endothelial Cells
- Author
-
Jean K. Gustin, Ashlee V. Moses, and Sara Botto
- Subjects
0301 basic medicine ,Microbiology (medical) ,HO-1 ,Context (language use) ,KSHV ,Biology ,Microbiology ,carbon monoxide ,03 medical and health sciences ,Immune system ,Viral life cycle ,Downregulation and upregulation ,TLR4 ,innate immunity ,Original Research ,Innate immune system ,030102 biochemistry & molecular biology ,Effector ,Pattern recognition receptor ,heme oxygenase-1 ,Virology ,3. Good health ,Cell biology ,CO ,030104 developmental biology - Abstract
Kaposi sarcoma herpesvirus (KSHV) is the etiologic agent of Kaposi sarcoma (KS) and certain rare B cell lymphoproliferative disorders. KSHV infection of endothelial cells (EC) in vitro increases expression of the inducible host-encoded enzyme heme oxygenase-1 (HO-1), which is also strongly expressed in KS tumors. HO-1 catalyzes the rate-limiting step in the conversion of heme into iron, biliverdin and the gasotransmitter carbon monoxide (CO), all of which share anti-apoptotic, anti-inflammatory, pro-survival, and tumorigenic activities. Our previous work has shown that HO-1 expression in KSHV-infected EC is characterized by a rapid yet transient induction at early times post-infection, followed by a sustained upregulation co-incident with establishment of viral latency. These two phases of expression are independently regulated, suggesting distinct roles for HO-1 in the virus life cycle. Here, we investigated the role of HO-1 during acute infection, prior to the onset of viral gene expression. The early infection phase involves a series of events that culminate in delivery of the viral genome to the nucleus. Primary infection also leads to activation of host innate immune effectors, including the pattern recognition receptor TLR4, to induce an antiviral response. It has been shown that TLR4-deficient EC are more susceptible to KSHV infection than wild-type controls, suggesting an important inhibitory role for TLR4 in the KSHV life cycle. TLR4 signaling is in turn subject to regulation by several virus-encoded immune evasion factors. In this report we identify HO-1 as a host protein co-opted by KSHV as part of a rapid immune evasion strategy. Specifically, we show that early HO-1 induction by KSHV results in increased levels of endogenous CO, which functions as a TLR4 signaling inhibitor. In addition, we show that CO-mediated inhibition of TLR4 signaling leads to reduced expression of TLR4-induced antiviral genes, thus dampening the host antiviral response and facilitating KSHV infection. Conversely, inhibition of HO-1 activity decreases intracellular CO, enhances the host antiviral response and inhibits KSHV infection. In conclusion, this study identifies HO-1 as a novel innate immune evasion factor in the context of KSHV infection and supports HO-1 inhibition as a viable therapeutic strategy for KS.
- Published
- 2017
- Full Text
- View/download PDF
41. Evasion of adaptive and innate immune response mechanisms by γ-herpesviruses
- Author
-
Klaus Früh, Ashlee V. Moses, and Pinghui Feng
- Subjects
Innate immune system ,animal diseases ,Innate lymphoid cell ,CCL18 ,Immune Targeting ,chemical and pharmacologic phenomena ,biochemical phenomena, metabolism, and nutrition ,Biology ,Acquired immune system ,Immunity, Innate ,Article ,Virus Latency ,Classical complement pathway ,Gammaherpesvirinae ,Immune system ,Virology ,Immunology ,Antigenic variation ,Humans ,bacteria ,Immune Evasion - Abstract
γ-Herpesviral immune evasion mechanisms are optimized to support the acute, lytic and the longterm, latent phase of infection. During acute infection, specific immune modulatory proteins limit, but also exploit, the antiviral activities of cell intrinsic innate immune responses as well as those of innate and adaptive immune cells. During latent infection, a restricted gene expression program limits immune targeting and cis-acting mechanisms to reduce the antigen presentation as well as antigenicity of latency-associated proteins. Here, we will review recent progress in our understanding of γ-herpesviral immune evasion strategies.
- Published
- 2013
- Full Text
- View/download PDF
42. Remodeling of Endothelial Adherens Junctions by Kaposi's Sarcoma-Associated Herpesvirus
- Author
-
Ashlee V. Moses, Mandana Mansouri, Klaus Früh, and Patrick P. Rose
- Subjects
Gene Expression Regulation, Viral ,Cell Survival ,Angiogenesis ,Immunology ,Biology ,medicine.disease_cause ,Cell morphology ,Microbiology ,Adherens junction ,Vasculogenesis ,Virology ,Cell Adhesion ,Electric Impedance ,medicine ,Humans ,Biotinylation ,Kaposi's sarcoma-associated herpesvirus ,Cell adhesion ,Cytoskeleton ,Cell Proliferation ,Skin ,Ubiquitin ,Cell Membrane ,Catenins ,Adherens Junctions ,Actin cytoskeleton ,Actins ,Virus-Cell Interactions ,Cell biology ,Insect Science ,Catenin ,Herpesvirus 8, Human - Abstract
Vascular endothelial cadherin (VE-cadherin) connects neighboring endothelial cells (ECs) via interendothelial junctions and regulates EC proliferation and adhesion during vasculogenesis and angiogenesis. The cytoplasmic domain of VE-cadherin recruits α- and β-catenins and γ-catenin, which interact with the actin cytoskeleton, thus modulating cell morphology. Dysregulation of the adherens junction/cytoskeletal axis is a hallmark of invasive tumors. We now demonstrate that the transmembrane ubiquitin ligase K5/MIR-2 of Kaposi's sarcoma-associated herpesvirus targets VE-cadherin for ubiquitin-mediated destruction, thus disturbing EC adhesion. In contrast, N-cadherin levels in K5-expressing cells were increased compared to those in control cells. Steady-state levels of α- and β-catenins and γ-catenin in K5-expressing ECs were drastically reduced due to proteasomal destruction. Moreover, the actin cytoskeleton was rearranged, resulting in the dysregulation of EC barrier function as measured by electric cell-substrate impedance sensing. Our data represent the first example of a viral protein targeting adherens junction proteins and suggest that K5 contributes to EC proliferation, vascular leakage, and the reprogramming of the EC proteome during Kaposi's sarcoma tumorigenesis.
- Published
- 2008
- Full Text
- View/download PDF
43. The Role of Angiogenic and Wound Repair Factors During CMV-Accelerated Transplant Vascular Sclerosis in Rat Cardiac Transplants
- Author
-
Susan L. Orloff, Ashlee V. Moses, Patsy Smith, Daniel N. Streblow, T. Andoh, Jay A. Nelson, Victor R. DeFilippis, Craig N. Kreklywich, Jerome Dumortier, and Klaus Früh
- Subjects
Male ,Human cytomegalovirus ,Angiogenesis ,Cytomegalovirus ,Neovascularization, Physiologic ,Coronary Artery Disease ,Downregulation and upregulation ,Betaherpesvirinae ,medicine ,Animals ,Transplantation, Homologous ,Immunology and Allergy ,Pharmacology (medical) ,Oligonucleotide Array Sequence Analysis ,Wound Healing ,Transplantation ,Genome ,biology ,Reverse Transcriptase Polymerase Chain Reaction ,business.industry ,medicine.disease ,biology.organism_classification ,Matrix Metalloproteinases ,Rats, Inbred F344 ,Rats ,Endothelial stem cell ,Disease Models, Animal ,Viral replication ,Rats, Inbred Lew ,Cytomegalovirus Infections ,Immunology ,Cancer research ,Heart Transplantation ,Wound healing ,business - Abstract
Human cytomegalovirus (HCMV) accelerates transplant vascular sclerosis (TVS), a consequence of angiogenesis (AG) and wound repair (WR). While HCMV can be localized to TVS lesions, the low number of infected cells suggests a global effect on target tissues. We used microarray analysis followed by real-time-polymerase chain reaction (RT-PCR) in an RCMV-accelerated TVS rat cardiac transplant model to determine whether CMV activates host WR and AG factors. Dysregulated cellular genes in allografts from RCMV-infected recipients were compared to those from uninfected recipients and native hearts. We demonstrated that RCMV upregulates the genes involved in WR and AG, which was highest during the critical time of TVS acceleration (21-28 days). Using a standard in vitro AG assay, virus and serum-free supernatants collected at 48 h postinfection significantly induced endothelial cell (EC) migration, branching and tubule formation compared to supernatants from mock-infected cells. Supernatants from ultraviolet (UV)-inactivated RCMV-infected cells failed to induce AG, indicating that virus replication is required. Upregulation of WR and AG genes occurs during the critical period of CMV-accelerated TVS. Targeting these genes may prevent this process and improve allograft survival.
- Published
- 2008
- Full Text
- View/download PDF
44. Kaposi Sarcoma Herpesvirus Induces HO-1 during De Novo Infection of Endothelial Cells via Viral miRNA-Dependent and -Independent Mechanisms
- Author
-
Jean K. Gustin, Ashlee V. Moses, Jennifer Totonchy, and Sara Botto
- Subjects
viruses ,Cell ,Biology ,medicine.disease_cause ,Microbiology ,Proinflammatory cytokine ,03 medical and health sciences ,chemistry.chemical_compound ,0302 clinical medicine ,Downregulation and upregulation ,Virology ,Gene expression ,Virus latency ,medicine ,Heme ,030304 developmental biology ,Regulation of gene expression ,0303 health sciences ,Endothelial Cells ,medicine.disease ,QR1-502 ,Up-Regulation ,Virus Latency ,3. Good health ,Cell biology ,MicroRNAs ,medicine.anatomical_structure ,Gene Expression Regulation ,Biochemistry ,chemistry ,030220 oncology & carcinogenesis ,Herpesvirus 8, Human ,Host-Pathogen Interactions ,RNA, Viral ,Carcinogenesis ,Gene Deletion ,Heme Oxygenase-1 ,Research Article - Abstract
Kaposi sarcoma (KS) herpesvirus (KSHV) infection of endothelial cells (EC) is associated with strong induction of heme oxygenase-1 (HO-1), a stress-inducible host gene that encodes the rate-limiting enzyme responsible for heme catabolism. KS is an angioproliferative tumor characterized by the proliferation of KSHV-infected spindle cells, and HO-1 is highly expressed in such cells. HO-1 converts the pro-oxidant, proinflammatory heme molecule into metabolites with antioxidant, anti-inflammatory, and proliferative activities. Previously published work has shown that KSHV-infected EC in vitro proliferate in response to free heme in a HO-1-dependent manner, thus implicating virus-enhanced HO-1 activity in KS tumorigenesis. The present study investigated the molecular mechanisms underlying KSHV induction of HO-1 in lymphatic EC (LEC), which are the likely spindle cell precursors. In a time course analysis of KSHV-infected cells, HO-1 expression displays biphasic kinetics characterized by an early transient induction that is followed by a more sustained upregulation coincident with the establishment of viral latency. A viral microRNA miR-K12-11 deletion mutant of KSHV was found to be defective for induction of HO-1 during latency. A potential mechanism for this phenotype was provided by BACH1, a cellular HO-1 transcriptional repressor targeted by miR-K12-11. In fact, in KSHV-infected LEC, the BACH1 message level is reduced, BACH1 subcellular localization is altered, and miR-K12-11 mediates the inverse regulation of HO-1 and BACH1 during viral latency. Interestingly, the data indicate that neither miR-K12-11 nor de novo KSHV gene expression is required for the burst of HO-1 expression observed at early times postinfection, which suggests that additional virion components promote this phenotype., IMPORTANCE While the mechanisms underlying KSHV induction of HO-1 remain unknown, the cellular mechanisms that regulate HO-1 expression have been extensively investigated in the context of basal and pathophysiological states. The detoxifying action of HO-1 is critical for the protection of cells exposed to high heme levels. KS spindle cells are erythrophagocytic and contain erythrocyte ghosts. Erythrocyte degeneration leads to the localized release of heme, creating oxidative stress that may be further exacerbated by environmental or other cofactors. Our previous work showed that KSHV-infected cells proliferate in response to heme and that this occurs in a HO-1-dependent manner. We therefore hypothesize that KSHV induction of HO-1 contributes to KS tumor development via heme metabolism and propose that HO-1 be evaluated as a therapeutic target for KS. Our present work, which aimed to understand the mechanisms whereby KSHV induces HO-1, will be important for the design and implementation of such a strategy.
- Published
- 2015
- Full Text
- View/download PDF
45. Ebola Virus Glycoprotein Promotes Enhanced Viral Egress by Preventing Ebola VP40 From Associating With the Host Restriction Factor BST2/Tetherin
- Author
-
Jean K. Gustin, Janet L. Douglas, Ashlee V. Moses, and Ying Bai
- Subjects
viruses ,Down-Regulation ,Receptors, Cell Surface ,Biology ,medicine.disease_cause ,GPI-Linked Proteins ,Cell Line ,Viral Matrix Proteins ,Viral Proteins ,Immune system ,VP40 ,Viral envelope ,Antigens, CD ,medicine ,Immunology and Allergy ,Humans ,Ebola and Marburg Viruses-Research, Outbreak Management, Epidemiology and Ecology ,Receptor ,Virus Release ,Glycoproteins ,chemistry.chemical_classification ,Innate immune system ,Ebola virus ,Mucins ,virus diseases ,Ebolavirus ,Virology ,Infectious Diseases ,HEK293 Cells ,chemistry ,Mutation ,Tetherin ,Glycoprotein - Abstract
Background BST2/tetherin is an innate immune molecule with the unique ability to restrict the egress of human immunodeficiency virus (HIV) and other enveloped viruses, including Ebola virus (EBOV). Coincident with this discovery was the finding that the HIV Vpu protein down-regulates BST2 from the cell surface, thereby promoting viral release. Evidence suggests that the EBOV envelope glycoprotein (GP) also counteracts BST2, although the mechanism is unclear. Results We find that total levels of BST2 remain unchanged in the presence of GP, whereas surface BST2 is significantly reduced. GP is known to sterically mask surface receptors via its mucin domain. Our evaluation of mutant GP molecules indicate that masking of BST2 by GP is probably responsible for the apparent surface BST2 down-regulation; however, this masking does not explain the observed virus-like particle egress enhancement. We discovered that VP40 coimmunoprecipitates and colocalizes with BST2 in the absence but not in the presence of GP. Conclusions These results suggest that GP may overcome the BST2 restriction by blocking an interaction between VP40 and BST2. Furthermore, we have observed that GP may enhance BST2 incorporation into virus-like particles. Understanding this novel EBOV immune evasion strategy will provide valuable insights into the pathogenicity of this deadly pathogen.
- Published
- 2015
46. The insulin receptor is essential for virus-induced tumorigenesis of Kaposi's sarcoma
- Author
-
Victor R. DeFilippis, J M Carroll, Patrick P. Rose, Klaus Früh, Ashlee V. Moses, M Lagunoff, Charles T. Roberts, and P A Carroll
- Subjects
Cancer Research ,medicine.medical_treatment ,Organophosphonates ,Naphthalenes ,Receptor, IGF Type 1 ,Insulin-like growth factor ,Growth factor receptor ,Genetics ,medicine ,Humans ,Gammaherpesvirinae ,RNA, Small Interfering ,Receptor ,Sarcoma, Kaposi ,Molecular Biology ,Kaposi's sarcoma ,Cell Line, Transformed ,biology ,Growth factor ,Endothelial Cells ,virus diseases ,Cell Transformation, Viral ,medicine.disease ,biology.organism_classification ,Receptor, Insulin ,Insulin receptor ,Herpesvirus 8, Human ,biology.protein ,Cancer research ,Primary effusion lymphoma ,Mitogen-Activated Protein Kinases - Abstract
Kaposi sarcoma (KS), a multifocal neoplasm of the skin that can spread to visceral organs, is the most prevalent malignant tumor in acquired immuno deficiency syndrome (AIDS) patients. KS-associated herpesvirus (KSHV or HHV8) is considered the primary etiological factor of this malignancy, as well as of primary effusion lymphoma and multicentric Castleman's disease. KS lesions are characterized by proliferating spindle cells of endothelial cell (EC) origin. The action of the insulin-like growth factor (IGF) system has been implicated in many malignancies, and recent data have demonstrated that the IGF-I receptor (IGF-IR) is required for in vitro growth of the KS-derived KSIMM cell line. To examine whether the IGF pathway is also involved in KSHV-mediated transformation of ECs, we examined the expression and function of the IGF system in KSHV-infected, immortalized dermal microvascular EC (E-DMVEC). The expression of the insulin receptor (IR) was strongly induced in latently infected E-DMVEC, whereas the expression levels of the IGF-IR remained unchanged. Gene knockdown of IR, but not IGF-IR, prevented the characteristic focus formation seen in KSHV-infected E-DMVEC. Similarly, treatment with the IR-specific small-molecule inhibitor HNMPA-(AM(3)) inhibited postconfluent growth. These data suggest a role for the IR, but not the IGF-IR, in KSHV-induced transformation of vascular ECs.
- Published
- 2006
- Full Text
- View/download PDF
47. Kaposi sarcoma herpesvirus K5 removes CD31/PECAM from endothelial cells
- Author
-
Gary Thomas, Janet Douglas, Ashlee V. Moses, Patrick P. Rose, Klaus Früh, Robert E. Means, Kristine Gouveia, and Mandana Mansouri
- Subjects
CD31 ,Proteasome Endopeptidase Complex ,Ubiquitin-Protein Ligases ,Immunology ,Antigen presentation ,Vesicular Transport Proteins ,Down-Regulation ,Biology ,Endocytosis ,Biochemistry ,Substrate Specificity ,Viral Proteins ,Ubiquitin ,Cell Movement ,Humans ,Sarcoma, Kaposi ,Cells, Cultured ,Adaptor Proteins, Signal Transducing ,Immunobiology ,Cell adhesion molecule ,Endoplasmic reticulum ,Endothelial Cells ,Cell Biology ,Hematology ,Cell biology ,Ubiquitin ligase ,Platelet Endothelial Cell Adhesion Molecule-1 ,Proteasome ,Herpesvirus 8, Human ,cardiovascular system ,biology.protein - Abstract
The transmembrane ubiquitin ligase K5/MIR2 of Kaposi sarcoma herpesvirus (KSHV) mediates internalization and lysosomal degradation of glycoproteins involved in antigen presentation and co-stimulation. In endothelial cells (ECs), K5 additionally reduced expression of CD31/platelet–endothelial cell adhesion molecule (PECAM), an adhesion molecule regulating cell-cell interactions of ECs, platelets, monocytes, and T cells. K5 also reduced EC migration, a CD31-dependent process. Unlike other K5 substrates, both newly synthesized and pre-existing CD31 molecules were targeted by K5. K5 was transported to the cell surface and ubiquitinated pre-existing CD31, resulting in endocytosis and lysosomal degradation. In the endoplasmic reticulum, newly synthesized CD31 was degraded by proteasomes, which required binding of phosphofurin acidic cluster sorting protein-2 (PACS-2) to acidic residues in the carboxyterminal tail of K5. Thus, CD31, a novel target of K5, is efficiently removed from ECs by a dual degradation mechanism that is regulated by the subcellular sorting of the ubiquitin ligase. K5-mediated degradation of CD31 is likely to affect EC function in KS tumors.
- Published
- 2006
- Full Text
- View/download PDF
48. Novel Cellular Genes Essential for Transformation of Endothelial Cells by Kaposi's Sarcoma–Associated Herpesvirus
- Author
-
Ashlee V. Moses, Klaus Früh, Shane C McAllister, Bruce J. Dezube, Henry B. Koon, Rebecca Ruhl, and Camilo Raggo
- Subjects
Cancer Research ,Small interfering RNA ,Sialoglycoproteins ,Mice, Nude ,Biology ,GPI-Linked Proteins ,medicine.disease_cause ,3T3 cells ,Receptors, G-Protein-Coupled ,Transcriptome ,Mice ,Proto-Oncogene Proteins ,Metalloproteins ,medicine ,Animals ,Humans ,RNA, Small Interfering ,Kaposi's sarcoma-associated herpesvirus ,Sarcoma, Kaposi ,Adaptor Proteins, Signal Transducing ,Oligonucleotide Array Sequence Analysis ,Receptors, CXCR ,Cell growth ,Gene Expression Profiling ,Neuropeptides ,Endothelial Cells ,Oncogenes ,LIM Domain Proteins ,Oligonucleotides, Antisense ,Cell Transformation, Viral ,Virology ,Cell biology ,DNA-Binding Proteins ,Endothelial stem cell ,medicine.anatomical_structure ,Oncology ,Herpesvirus 8, Human ,NIH 3T3 Cells ,Osteopontin ,Receptors, Chemokine ,Ectopic expression ,Carcinogenesis - Abstract
Kaposi's sarcoma–associated herpesvirus (KSHV) is involved in the development of lymphoproliferative diseases and Kaposi's sarcoma. The oncogenicity of this virus is reflected in vitro by its ability to transform B cells and endothelial cells. Infection of dermal microvascular endothelial cells (DMVEC) transforms the cells from a cobblestone-like monolayer to foci-forming spindle cells. This transformation is accompanied by dramatic changes in the cellular transcriptome. Known oncogenes, such as c-Kit, are among the KSHV-induced host genes. We previously showed that c-Kit is an essential cellular component of the KSHV-mediated transformation of DMVEC. Here, we test the hypothesis that the transformation process can be used to discover novel oncogenes. When expression of a panel of KSHV-induced cellular transcripts was inhibited with antisense oligomers, we observed inhibition of DMVEC proliferation and foci formation using antisense molecules to RDC1 and Neuritin. We further showed that transformation of KSHV-infected DMVEC was inhibited by small interfering RNA directed at RDC1 or Neuritin. Ectopic expression of Neuritin in NIH 3T3 cells resulted in changes in cell morphology and anchorage-independent growth, whereas RDC1 ectopic expression significantly increased cell proliferation. In addition, both RDC1- and Neuritin-expressing cells formed tumors in nude mice. RDC1 is an orphan G protein–coupled receptor, whereas Neuritin is a growth-promoting protein known to mediate neurite outgrowth. Neither gene has been previously implicated in tumorigenesis. Our data suggest that KSHV-mediated transformation involves exploitation of the hitherto unrealized oncogenic properties of RDC1 and Neuritin.
- Published
- 2005
- Full Text
- View/download PDF
49. Increased Efficiency of Phorbol Ester-Induced Lytic Reactivation of Kaposi's Sarcoma-Associated Herpesvirus during S Phase
- Author
-
Janko Nikolich-Zugich, Ashlee V. Moses, Shane C McAllister, Scott G. Hansen, and Ilhem Messaoudi
- Subjects
DNA Replication ,Gene Expression Regulation, Viral ,Genes, Viral ,viruses ,Immunology ,Replication ,Context (language use) ,Virus Replication ,medicine.disease_cause ,Microbiology ,Herpesviridae ,Virus ,S Phase ,Virology ,Phorbol Esters ,Tumor Cells, Cultured ,medicine ,Gammaherpesvirinae ,Kaposi's sarcoma-associated herpesvirus ,Sarcoma, Kaposi ,S phase ,biology ,virus diseases ,Fibroblasts ,biology.organism_classification ,Viral replication ,Lytic cycle ,Insect Science ,DNA, Viral ,Herpesvirus 8, Human - Abstract
Expression of Kaposi's sarcoma-associated herpesvirus (KSHV) lytic genes is thought to be essential for the establishment and progression of KSHV-induced diseases. The inefficiency of lytic reactivation in various in vitro systems hampers the study of lytic genes in the context of whole virus. We report here increased expression of KSHV lytic genes and increased release of progeny virus when synchronized cultures of body cavity-based lymphoma-1 cells are treated with a phorbol ester during S phase of the cell cycle.
- Published
- 2005
- Full Text
- View/download PDF
50. Transendothelial migration of CD16+ monocytes in response to fractalkine under constitutive and inflammatory conditions
- Author
-
Dana Gabuzda, Petronela Ancuta, and Ashlee V. Moses
- Subjects
Umbilical Veins ,Chemokine ,Receptors, CCR2 ,Immunology ,Inflammation ,CD16 ,Monocytes ,Interferon-gamma ,chemistry.chemical_compound ,Cell Movement ,Cell Adhesion ,medicine ,Humans ,Immunology and Allergy ,VCAM-1 ,CX3CL1 ,Cells, Cultured ,ICAM-1 ,biology ,Chemokine CX3CL1 ,Tumor Necrosis Factor-alpha ,Monocyte ,Receptors, IgG ,Brain ,Membrane Proteins ,Hematology ,Chemokines, CX3C ,Cell biology ,medicine.anatomical_structure ,chemistry ,biology.protein ,Receptors, Chemokine ,Tumor necrosis factor alpha ,Endothelium, Vascular ,medicine.symptom ,Cell Adhesion Molecules - Abstract
CD16+ monocytes represent 5-10% of circulating monocytes in healthy individuals and are dramatically expanded in several pathological conditions including AIDS and HIV-1-associated dementia (HAD). CD16+ monocytes constitutively produce high levels of pro-inflammatory cytokines and neurotoxic factors that may contribute to the pathogenesis of these disorders. Monocyte recruitment into the central nervous system (CNS) and other peripheral tissues in response to locally produced chemokines is a critical event in immune surveillance and inflammation and involves monocyte arrest onto vascular beds and subsequent diapedesis. Here we investigate the ability of CD16+ monocytes to undergo transendothelial migration (TEM) under constitutive and inflammatory conditions. CD16+ monocytes underwent TEM across unstimulated human umbilical vascular (HUVEC) and brain microvascular endothelial (BMVEC) cell monolayers in response to soluble fractalkine (FKN/CX3CL1). Stimulation with tumor necrosis factor (TNF) and interferon-gamma (IFN-gamma) induced high and low expression of membrane-bound FKN on HUVEC and BMVEC, respectively, together with expression of VCAM-1 and intercellular adhesion molecule-1 (ICAM)-1. By contrast, only HUVEC expressed CD62E while BMVEC remained negative. Both CD16- and CD16+ monocyte subsets adhered to TNF/IFN-gamma-stimulated HUVEC with higher frequency than to unstimulated HUVEC. Monocyte chemoattractant protein-1 (MCP-1) triggered efficient TEM of CD16- monocytes across TNF/IFN-gamma-stimulated HUVEC, whereas soluble FKN failed to induce TEM of CD16+ monocytes across stimulated HUVEC. These results demonstrate that stimulation with TNF and IFN-gamma triggers expression of membrane-bound FKN on both HUVEC and BMVEC, but prevents TEM of CD16+ monocytes in response to soluble FKN. Thus, pro-inflammatory CD16+ monocytes may contribute to the pathogenesis of HAD and other inflammatory CNS diseases by affecting the integrity of the blood-brain barrier as a consequence of their massive accumulation onto inflamed brain vascular endothelial cells expressing FKN and other adhesion molecules.
- Published
- 2004
- Full Text
- View/download PDF
Catalog
Discovery Service for Jio Institute Digital Library
For full access to our library's resources, please sign in.