Your search keyword '"Gene Products, env analysis"' showing total 105 results

1. Monitoring the Transcriptional Activity of Human Endogenous Retroviral HERV-W Family Using PNA Strand Invasion into Double-Stranded DNA.

Author

Machnik G, Skudrzyk E, Bułdak Ł, Ruczyński J, Kozłowska A, Mucha P, Rekowski P, Szkróbka W, Basiak M, Bołdys A, Sławska H, and Okopień B

Subjects

Adult, Cell Line, Cell Line, Tumor, DNA genetics, DNA metabolism, Endogenous Retroviruses growth & development, Endogenous Retroviruses metabolism, Female, Gene Products, env genetics, Gene Products, env metabolism, Humans, Peptide Nucleic Acids metabolism, Plasmids chemistry, Plasmids metabolism, Polymerase Chain Reaction methods, Pregnancy, Pregnancy Proteins genetics, Pregnancy Proteins metabolism, Transcription, Genetic, Astrocytes virology, Endogenous Retroviruses genetics, Gene Products, env analysis, Peptide Nucleic Acids genetics, Placenta virology, Pregnancy Proteins analysis, Virus Replication genetics

Abstract

In the presented assay, we elaborated a method for distinguishing sequences that are genetically closely related to each other. This is particularly important in a situation where a fine balance of the allele abundance is a point of research interest. We developed a peptide nucleic acid (PNA) strand invasion technique for the differentiation between multiple sclerosis-associated retrovirus (MSRV) and ERVWE1 sequences, both molecularly similar, belonging to the human endogenous retrovirus HERV-W family. We have found that this method may support the PCR technique in screening for minor alleles which, in certain conditions, may be undetected by the standard PCR technique. We performed the analysis of different ERVWE1 and MSRV template mixtures ranging from 0 to 100% of ERVWE1 in the studied samples, finding the linear correlation between template composition and signal intensity of final reaction products. Using the PNA strand invasion assay, we were able to estimate the relative ERVWE1 expression level in human specimens such as U-87 MG, normal human astrocytes cell lines and placental tissue. The results remained in concordance with those obtained by semi-quantitative or quantitative PCR.

Published

2018

2. Transmission of Porcine Endogenous Retrovirus Produced from Different Recipient Cells In Vivo.

Author

Kim N, Choi J, Kim S, Gwon YD, Cho Y, Yang JM, Oh YK, and Kim YB

Subjects

Animals, CD4-Positive T-Lymphocytes immunology, CD4-Positive T-Lymphocytes virology, CD8-Positive T-Lymphocytes immunology, CD8-Positive T-Lymphocytes virology, Endogenous Retroviruses isolation & purification, Gene Products, env analysis, Genome, Viral, Humans, Immunity, Cellular, Mice, Mice, Inbred NOD, NIH 3T3 Cells transplantation, NIH 3T3 Cells virology, Swine genetics, Zoonoses immunology, Zoonoses virology, Cell Transplantation, Endogenous Retroviruses genetics, Swine virology, Transplantation, Heterologous, Zoonoses genetics, Zoonoses transmission

Abstract

Humanized pigs have been developed to reduce the incidence of immune rejection in xenotransplantation, but significant concerns remain, such as transmission of viral zoonosis. Porcine endogenous retroviruses (PERV), which exist in the genome of pigs, are produced as infectious virions from all porcine cells and cause zoonosis. Here, we examined the possibility of zoonosis of hosts under conditions of immune suppression or xenotransplantation of cells producing host-adapted viruses. Upon transplantation of PERV-producing porcine cells into mice, no transmission of PERV was detected, whereas, transmission of PERV from mice transplanted with mouse-adapted PERV-producing cells was detected. In addition, the frequency of PERV transmission was increased in CsA treated mice transplanted with PERV-producing murine cells, compared with PERV-producing porcine cells. Transmission of PERV to host animals did not affect weight but immune responses, in particular, the number of T cells from PERV-transmitted mice, were notably reduced. The observed risk of PERV zoonosis highlights the requirement for thorough evaluation of viral zoonosis under particular host conditions, such as immunosuppressive treatment and transplantation with host-adapted virus-producing cells., Competing Interests: The authors have declared that no competing interests exist.

Published

2016

3. Expression of Syncytin 1 (HERV-W), in the preimplantation human blastocyst, embryonic stem cells and trophoblast cells derived in vitro.

Author

Soygur B and Moore H

Subjects

Blotting, Western, Cell Differentiation, Gene Products, env analysis, Humans, Microscopy, Fluorescence, Pregnancy Proteins analysis, Blastocyst metabolism, Embryonic Stem Cells metabolism, Gene Products, env metabolism, Pregnancy Proteins metabolism, Trophoblasts metabolism

Abstract

Study Question: As Syncytin 1 (human endogenous retrovirus (HERV-W)) is crucial for human embryo placentation is it expressed during preimplantation embryo development?, Summary Answer: Syncytin 1 was expressed mainly in trophoblast cells of the blastocyst particularly in cells underlying the inner cell mass (ICM)., What Is Known Already: Syncytin 1 (along with HERV-FRD or Syncytin 2) is expressed in first-trimester placenta and required for cell-cell fusion to enable formation of syncytiotrophoblast and effective placentation., Study Design, Size and Duration: Preimplantation human embryos donated for research were cultured in vitro and protein expression of Syncytin 1 at the blastocyst stage of development investigated. Comparisons were made with protein (Syncytin 1) and mRNA (Syncytin 1 and 2) expression in human embryonic stem cells (hESCs) undergoing differentiation to trophoblast-like cells in vitro. In total, 10 blastocysts (×3 or 4 replicates) were analysed and 4 hESC lines. The study was terminated after consistent observations of embryos were made., Participants/materials, Setting, Methods: Donated embryos were thawed and cultured to blastocyst, fixed with 4% w/v paraformaldehyde. Syncytin 1 protein expression was determined by immunofluorescent localisation and confocal microscopy. Additionally, hESCs were differentiated to trophoblast-like cells in standard and conditioned culture medium with growth factors (bone morphogenetic protein 4 (BMP4) or fibroblast growth factor 4 (FGF4) and assessed for mRNA (Syncytin 1 and 2) by quantitative polymerase chain reaction (qPCR) and protein expression by immunolocalization and western blot., Main Results and Role of Chance: Syncytin 1 was expressed in cytoplasm and on the cell surface of some trophoblast cells, and consistently the trophectoderm underlying the ICM of the blastocyst. There was weak but consistent expression of Syncytin 1 in cells on the periphery of the ICM also displaying pluripotency antibody marker (Tra-1-60). Three-dimensional reconstruction of confocal slice data provided good visualization of expression. The time course of expression of Syncytin 1 was replicated in hESCs differentiated in vitro confirming the embryo observations and providing statistically significant differences in protein and mRNA level (P= 0.002) and (P< 0.05), respectively., Limitation, Reasons for Caution: Culture of a limited number of embryos to blastocyst in vitro may not replicate the range and quality of development in situ. Probes (antibodies, PCR) were tested for specificity, but might have non-specific reactions., Wider Implications of Findings: Syncytin expression is a prerequisite for embryo implantation and placentation. Understanding when expression first occurs during embryo development may be informative for understanding conditions of abnormal gestations such as pre-clampsia., Study Funding/competing Interests: The study was supported partly by an ERASMUS training grant and grant G0801059 from the Medical Research Council, U.K. There were no competing interests., (© The Author 2016. Published by Oxford University Press on behalf of the European Society of Human Reproduction and Embryology. All rights reserved. For Permissions, please email: journals.permissions@oup.com.)

Published

2016

4. Human endogenous retrovirus (HERV) expression is not induced by treatment with the histone deacetylase (HDAC) inhibitors in cellular models of HIV-1 latency.

Author

Hurst T, Pace M, Katzourakis A, Phillips R, Klenerman P, Frater J, and Magiorkinis G

Subjects

Cell Line, Gene Products, env analysis, Gene Products, env genetics, Gene Products, pol analysis, Gene Products, pol genetics, Humans, Monocytes drug effects, Monocytes virology, T-Lymphocytes drug effects, T-Lymphocytes virology, Transcription, Genetic, Endogenous Retroviruses drug effects, Endogenous Retroviruses physiology, HIV-1 drug effects, Histone Deacetylase Inhibitors metabolism, Proviruses drug effects, Proviruses physiology, Virus Activation drug effects

Abstract

Background: While antiretroviral therapies have improved life expectancy and reduced viral loads in HIV-1-positive individuals, the cessation of treatment results in a rebound of viral replication. This suggests that a reservoir of latently-infected cells remains within these patients, the identity of which is ill-defined and therefore difficult to target therapeutically. Current strategies are aimed at using drugs such as histone deacetylase (HDAC) inhibitors to induce the expression of latent HIV-1 proviruses in order to activate and ultimately eradicate this reservoir of infected cells. One concern with the use of HDAC inhibitors is that they could up-regulate human endogenous retroviruses (HERVs), as well as HIV-1, with potentially pathophysiological consequences., Results: In this study, we analysed the transcription of HERV genes in HIV-1 latency T cell (J-LAT 8.4) and monocyte (U1) models following treatment with the HDAC inhibitors, vorinostat, panobinostat and romidepsin. We examined the expression of HERV-K (HML-2) env and pol, as well as the co-opted genes HERV-W env (syncytin-1), HERV-FRD env (syncytin-2), in these cell lines. Finally, we investigated HERV expression in primary human T cells., Conclusions: We show that HDAC inhibitors did not substantially increase the transcription of the analysed HERV env or pol genes, suggesting that histone acetylation is not crucial for controlling HERV expression in these experimental models and in ex vivo primary human T cells. Importantly, this indicates that unwanted HERV expression does not appear to be a barrier to the use of HDAC inhibitors in HIV-1 cure strategies.

Published

2016

5. Morphological changes of placental syncytium and their implications for the pathogenesis of preeclampsia.

Author

Roland CS, Hu J, Ren CE, Chen H, Li J, Varvoutis MS, Leaphart LW, Byck DB, Zhu X, and Jiang SW

Subjects

Animals, Apoptosis, Cell Fusion, Cell Proliferation, Female, Gene Products, env analysis, Gene Products, env metabolism, Giant Cells cytology, Giant Cells metabolism, Humans, Placenta cytology, Placenta metabolism, Pre-Eclampsia metabolism, Pregnancy, Pregnancy Proteins analysis, Pregnancy Proteins metabolism, Trophoblasts cytology, Trophoblasts metabolism, Giant Cells pathology, Placenta pathology, Pre-Eclampsia pathology, Trophoblasts pathology

Abstract

Preeclampsia is a hypertensive disease that complicates many pregnancies, typically presenting with new-onset or worsening hypertension and proteinuria. It is well recognized that the placental syncytium plays a key role in the pathogenesis of preeclampsia. This review summarizes the findings pertaining to the structural alterations in the syncytium of preeclamptic placentas and analyzes their pathological implications for the development of preeclampsia. Changes in the trophoblastic lineage, including those in the proliferation of cytotrophoblasts, the formation of syncytiotrophoblast through cell fusion, cell apoptosis and syncytial deportation, are discussed in the context of preeclampsia. Extensive correlations are made between functional deficiencies and the alterations on the levels of gross anatomy, tissue histology, cellular events, ultrastructure, molecular pathways, and gene expression. Attention is given to the significance of dynamic changes in the syncytial turnover in preeclamptic placentas. Specifically, experimental evidences for the complex and obligatory role of syncytin-1 in cell fusion, cell-cycle regulation at the G1/S transition, and apoptosis through AIF-mediated pathway, are discussed in detail in the context of syncytium homeostasis. Finally, the recent observations on the aberrant fibrin deposition in the trophoblastic layer and the trophoblast immature phenotype in preeclamptic placentas and their potential pathogenic impact are also reviewed.

Published

2016

6. Natalizumab inhibits the expression of human endogenous retroviruses of the W family in multiple sclerosis patients: a longitudinal cohort study.

Author

Arru G, Leoni S, Pugliatti M, Mei A, Serra C, Delogu LG, Manetti R, Dolei A, Sotgiu S, and Mameli G

Subjects

Adult, Cohort Studies, Female, Flow Cytometry, Humans, Leukocytes, Mononuclear virology, Longitudinal Studies, Male, Middle Aged, Natalizumab, Real-Time Polymerase Chain Reaction, Reverse Transcriptase Polymerase Chain Reaction, Young Adult, Antibodies, Monoclonal, Humanized therapeutic use, Endogenous Retroviruses drug effects, Gene Products, env analysis, Multiple Sclerosis, Relapsing-Remitting drug therapy, Multiple Sclerosis, Relapsing-Remitting virology, Pregnancy Proteins analysis

Abstract

Background: Several viruses were reported as co-factors triggering the pathogenesis of multiple sclerosis (MS), including the endogenous retroviruses of the HERV-W family, that were also proposed as biomarkers of disease progression and therapy outcome., Objective: The objective of this article is to clarify whether in MS patients treatment with natalizumab has effects on MSRV/syncytin-1/HERV-W expression and the possible relationship with disease outcome., Methods: Peripheral blood mononuclear cells were collected from 22 patients with relapsing-remitting disease, at entry and after three, six and 12 months of treatment with natalizumab. The cell subpopulations and the expression of MSRVenv/syncytin-1/HERV-Wenv were analyzed by flow cytometry and by discriminatory env-specific RT-PCR assays., Results: By flow cytometry the relative amounts of T, NK and monocyte subpopulations were shown to remain fairly constant. A relative increase of B lymphocytes was observed at three to six months (p = 0.033). The MSRVenv and syncitin-1 transcripts were reduced at six to 12 months of therapy (p = 0.0001). Accordingly, at month 12, the plasma-membrane levels of the HERV-Wenv protein were reduced (p = 0.0001). B cells, NK and monocytes but not T cells expressed the HERV-Wenv protein. None of the patients relapsed during therapy., Conclusion: Effective therapy with natalizumab downregulates MSRV/syncytin-1/HERV-W expression.

Published

2014

7. Human ERV3-1 env protein expression in various human tissues and tumours.

Author

Kang YJ, Jo JO, Ock MS, Chang HK, Baek KW, Lee JR, Choi YH, Kim WJ, Leem SH, Kim HS, and Cha HJ

Subjects

Blotting, Western, Humans, Immunohistochemistry, Tissue Array Analysis, Gene Products, env analysis, Neoplasms virology, Retroviridae Infections

Published

2014

8. Identification and characterization of a nuclear factor-κ B-p65 proteolytic fragment in nuclei of porcine hepatocytes in monolayer culture.

Author

Caperna TJ, Shannon AE, Garrett WM, Ramsay TG, Blomberg LA, and Elsasser TH

Subjects

Animals, Blotting, Western, Cells, Cultured, Chymotrypsin metabolism, Hepatocytes chemistry, NF-kappa B metabolism, Trypsin metabolism, Tumor Necrosis Factor-alpha pharmacology, Cell Nucleus chemistry, Gene Products, env analysis, Hepatocytes ultrastructure, NF-kappa B chemistry, Peptide Fragments analysis, Swine

Abstract

Hepatic responses to proinflammatory signals are controlled by the activation of several transcription factors, including, nuclear factor-κ B (NF-κB). In this study, hepatocytes prepared from suckling pigs and maintained in serum-free monolayer culture were used to define a novel proinflammatory cytokine-specific NF-κB subunit modification. The immunoreactive p65 protein was detected by Western blot analysis at the appropriate molecular weight in the cytosol of control cultures and those incubated with tumor necrosis factor-α (TNF). However, in nuclei, the p65 antisera cross-reacted with a protein of approximately 38 kDa (termed p38) after TNF addition, which was not observed in the cytosol of control or cytokine-treated cells. Specifically, incubation with TNF also resulted in phosphorylation (P < 0.05) of the inhibitor complex protein (IκB), whereas incubation with other cytokines, IL-6, IL-17a, or oncostatin M was not associated with either phosphorylation of IκB or nuclear translocation of p65. Intracellular endothelial nitric oxide synthase was deceased (P < 0.05) and plasminogen activator inhibitor-1 secretion was increased (P < 0.05) after TNF incubation. The TNF-induced p38 protein was purified from hepatocyte nuclei by immunoprecipitation, concentrated by electrophoresis, and subsequently analyzed by mass spectrometry. Ten unique NF-κB p65 peptides were identified after digestion with trypsin and chymotrypsin; however, all were mapped to the N-terminus and within the first 310 amino acid residues of the intact p65 protein. Although low molecular weight immunoreactive p65 molecules were previously observed in various human and rodent systems, this is the first report to positively identify the p38 fragment within hepatocyte nuclei or after specific cytokine (TNF) induction., (Published by Elsevier Inc.)

Published

2013

9. Expression of human endogenous retrovirus-K coincides with that of micro-RNA-663 and -638 in germ-cell tumor cells.

Author

Kraus B, Mönk B, Sliva K, and Schnierle BS

Subjects

Blotting, Northern, Blotting, Western, Endogenous Retroviruses, Gene Products, env analysis, Gene Products, env biosynthesis, Humans, MicroRNAs genetics, Prognosis, Transcriptome, MicroRNAs biosynthesis, Neoplasms, Germ Cell and Embryonal genetics, Neoplasms, Germ Cell and Embryonal virology

Abstract

Background/aim: The cell line GH was established from germ-cell tumor tissue; human endogenous retrovirus-K (HERV-K) expression was detectable after prolonged culture of the cells, particularly in cells that formed domes and vesicles. In addition, keeping GH cells in culture at high cell densities increased HERV-K expression. Here, we studied whether this inducible HERV-K expression is accompanied by differences in microRNA (miRNA) expression patterns of GH cells., Materials and Methods: The global miRNA expression pattern of GH cell samples (HERV-K high versus low) was analyzed by miRNA arrays., Results: Two miRNAs were found to be differentially regulated and to exhibit expression parallel to that of HERV-K. The identified miRNAs-663 and -638, have been reported to be involved in multiple processes, including cellular senescence. However, induction of HERV-K expression did not change the cellular senescence status of GH cells., Conclusion: The expression of these two miRNAs might be useful as novel diagnostic and prognostic markers in patients with tumors.

Published

2012

10. Reduced expression of both syncytin 1 and syncytin 2 correlates with severity of preeclampsia.

Author

Vargas A, Toufaily C, LeBellego F, Rassart É, Lafond J, and Barbeau B

Subjects

Blotting, Western, Cells, Cultured cytology, Endogenous Retroviruses, Female, Gene Products, env analysis, Humans, Placenta chemistry, Pregnancy, Pregnancy Proteins analysis, RNA, Messenger analysis, Reverse Transcriptase Polymerase Chain Reaction, Trophoblasts, Gene Expression, Gene Products, env genetics, Pre-Eclampsia physiopathology, Pregnancy Proteins genetics

Abstract

Human endogenous retroviruses (HERVs) represent up to 8% of the human genome and express several of its genes in the placenta. Studies have demonstrated that HERV envelope proteins syncytins 1 and 2 play a crucial role in trophoblast fusion and placenta development. Here, we compared the levels of placental expression of syncytins with the severity of preeclampsia (PE) symptoms. Confocal microscopy experiments indicated a pronounced deficiency in cellular fusion in trophoblast cells from patients with PE when compared to controls. As determined by quantitative reverse transcriptase polymerase chain reaction (qRT-PCR) and Western blot analyses, syncytin mRNA and protein levels were decreased in PE placentas versus controls. Interestingly, syncytin 2 levels were more importantly impaired than syncytin 1. Our results further highlighted the existence of a correlation between the extent of the decrease in the expression levels of both fusogenic proteins and the degree of severity of PE symptoms. These HERV proteins could thereby be used as potential markers for the early diagnosis of PE.

Published

2011

11. Accelerated evolution of SIV env within the cerebral compartment in the setting of morphine-dependent rapid disease progression.

Author

Rivera-Amill V, Noel RJ Jr, García Y, Rivera I, Iszard M, Buch S, and Kumar A

Subjects

Animals, Brain Chemistry, Evolution, Molecular, Genotype, Macaca virology, Molecular Sequence Data, Morphine Dependence virology, Phenotype, Simian Acquired Immunodeficiency Syndrome genetics, Simian Acquired Immunodeficiency Syndrome virology, Brain virology, Disease Progression, Gene Products, env analysis, Gene Products, env genetics, Morphine Dependence complications, Simian Acquired Immunodeficiency Syndrome complications, Simian Immunodeficiency Virus genetics

Abstract

Human immunodeficiency virus-1 (HIV-1) and simian immunodeficiency virus (SIV) have been shown to compartmentalize within various tissues, including the brain. However, the evolution of viral quasispecies in the setting of drug abuse has not been characterized. The goal of this study was to examine viral evolution in the cerebral compartment of morphine-dependent and control macaques to determine its role in rapid disease progression. To address this issue, we analyzed the envelope (env) gene from proviral DNA in our SIV/SHIV macaque model of morphine dependence and AIDS. Analyses of proviral DNA revealed a direct correlation between total genetic changes and survival time. However, the rate of evolution during disease progression was higher in morphine-dependent and rapid-progressor macaques than was the rate of evolution in the control animals. This study provides additional insight into SIV envelope variation in the CNS of morphine-dependent macaques and genotypes that may have evolved in the brain and contributed to disease progression., (Copyright 2009 Elsevier Inc. All rights reserved.)

Published

2010

12. Detection of human mammary tumor virus proteins in human breast cancer cells.

Author

Melana SM, Nepomnaschy I, Hasa J, Djougarian A, Djougarian A, Holland JF, and Pogo BG

Subjects

Animals, Antibodies, Monoclonal immunology, Betaretrovirus isolation & purification, Breast Neoplasms immunology, Capsid Proteins immunology, Cross Reactions, Female, Gene Products, env immunology, Humans, Mammary Tumor Virus, Mouse isolation & purification, Mice, Tumor Cells, Cultured, Tumor Virus Infections immunology, Betaretrovirus immunology, Breast Neoplasms virology, Capsid Proteins analysis, Gene Products, env analysis, Mammary Tumor Virus, Mouse immunology, Tumor Virus Infections virology

Abstract

Mouse mammary tumor virus (MMTV) has been proven to induce mammary cancer in mice. MMTV-like env gene sequences have been detected in one-third of the human breast tumors studied. The whole proviral structure with 95% homology to MMTV was found in two human breast tumors and was designated as human mammary tumor virus (HMTV). HMTV viral particles with betaretroviral features have been isolated. In addition, a retrovirus called human betaretrovirus (HBRV), homologous to the mentioned retroviruses, has been isolated from tissues of patients with primary biliary cirrhosis. In this report, the expression of HMTV envelope (Env) and capsid (Ca) was detected in 10 primary cultures of human breast cancer containing HMTV sequences (MSSM) by Western blot and fluorescence activated cell sorting (FACS), using a panel of antibodies against HMTV Env, HBRV Env and Ca and the MMTV Env Gp36 and Ca P27 proteins. By contrast, HMTV proteins did not react with antibody against the MMTV Env Gp52 protein. All the antibodies detected MMTV proteins with exception of two out of four monoclonal antibodies against HMTV Env. Approximately 13% of the MSSM cells showed HMTV protein expression by FACS analysis. This report shows the expression of HMTV proteins for the first time in human breast cancer cells using a panel of antibodies against HMTV, HBRV and MMTV proteins. This should be taken into consideration when MMTV antibodies are used to detect HMTV proteins in human tissues.

Published

2010

13. Detection of an infectious retrovirus, XMRV, in blood cells of patients with chronic fatigue syndrome.

Author

Lombardi VC, Ruscetti FW, Das Gupta J, Pfost MA, Hagen KS, Peterson DL, Ruscetti SK, Bagni RK, Petrow-Sadowski C, Gold B, Dean M, Silverman RH, and Mikovits JA

Subjects

Animals, Antibodies, Viral blood, B-Lymphocytes immunology, B-Lymphocytes virology, Base Sequence, Cell Line, Cell Line, Tumor, Coculture Techniques, DNA genetics, Gammaretrovirus genetics, Gammaretrovirus immunology, Gammaretrovirus physiology, Gene Products, env analysis, Gene Products, gag analysis, Genome, Viral, Humans, Lymphocyte Activation, Male, Mice, Molecular Sequence Data, Prostatic Neoplasms virology, Retroviridae Infections epidemiology, Retroviridae Infections transmission, T-Lymphocytes immunology, T-Lymphocytes virology, Tumor Virus Infections epidemiology, Tumor Virus Infections transmission, Fatigue Syndrome, Chronic virology, Gammaretrovirus isolation & purification, Leukocytes, Mononuclear virology, Retroviridae Infections virology, Tumor Virus Infections virology

Abstract

Chronic fatigue syndrome (CFS) is a debilitating disease of unknown etiology that is estimated to affect 17 million people worldwide. Studying peripheral blood mononuclear cells (PBMCs) from CFS patients, we identified DNA from a human gammaretrovirus, xenotropic murine leukemia virus-related virus (XMRV), in 68 of 101 patients (67%) as compared to 8 of 218 (3.7%) healthy controls. Cell culture experiments revealed that patient-derived XMRV is infectious and that both cell-associated and cell-free transmission of the virus are possible. Secondary viral infections were established in uninfected primary lymphocytes and indicator cell lines after their exposure to activated PBMCs, B cells, T cells, or plasma derived from CFS patients. These findings raise the possibility that XMRV may be a contributing factor in the pathogenesis of CFS.

Published

2009

14. Response of HEK293 and CHO cells overexpressing fusiogenic syncytin-1 to mitochondrion-mediated apoptosis induced by antimycin A.

Author

Knerr I, Söder S, Licha E, Aigner T, and Rascher W

Subjects

Animals, CHO Cells, Caspase 9 metabolism, Cell Fusion, Cells, Cultured, Cricetinae, Cricetulus, Gene Products, env analysis, Gene Products, env genetics, Humans, Microscopy, Confocal, Pregnancy Proteins analysis, Pregnancy Proteins genetics, Transfection, Antimycin A pharmacology, Apoptosis drug effects, Gene Products, env metabolism, Mitochondria metabolism, Pregnancy Proteins metabolism

Abstract

Apoptosis is essential for the regulation of cellular homeostasis in the placenta and is also involved in the pathophysiology of pregnancy-related diseases such as pre-eclampsia and intrauterine growth restriction (IUGR). Syncytin-1, a fusiogenic glycoprotein of endogenous-retroviral origin expressed in human trophoblasts, facilitates placental syncytium formation and is found reduced in pre-eclamptic placentas. We focus here on the mitochondrial apoptotic pathway and investigate whether the overexpression of syncytin-1 in HEK293-52 (human embryonic kidney cells) and CHO-52 cells influences the apoptotic response to the mitochondrial inhibitor antimycin A (AA). After the induction of apoptosis by 5 microM AA and incubation for up to 36 h in the absence of serum, the mean apoptotic rate was reduced by 15-30% in syncytin-1 transfected cells compared with mock-transfectants. After 12 h of challenge with AA we found lower cytochrome c levels in the cytoplasmic protein fraction and higher amounts in the mitochondrial fraction in syncytin-1 transfectants compared with mock-transfectants. We observed a decreased Mitotracker Red staining of mitochondria following AA challenge for 24 h in mock-treated CHO cells, in particular, compared with syncytin-1 transfectants. Moreover, we found a reduced activation of caspase 9 in syncytin-1 transfected HEK293-52 cells after 48 h of apoptotic challenge compared to mock-transfectants. However, a high expression of anti-apoptotic Bcl-x(L) was found in both cell types. Using syncytin-1 transfected HEK293-52 cells and CHO-52 cells, we provide initial evidence that syncytin-1 may exert its anti-apoptotic function at the mitochondrial level. A reduced release of cytochrome c followed by a diminished activation of caspase 9 is a possible mechanism., ((c) 2008 Wiley-Liss, Inc.)

Published

2008

15. Cell fusions in mammals.

Author

Larsson LI, Bjerregaard B, and Talts JF

Subjects

Animals, Cell Fusion, Female, Gene Products, env physiology, Humans, Immunohistochemistry, Neoplasms metabolism, Neoplasms pathology, Placenta cytology, Placenta metabolism, Pregnancy, Pregnancy Proteins physiology, Gene Products, env analysis, Mammals metabolism, Pregnancy Proteins analysis

Abstract

Cell fusions are important to fertilization, placentation, development of skeletal muscle and bone, calcium homeostasis and the immune defense system. Additionally, cell fusions participate in tissue repair and may be important to cancer development and progression. A large number of factors appear to regulate cell fusions, including receptors and ligands, membrane domain organizing proteins, proteases, signaling molecules and fusogenic proteins forming alpha-helical bundles that bring membranes close together. The syncytin family of proteins represent true fusogens and the founding member, syncytin-1, has been documented to be involved in fusions between placental trophoblasts, between cancer cells and between cancer cells and host cells. We review the literature with emphasis on the syncytin family and propose that syncytins may represent universal fusogens in primates and rodents, which work together with a number of other proteins to regulate the cell fusion machinery.

Published

2008

16. An optimized nested polymerase chain reaction (PCR) approach allows detection and characterization of human immunodeficiency virus type 1 (HIV-1) env and gag genes from clinical samples.

Author

Locateli D, Stoco PH, Zanetti CR, Pinto AR, and Grisard EC

Subjects

Electrophoresis, Agar Gel, Ethidium, Genes, Viral genetics, Humans, Sensitivity and Specificity, Gene Products, env analysis, Gene Products, env genetics, Gene Products, gag analysis, Gene Products, gag genetics, HIV Infections virology, HIV-1 genetics, HIV-1 isolation & purification, Polymerase Chain Reaction methods

Abstract

The needs for development and/or improvement of molecular approaches for microorganism detection and characterization such as polymerase chain reaction (PCR) are of high interest due their sensitivity and specificity when compared to traditional microbiological techniques. Considering the worldwide importance of human immunodeficiency virus type 1 (HIV-1) infection, it is essential that such approaches consider the genetic variability of the virus, the heterogeneous nature of the clinical samples, the existence of contaminants and inhibitors, and the consequent needs for standardization in order to guarantee the reproducibility of the methods. In this work we describe a nested PCR assay targeting HIV-1 virus gag and env genes, allowing specific and sensitive diagnosis and further direct characterization of clinical samples. The method described herein was tested on clinical samples and allowed the detection of HIV-1 presence in all samples tested for the gag gene and 90.9% for the env gene, revealing sensitivities of 1 fg and 100 fg, respectively. Also, no cross-reactions were observed with DNA from infected and noninfected patients and the method allowed detection of the env and gag genes on an excess of 10(8) and 10(4) of human deoxyribonucleic acid (DNA), respectively. Furthermore, it was possible to direct sequence all amplified products, which allowed the sub typing of the virus in clinical samples., ((Copyright ) 2008 Wiley-Liss, Inc.)

Published

2008

17. A conserved dileucine motif mediates clathrin and AP-2-dependent endocytosis of the HIV-1 envelope protein.

Author

Byland R, Vance PJ, Hoxie JA, and Marsh M

Subjects

Adaptor Protein Complex 2 antagonists & inhibitors, Adaptor Protein Complex 2 genetics, Amino Acid Motifs, Amino Acid Sequence, CD4 Antigens analysis, CD4 Antigens genetics, CD4 Antigens metabolism, Cell Membrane chemistry, Cell Membrane metabolism, Conserved Sequence, Gene Products, env analysis, Gene Products, env genetics, HeLa Cells, Humans, Leucine chemistry, Leucine genetics, Molecular Sequence Data, Mutation, Protein Structure, Tertiary, RNA Interference, Recombinant Fusion Proteins analysis, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Adaptor Protein Complex 2 metabolism, Clathrin metabolism, Endocytosis, Gene Products, env metabolism, HIV-1

Abstract

During the assembly of enveloped viruses viral and cellular components essential for infectious particles must colocalize at specific membrane locations. For the human and simian immunodeficiency viruses (HIV and SIV), sorting of the viral envelope proteins (Env) to assembly sites is directed by trafficking signals located in the cytoplasmic domain of the transmembrane protein gp41 (TM). A membrane proximal conserved GYxxØ motif mediates endocytosis through interaction with the clathrin adaptor AP-2. However, experiments with SIV(mac239) Env indicate the presence of additional signals. Here we show that a conserved C-terminal dileucine in HIV(HxB2) also mediates endocytosis. Biochemical and morphological assays demonstrate that the C-terminal dileucine motif mediates internalization as efficiently as the GYxxØ motif and that both must be removed to prevent Env internalization. RNAi experiments show that depletion of the clathrin adaptor AP-2 leads to increased plasma membrane expression of HIV Env and that this adaptor is required for efficient internalization mediated by both signals. The redundancy of conserved endocytosis signals and the role of the SIV(mac239) Env GYxxØ motif in SIV pathogenesis, suggest that these motifs have functions in addition to endocytosis, possibly related to Env delivery to the site of viral assembly and/or incorporation into budding virions.

Published

2007

18. Impact of natural polymorphism within the gp41 cytoplasmic tail of human immunodeficiency virus type 1 on the intracellular distribution of envelope glycoproteins and viral assembly.

Author

Lambelé M, Labrosse B, Roch E, Moreau A, Verrier B, Barin F, Roingeard P, Mammano F, and Brand D

Subjects

Amino Acid Motifs, Amino Acid Sequence, Gene Products, gag metabolism, HIV Envelope Protein gp41 analysis, HIV Envelope Protein gp41 metabolism, HIV Infections virology, HIV-1 physiology, HIV-1 ultrastructure, HeLa Cells, Humans, Kinetics, Molecular Sequence Data, Protein Transport, Sequence Alignment, Virion metabolism, Virus Replication, Gene Products, env analysis, HIV Envelope Protein gp41 genetics, HIV-1 genetics, Polymorphism, Genetic, Virus Assembly genetics

Abstract

The motifs involved in the various functions of the human immunodeficiency virus type 1 (HIV-1) gp41 cytoplasmic tail (CT), particularly those related to the intracellular trafficking and assembly of envelope glycoproteins (Env) onto core particles, have generally been assessed with a restricted panel of T-cell laboratory-adapted virus strains. Here, we investigated gp41 CT sequences derived from individuals infected with HIV-1 viruses of various subtypes. We identified four patients harboring HIV variants with a natural polymorphism in the membrane-proximal tyrosine-based signal Y(712)SPL or the Y(802)W(803) diaromatic motif, which are two major determinants of Env intracellular trafficking. Confocal microscopy showed that the intracellular distribution of Env with a mutation in the tyrosine or diaromatic motif differed from that of Env with no mutation in these motifs. Surprisingly, the gp41 CTs of the primary viruses also had differential effects on the intracellular distribution of Env, independently of mutations in the tyrosine or diaromatic motifs, suggesting the involvement of additional determinants. Furthermore, analyses of virus replication kinetics indicated that the effects of mutations in the tyrosine or diaromatic motifs on viral replication depended on the gp41 CT context. These effects were at least partly due to differences in the efficiency of Env incorporation into virions. Thus, polymorphisms in primary HIV-1 gp41 CTs at the quasispecies or subtype level can influence the intracellular distribution of Env, its incorporation into virions, and viral replication capacity.

Published

2007

19. Expression of the jaagsiekte sheep retrovirus envelope glycoprotein is sufficient to induce lung tumors in sheep.

Author

Caporale M, Cousens C, Centorame P, Pinoni C, De las Heras M, and Palmarini M

Subjects

Adenocarcinoma pathology, Adenocarcinoma virology, Animals, Gene Products, env analysis, Gene Products, env genetics, Glycoproteins genetics, Glycoproteins metabolism, Jaagsiekte sheep retrovirus genetics, Lung Neoplasms pathology, Lung Neoplasms virology, Sheep Diseases metabolism, Sheep Diseases pathology, Adenocarcinoma veterinary, Gene Products, env metabolism, Jaagsiekte sheep retrovirus metabolism, Lung Neoplasms veterinary, Sheep Diseases virology, Sheep, Domestic virology

Abstract

Jaagsiekte sheep retrovirus (JSRV) is the causative agent of ovine pulmonary adenocarcinoma (OPA). The expression of the JSRV envelope (Env) alone is sufficient to transform a variety of cell lines in vitro and induce lung cancer in immunodeficient mice. In order to determine the role of the JSRV Env in OPA tumorigenesis in sheep, we derived a JSRV replication-defective virus (JS-RD) which expresses env under the control of its own long terminal repeat (LTR). JS-RD was produced by transiently transfecting 293T cells with a two plasmid system, involving (i) a packaging plasmid, with the putative JSRV packaging signal deleted, expressing the structural and enzymatic proteins Gag, Pro, and Pol, and (ii) a plasmid which expresses env in trans for JS-RD particles and provides the genomes necessary to deliver JSRV env upon infection. During the optimization of the JS-RD system we determined that both R-U5 (in the viral 5' LTR) and the env region are important for JSRV particle production. Two independent experimental transmission studies were carried out with newborn lambs. Four of five lambs inoculated with JS-RD showed OPA lesions in the lungs at various times between 4 and 12 months postinoculation. Abundant expression of JSRV Env was detected in tumor cells of JS-RD-infected animals and PCR assays confirmed the presence of the deleted JS-RD genome. These data strongly suggest that the JSRV Env functions as a dominant oncoprotein in the natural immunocompetent host and that JSRV can induce OPA in the absence of viral spread.

Published

2006

20. Mutational analysis of the cytoplasmic tail of jaagsiekte sheep retrovirus envelope protein.

Author

Hull S and Fan H

Subjects

Amino Acid Motifs, Amino Acid Substitution, Animals, Cell Membrane chemistry, Cell Membrane metabolism, Cytoplasm chemistry, Cytoplasm virology, DNA Mutational Analysis, Enzyme Activation, Gene Products, env analysis, Gene Products, env genetics, MAP Kinase Kinase 1 metabolism, Mice, NIH 3T3 Cells, Phosphorylation, Protein Kinases metabolism, Protein Structure, Tertiary, Proto-Oncogene Proteins c-akt metabolism, TOR Serine-Threonine Kinases, p38 Mitogen-Activated Protein Kinases metabolism, Cell Transformation, Viral genetics, Gene Products, env physiology, Jaagsiekte sheep retrovirus physiology

Abstract

Jaagsiekte sheep retrovirus (JSRV) is the etiologic agent of a transmissible lung cancer in sheep, ovine pulmonary adenocarcinoma. JSRV is unique in that the envelope protein functions as an oncogene, since it can morphologically transform fibroblast and epithelial cells in culture and can induce lung tumors in mice. Previous studies indicated that the transmembrane (TM) protein is essential for transformation, and particular attention has focused on a YXXM motif in the cytoplasmic tail. In this study, we carried out systematic mutagenesis of the cytoplasmic tail of JSRV Env. Alanine scanning mutagenesis revealed four classes of mutants: mutants in which transformation was abrogated, those in which transformation was not affected, those with reduced transformation, and those with increased transformation (supertransformers). In general, the alanine mutations did not affect Env protein production or its localization to the plasma membrane. Three functional domains of the cytoplasmic tail were identified: an amphipathic helix at the N-terminal (juxtamembrane) side, a nonessential C-terminal region, and an internal region (including the YXXM motif) where mutations resulted in abrogation, decreases, or increases in transformation. Alanine mutations in the amphipathic helix in both the hydrophobic and hydrophilic faces generally abolished transformation. The mutation R591A showed partial transformation that was consistent with loss of signaling through the Akt-mTOR pathway and signaling predominantly through the Ras-Raf-MEK1/2-extracellular signal-regulated kinase 1/2 pathway. The supertransforming mutants generally showed increased signaling through Akt and reduced activation of p38 MAPK that is inhibitory for transformation. These mutants provide further insight into the role of the TM cytoplasmic tail in JSRV transformation.

Published

2006

21. Targeted infection of HIV-1 Env expressing cells by HIV(CD4/CXCR4) vectors reveals a potential new rationale for HIV-1 mediated down-modulation of CD4.

Author

Ye Z, Harmison GG, Ragheb JA, and Schubert M

Subjects

Animals, COS Cells, Cell Adhesion, Chlorocebus aethiops, Down-Regulation, Gene Products, env analysis, Genetic Vectors, HeLa Cells, Humans, Mice, NIH 3T3 Cells, Transduction, Genetic, Virion physiology, Virus Assembly, CD4 Antigens physiology, Gene Products, env physiology, HIV-1 pathogenicity, Receptors, CXCR4 physiology

Abstract

Background: Efficient targeted gene transfer and cell type specific transgene expression are important for the safe and effective expression of transgenes in vivo. Enveloped viral vectors allow insertion of exogenous membrane proteins into their envelopes, which could potentially aid in the targeted transduction of specific cell types. Our goal was to specifically target cells that express the T cell tropic HIV-1 envelope protein (Env) using the highly specific interaction of Env with its cellular receptor (CD4) inserted into the envelope of an HIV-1-based viral vector., Results: To generate HIV-1-based vectors carrying the CD4 molecule in their envelope, the CD4 ectodomain was fused to diverse membrane anchors and inserted together with the HIV-1 coreceptor CXCR4 into the envelopes of HIV-1 vector particles. Independent of the type of CD4 anchor, all chimeric CD4 proteins inserted into HIV-1 vector envelopes and the resultant HIV(CD4/CXCR4) particles were able to selectively confer neomycin resistance to cells expressing the fusogenic T cell tropic HIV-1 Env protein. Unexpectedly, in the absence of Env on the target cells, all vector particles carrying the CD4 ectodomain anchored in their envelope adhered to various cell types without infecting these cells. This cell adhesion was very avid. It was independent of the presence of Env on the target cell, the type of CD4 anchor or the presence of CXCR4 on the particle. In mixed cell populations with defined ratios of Env+/Env- cells, the targeted transduction of Env+ cells by HIV(CD4/CXCR4) particles was diminished in proportion to the number of Env- cells., Conclusion: Vector diversion caused by a strong, non-selective cell binding of CD4+-vector particles effectively prevents the targeted transduction of HIV-1 Env expressing cells in mixed cell populations. This Env-independent cell adhesion severely limits the effective use of targeted HIV(CD4/CXCR4) vectors designed to interfere with HIV-1 replication in vivo. Importantly, the existence of this newly described and remarkably strong CD4-dependent cell adhesion suggests that the multiple viral efforts to reduce CD4 cell surface expression may, in part, be to prevent cell adhesion to non-target cells and thereby to increase the infectivity of viral progeny. Preventing CD4 down-modulation by HIV-1 might be an effective component of a multi-faceted antiviral strategy.

Published

2005

22. In vivo expression of GFP transgene delivered via a replicating feline leukemia virus.

Author

Pan J, Al-Dubaib M, Liao CP, Fujino Y, Hinton DR, Hayes KA, Mathes LE, and Roy-Burman P

Subjects

Animals, Animals, Newborn, Cats, Gene Products, env analysis, Gene Products, env biosynthesis, Gene Products, env genetics, Green Fluorescent Proteins metabolism, RNA, Viral blood, Viremia, Gene Expression, Genetic Vectors genetics, Green Fluorescent Proteins genetics, Leukemia Virus, Feline genetics, Leukemia Virus, Feline physiology, Transgenes genetics, Virus Replication

Abstract

We previously described replication-competent feline leukemia virus (FeLV) vectors with high-level and stable expression of a green fluorescent protein (GFP) or a suicide transgene in cell cultures in vitro. Considering that FeLV might potentially be used to deliver therapeutic genes in vivo, we first evaluated the expression of the GFP gene introduced in cats by the FeLV, Rickard subgroup A (FRA) construct. Eight newborn kittens were either inoculated with pFRA-GFP plasmid DNA intradermally, or challenged intraperitoneally with FRA-GFP-infected feline fibroblasts. During a 12-week observation period, five cats were shown to be progressively viremic. Quantitative PCR and RT-PCR analyses of plasma and tissue samples from these cats showed that GFP was retained in FeLV DNA or RNA to a variable degree, ranging from 0.002 to 27.890%. Tissue DNA samples were analyzed by PCR for the status of GFP and the env-transgene complex. While the proviruses carrying the GFP transgene were shown to be minor species, all tissues, however, retained the full-length GFP transgene. Despite the occurrence of predominant species with various deletions in the viral genome, approximately 1-3% of the total cell population was GFP-positive in the lymphoid tissues as visualized by laser confocal microscopy. Co-localization of immunofluorescent cells indicated that CD3-positive T cells, dendritic cells and macrophages were the major targets for GFP expression. These findings on the detectable in vivo expression of GFP for as long as a period of 3 months could be viewed positively for contemplating a therapeutic strategy for control of FeLV infection in the cats.

Published

2005

23. Long-term protection against SHIV89.6P replication in HIV-1 Tat vaccinated cynomolgus monkeys.

Author

Maggiorella MT, Baroncelli S, Michelini Z, Fanales-Belasio E, Moretti S, Sernicola L, Cara A, Negri DR, Buttò S, Fiorelli V, Tripiciano A, Scoglio A, Caputo A, Borsetti A, Ridolfi B, Bona R, ten Haaft P, Macchia I, Leone P, Pavone-Cossut MR, Nappi F, Ciccozzi M, Heeney J, Titti F, Cafaro A, and Ensoli B

Subjects

Animals, B-Lymphocytes immunology, CD4-Positive T-Lymphocytes immunology, CD8-Positive T-Lymphocytes immunology, DNA, Viral biosynthesis, DNA, Viral immunology, Gene Products, env analysis, Gene Products, env biosynthesis, Gene Products, gag analysis, Gene Products, gag biosynthesis, Humans, Interferon-gamma analysis, Interferon-gamma biosynthesis, Lymph Nodes pathology, Macaca fascicularis, Male, RNA, Viral biosynthesis, Recombinant Proteins biosynthesis, Recombinant Proteins immunology, Simian Acquired Immunodeficiency Syndrome immunology, Simian Acquired Immunodeficiency Syndrome pathology, Simian Acquired Immunodeficiency Syndrome virology, Simian Immunodeficiency Virus immunology, Vaccination, Viral Load, tat Gene Products, Human Immunodeficiency Virus, AIDS Vaccines therapeutic use, Gene Products, tat immunology, HIV-1 immunology, Simian Acquired Immunodeficiency Syndrome prevention & control, Simian Immunodeficiency Virus physiology, Virus Replication drug effects

Abstract

Vaccination with a biologically active Tat protein or tat DNA contained infection with the highly pathogenic SHIV89.6P virus, preventing CD4 T-cell decline and disease onset. Here we show that protection was prolonged, since neither CD4 T-cell decline nor active virus replication was observed in all vaccinated animals that controlled virus replication up to week 104 after the challenge. In contrast, virus persisted and replicated in peripheral blood mononuclear cells and lymph nodes of infected animals, two of which died. Tat-specific antibody, CD4 and CD8 T-cell responses were high and stable only in the animals controlling the infection. In contrast, Gag-specific antibody production and CD4 and CD8 T-cell responses were consistently and persistently positive only in the monkeys that did not control primary virus replication. These results indicate that vaccination with Tat protein or DNA induced long-term memory Tat-specific immune responses and controlled primary infection at its early stages allowing a long-term containment of virus replication and spread in blood and tissues.

Published

2004

24. Identification in gelada baboons (Theropithecus gelada) of a distinct simian T-cell lymphotropic virus type 3 with a broad range of Western blot reactivity.

Author

Van Dooren S, Shanmugam V, Bhullar V, Parekh B, Vandamme AM, Heneine W, and Switzer WM

Subjects

Animals, Blotting, Western, Carrier State blood, Carrier State transmission, Deltaretrovirus Infections blood, Deltaretrovirus Infections transmission, Evolution, Molecular, Female, Gene Products, env analysis, Gene Products, tax analysis, Human T-lymphotropic virus 1 chemistry, Human T-lymphotropic virus 1 genetics, Human T-lymphotropic virus 1 immunology, Human T-lymphotropic virus 2 chemistry, Human T-lymphotropic virus 2 genetics, Human T-lymphotropic virus 2 immunology, Likelihood Functions, Male, Molecular Sequence Data, Phylogeny, Primate T-lymphotropic virus 3 genetics, Primate T-lymphotropic virus 3 immunology, Sequence Homology, Nucleic Acid, United States, Animals, Zoo virology, Carrier State virology, Primate T-lymphotropic virus 3 isolation & purification, Theropithecus virology

Abstract

Antibodies to simian T-cell lymphotropic virus (STLV) were found in serum or plasma from 12 of 23 (52.2 %) gelada baboons (Theropithecus gelada) captive in US zoos. A variety of Western blot (WB) profiles was seen in the 12 seroreactive samples, including human T-cell lymphotropic virus (HTLV)-1-like (n=5, 41.7 %), HTLV-2-like (n=1, 8.3 %), HTLV-untypable (n=4, 33.3 %) and indeterminate (n=2, 16.6 %) profiles. Phylogenetic analysis of tax or env sequences that had been PCR amplified from peripheral blood lymphocyte DNA available from nine seropositive geladas showed that four were infected with identical STLV-1s; these sequences clustered with STLV-1 from Celebes macaques and probably represent recent cross-species infections. The tax sequences from the five remaining geladas were also identical and clustered with STLV-3. Analysis of the complete STLV-3 genome (8917 bp) from one gelada, TGE-2117, revealed that it is unique, sharing only 62 % similarity with HTLV-1/ATK and HTLV-2/Mo. STLV-3/TGE-2117 was closest genetically to STLV-3 from an Eritrean baboon (STLV-3/PH969, 95.6 %) but more distant from STLV-3s from red-capped mangabeys from Cameroon and Nigeria (STLV-3/CTO-604, 87.7 %, and STLV-3/CTO-NG409, 87.2 %, respectively) and Senegalese baboons (STLV-3/PPA-F3, 88.4 %). The genetic relatedness of STLV-3/TGE-2117 to STLV-3 was confirmed by phylogenetic analysis of a concatenated gag-pol-env-tax sequence (6795 bp). An ancient origin of 73 628-109 809 years ago for STLV-3 was estimated by molecular clock analysis of third-codon positions of gag-pol-env-tax sequences. LTR sequences from five STLV-3-positive geladas were >99 % identical and clustered with that from a Papio anubisxP. hamadryas hybrid Ethiopian baboon, suggesting a common source of STLV-3 in these sympatric animals. LTR sequences obtained 20 years apart from a mother-infant pair were identical, providing evidence of both mother-to-offspring transmission and a high genetic stability of STLV-3. Since STLV-3-infected primates show a range of HTLV-like WB profiles and have an ancient origin, further studies using STLV-3-specific testing are required to determine whether STLV-3 infects humans, especially in regions of Africa where STLV-3 is endemic.

Published

2004

25. Electron tomography analysis of envelope glycoprotein trimers on HIV and simian immunodeficiency virus virions.

Author

Zhu P, Chertova E, Bess J Jr, Lifson JD, Arthur LO, Liu J, Taylor KA, and Roux KH

Subjects

AIDS Vaccines, Image Processing, Computer-Assisted, Tomography, X-Ray Computed, Virion ultrastructure, Gene Products, env analysis, HIV ultrastructure, Simian Immunodeficiency Virus ultrastructure

Abstract

We used electron tomography to directly visualize trilobed presumptive envelope (env) glycoprotein structures on the surface of negatively stained HIV type 1 (HIV-1) and simian immunodeficiency virus (SIV) virions. Wild-type HIV-1 and SIV virions had an average of 8-10 trimers per virion, consistent with predictions based on biochemical evidence. Mutant SIVs, biochemically demonstrated to contain high levels of the viral env proteins, averaged 70-79 trimers per virion in tomograms. These correlations strongly indicate that the visualized trimers represent env spikes. The env trimers were without obvious geometric distribution pattern or preferred rotational orientation. Combined with biochemical analysis of gag/env ratios in virions, these trimer counts allow calculation of the number of gag molecules per virion, yielding an average value of approximately 1400. Virion and env dimensions were also determined. Image-averaging analysis of SIV env trimers revealed a distinct chirality and strong concordance with recent molecular models. The results directly demonstrate the presence of env trimers on the surface of AIDS virus virions, albeit at numbers much lower than generally appreciated, and have important implications for understanding virion formation, virus interactions with host cells, and virus neutralization.

Published

2003

26. The immune control and cell-to-cell spread of human T-lymphotropic virus type 1.

Author

Bangham CRM

Subjects

CD4-Positive T-Lymphocytes immunology, CD8-Positive T-Lymphocytes immunology, Gene Products, env analysis, Gene Products, gag analysis, Human T-lymphotropic virus 1 physiology, Humans, Immunity, Cellular, Intercellular Junctions virology, Logistic Models, Lymphocyte Count, Paraparesis, Tropical Spastic etiology, Paraparesis, Tropical Spastic virology, Proviruses pathogenicity, RNA-Directed DNA Polymerase immunology, Viral Load, Virus Latency, Human T-lymphotropic virus 1 pathogenicity, Paraparesis, Tropical Spastic immunology, T-Lymphocytes immunology, T-Lymphocytes virology

Abstract

Human T-lymphotropic virus type 1 (HTLV-1) varies little in sequence compared with human immunodeficiency virus type 1 (HIV) and it is difficult to detect HTLV-1 mRNA, proteins or virions in fresh blood. But the strong and chronically activated T cell response to the virus indicates that HTLV-1 proteins are expressed persistently. It now appears that the efficiency of an individual's cytotoxic T cell (CTL) response to HTLV-1 is the chief single determinant of that person's provirus load, which can differ between HTLV-1-infected people by more than 10 000-fold. Progress is now being made towards defining this CTL 'efficiency' in terms of host genetics, T cell function, T cell gene expression and mathematical dynamics. Lymphocytes that are naturally infected with HTLV-1 do not produce enveloped extracellular virions in short-term culture and this has reinforced the erroneous conclusion that the virus is latent. But recent evidence shows that HTLV-1 can spread directly between lymphocytes across a specialized, virus-induced cell-cell contact - a 'viral synapse'. Instead of making extracellular virions, HTLV-1 uses the mobility of the host cell to spread within and between hosts. In this review the evidence is summarized on the persistent gene expression of HTLV-1 in vivo, the role of the immune system in protection and pathogenesis in HTLV-1 infection, and the mechanism of cell-to-cell spread of HTLV-1.

Published

2003

27. [Expression of retroviral env protein and its antigenisity in the transgenic rat carrying human endogenous retrovirus gene, HERV-R].

Author

Otsuka N

Subjects

Animals, Animals, Genetically Modified, Blotting, Western, Immunohistochemistry, RNA, Viral analysis, Rats, Skin Transplantation immunology, Endogenous Retroviruses genetics, Gene Products, env analysis, Gene Products, env immunology

Published

2003

28. Detecting the expression of human endogenous retrovirus E envelope transcripts in human prostate adenocarcinoma.

Author

Wang-Johanning F, Frost AR, Jian B, Azerou R, Lu DW, Chen DT, and Johanning GL

Subjects

Blotting, Northern, DNA, Complementary analysis, DNA, Complementary metabolism, Endogenous Retroviruses metabolism, Gene Products, env analysis, Genetic Vectors, Humans, Male, Molecular Sequence Data, Prostatic Neoplasms metabolism, RNA, Messenger biosynthesis, Reverse Transcriptase Polymerase Chain Reaction, Tumor Cells, Cultured, Endogenous Retroviruses genetics, Gene Products, env biosynthesis, Prostatic Neoplasms genetics

Abstract

Background: The expression of human endogenous retrovirus (HERV) mRNA and proteins was associated recently with diseases that include human malignancies. The authors report that, in the current study, transcripts encoding the envelope region of an HERV family, HERV-E, were expressed in human prostate carcinoma., Methods: RNA was isolated from various prostate tissues and was tested for the expression of various HERV envelope (env) genes by reverse transcriptase-polymerase chain reaction (RT-PCR) analysis, RNA in situ hybridization (ISH), and Northern blot analysis. Variants of HERV that appeared in prostate carcinoma tissues were sequenced, and HERV-E was expressed in prokaryotic and eukaryotic systems., Results: In the current study, the authors found that the mRNA of the env gene of one particular family of HERVs, HERV-E, was expressed in some prostate carcinoma tissues (38.8% positive; n = 49 specimens) but not in normal prostate tissues using RT-PCR, RNA ISH, and Northern blot assays. The expression of HERV-E transcripts in prostate tumor epithelial cells was confirmed further by ISH using an HERV-E specific antisense probe. Approximately 50% of the cDNA of HERV-E obtained from prostate carcinoma specimens contained no stop codon and expressed proteins in prokaryotic or eukaryotic expression systems. Furthermore, the expression of both HERV-E and ERV3 (another class of HERV) was detected in the same prostate carcinoma tissues., Conclusions: The expression and distribution of multiple HERV-E endogenous retroviral elements in prostate carcinoma, but not in normal control specimens, suggests that they may serve as novel tumor markers for the early diagnosis and immunotherapy of patients with prostate carcinoma., (Copyright 2003 American Cancer Society.DOI 10.1002/cncr.11451)

Published

2003

29. Detection of porcine endogenous retrovirus (PERV) using highly specific antisera against Gag and Env.

Author

Fischer N, Krach U, Niebert M, and Tönjes RR

Subjects

Amino Acid Sequence, Animals, Antibodies, Viral, Cell Line, Endogenous Retroviruses immunology, Gene Products, env genetics, Gene Products, gag genetics, Humans, Immunoassay, Microscopy, Immunoelectron, Molecular Sequence Data, Retroviridae Proteins, Oncogenic analysis, Swine, Viral Envelope Proteins analysis, Endogenous Retroviruses isolation & purification, Gene Products, env analysis, Gene Products, gag analysis, Immune Sera

Abstract

Porcine endogenous retroviruses (PERV) are considered an obstacle to the safe use of cells, tissues, and organs from pigs in the course of xenotransplantation. Thus, the detection of viral proteins and of a potential PERV infection is of major interest. Recently, we have published the generation of a highly specific antiserum directed against the nucleocapsid (p10) of PERV (Xenotransplantation 7 (2000), 221). Here we present new peptide-antisera specific to the capsid protein (p30) and the surface molecule of PERV class B (SU, gp70(B)) as well as the transmembrane moiety of the envelope protein (TM, p15E) of PERV which showed functionality in several immunological assays, such as immunoblots, immunofluorescence, and immunogold staining. Thus, these antisera can be used as tools for the identification of viral proteins in basic research as well as clinical trials.

Published

2003

30. Quantitation of HERV-K env gene expression and splicing in human breast cancer.

Author

Wang-Johanning F, Frost AR, Jian B, Epp L, Lu DW, and Johanning GL

Subjects

Breast Neoplasms drug therapy, Breast Neoplasms pathology, Carcinoma, Intraductal, Noninfiltrating drug therapy, Carcinoma, Intraductal, Noninfiltrating pathology, Codon, Terminator, Epithelial Cells physiology, Estradiol pharmacology, Female, Gene Expression Regulation, Neoplastic drug effects, Gene Products, env analysis, Humans, Progesterone pharmacology, RNA Splicing, Reference Values, Reverse Transcriptase Polymerase Chain Reaction methods, Tumor Cells, Cultured, Breast Neoplasms genetics, Carcinoma, Intraductal, Noninfiltrating genetics, Endogenous Retroviruses genetics, Gene Products, env genetics

Abstract

Human endogenous retroviruses (HERVs) comprise up to 8% of the human genome. In previous studies, we demonstrated that type 1 HERV-K envelope (env) transcripts are expressed in most human breast cancers, but not in normal breast tissues. In the current study, we report that type 2 HERV-K env transcripts are also present in human breast cancers. By real-time RT-PCR, the expression of HERV-K env transcripts was 5-10-fold higher in breast cancer cell lines treated with estradiol and progesterone than in cells without treatment, and expression was significantly higher in most breast cancer tissues than in normal breast tissues. Furthermore, both types of HERV-K env transcripts were capable of being spliced into subgenomic env transcripts and various splice donor and acceptor sites were detected in breast cancers. The selective expression and distribution of multiple HERV-K endogenous retroviral element splice variants in breast cancer, but not in normal controls, suggests that they are novel breast tumor markers.

Published

2003

31. Rapid reconstitution of humoral immunity against cytomegalovirus but not HIV following highly active antiretroviral therapy.

Author

Deayton JR, Sabin CA, Britt WB, Jones IM, Wilson P, Johnson MA, Griffiths PD, and Emery VC

Subjects

AIDS-Related Opportunistic Infections immunology, Acquired Immunodeficiency Syndrome drug therapy, Antibodies, Viral immunology, Cytomegalovirus physiology, Cytomegalovirus Infections complications, DNA, Viral blood, Female, Gene Products, env analysis, Gene Products, env immunology, Gene Products, gag analysis, Gene Products, gag immunology, HIV-1 immunology, HIV-1 physiology, Humans, Male, RNA, Viral blood, Viral Envelope Proteins immunology, Viral Load, Virus Replication drug effects, AIDS-Related Opportunistic Infections complications, Acquired Immunodeficiency Syndrome immunology, Antibody Formation immunology, Antiretroviral Therapy, Highly Active, Cytomegalovirus Infections immunology

Abstract

Objective: To determine the kinetics of reduction in human cytomegalovirus (HCMV) load and specific anti-glycoprotein B (gB) immune responses in patients with concurrent HCMV DNAaemia following the initiation of highly active antiretroviral therapy (HAART)., Design: Sequential analysis of eleven patients with HCMV DNAaemia who received HAART and eleven control patients with HCMV DNAaemia., Methods: HCMV load was measured by quantitative competitive polymerase chain reaction and anti-gB, anti-HIV Env and Gag responses by an end-point dilution immunofluorescence assay using recombinant antigens expressed in insect cells. Estimates of the efficacy of the reconstituting immune system at controlling HCMV replication were based on previous dynamic models., Results: In patients initiating HAART, HCMV DNA levels in blood declined rapidly, with a median half-life of 5.2 days, consistent with an efficacy of the reconstituting immune system at inhibiting HCMV replication of 52.8-85% (median, 61%). Commensurate with this decrease, a significant increase in anti-gB titres was observed in the post-HAART period (corresponding to an average fourfold increase in titre by 1 month rising to an eightfold increase at month 3; = 0.01). No changes in titre were observed in the control group or for anti-HIV Gag antibody levels, while anti-HIV Env antibody levels decreased after HAART., Conclusions: In patients with HCMV DNAaemia, reconstitution of humoral immunity to HCMV gB occurs rapidly following the initiation of HAART. These changes contrast with the patterns observed for anti-HIV humoral immune responses.

Published

2002

32. Purification and reactiongenicity of human immunodeficiency virus type 2 total external glycoprotein expressed in Pichia Pastoris.

Author

Zhang YJ, Jin NY, Jin HT, and Shen JC

Subjects

Cloning, Molecular methods, Enzyme-Linked Immunosorbent Assay, Fermentation, Gene Products, env genetics, Humans, Pichia growth & development, Polymerase Chain Reaction methods, Sensitivity and Specificity, env Gene Products, Human Immunodeficiency Virus, Gene Products, env analysis, HIV-2 isolation & purification, Pichia genetics

Abstract

The purification of human immunodeficiency virus type 2 total external glycoprotein gp105 expressed in Pichia pastoris was investigated. Expression conditions were optimized by an orthogonal test. The results from tests of variance analyses showed that the most important parameter for efficient expression of total gp105 in P. pastoris is adequate aeration during methanol induction. The optimum induction conditions for gp105 expression were: more than 85% aeration, induction for 3 days, the initial pH 6.0-7.0 and a final methanol concentration of 1.0%. Under these conditions, the expressed total gp105 was secreted into fermentation broth and reached a yield of 23%, approximately 141 mg/l. Expressed gp105 was isolated and purified by salting out and Sephadex G-100 chromatography and the yield of gp105 was 40%. gp105 was purified to electrophoretic purity and its isoelectric point (pI) was about 5.2 by SDS-PAGE and isoelectrofocusing. The purified gp105 contained approximately 35% carbohydrate, which proved that the expressed gp105 was a glycoprotein. Its N-terminal amino acid was arginine by Dansyl-Cl and the result indicated that expressed gp105 was secreted and cleaved correctly. The results from gp105 ELISA demonstrated that the purified total gp105 showed good reactiongenicity and antigenic specificity.

Published

2002

33. Detailed analysis of CD4+ Th responses to envelope and Gag proteins of simian immunodeficiency virus reveals an exclusion of broadly reactive Th epitopes from the glycosylated regions of envelope.

Author

Sarkar S, Kalia V, Murphey-Corb M, and Montelaro RC

Subjects

Aging immunology, Amino Acid Sequence, Animals, Antigen-Antibody Reactions, Antigens, Viral immunology, Antigens, Viral metabolism, Biomarkers analysis, CD4-Positive T-Lymphocytes metabolism, CD4-Positive T-Lymphocytes virology, Conserved Sequence, Epitopes, T-Lymphocyte analysis, Fluoresceins analysis, Gene Products, env analysis, Gene Products, gag analysis, Glycosylation, Histocompatibility Antigens Class II immunology, Immunity, Cellular physiology, Ki-67 Antigen analysis, Lymphocyte Activation immunology, Macaca mulatta, Membrane Glycoproteins immunology, Mitogens immunology, Molecular Sequence Data, Peptide Fragments analysis, Peptide Fragments immunology, Peptide Mapping, Protein Structure, Secondary, SAIDS Vaccines administration & dosage, SAIDS Vaccines immunology, Simian Immunodeficiency Virus metabolism, Succinimides analysis, Vaccines, Attenuated administration & dosage, Vaccines, Attenuated immunology, CD4-Positive T-Lymphocytes immunology, Epitopes, T-Lymphocyte immunology, Epitopes, T-Lymphocyte metabolism, Gene Products, env immunology, Gene Products, env metabolism, Gene Products, gag immunology, Gene Products, gag metabolism, Simian Immunodeficiency Virus immunology

Abstract

Ag-specific CD4(+) Th cells play a key role in the development, maturation, and maintenance of pathogen-specific humoral and cellular immune responses. To define the fine specificity of broadly reactive Th responses associated with mature immunity in a lentiviral system, we analyzed peptide-specific Th responses in eight macaques chronically infected with a reference live attenuated SIV at 12-14 mo postinoculation. All macaques had stable immunocompetent Th cells at the time of analysis, and a unique array of Th responses to 20-mer overlapping peptides from envelope (Env) and Gag was identified for each macaque, which were then used to define a set of 31 broadly reactive peptide epitopes. Only 5 of the 31 broadly reactive Th epitope peptides mapped to the surface (SU) domain of Env. Interestingly, these were all confined to two conserved nonglycosylated regions toward the carboxyl terminus of SU, suggesting a structural influence of glycosylation on development of Th responses. Gag and the Env transmembrane proteins contained the majority of broadly reactive peptide epitopes (12 and 14 peptides, respectively), which were uniformly distributed throughout their sequence. This study defines for the first time broadly reactive Th epitope peptides of SIV Env and Gag proteins that are associated with enduring broadly protective vaccine immunity to attenuated SIV, which may be used for the design and evaluation of experimental vaccines. Moreover, the data suggest that extensive glycosylation of SU may provide yet another immune escape mechanism developed by lentiviruses to restrict the breadth of Th repertoire to SU, a major immunologically exposed protein of the virus.

Published

2002

34. Deletion of the vpu sequences prior to the env in a simian-human immunodeficiency virus results in enhanced Env precursor synthesis but is less pathogenic for pig-tailed macaques.

Author

Stephens EB, McCormick C, Pacyniak E, Griffin D, Pinson DM, Sun F, Nothnick W, Wong SW, Gunderson R, Berman NE, and Singh DK

Subjects

Animals, Atrophy, Base Sequence, CD4 Lymphocyte Count, DNA, Viral analysis, Gene Deletion, Gene Products, env analysis, HIV Infections immunology, HIV-1 genetics, Human Immunodeficiency Virus Proteins, Lymph Nodes virology, Macaca nemestrina, Molecular Sequence Data, Protein Precursors analysis, Reassortant Viruses genetics, Simian Immunodeficiency Virus genetics, Spleen virology, Thymus Gland pathology, Thymus Gland virology, Viral Regulatory and Accessory Proteins genetics, Virulence, Virus Replication, Gene Products, env biosynthesis, HIV Infections virology, HIV-1 pathogenicity, Protein Precursors biosynthesis, Reassortant Viruses pathogenicity, Simian Immunodeficiency Virus pathogenicity

Abstract

The Vpu protein of human immunodeficiency virus type 1 (HIV-1) has been reported to enhance virion release from infected cells and to down-regulate the expression of CD4 on infected cells. Previous studies have shown that Vpu and the envelope glycoprotein precursor (gp160) are translated from different reading frames of the same bicistronic messenger RNA (mRNA). In order to assess the effect of the Vpu sequences 5' to the Env open reading frame on Env biosynthesis and pathogenesis, we have constructed a deletion mutant of a molecularly cloned chimeric simian--human immunodeficiency virus (SHIV(KU-1bMC33)) in which the entire coding region of vpu upstream of env had been deleted (novpuSHIV(KU-1bMC33)). While both SHIV(KU-1bMC33) and novpuSHIV(KU-1bMC33) synthesized comparable amounts of env mRNA in infected cells, the novpuSHIV(KU-1bMC33)-infected cells synthesized more Env precursor when standardized against the p57 Gag precursor protein. While more Env was synthesized than Gag in novpuSHIV(KU-1bMC33)-infected cells, pulse--chase analysis revealed that p27 Gag protein was released from infected cells with delayed kinetics, a reflection of the lack of a Vpu protein. Inoculation of novpuSHIV(KU-1bMC33) into two pig-tailed macaques resulted in no loss of circulating CD4(+) T cells. However, replicating virus could be detected in the lymphoid tissues (lymph nodes, spleen, thymus) 1 year after inoculation and the thymus of one of the macaques exhibited severe atrophy. The results of these studies indicate that the Vpu coding sequences upstream of Env may attenuate the level of Env precursor biosynthesis but significantly contribute to the pathogenesis of this SHIV in pig-tailed macaques.

Published

2002

35. Downregulation of placental syncytin expression and abnormal protein localization in pre-eclampsia.

Author

Lee X, Keith JC Jr, Stumm N, Moutsatsos I, McCoy JM, Crum CP, Genest D, Chin D, Ehrenfels C, Pijnenborg R, van Assche FA, and Mi S

Subjects

Female, Humans, Immunohistochemistry, In Situ Hybridization, Pregnancy, RNA, Messenger analysis, Tissue Distribution, Gene Expression Regulation, Gene Products, env analysis, Gene Products, env genetics, Placenta chemistry, Pre-Eclampsia metabolism, Pregnancy Proteins analysis, Pregnancy Proteins genetics

Abstract

Development of placentation and successful pregnancy depend on co-ordinated interactions between the maternal decidua and myometrium, and the invasive properties of the fetal trophoblast. Syncytin, a protein encoded by the envelope gene of a recently identified human endogenous defective retrovirus, HERV-W, is highly expressed in placental tissue. Previously, we have shown that the major site of syncytin expression is the placental syncytiotrophoblast, a fused multinuclear syncytium originating from cytotrophoblast cells. Here we present the first evidence that in pre-eclampsia, syncytin gene expression levels are dramatically reduced. Additionally, immunohistochemical examination of normal placentae and placentae from women with pre-eclampsia reveals that the syncytin protein in placental tissue from women with pre-eclampsia is localized improperly to the apical syncytiotrophoblast microvillous membrane as opposed to its normal location on the basal syncytiotrophoblast cytoplasmic membrane. Our previous results suggest that syncytin may mediate placental cytotrophoblast fusion in vivo and may play an important role in human placental morphogenesis. The present study suggests that altered expression of the syncytin gene, and altered cellular location of its protein product, may contribute to the aetiology of pre-eclampsia., (Copyright 2001 Harcourt Publishers Ltd.)

Published

2001

36. HIV type 1 non-B subtype prevalence in Spain, 1997-1998.

Author

García-Albert L, Ortiz M, and García-Saiz A

Subjects

Gene Products, env analysis, HIV Envelope Protein gp41, HIV Infections epidemiology, Humans, Peptide Fragments, Prevalence, Serotyping, Spain epidemiology, Enzyme-Linked Immunosorbent Assay methods, HIV Infections virology, HIV-1 classification

Abstract

We have evaluated the prevalence of HIV-1 non-B subtypes in Spain by means of an enzyme immunoassay (EIA) for discrimination between B and non-B subtypes. Samples were obtained from newly diagnosed patients attended at internal medicine outpatient clinics between October 1997 and October 1998. Discrimination between HIV-1 B and non-B subtypes was carried out by means of the EIA, with V3 synthetic peptides specific to the different subtypes. Non-B-serotyped samples were genetically analyzed in the gp41 region from the original sera. During the study period, 909 samples were collected from 21 medical units located in various Spanish geographical regions. Serotyping was possible in 885 cases, of which 791 were assigned as B serotype (89.38%), 70 showed no reactivity to any of the peptides (7.91%), and the remaining samples displayed other reaction patterns (2.72%). Of the 94 non-B-assigned samples, 65 were genetically characterized in the gp41 region of the env gene: 55 were B subtype, 5 were A subtype (4 clustered with CRF02AG reference strains), 3 were C subtype, and 2 were G subtype. The prevalence rate for non-B subtypes in Spain was established at 1.13% (95% CI, 0.59-2.21). Although the B subtype is predominant in the Spanish population, other subtypes have been detected.

Published

2001

37. Comparison of early plasma RNA loads in different macaque species and the impact of different routes of exposure on SIV/SHIV infection.

Author

ten Haaft P, Almond N, Biberfeld G, Cafaro A, Cranage M, Ensoli B, Hunsmann G, Polyanskaya N, Stahl-Hennig C, Thortensson R, Titti F, and Heeney J

Subjects

Animals, Chimera, Gene Products, env analysis, HIV Infections immunology, Humans, Retroviridae Proteins, Oncogenic analysis, Simian Acquired Immunodeficiency Syndrome immunology, Viral Fusion Proteins analysis, Viral Load, AIDS Vaccines, Acquired Immunodeficiency Syndrome physiopathology, HIV Infections virology, Macaca fascicularis virology, Macaca mulatta virology, RNA analysis, Simian Acquired Immunodeficiency Syndrome virology, Simian Immunodeficiency Virus pathogenicity

Abstract

Various simian immunodeficiency virus (SIV)sm/mac and simian/human immunodeficiency virus (SHIV) strains are used in different macaque species to study AIDS pathogenesis, as well as to evaluate candidate vaccine and anti-retroviral drugs efficacy. In this study we investigated the effect of route of infection, species of macaques and nature of virus stock on early plasma viral RNA load. We monitored the plasma RNA concentrations of 63 rhesus (Macaca mulatta) and cynomolgus macaques (Macaca fascicularis) infected with well-characterised virus stocks administered either by oral, rectal, vaginal or intravenous (i.v.) routes. In SIV(mac)-infected macaques, no significant difference in plasma RNA loads was observed between the rectal, oral and i.v. routes of infection. Cynomolgus macaques developed lower steady state SIV plasma RNA concentrations compared with rhesus macaques and no significant difference was observed between rectal and i.v. routes of infection. In SHIV(89.6p)-infected macaques, no difference between species or between route of infection was observed with this particular chimeric virus.

Published

2001

38. A solid phase plate assay for HIV-1 genotyping.

Author

González-Villaseñor LI, Wu K, and Yang L

Subjects

Biotinylation, Color, DNA Primers genetics, DNA, Viral analysis, DNA, Viral genetics, Gene Products, env analysis, Gene Products, env genetics, Genetic Variation genetics, Genotype, HIV Infections blood, HIV Infections diagnosis, HIV-1 genetics, Humans, Molecular Probe Techniques, Oligonucleotide Probes genetics, Polymerase Chain Reaction, Reference Standards, Reproducibility of Results, Sensitivity and Specificity, Solubility, Genes, Viral genetics, HIV Infections virology, HIV-1 classification, HIV-1 isolation & purification, Nucleic Acid Hybridization methods

Abstract

A prototype solid phase plate assay (SPPA) for the detection and genotyping of HIV-1 subtypes was developed using a PCR-based capture hybridization format. Well characterized HIV-1 reference controls of known subtypes and subtype specific capture oligonucleotide probes targeting several regions of the envelope (env) gene of HIV-1 were selected to develop the assay. The subtype specific oligonucleotide probes were covalently bound to microtubes in an ordered pattern and biotin labelled primers were used to amplify the target sequences. The PCR products were hybridized to the corresponding oligonucleotide probes, and colorimetrically detected by a chromogenic reaction using a standard microplate reader. All the HIV-1 subtype reference controls specifically hybridized to the corresponding capture probes and negligible cross-hybridization between subtypes was observed. To demonstrate the performance and reproducibility of the SPPA system and its validation with clinical samples, several human plasma samples of unknown and known HIV-1 subtypes were tested. The SPPA is highly specific and unambiguously identify the major subtypes of the HIV-1 M and O groups. This assay could be a useful method for subtyping samples of HIV-1 infected individuals and for disease management., (Copyright 2000 Academic Press.)

Published

2000

39. Analysis of recombinant protein expression by MALDI-TOF mass spectrometry of bacterial colonies.

Author

Winkler MA, Hickman RK, Golden A, and Aboleneen H

Subjects

Bacteriological Techniques, Gene Expression Regulation, Viral, Gene Products, env analysis, Gene Products, env genetics, HIV-1 genetics, Mutagenesis genetics, Plasmids, Promoter Regions, Genetic, Transformation, Genetic, Cloning, Molecular methods, Escherichia coli genetics, Recombinant Proteins analysis, Recombinant Proteins genetics, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods

Abstract

E. coli expressing soluble recombinant HIV antigens were analyzed directly by MALDI-TOF mass spectrometry (MS) from bacterial colonies picked from agar plates. An HIV envelope (ENV) antigen construct, penvA, was expressed in E. coli by transformation of the plasmid pPL/penvA-M. The plasmid was co-transformed into E. coli DH5 alpha cells with an equal quantity of the plasmid pKRR826, the parent vector without the penvA insert, and plated at medium density on L-agar plus ampicillin plates. A total of 24 colonies from four agar plates (six colonies per plate) were picked and transferred into 50% acetonitrile--0.1% trifluoroacetic acid aliquots for analysis by MALDI-TOF MS. The MS analysis detected 10 of 24 colonies expressing the recombinant protein; one colony expressed a mutant penvA protein; eleven of 24 colonies showed ions only from E. coli; and two of 24 colonies showed no detectable proteins. When E. coli transformed only with plasmid pPL/penvA-M were examined, all (10 of 10) colonies showed the penv insert by the MALDI-TOF MS method. The method is fast (less than 1.5 h for 24 colonies) and allows identification of colonies expressing intact or mutant proteins directly from culture plates without sample purification.

Published

2000

40. Detection of the human immunodeficiency virus regulatory protein tat in CNS tissues.

Author

Hudson L, Liu J, Nath A, Jones M, Raghavan R, Narayan O, Male D, and Everall I

Subjects

AIDS Dementia Complex metabolism, AIDS Dementia Complex pathology, Adult, Aged, Animals, Blotting, Western, Encephalitis, Viral metabolism, Encephalitis, Viral pathology, Enzyme-Linked Immunosorbent Assay, Female, Frontal Lobe pathology, Frontal Lobe virology, Gene Products, env analysis, Gene Products, vif analysis, HIV-1 isolation & purification, Humans, Lung chemistry, Lung pathology, Lung virology, Macaca mulatta, Male, Middle Aged, Postmortem Changes, Reverse Transcriptase Polymerase Chain Reaction, Sensitivity and Specificity, Simian Immunodeficiency Virus genetics, tat Gene Products, Human Immunodeficiency Virus, vif Gene Products, Human Immunodeficiency Virus, AIDS Dementia Complex virology, Encephalitis, Viral virology, Frontal Lobe chemistry, Gene Products, tat analysis, Genes, tat, HIV Infections virology, HIV-1 genetics, RNA, Messenger analysis, RNA, Viral analysis

Abstract

Neuropathologically, human immunodeficiency virus (HIV) is associated with a range of inflammatory disorders, extensive cortical neuronal loss, and dendritic and synaptic damage. Although the mechanisms resulting in these abnormalities are still unclear, the neurotoxic effects are thought to be due in part to viral products including the tat gene product. We have previously shown that Tat when presented to neurons extracellularly interacts with neuronal cell membranes to cause neuronal excitation and toxicity in fmole amounts. To determine the role of Tat in mediating HIV encephalitis (HIVE), we detected tat mRNA and protein in tissue extracts of nine patients with HIVE and seven patients without HIVE. Despite long autopsy times and significant degradation, tat mRNA was detected in 4/9 patients with HIVE but not in any of the seven patients without dementia. Similarly, the env mRNA was also detected in 5/9 patients with HIVE but not in the patients without HIVE. However, vif mRNA was detected in both groups of patients with (5/9) or without (2/7) HIVE. Using protein extracts from the brains of the same groups of patients we were unable to detect Tat by enzyme linked immunosorbant assay (ELISA) (sensitivity of 2 ng Tat/ml of brain tissue). However, Tat could be detected immunohistochemically and in protein extracts from the brains of rhesus macaques with encephalitis due to a chimeric strain of HIV and simian immunodeficiency virus (SHIV). Our observations support the role of Tat in the neuropathogenesis of HIV and SHIV encephalitis.

Published

2000

41. High frequency of non-B subtypes in newly diagnosed HIV-1 infections in Switzerland.

Author

Böni J, Pyra H, Gebhardt M, Perrin L, Bürgisser P, Matter L, Fierz W, Erb P, Piffaretti JC, Minder E, Grob P, Burckhardt JJ, Zwahlen M, and Schüpbach J

Subjects

Adult, Female, Gene Products, env analysis, HIV Infections epidemiology, Heterosexuality, Homosexuality, Humans, Male, Prevalence, Risk Factors, Substance Abuse, Intravenous complications, Switzerland epidemiology, HIV Infections virology, HIV-1 classification

Abstract

HIV-1 subtypes were determined in newly diagnosed residents of Switzerland. Blood was anonymously collected from patients with a first confirmed positive HIV-1 test result. Viral DNA from the env V3-V5 region was amplified by nested polymerase chain reaction (PCR) and screened for subtype B by heteroduplex mobility assay. All amplicons not identified as B were sequenced. From November 1996 to February 1998, 206 samples were analyzed. Main transmission risks were unprotected heterosexual (55.7%) or homosexual (27.1%) sexual contact or intravenous drug use (12.9%). Subtype B dominated in patients of Swiss, other European, American, or Asian citizenship; particularly high frequencies were found in homosexuals (97%) and drug users (94%). Non-B subtypes including A, C, D, E, F, G, H, a possible B/F recombinant, and a sequence related to J were present in 28.2% (95% confidence interval [CI], 22.9%-35.0%). Non-B were frequent in African citizens (95%), heterosexually infected individuals (44%), and women (43%). Heterosexually infected Swiss males harbored non-B strains in 18% and females in 33%. The results document a change in the epidemiology of newly diagnosed HIV-1 infections in Switzerland: predominance of heterosexual transmission and a high frequency of non-B subtypes.

Published

1999

42. A new sensitive serological assay for detection of lentivirus infections in small ruminants.

Author

Saman E, Van Eynde G, Lujan L, Extramiana B, Harkiss G, Tolari F, Gonzàlez L, Amorena B, Watt N, and Badiola J

Subjects

Amino Acid Sequence, Animals, Antibodies, Viral analysis, Antibodies, Viral blood, Antibody Specificity, Antisense Elements (Genetics), Arthritis-Encephalitis Virus, Caprine genetics, Arthritis-Encephalitis Virus, Caprine immunology, Blotting, Western, Europe, Female, Gene Products, env analysis, Gene Products, env genetics, Gene Products, env immunology, Gene Products, gag analysis, Gene Products, gag genetics, Gene Products, gag immunology, Glutathione Transferase genetics, Goats, Immunodominant Epitopes analysis, Immunodominant Epitopes immunology, Lentivirus Infections immunology, Mass Screening methods, Milk virology, Molecular Sequence Data, Pneumonia, Progressive Interstitial, of Sheep diagnosis, Recombinant Proteins immunology, Sensitivity and Specificity, Sheep, Viral Proteins analysis, Viral Proteins genetics, Visna-maedi virus genetics, Visna-maedi virus immunology, Visna-maedi virus isolation & purification, Arthritis-Encephalitis Virus, Caprine isolation & purification, Enzyme-Linked Immunosorbent Assay methods, Lentivirus Infections diagnosis, Sheep Diseases diagnosis, Sheep Diseases virology

Abstract

Lentivirus infections in small ruminants represent an economic problem affecting several European countries with important sheep-breeding industries. Programs for control and eradication of these infections are being initiated and require reliable screening assays. This communication describes the construction and evaluation of a new serological screening enzyme-linked immunosorbent assay (ELISA) for the detection of antibodies to maedi-visna virus (MVV) in sheep and to caprine arthritis encephalitis virus (CAEV) in goats. The solid phase is sensitized with a combination of the major core protein p25 of MVV produced in Escherichia coli and a peptide derived from the immunodominant region of the viral transmembrane protein gp46. The peptide carries an N-terminal biotin residue and is complexed with streptavidin prior to being coated. The new assay was evaluated with 2,336 sheep serum samples from different European countries with large differences in the levels of prevalence of MVV infections, and the results have been compared to those of the standard agar gel immunodiffusion test. Discrepant samples were analyzed by Western blotting with viral lysate, and most sera could be classified unambiguously. The estimated overall sensitivity of the new ELISA was 99.4% (95% confidence interval [CI], 98.4 to 99. 8%) and the specificity was 99.3% (95% CI, 98.7 to 99.6%). A limited set of goat sera (n = 212) was also analyzed, with similar results. These data indicate that the new assay is a reliable tool that can be used in control and eradication programs for small ruminant lentivirus infections.

Published

1999

43. Establishment of a seronegative human T-cell leukemia virus type 1 (HTLV-1) carrier state in rats inoculated with a syngeneic HTLV-1-immortalized T-cell line preferentially expressing Tax.

Author

Koya Y, Ohashi T, Kato H, Hanabuchi S, Tsukahara T, Takemura F, Etoh K, Matsuoka M, Fujii M, and Kannagi M

Subjects

Animals, Antibodies, Viral blood, Cell Line, Transformed, Deltaretrovirus Antigens analysis, Disease Models, Animal, Female, Gene Expression, Gene Products, env analysis, Gene Products, gag analysis, HTLV-I Infections blood, HTLV-I Infections immunology, Human T-lymphotropic virus 1 immunology, Humans, Phenotype, Proviruses, RNA, Viral, Rats, Rats, Inbred F344, Retroviridae Proteins, Oncogenic analysis, Virus Integration, Virus Latency, gag Gene Products, Human Immunodeficiency Virus, Carrier State, Gene Products, tax biosynthesis, HTLV-I Infections virology, Human T-lymphotropic virus 1 physiology

Abstract

Human T-cell leukemia virus type 1 (HTLV-1) causes T-cell malignancies in a small percentage of the population infected with the virus after a long carrier state. In the present study, we established a seronegative HTLV-1 carrier state in rats inoculated with a newly established HTLV-1-infected rat T cell line, FPM1. FPM1 originated from rat thymocytes cocultured with a human HTLV-1 producer, MT-2 cells, and expressed rat CD4, CD5, CD25, and HTLV-1 Tax. However, FPM1 scarcely expressed other major HTLV-1 structural proteins and failed to induce typical antibody responses against HTLV-1 in inoculated rats. In contrast, control rats inoculated with MT-2 cells generated significant levels of anti-HTLV-1 antibodies. HTLV-1 proviruses were detected in peripheral blood cells of syngeneic rats inoculated with FPM1 for more than 1 year. Analysis of the flanking region of HTLV-1 provirus integrated into host cells suggested that FPM1 cells remained in these animals over a relatively long period of time. However, a similar seronegative HTLV-1 carrier state was induced in the rats inoculated with mitomycin C-treated FPM1 cells and also in FPM1-inoculated allogeneic rats, suggesting that FPM1 could also transmit HTLV-1 into host cells in vivo. Our findings indicated that (i) HTLV-1-immortalized T cells which preferentially express HTLV-1 Tax persisted in vivo but failed to induce any diseases in immunocompetent syngeneic rats and that (ii) suboptimal levels of HTLV-1 for antibody responses allowed the establishment of persistent HTLV-1 infection.

Published

1999

44. Comparison of four tests to evaluate the reactivity of rabbit sera against envelope or Gag-related proteins of bovine leukemia virus (BLV).

Author

Doménech A, Llames L, Goyache J, Suárez G, and Gómez-Lucía E

Subjects

Animals, Blotting, Western, Cattle, Cell Line, Enzootic Bovine Leukosis blood, Enzootic Bovine Leukosis immunology, Enzyme-Linked Immunosorbent Assay, Giant Cells, Immunodiffusion, Leukemia Virus, Bovine physiology, Rabbits, Reproducibility of Results, Sensitivity and Specificity, Virology methods, Virus Latency, Antibodies, Viral blood, Enzootic Bovine Leukosis diagnosis, Gene Products, env analysis, Gene Products, gag analysis, Leukemia Virus, Bovine isolation & purification

Abstract

Bovine leukemia virus (BLV) has a long latency period during which animals are inapparently infected, may spread the disease, and are only detected by serological techniques or by the most cumbersome molecular biology techniques. We have compared techniques for detecting either total antibodies (ELISA), anti-p24 and Gag-related proteins (Western blot), or anti-gp51 (agar gel immunodiffusion, AGID, and syncytia inhibition, SI) in rabbits inoculated experimentally with inocula of variable immunogenicity. The two tests to detect antibodies to gp51 correlated well in sera clearly positive or clearly negative by either one, but correlation was poor in the intermediate groups. All sera positive by AGID were also positive by ELISA, but results did not agree in sera negative by AGID, ELISA proving to be more sensitive. Western blot was a good technique for detecting antibodies against Gag-related proteins. However, no band was identified to clearly correspond to anti-Env-related proteins. As for other retroviruses, testing of animals for infection with BLV should include the detection of antibodies anti-Gag and anti-Env proteins.

Published

1998

45. Detection of endogenous retrovirus antigens in NOD mouse pancreatic beta-cells.

Author

Tsumura H, Miyazawa M, Ogawa S, Wang JZ, Ito Y, and Shimura K

Subjects

Animals, Antibodies, Heterophile pharmacology, Antibodies, Monoclonal immunology, Antigens, Viral immunology, Female, Gammaretrovirus genetics, Gammaretrovirus physiology, Gene Products, env analysis, Gene Products, gag analysis, Immunoenzyme Techniques, Islets of Langerhans immunology, Islets of Langerhans pathology, Male, Mice, Mice, Inbred NOD, Microscopy, Electron, Microscopy, Fluorescence, Oligonucleotides, Antisense chemistry, Oligonucleotides, Antisense immunology, Oligonucleotides, Antisense pharmacology, Specific Pathogen-Free Organisms, Thionucleotides immunology, Thionucleotides pharmacology, Virion genetics, Virion physiology, Antigens, Viral analysis, Diabetes Mellitus, Type 1 virology, Gammaretrovirus immunology, Islets of Langerhans virology, Virion immunology

Abstract

We characterized C-type retroviruses expressed in the pancreatic beta-cells of non-obese diabetic (NOD) mice by immunohistochemical techniques and by inhibiting the production of viral particles using antisense oligonucleotides. Some cells in the pancreatic islets from both NOD and diabetes-resistant NOD-related mice (NON) reacted with a monoclonal antibody directed against the envelope protein(s) of polytropic viruses. On the other hand, NOD islet cells also showed strong immunoreactivity with an anti-gag protein monoclonal antibody and another anti-envelope protein(s) monoclonal antibody that is specific for xenotropic viruses. In antisense oligodeoxynucleotide inhibition assays, a xenotropic virus-specific phosphorothionate-particles antisense oligodeoxynucleotide significantly inhibited the occurrence of C-type virus particles in NOD mouse islet beta-cells. Therefore, C-type retrovirus-like particles expressed in NOD mouse pancreatic beta-cells were considered to be endogenous xenotropic virus. The expression of the xenotropic viral genome may be involved in the pathogenesis of the diabetic syndrome in NOD mice.

Published

1998

46. In vitro characterization of adult primary human immunodeficiency virus type 1: demonstration of distinctive single-cell killing phenotypes in spite of similar levels of viral replication.

Author

Pal A, Greenough TC, Sullivan JL, and Somasundaran M

Subjects

Acquired Immunodeficiency Syndrome virology, Adult, CD4 Antigens immunology, CD4 Lymphocyte Count, CD4-Positive T-Lymphocytes immunology, CD4-Positive T-Lymphocytes virology, CD8-Positive T-Lymphocytes immunology, Cell Death physiology, Cells, Cultured, Cytopathogenic Effect, Viral, Gene Products, env analysis, Gene Products, env genetics, Giant Cells virology, HIV-1 growth & development, HIV-1 pathogenicity, Hemophilia A virology, Humans, Kinetics, Leukocytes, Mononuclear virology, Mitochondria physiology, Polymerase Chain Reaction, Proviruses growth & development, Survivors, HIV Infections virology, HIV-1 physiology, Virus Replication

Abstract

Two primary human immunodeficiency virus (HIV)-1 biologic clones have been studied extensively in a system using CD4 T cell-enriched peripheral blood lymphocytes and anti-CD4 antibody to measure viral replication kinetics and single-cell cytopathicity. Biologic clones from a person with AIDS replicated to high levels and were cytopathic in the absence of syncytium formation. Unexpectedly, biologic clones from an adult long-term nonprogressor were noncytopathic in spite of similar levels of viral replication. A correlation has recently been demonstrated between reduced mitochondrial viability and cell death in HIV-1-infected cultures. Peripheral blood-derived CD4 T cells infected with the cytopathic clone showed a progressive reduction in mitochondrial viability, while those infected with the noncytopathic clone demonstrated functionally viable mitochondria. These studies demonstrate that primary HIV-1-induced cytopathicity is separable from syncytium formation and replication rate.

Published

1997

47. An HIV type 1 epidemic among injecting drug users in the former Soviet Union caused by a homogeneous subtype A strain.

Author

Bobkov A, Cheingsong-Popov R, Selimova L, Ladnaya N, Kazennova E, Kravchenko A, Fedotov E, Saukhat S, Zverev S, Pokrovsky V, and Weber J

Subjects

Adolescent, Adult, Amino Acid Sequence, Female, Gene Products, env analysis, Gene Products, env chemistry, Gene Products, env genetics, Gene Products, gag analysis, Gene Products, gag chemistry, Gene Products, gag genetics, HIV Infections blood, HIV Infections genetics, HIV-1 classification, HIV-1 isolation & purification, Humans, Male, Molecular Sequence Data, Phylogeny, Russia epidemiology, Sequence Homology, Amino Acid, Substance Abuse, Intravenous physiopathology, Ukraine epidemiology, Disease Outbreaks, HIV Infections epidemiology, HIV-1 genetics, Substance Abuse, Intravenous virology

Abstract

Epidemiological data have demonstrated rapid growth of HIV-1 infections among injecting drug users (IDUs) in the Ukraine and Russia, during 1996. Here we describe the results of genetic analysis of isolates derived from 12 HIV-1-infected IDUs in different sites of Russia and the Ukraine. The blood samples were taken within a 1- to 2-month period after the first HIV-1-positive test. The results of the heteroduplex mobility assay as well as gag/env phylogenetic analysis reveal that all sequences belong to gag/env genetic subtype A. Moreover, interpatient genetic distances between the nucleotide sequences encompassing the C2-V3, the V4-V5, and p17-encoding regions within this group were low (the average means were 0.9, 1.3, and 0.4%, respectively). These data show a marked homogeneity of HIV-1, probably spreading during primary infection. It is possible that the current epidemic of subtype A HIV-1 among IDUs in the former Soviet Union is caused by a point source exposure.

Published

1997

48. Human immunodeficiency virus type 2 (HIV-2) seroprevalence and characterization of a distinct HIV-2 genetic subtype from the natural range of simian immunodeficiency virus-infected sooty mangabeys.

Author

Chen Z, Luckay A, Sodora DL, Telfer P, Reed P, Gettie A, Kanu JM, Sadek RF, Yee J, Ho DD, Zhang L, and Marx PA

Subjects

Adolescent, Adult, Aged, Amino Acid Sequence, Animals, Blotting, Western, Child, Female, Gene Products, env analysis, Gene Products, gag analysis, Genotype, HIV-2 genetics, HIV-2 immunology, Humans, Male, Middle Aged, Molecular Sequence Data, Phylogeny, Cercocebus atys virology, HIV Seroprevalence, HIV-2 classification, Simian Immunodeficiency Virus classification

Abstract

The extent of zoonotic infections in rural Sierra Leone, where both feral and pet sooty mangabeys harbor divergent members of the human immunodeficiency virus type 2 (HIV-2)-sooty mangabey simian immunodeficiency virus (SIVsm) family, was tested in blood samples collected from 9,309 human subjects in 1993. Using HIV-1- and HIV-2-specific enzyme immunoassays and confirmatory Western blot analysis to test for antibodies to SIVsm-related lentiviruses, we found only nine subjects (0.096%) who tested positive for HIV: seven tested positive for HIV-1 and two tested positive for HIV-2. Compared with other rural West African communities, Sierra Leone displayed the lowest seroprevalence (0.021%) of HIV-2 infection yet reported, much lower than the previously reported seroprevalence in SIVsm-infected feral and household pet sooty mangabeys. Heteroduplex analysis demonstrated that two of the newly found HIV-1 strains belonged to subtype A, the most common HIV-1 subtype in Africa, but this is the first report of subtype A in Sierra Leone. The two HIV-2-infected individuals harbored two distinct HIV-2 strains, designated 93SL1 and 93SL2. Phylogenetic analysis indicated that HIV-2 93SL1 is a member of HIV-2 subtype A, the first strain of this HIV-2 subtype found in Sierra Leone. In contrast, HIV-2 93SL2 belongs to none of the five previously characterized HIV-2 subtypes (A to E) but is a new subtype, herein designated F, having the most divergent transmembrane sequences yet reported for HIV-2. The fact that both of the two most divergent HIV-2 subtypes known, E and F, are rare and found as single occurrences in persons from Sierra Leone may be related to the fact that this small region of West Africa also contains free-living and household pet sooty mangabeys with highly divergent variants of SIVsm. This finding provides support for the hypotheses that new HIV-2 subtypes result from independent cross-species transmission of SIVsm to the human population and that these single-occurrence transmission events had not spread widely into the population by 1993.

Published

1997

49. [Gene products of human endogenous retrovirus (HERV)-K in germ cell and trophoblastic tumors].

Author

Herbst H, Sauter M, Fuchs H, Kühler-Obbarius C, Löning T, and Mueller-Lantzsch N

Subjects

Adult, Female, Gene Products, env analysis, Gene Products, gag analysis, Genes, env, Genes, gag, Germinoma pathology, Humans, Male, Ovarian Neoplasms classification, Ovarian Neoplasms pathology, Pregnancy, Testicular Neoplasms classification, Testicular Neoplasms pathology, Trophoblastic Neoplasms pathology, Germinoma virology, Ovarian Neoplasms virology, Retroviridae genetics, Retroviridae isolation & purification, Testicular Neoplasms virology, Trophoblastic Neoplasms virology

Abstract

Antibodies against Gag and Env proteins encoded by human endogenous retrovirus (HERV)-K genomes are found in the sera of patients with classical seminoma. This prompted us to study ovarian and testicular germ cell tumors, their precursor lesions, dysgenetic gonads, and trophoblast lesions for expression of HERV-K sequences by in situ hybridization using radioactive and non-radioactive probes. Expression of HERV-K sequences was found in all testicular and ovarian germ cell tumors with the exception of teratomas and spermatocytic seminomas. HERV-K expression was also found in testicular intraepithelial neoplasia (so-called carcinoma in situ) as well as in gonocytes of dysgenetic gonads. Among gestational trophoblastic lesions, HERV-K expression was regularly found in choriocarcinomas, but not in non-invasive molar lesions. There was no evidence for HERV-K expression in differentiated embryonal and adult tissues. The findings point to a common molecular pathogenesis of most germ cell tumor entities and malignant gestational trophoblastic disease. They furthermore support the concept of carcinoma in situ as a precursor lesion common to most testicular germ cell tumors. Conceivably, the detection of HERV-K gene products in body fluids and tissues will aid diagnosis and monitoring of germ cell tumors and related lesions.

Published

1997

50. Characterization of a putative retroviral env-related human protein.

Author

Turbeville MA, Rhodes JC, Hyams DM, Distler CM, and Steele PE

Subjects

Adenocarcinoma chemistry, Animals, Antibody Formation, Antibody Specificity, Colonic Neoplasms chemistry, Endothelium chemistry, Gene Products, env immunology, Humans, Male, Prostatic Neoplasms chemistry, Rabbits, Recombinant Fusion Proteins analysis, Recombinant Fusion Proteins immunology, Retroviridae Proteins immunology, Seminoma chemistry, Testicular Neoplasms chemistry, Tumor Cells, Cultured chemistry, Viral Envelope Proteins immunology, Gene Products, env analysis, Neoplasm Proteins, Neoplasms chemistry, Retroviridae, Retroviridae Proteins analysis, Viral Envelope Proteins analysis

Abstract

In this study, we developed a rabbit polyclonal antibody to a fusion protein containing the envelope (env) transmembrane (TM) region from the human endogenous retroviral family, HERV-E. We used this reagent to document the expression of TM-related protein by Western blot in endothelial, colon and prostate carcinoma and seminoma cell lines and in peripheral blood mononuclear cells from a healthy donor. We detected a 58-kD protein (as compared to murine TM of 15 kD) that had specificity for the env-related antibodies of the polyclonal antiserum.

Published

1997