Your search keyword '"Adenovirus E3 Proteins biosynthesis"' showing total 26 results

1. The tripartite leader sequence is required for ectopic expression of HAdV-B and HAdV-E E3 CR1 genes.

Author

Bair CR, Kotha Lakshmi Narayan P, and Kajon AE

Subjects

Adenoviruses, Human classification, Electroporation, Genetic Vectors genetics, HEK293 Cells, HeLa Cells, Humans, Microscopy, Fluorescence, Open Reading Frames genetics, Protein Sorting Signals, Transfection, Viral Proteins genetics, 5' Untranslated Regions genetics, Adenovirus E3 Proteins biosynthesis, Adenovirus E3 Proteins genetics, Adenoviruses, Human genetics, Ectopic Gene Expression genetics, Genome, Viral genetics

Abstract

The unique repertoire of genes that characterizes the early region 3 (E3) of the different species of human adenovirus (HAdV) likely contributes to their distinct pathogenic traits. The function of many E3 CR1 proteins remains unknown possibly due to unidentified intrinsic properties that make them difficult to express ectopically. This study shows that the species HAdV-B- and HAdV-E-specific E3 CR1 genes can be expressed from vectors carrying the HAdV tripartite leader (TPL) sequence but not from traditional mammalian expression vectors. Insertion of the TPL sequence upstream of the HAdV-B and HAdV-E E3 CR1 open reading frames was sufficient to rescue protein expression from pCI-neo constructs in transfected 293T cells. The detection of higher levels of HAdV-B and HAdV-E E3 CR1 transcripts suggests that the TPL sequence may enhance gene expression at both the transcriptional and translational levels. Our findings will facilitate the characterization of additional AdV E3 proteins., (Copyright © 2017 Elsevier Inc. All rights reserved.)

Published

2017

2. Fluorescent site-specific labeling of Escherichia coli expressed proteins with Sfp phosphopantetheinyl transferase.

Author

Zhang A, Sun L, Buswell J, Considine N, Ghosh I, Masharina A, Noren C, and Xu MQ

Subjects

Bacterial Proteins chemistry, Bacterial Proteins genetics, Escherichia coli genetics, Transferases (Other Substituted Phosphate Groups) chemistry, Transferases (Other Substituted Phosphate Groups) genetics, Adenovirus E3 Proteins biosynthesis, Adenovirus E3 Proteins chemistry, Adenovirus E3 Proteins genetics, Bacterial Proteins metabolism, Escherichia coli metabolism, Fluorescent Dyes chemistry, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Transferases (Other Substituted Phosphate Groups) metabolism

Abstract

Fluorescent tagging of proteins has become a critical step in optical analysis of protein function in vitro and in living cells. Here we describe a two-tag system for expression and isolation of a protein of interest from Escherichia coli and subsequent site-specific fluorescent labeling with Sfp phosphopantetheinyl transferase (Sfp synthase). In the example presented, adenoviral protein E3-14.7 K (E14.7) was expressed as a tripartite fusion protein with a fluorophore-targeting peptide tag and a chitin-binding domain. This system allows for rapid isolation of the recombinant fusion protein from crude bacterial cell lysate via a single chitin column. Sfp synthase-mediated labeling with fluorophore conjugated to coenzyme A-SH (CoA-SH) resulted in covalent attachment of a fluorescent dye to a specific residue of the peptide tag via a phosphopantetheinyl linker. The fluorescently labeled E14.7 fusion protein was analyzed with a fluorescence imager and subsequently transfected into mammalian cells for imaging with a fluorescence microscope.

Published

2011

3. An acute toxicology study with INGN 007, an oncolytic adenovirus vector, in mice and permissive Syrian hamsters; comparisons with wild-type Ad5 and a replication-defective adenovirus vector.

Author

Lichtenstein DL, Spencer JF, Doronin K, Patra D, Meyer JM, Shashkova EV, Kuppuswamy M, Dhar D, Thomas MA, Tollefson AE, Zumstein LA, Wold WS, and Toth K

Subjects

Adenovirus E3 Proteins biosynthesis, Animals, Blood Cell Count, Cell Line, Cricetinae, Erythropoiesis, Genetic Vectors administration & dosage, Humans, Injections, Intravenous, Liver pathology, Liver virology, Mesocricetus, Mice, Mice, Inbred C57BL, Oncolytic Viruses, Virus Replication, Adenoviridae physiology, Genetic Vectors adverse effects

Abstract

Oncolytic (replication-competent) adenoviruses as anticancer agents provide new, promising tools to fight cancer. In support of a Phase I clinical trial, here we report safety data with INGN 007 (VRX-007), an oncolytic adenovirus with increased anti-tumor efficacy due to overexpression of the adenovirus-encoded ADP protein. Wild-type adenovirus type 5 (Ad5) and a replication-defective version of Ad5 were also studied as controls. A parallel study investigating the biodistribution of these viruses is described elsewhere in this issue. The toxicology experiments were conducted in two species, the Syrian hamster, which is permissive for INGN 007 and Ad5 replication and the poorly permissive mouse. The studies demonstrated that the safety profile of INGN 007 is similar to Ad5. Both viruses caused transient liver damage upon intravenous injection that resolved by 28 days post-infection. The No-Observable-Adverse-Effect-Level (NOAEL) for INGN 007 in hamsters was 3 x 10(10) viral particles per kg. In hamsters, the replication-defective vector caused less toxicity, indicating that replication of Ad vectors in the host is an important factor in pathogenesis. With mice, INGN 007 and Ad5 caused toxicity comparable to the replication-defective adenovirus vector. Partially based on these results, the FDA granted permission to enter into a Phase I clinical trial with INGN 007.

Published

2009

4. Anticancer activity of oncolytic adenovirus vector armed with IFN-alpha and ADP is enhanced by pharmacologically controlled expression of TRAIL.

Author

Shashkova EV, Kuppuswamy MN, Wold WS, and Doronin K

Subjects

Adenoviridae physiology, Adenovirus E3 Proteins biosynthesis, Adenovirus E3 Proteins physiology, Animals, Apoptosis genetics, Cell Line, Tumor, Doxycycline pharmacology, Gene Expression Regulation, Neoplastic drug effects, Gene Expression Regulation, Neoplastic physiology, Humans, Interferon-alpha biosynthesis, Interferon-alpha physiology, Mice, Mutation, Neoplasms genetics, Neoplasms pathology, TNF-Related Apoptosis-Inducing Ligand physiology, Tetracycline pharmacology, Adenoviridae genetics, Adenovirus E3 Proteins genetics, Genetic Therapy, Genetic Vectors, Interferon-alpha genetics, Neoplasms therapy, TNF-Related Apoptosis-Inducing Ligand biosynthesis, TNF-Related Apoptosis-Inducing Ligand genetics

Abstract

We have previously described oncolytic adenovirus (Ad) vectors KD3 and KD3-interferon (IFN) that were rendered cancer-specific by mutations in the E1A region of Ad; these mutations abolish binding of E1A proteins to p300/CBP and pRB. The antitumor activity of the vectors was enhanced by overexpression of the Adenovirus Death Protein (ADP, E3-11.6K) and by replication-linked expression of IFN-alpha. We hypothesized that the anticancer efficacy of the KD3-IFN vector could be further improved by expression of tumor necrosis factor-related apoptosis-inducing ligand (TRAIL). E1-deleted Ad vectors were constructed carrying reporter genes for enhanced green fluorescent protein or secreted placental alkaline phosphatase (SEAP) and a therapeutic gene for TRAIL under control of the TetON system. Expression of the genes was increased in the presence of a helper virus and the inducer doxycycline such that up to 231-fold activation of expression for the TetON-SEAP vector was obtained. Coinfection with TetON-TRAIL augmented oncolytic activity of KD3 and KD3-IFN in vitro. Induction of TRAIL expression did not reduce the yield of progeny virus. Combination of TetON-TRAIL and KD3-IFN produced superior antitumor activity in vivo as compared with either vector alone demonstrating the efficacy of a four-pronged cancer gene therapy approach, which includes Ad oncolysis, ADP overexpression, IFN-alpha-mediated immunotherapy, and pharmacologically controlled TRAIL activity.

Published

2008

5. Noninvasive visualization of adenovirus replication with a fluorescent reporter in the E3 region.

Author

Ono HA, Le LP, Davydova JG, Gavrikova T, and Yamamoto M

Subjects

Adenocarcinoma virology, Adenoviridae genetics, Adenovirus E3 Proteins biosynthesis, Animals, Cell Line, Transformed, Cell Line, Tumor, DNA Replication, Fluorescence, Genes, Reporter, Genetic Vectors genetics, Genetic Vectors physiology, Green Fluorescent Proteins biosynthesis, Green Fluorescent Proteins genetics, Humans, Lung Neoplasms virology, Male, Mice, Mice, Inbred BALB C, Mice, Nude, Virus Replication genetics, Adenoviridae physiology, Adenovirus E3 Proteins genetics, Green Fluorescent Proteins analysis, Virus Replication physiology

Abstract

To overcome the inefficacy and undesirable side effects of current cancer treatment strategies, conditionally replicative adenoviruses have been developed to exploit the unique mechanism of oncolysis afforded by tumor-specific viral replication. Despite rapid translation into clinical trials and the established safety of oncolytic adenoviruses, the in vivo function of these agents is not well understood due to lack of a noninvasive detection system for adenovirus replication. To address this issue, we propose the expression of a reporter from the adenovirus E3 region as a means to monitor replication. Adenovirus replication reporter vectors were constructed with the enhanced green fluorescent protein (EGFP) gene placed in the deleted E3 region under the control of the adenoviral major late promoter while retaining expression of the adenovirus death protein to conserve the native oncolytic capability of the virus. Strong EGFP fluorescence was detected from these vectors in a replication-dependent manner, which correlated with viral DNA replication. Fluorescence imaging in vivo confirmed the ability to noninvasively detect fluorescent signal during replication, which generally corresponded with the underlying level of viral DNA replication. EGFP representation of viral replication was further confirmed by Western blot comparison with the viral DNA content in the tumors. Imaging reporter expression controlled by the adenoviral major late promoter provides a viable approach to noninvasively monitor adenovirus replication in preclinical studies and has the potential for human application with clinically relevant imaging reporters.

Published

2005

6. The endoplasmic reticulum lumenal domain of the adenovirus type 2 E3-19K protein binds to peptide-filled and peptide-deficient HLA-A*1101 molecules.

Author

Liu H, Stafford WF, and Bouvier M

Subjects

Adenovirus E3 Proteins biosynthesis, Adenovirus E3 Proteins chemistry, Baculoviridae metabolism, Electrophoretic Mobility Shift Assay, Endoplasmic Reticulum, HLA-A Antigens biosynthesis, HLA-A Antigens chemistry, In Vitro Techniques, Peptide Fragments, Protein Binding, Recombinant Proteins biosynthesis, Recombinant Proteins metabolism, Solubility, Adenoviridae immunology, Adenovirus E3 Proteins metabolism, HLA-A Antigens metabolism

Abstract

E3-19K is a type I membrane glycoprotein expressed by adenoviruses (Ads) to modulate host antiviral immune responses. We have developed an expression system for the endoplasmic reticulum lumenal domain (residues 1 to 100) of Ad type 2 E3-19K tagged with a C-terminal His6 sequence in baculovirus-infected insect cells. In this system, recombinant E3-19K is secreted into the culture medium. A characterization of soluble E3-19K by analytical ultracentrifugation and circular dichroism showed that the protein is monomeric and adopts a stable and correctly folded tertiary structure. Using a gel mobility shift assay and analytical ultracentrifugation, we showed that soluble E3-19K associates with soluble peptide-filled and peptide-deficient HLA-A*1101 molecules. This is the first example of a viral immunomodulatory protein that interacts with conformationally distinct forms of class I major histocompatibility complex molecules. The E3-19K/HLA-A*1101 complexes formed in a 1:1 stoichiometry with equilibrium dissociation constants (Kd) of 50 +/- 10 nM for peptide-filled molecules and of about 10 microM for peptide-deficient molecules. A temperature-dependent proteolysis study revealed that the association of E3-19K with peptide-deficient HLA-A*1101 molecules stabilizes the binding groove. Importantly, our studies showed that peptide-deficient HLA-A*1101 molecules sequestered by E3-19K are capable of binding antigenic peptides and maturing into peptide-filled molecules. This firmly establishes that E3-19K does not block binding of antigenic peptides. Together, our results suggest that Ads have evolved to exploit the late and early stages of the class I antigen presentation pathway.

Published

2005

7. ADP-overexpressing adenovirus elicits enhanced cytopathic effect by induction of apoptosis.

Author

Yun CO, Kim E, Koo T, Kim H, Lee YS, and Kim JH

Subjects

Adenoviridae pathogenicity, Adenovirus E3 Proteins pharmacology, Animals, Carcinoma, Hepatocellular genetics, Carcinoma, Hepatocellular pathology, Drug Screening Assays, Antitumor, Female, Fibroblasts, Humans, Liver Neoplasms genetics, Liver Neoplasms pathology, Liver Neoplasms therapy, Male, Membrane Glycoproteins, Mice, Mice, Nude, RNA, Messenger analysis, RNA, Messenger biosynthesis, Transplantation, Heterologous, Tumor Cells, Cultured, Uterine Cervical Neoplasms genetics, Uterine Cervical Neoplasms pathology, Virus Replication, Adenoviridae genetics, Adenovirus E3 Proteins biosynthesis, Adenovirus E3 Proteins genetics, Apoptosis genetics, Carcinoma, Hepatocellular therapy, Genetic Therapy methods, Uterine Cervical Neoplasms therapy

Abstract

Replication-competent adenoviruses (Ad's) are emerging as a promising new modality for treatment of cancer. Selective replication of viral agents in tumor may lead to improved efficacy over nonreplicating Ad's due to their inherent ability to multiply, lyse, and spread to surrounding cells. We have previously shown that an E1B 55 kDa-deleted adenovirus (YKL-1) exhibits tumor-specific replication and cell lysis, but its cytolytic effects were reduced in comparison to the wild-type adenovirus. To increase the oncolytic potency of YKL-1, we have reintroduced the Ad death protein (ADP) gene under the control of either a CMV or an MLP promoter at the E3 region of YKL-1, generating YKL-cADP and YKL-mADP Ad's, respectively. ADP is an 11.6 kDa protein encoded by the E3 transcription unit, and is required to kill adenovirus-infected cells efficiently. However, to date, the mechanism by which ADP mediates cell death has not been clearly defined. In this study, we report that ADP-overexpressing Ad markedly enhanced cytolytic effect (up to 100-fold) against all tumor cell lines tested, but did not increase cytopathic effect in normal skin fibroblast, BJ. Moreover, plaque size formed by YKL-cADP was substantially larger than that of YKL-1, indicating an enhancement in cell lysis. TUNEL (terminal deoxynucleotidyl transferase-mediated dUTP nick-end labeling) assay and Annexin-V/PI double staining indicate that ADP-mediated cytotoxicity was largely driven by apoptosis. Finally, YKL-cADP adenovirus also showed superior antitumor effect than YKL-1 and YKL-mADP in C33A cervical and Hep3B hepatoma xenograft tumor models. Taken together, these lines of evidence demonstrate that the newly generated adenovirus expressing ADP under the CMV promoter induces efficient but tumor-selective cell lysis, which is critical for adding therapeutic value to replicating adenovirus for its use in cancer gene therapy.

Published

2005

8. Overexpression of adenovirus E3-11.6K protein induces cell killing by both caspase-dependent and caspase-independent mechanisms.

Author

Zou A, Atencio I, Huang WM, Horn M, and Ramachandra M

Subjects

Adenoviridae genetics, Adenovirus E3 Proteins genetics, Apoptosis, Cell Line, Tumor, Cytopathogenic Effect, Viral, Humans, Promoter Regions, Genetic, Recombinant Proteins biosynthesis, Adenoviridae metabolism, Adenovirus E3 Proteins biosynthesis, Caspases metabolism

Abstract

Recent studies have shown enhanced antitumor efficacy with adenoviruses that either lack E1B-19K or overexpress E3-11.6K (also known as adenoviral death protein). E1B-19K is a well-characterized anti-apoptotic protein, and viruses with E1B-19K deletions show increased cytopathicity. However, the mechanism of cell killing by E3-11.6K, which plays an important role in killing infected cells and virion release, is not well characterized. To understand the mechanism of cell killing following E3-11.6K overexpression, we constructed a recombinant adenovirus, Ad-ME, by introducing viral major late promoter upstream of the E3-11.6K sequence. Similar to the E1B-19K-deleted virus, E1B/19K-, Ad-ME induced cell death to a greater extent than the wild-type virus. Cell shrinkage, membrane blebbing, activation of caspases 3 and 9, cleavage of poly(ADP-ribose)polymerase (PARP), DNA degradation, and ratio of ADP to ATP in Ad-ME-infected cells indicated that apoptosis contributes to cell death following E3-11.6K overexpression. However, the levels of activation of caspases 3 and 9 were lower in cells infected with Ad-ME compared to those infected with E1B/19K-. Furthermore, cell killing by Ad-ME was not effectively inhibited by Z-VAD-FMK, a general caspase inhibitor. Taken together, our results suggest both caspase-dependent and caspase-independent mechanisms of cell killing due to overexpression of E3-11.6K.

Published

2004

9. An oncolytic adenovirus vector combining enhanced cell-to-cell spreading, mediated by the ADP cytolytic protein, with selective replication in cancer cells with deregulated wnt signaling.

Author

Toth K, Djeha H, Ying B, Tollefson AE, Kuppuswamy M, Doronin K, Krajcsi P, Lipinski K, Wrighton CJ, and Wold WS

Subjects

Adenoviridae genetics, Adenovirus E3 Proteins biosynthesis, Adenovirus E3 Proteins genetics, Adenovirus E4 Proteins biosynthesis, Adenovirus E4 Proteins genetics, Animals, Cell Division physiology, Cell Line, Tumor, Cytopathogenic Effect, Viral, Endothelium, Vascular metabolism, Endothelium, Vascular virology, Genetic Vectors genetics, Humans, Mice, Neoplasms genetics, Plasmids genetics, Proto-Oncogene Proteins physiology, Signal Transduction, Virus Replication, Wnt Proteins, Xenograft Model Antitumor Assays, Adenoviridae physiology, Adenovirus E3 Proteins physiology, Neoplasms therapy, Neoplasms virology, Proto-Oncogene Proteins genetics

Abstract

We have constructed a novel oncolytic adenovirus (Ad) vector named VRX-009 that combines enhanced cell spread with tumor-specific replication. Enhanced spread, which could significantly increase antitumor efficacy, is mediated by overexpression of the Ad cytolytic protein named ADP (also known as E3-11.6K). Replication of VRX-009 is restricted to cells with a deregulated wnt signal transduction pathway by replacement of the wild-type Ad E4 promoter with a synthetic promoter consisting of five consensus binding sites for the T-cell factor transcription factor. Tumor-selective replication is indicated by several lines of evidence. VRX-009 expresses E4ORF3, a representative Ad E4 protein, only in colon cancer cell lines. Furthermore, VRX-009 replicates preferentially in colon cancer cell lines as evidenced by virus productivity 2 orders of magnitude higher in SW480 colon cancer cells than in A549 lung cancer cells. Replication in primary human bronchial epithelial cells and human umbilical vein endothelial cells was also significantly lower than in SW480 cells. When tested in human tumor xenografts in nude mice, VRX-009 effectively suppressed the growth of SW480 colon tumors but not of A549 lung tumors. VRX-009 may provide greater level of antitumor efficacy than standard oncolytic Ad vectors in tumors in which a defect in wnt signaling increases the level of nuclear beta-catenin.

Published

2004

10. Early adenoviral gene expression mediates immunosuppression by transduced dendritic cell (DC): implications for immunotherapy using genetically modified DC.

Author

Tuettenberg A, Jonuleit H, Tüting T, Brück J, Biermann V, Kochanek S, Knop J, and Enk AH

Subjects

Adenovirus E1 Proteins biosynthesis, Adenovirus E1 Proteins genetics, Adenovirus E3 Proteins biosynthesis, Adenovirus E3 Proteins genetics, Adenoviruses, Human immunology, CD4-Positive T-Lymphocytes immunology, CD4-Positive T-Lymphocytes pathology, CD4-Positive T-Lymphocytes virology, CD8-Positive T-Lymphocytes immunology, CD8-Positive T-Lymphocytes pathology, CD8-Positive T-Lymphocytes virology, Cell Cycle genetics, Cell Cycle immunology, Cell Differentiation genetics, Cell Differentiation immunology, Cells, Cultured, Cytokines biosynthesis, Dendritic Cells cytology, Dendritic Cells virology, Genetic Vectors chemical synthesis, Growth Inhibitors genetics, Growth Inhibitors immunology, Humans, Immunophenotyping, Intestinal Mucosa immunology, Intestinal Mucosa pathology, Intestinal Mucosa virology, Lymphocyte Activation genetics, Lymphocyte Activation immunology, Recombination, Genetic, Adenoviruses, Human genetics, Dendritic Cells immunology, Dendritic Cells metabolism, Gene Expression Regulation, Viral immunology, Genetic Vectors immunology, Immunosuppression Therapy methods, Transduction, Genetic methods

Abstract

Long-lasting, high-level gene expression in the absence of a toxic or inflammatory response to viral Ags is necessary for the successful application of genetically modified dendritic cell (DC). We previously demonstrated that efficient transduction of mature DC using DeltaE1DeltaE3 adenoviruses suppressed their stimulatory capacity for T cells. The current study was designed to investigate in more detail the suppressive effect of Ad-DC. We demonstrate that immunosuppression is not mediated by alterations in the T cell phenotype or cytokine profiles released by stimulated T cells. Also DC phenotypes are not affected. However, we demonstrate a cell cycle arrest of the T cell population stimulated by adenovirally transduced DC. Surprisingly, only freshly transduced DC are perturbed in their stimulatory capacity. Experiments using cycloheximide to block early intracellular viral gene expression showed that viral genes expressed in DC are responsible for this transient immunosuppression. In agreement with these findings, high-capacity (gutless) Ad-vectors that differ in viral gene expression from conventional DeltaE1DeltaE3 adenovirus are suitable for an efficient transduction of human DC. DC transduced with gutless Ad-vectors showed a high allostimulatory capacity for CD4(+) and CD8(+) T cells. Thus, the immunosuppressive effect of DeltaE1DeltaE3 Ad-transduced mature DC seems to be the result of early viral gene expression in DC that can be prevented using gutless Ad-vectors for transduction. These results have important implications for the use of genetically modified DC for therapeutic application.

Published

2004

11. Immune evasion by adenovirus E3 proteins: exploitation of intracellular trafficking pathways.

Author

Windheim M, Hilgendorf A, and Burgert HG

Subjects

Adenoviridae Infections virology, Adenovirus E3 Proteins biosynthesis, Adenovirus E3 Proteins metabolism, Adenoviruses, Human chemistry, Adenoviruses, Human physiology, Animals, Biological Transport, Humans, Immunity, Innate, Adenoviridae Infections immunology, Adenovirus E3 Proteins immunology, Adenoviruses, Human immunology

Abstract

Adenoviruses (Ads) are nonenveloped viruses which replicate and assemble in the nucleus. Therefore, viral membrane proteins are not directly required for their multiplication. Yet, all human Ads encode integral membrane proteins in the early transcription unit 3 (E3). Previous studies on subgenus C Ads demonstrated that most E3 proteins exhibit immunomodulatory functions. In this review we focus on the E3 membrane proteins, which appear to be primarily devoted to remove critical recognition structures for the host immune system from the cell surface. The molecular mechanism for removal depends on the E3 protein involved: E3/19K prevents expression of newly synthesized MHC molecules by inhibition of ER export, whereas E3/10.4-14.5K down-regulate apoptosis receptors by rerouting them into lysosomes. The viral proteins mediating these processes contain typical transport motifs, such as KKXX, YXXphi, or LL. E3/49K, another recently discovered E3 protein, may require such motifs to reach a processing compartment essential for its presumed immunomodulatory activity. Thus, E3 membrane proteins exploit the intracellular trafficking machinery for immune evasion. Conspicuously, many E3 membrane proteins from Ads other than subgenus C also contain putative transport motifs. Close inspection of surrounding amino acids suggests that many of these are likely to be functional. Therefore, Ads might harbor more E3 proteins that exploit intracellular trafficking pathways as a means to manipulate immunologically important key molecules. Differential expression of such functions by Ads of different subgenera may contribute to their differential pathogenesis. Thus, an unexpected link emerges between viral manipulation of intracellular transport pathways and immune evasion.

Published

2004

12. [Recombinant replication-defective adenovirus based rabies vaccine].

Author

Li WH, Zhang Y, Wang SH, Liu L, and Yang F

Subjects

Adenovirus E3 Proteins biosynthesis, Adenovirus E3 Proteins genetics, Adenovirus E3 Proteins immunology, Animals, Antibodies, Viral biosynthesis, Antibodies, Viral genetics, Antibodies, Viral immunology, Base Sequence, Genetic Vectors, Glycoproteins genetics, Glycoproteins immunology, Humans, Mice, Molecular Sequence Data, Nucleoproteins biosynthesis, Nucleoproteins genetics, Nucleoproteins immunology, Rabies immunology, Rabies Vaccines genetics, Rabies Vaccines immunology, Rabies virus genetics, Rabies virus immunology, Vaccines, Synthetic genetics, Vaccines, Synthetic immunology, Viral Envelope Proteins genetics, Viral Envelope Proteins immunology, Virus Replication, Adenoviruses, Human genetics, Antigens, Viral, Glycoproteins biosynthesis, Rabies prevention & control, Rabies Vaccines biosynthesis, Vaccines, Synthetic biosynthesis, Viral Envelope Proteins biosynthesis

Abstract

Objective: To construct and characterize recombinant adenoviruses containing glycoprotein (GP) gene from rabies virus CVS-N2C strain., Methods: To obtain the recombinant adenovirus by pAdEasy system, identify recombinant virus with cDNA sequencing, Northern blot, Dot blot, Western blot and challenge-protection experiment of mice., Results: Recombinant adenovirus showed typical adenovirus morphological characteristics; the viral genome was stable; GP specific mRNA and presence of glycoprotein were determined in rAdGPcvs and rAdGPcvs' infected cells. The glycoprotein produced by recombinant adenovirus had a molecular mass of 66,000, which was similar to that of natural glycoprotein. In the group of rAdGPcvs immunized mice, 87.5%-100% of mice survived from a 35.8LD50/38.0LD50 lethal rabies intracerebral challenge. Finally 73.3%-83.3% of the mice that had received eAdGPcvs survived, and all the Ad5 immunized mice succumbed to rabies., Conclusion: Recombinant adenovirus rAdGPcvs and rAdGPcvs' hold great potential to be developed as recombinant rabies vaccines, and at the same time, it is actually the first study that on high neuropathogenicity rabies CVS-N2C glycoprotein based adenoviral recombinants.

Published

2003

13. Construction and characterization of E1-minus replication-defective adenovirus vectors that express E3 proteins from the E1 region.

Author

Toth K, Kuppuswamy M, Doronin K, Doronina O, Lichtenstein D, Tollefson A, and Wold W

Subjects

Adenoviridae genetics, Adenovirus E3 Proteins analysis, Adenovirus E3 Proteins genetics, Apoptosis, Endosomes metabolism, ErbB Receptors metabolism, HeLa Cells, Humans, Lysosomes metabolism, fas Receptor metabolism, Adenoviridae metabolism, Adenovirus E1 Proteins genetics, Adenovirus E3 Proteins biosynthesis, Defective Viruses metabolism, Genetic Vectors, Virus Replication

Abstract

Previous research has indicated that the adenovirus protein complex named RID, derived from the E3 transcription unit, functions to remove the receptors named Fas/Apo1/CD95 (Fas) and epidermal growth factor receptor (EGFR) from the surface of cells. (The RID complex is composed of the RIDalpha and RIDbeta polypeptides, previously named 10.4K and 14.5K, respectively.) In response to RID, Fas and EGFR appear to be internalized into endosomes and degraded in lysosomes. Fas is a death receptor in the tumor necrosis factor (TNF) receptor superfamily. RID inhibits apoptosis via the Fas pathway, presumably because RID gets rid of Fas. Earlier work further showed that another adenovirus E3-coded protein, E3-14.7K, inhibits apoptosis induced by TNF. Most of the above studies have been conducted using viable virus mutants that lack one or more of the genes for RID, E3-14.7K, or E1B-19K (this protein, coded by the E1B transcription unit, also inhibits apoptosis via the TNF and Fas pathways). Some studies have also been conducted with the genes for RID or E3-14.7K transiently or stably transfected into cells. We now report a new approach to studying the E3 genes. We have constructed four E1-minus replication-defective vectors that have all the E3 genes deleted from their natural position and then reinserted, in different permutations, into the deleted E1 region under control of the cytomegalovirus immediate early promoter. Vector Ad/RID only has the genes for RIDalpha and RIDbeta. Vector Ad/14.7K only has the gene for E3-14.7K. Vector Ad/RID/14.7K only has the genes for RIDalpha, RIDbeta, and E3-14.7K. Vector Ad/E3 has all E3 genes, but there are two missense mutations in the gene for Adenovirus Death Protein. These vectors expressed RID and/or E3-14.7K, as expected. The RID-expressing vectors forced the internalization and degradation of Fas and EGFR, and they inhibited apoptosis induced through the Fas pathway. These vectors should be useful reagents to study the E3 proteins.

Published

2002

14. Characterization of E3/49K, a novel, highly glycosylated E3 protein of the epidemic keratoconjunctivitis-causing adenovirus type 19a.

Author

Windheim M and Burgert HG

Subjects

Adenovirus E3 Proteins biosynthesis, Adenoviruses, Human physiology, Amino Acid Sequence, Cells, Cultured, Cloning, Molecular, Disulfides metabolism, Endosomes metabolism, Endosomes virology, Fibroblasts, Glycosylation, Humans, Mannose analysis, Molecular Sequence Data, Molecular Weight, Polysaccharides analysis, Protein Processing, Post-Translational, Tumor Cells, Cultured, trans-Golgi Network metabolism, trans-Golgi Network virology, Adenovirus E3 Proteins chemistry, Adenovirus E3 Proteins metabolism, Adenoviruses, Human chemistry, Conjunctivitis, Viral virology

Abstract

The early transcription unit 3 (E3) of human adenoviruses (Ads) encodes proteins with various immunomodulatory functions. Ads from different subgenera differ considerably in their E3 coding capacity, suggesting that distinct sets of immunomodulatory E3 proteins may influence the disease pattern associated with different Ad subgenera. Interestingly, the E3 region of Ads classified in subgenus D, which are often isolated from AIDS patients and have the propensity to cause eye infections, contains a unique gene, named E3/49K, that may encode a protein with a calculated molecular weight of 48,984 that might be implicated in diseases caused by this subgenus. The 49K sequence predicts a highly glycosylated type I transmembrane protein with a short cytoplasmic tail containing two motifs, YXXPhi and LL, potentially involved in targeting the protein to endosomal or lysosomal compartments. Remarkably, the 49K protein is predicted to contain an unusual immunoglobulin-like fold. Here we have characterized the E3/49K protein of Ad type 19a, an Ad of subgenus D which causes epidemic keratoconjunctivitis. E3/49K was synthesized as an 80- to 100-kDa protein, which is unusually large for an E3 protein. In contrast to another early protein, E3/19K, the expression of E3/49K started early but continued throughout the infection cycle. Analysis of the 49K glycosylation revealed that the majority of 49K molecules contained only 12 of the predicted 14 N-glycans. Furthermore, we provide evidence that 49K is O-glycosylated. At steady state, E3/49K was localized in the Golgi-trans-Golgi network and in early endosomes. Interestingly, the 49K protein has a rather short half-life and seems to be proteolytically cleaved. A processing pattern similar to that in the early stages of infection is seen in transfected cells, constitutively expressing 49K in the absence of other Ad proteins. Together, our data provide the first biochemical and cell biological characterization of an unique E3 protein of subgenus D Ads.

Published

2002

15. Inclusion of the E3 region in an adenoviral vector decreases inflammation and neointima formation after arterial gene transfer.

Author

Wen S, Driscoll RM, Schneider DB, and Dichek DA

Subjects

Adenoviridae immunology, Adenoviridae metabolism, Adenovirus E3 Proteins biosynthesis, Animals, Antibodies, Viral biosynthesis, Arterial Occlusive Diseases metabolism, Arterial Occlusive Diseases pathology, Arteries metabolism, Arteries pathology, Arteritis immunology, Arteritis pathology, CHO Cells, Cell Adhesion Molecules metabolism, Cell Line, Cricetinae, DNA, Viral genetics, Genetic Vectors, Luciferases biosynthesis, Luciferases genetics, RNA, Viral biosynthesis, Rabbits, Transduction, Genetic, Adenoviridae genetics, Adenovirus E3 Proteins genetics, Arterial Occlusive Diseases therapy, Arteritis therapy, Genetic Therapy methods

Abstract

Adenoviral vectors are promising agents for vascular gene transfer. Their use, however, is limited by inflammatory host responses, neointima formation, and brevity of transgene expression. Inclusion of the immunomodulatory adenoviral E3 genes in a vector might prevent inflammation and neointima formation and prolong transgene expression. We compared 2 adenoviral vectors in a model of in vivo gene transfer to rabbit arteries. Both vectors expressed a luciferase reporter gene. One vector (AdE3Luc) contained the adenovirus early 3 (E3) region and the other (AdRSVLuc) lacked E3. Expression of E3 genes by AdE3Luc was confirmed in vitro and in vivo. Arteries transduced with AdE3Luc had substantially and significantly less inflammation (fewer T cells and lower levels of vascular cell adhesion molecule-1 and intercellular adhesion molecule 1 expression) and decreased neointima formation 14 days after gene transfer. Luciferase expression from the 2 vectors was equivalent, however, at both 3 and 14 days after gene transfer. Expression of E3 had no systemic immunosuppressive effects, as measured by peripheral blood counts and by assays for serum antibodies to adenovirus. We conclude that expression of E3 significantly decreases adenovirus-induced arterial wall inflammation and neointima formation. Because inflammation and neointima formation are major barriers to the clinical application of adenoviral vectors, use of E3-containing vectors improves the promise of adenovirus-mediated arterial gene transfer.

Published

2001

16. Expression of gp19K increases the persistence of transgene expression from an adenovirus vector in the mouse lung and liver.

Author

Bruder JT, Jie T, McVey DL, and Kovesdi I

Subjects

Adenoviridae genetics, Animals, Cell Line, Female, Genes, MHC Class I, Genetic Therapy, Glucuronidase biosynthesis, Histocompatibility Antigens Class I metabolism, Humans, Kidney, Liver metabolism, Lung metabolism, Lung Neoplasms, Mice, Mice, Inbred BALB C, Recombinant Fusion Proteins biosynthesis, Tumor Cells, Cultured, Adenoviridae physiology, Adenovirus E3 Proteins biosynthesis, Genetic Vectors, Liver virology, Lung virology, Mice, Transgenic

Abstract

Activation of the cellular immune system and subsequent lysis of vector-transduced cells by adenovirus- or transgene-specific cytotoxic T lymphocytes have been shown to limit transgene expression in animal models. The adenovirus gp19K gene product associates with major histocompatibility complex class I proteins and prevents their maturation by sequestering them in the endoplasmic reticulum. gp19K has been shown to block the ability of adenovirus-specific cytotoxic T lymphocytes to recognize virus-infected cells in vitro. To determine if gp19K expression in an adenovirus vector would increase transgene persistence, a vector that replaces the E1 region of adenovirus with an expression cassette encoding both gp19K and beta-glucuronidase was constructed. This vector produced high levels of functional gp19K in infected cells. RNase protection analysis revealed efficient expression of the gp19K gene in the mouse lung. Enhanced persistence and increased beta-glucuronidase activity were observed in the lung and liver following delivery of the gp19K-expressing adenovirus vector in B10.HTG mice but not in BALB/c mice. Since gp19K binds to both class I alleles on B10.HTG mice but only one allele on BALB/c mice, these results suggest that the major histocompatibility complex class I haplotype of mice is important in determining the effectiveness of gp19K in vivo. Since gp19K has previously been shown to interact with every human major histocompatibility complex class I allele tested, the inclusion of gp19K in gene therapy vectors may increase vector persistence in human gene therapy trials.

Published

1997

17. Insertion of the adenoviral E3 region into a recombinant viral vector prevents antiviral humoral and cellular immune responses and permits long-term gene expression.

Author

Ilan Y, Droguett G, Chowdhury NR, Li Y, Sengupta K, Thummala NR, Davidson A, Chowdhury JR, and Horwitz MS

Subjects

Adenovirus E3 Proteins biosynthesis, Animals, Antibody Formation, Bile metabolism, Bilirubin analogs & derivatives, Bilirubin blood, Bilirubin metabolism, Genetic Therapy methods, Genetic Vectors, Glucuronosyltransferase biosynthesis, Glucuronosyltransferase genetics, Humans, Hyperbilirubinemia physiopathology, Immunity, Cellular, Inflammation, Liver enzymology, Liver pathology, Rats, Rats, Inbred Strains, Time Factors, Adenoviridae, Adenovirus E3 Proteins genetics, Adenovirus E3 Proteins immunology, Hyperbilirubinemia immunology, Hyperbilirubinemia therapy

Abstract

Recombinant adenoviruses (Ads) are highly efficient at transferring foreign genes to the liver in vivo; however, the duration of gene expression is limited by the host antiviral immune response, which prevents expression upon readministration of the virus. To test whether overexpression of the immunomodulatory products of the early Ad genome region 3 (E3) could prevent the antiviral immune response and prolong expression of foreign genes delivered by Ad vectors, we injected a recombinant Ad (Ad-E3-hBUGT), containing both E3 and the human bilirubin-uridine-diphosphoglucuronate-glucuronosyltransferase (BUGT) genes, into BUGT-deficient hyperbilirubinemic Gunn rats. Control Gunn rats received Ad-hBUGT, which expresses human BUGT alone. An initial injection of either virus resulted in hepatic expression of human BUGT as evidenced by excretion of bilirubin glucuronides in bile and a reduction of mean serum bilirubin levels from 7.0 mg/dl to 1.9-2.7 mg/dl within 7 days. In Ad-E3-hBUGT-injected rats, serum bilirubin levels increased to 4.5 mg/dl by 84 days after infection, but a second administration of the virus on that day resulted in a hypobilirubinemic response similar to that seen with the first injection. In contrast, rats receiving Ad-hBUGT had serum bilirubin levels of 7 mg/dl on day 84 after infection, but showed no reduction of serum bilirubin by reinjection of the virus on that day. In the rats injected with Ad-E3-hBUGT, but not in the ones injected with Ad-hBUGT, there was a marked inhibition of the antiviral antibody and Ad-specific cytotoxic T lymphocyte responses. This is the first demonstration that insertion of E3 genes in recombinant Ads facilitates readministration of a functional vector for long-term correction of an inherited metabolic disorder.

Published

1997

18. Human adenovirus-specific CD8+ T-cell responses are not inhibited by E3-19K in the presence of gamma interferon.

Author

Flomenberg P, Piaskowski V, Truitt RL, and Casper JT

Subjects

Adenovirus E3 Proteins biosynthesis, Adenoviruses, Human genetics, Adult, Animals, Antibodies, Monoclonal, Callithrix, Cell Line, Cytotoxicity, Immunologic, Endoplasmic Reticulum drug effects, Endoplasmic Reticulum immunology, Histocompatibility Antigens Class I biosynthesis, Histocompatibility Antigens Class I immunology, Humans, Mutagenesis, Recombinant Proteins biosynthesis, Recombinant Proteins immunology, Sequence Deletion, T-Lymphocytes, Cytotoxic drug effects, Tumor Cells, Cultured, Virion immunology, Adenovirus E3 Proteins immunology, Adenoviruses, Human immunology, Interferon-gamma pharmacology, Skin immunology, T-Lymphocytes, Cytotoxic immunology

Abstract

Adenovirus has considerable potential as a gene therapy vector, but recent animal data suggest that transduced cells are destroyed by adenovirus-specific cytotoxic T-lymphocyte (CTL) responses. Therefore, it will be important to develop strategies to evade adenovirus-specific CTL responses in humans. As a first step, an assay was developed to detect and characterize human CTLs directed against adenovirus. Adenovirus-specific CTL responses were demonstrated to be present in four of five healthy adults by in vitro stimulation of peripheral blood mononuclear cells with autologous fibroblasts infected with the adenovirus type 2 (Ad2) E3 deletion mutant Ad2+ND1. Killing by adenovirus-specific CTLs was major histocompatibility complex class I restricted and was documented to be mediated by CD8+ T cells. Wild-type-Ad2-infected cells were poor CTL targets compared with cells infected with the E3 deletion mutant because of the expression of E3-19K, an early viral glycoprotein which prevents transport of major histocompatibility complex class I antigens out of the endoplasmic reticulum to the cell surface. However, preincubation of targets with gamma interferon resulted in enhanced killing of wild-type-Ad2-infected cells, to levels comparable to those obtained with Ad2+ ND1-infected cells. Radioimmunoprecipitation analysis revealed that gamma interferon not only increased the synthesis of class I antigens but also allowed excess molecules to escape from the endoplasmic reticulum. It is concluded that E3-19K expression in adenovirus-infected cells inhibits human CTL recognition in vitro but that gamma interferon may help overcome the E3-19K effect during acute infection in vivo.

Published

1996

19. Analysis of early region 3 mutants of mouse adenovirus type 1.

Author

Beard CW and Spindler KR

Subjects

Adenoviridae ultrastructure, Animals, Base Sequence, Cell Line, DNA Primers, Mice, Microscopy, Electron, Molecular Sequence Data, Mutagenesis, Site-Directed, Polymerase Chain Reaction, RNA, Messenger biosynthesis, RNA, Viral biosynthesis, Recombination, Genetic, Restriction Mapping, Sequence Deletion, Transcription, Genetic, Adenoviridae genetics, Adenoviridae metabolism, Adenovirus E3 Proteins biosynthesis

Abstract

Early region 3 (E3) of mouse adenovirus type 1 has the potential to produce three proteins which have identical amino termini but unique carboxy-terminal sequences. Three recombinant deletion viruses were constructed so that each could produce only one of the three E3 proteins. A fourth mutant that should produce no E3 proteins was also constructed. These recombinants were able to grow in mouse 3T6 cells and produced wild-type levels of viral mRNAs and proteins except for those specifically deleted by the mutations. Early mRNA production from the mutant viruses was analyzed by reverse transcriptase PCR and confirmed that each deletion mutant would be able to produce only one of the three E3 proteins. Late mRNA production was analyzed by Northern (RNA) blotting and found to be similar in wild-type and mutant viruses. Capsid morphology was unaltered in the mutant viruses as seen by electron microscopy. Immunoprecipitation of E3 proteins from infections of mouse 3T6 cells using an antiserum specific for all three E3 proteins was used to examine the effect of the introduced mutations on protein expression. Two mutants produced only one class of E3 protein as predicted from their specific mutations and mRNA expression profiles. One mutant virus failed to produce any detectable E3 proteins. The predicted E3-null mutant was found to be leaky and could produce low levels of E3 proteins. Outbred Swiss mice were infected with the E3 mutant viruses to determine if the E3 proteins have an effect on the pathogenicity of the virus in mice. All of the mutants showed decreased pathogenicity as determined by increased 50% lethal doses, indicating that the proteins of the E3 region are important determinants of the pathogenesis of mouse adenovirus in its natural host.

Published

1996

20. Early region 3 of adenovirus type 19 (subgroup D) encodes an HLA-binding protein distinct from that of subgroups B and C.

Author

Deryckere F and Burgert HG

Subjects

Adenovirus E3 Proteins analysis, Adenoviruses, Human classification, Amino Acid Sequence, Base Sequence, Cell Line, Cell Membrane immunology, Cloning, Molecular, Conserved Sequence, DNA Primers, HLA Antigens, HeLa Cells, Histocompatibility Antigens Class I immunology, Humans, Keratoconjunctivitis virology, Molecular Sequence Data, Polymerase Chain Reaction, Restriction Mapping, Sequence Homology, Amino Acid, Transfection, Adenovirus E3 Proteins biosynthesis, Adenoviruses, Human genetics, Adenoviruses, Human immunology, Open Reading Frames

Abstract

Early region 3 (E3) of human adenoviruses (Ads) codes for proteins that appear to control viral interactions with the host. For example, the most abundant E3 protein, E3/19K, inhibits the transport of newly synthesized class I major histocompatibility molecules to the cell surface, thereby interfering with antigen presentation. So far, the E3 regions of Ad subgroups A, B, C, and F have been characterized. We have cloned the E3A region of Ad type 19a (Ad19a), which belongs to the largest subgroup, D, and causes epidemic keratoconjunctivitis in humans. The sequence reveals five open reading frames (ORFs) with the potential to encode the Ad19 equivalent of pVIII, as well as proteins 12.2K, 16.2K, and 18.6K. The last ORF predicts a novel 49K protein which has no counterpart in other subgroups. Both the sequence and the overall organization of the E3 region from Ad19a shows a closer relationship to group B than to group C Ads. The 18.6K ORF represents the Ad19 homolog of the Ad2 E3/19K protein. By using 293 cells stably transfected with the Adl9a E3A region, we showed by immunoprecipitation, pulse-chase experiments, and fluorescence-activated cell sorter analysis that the Ad19 E3/19K protein binds to and prevents the transport of major histocompatibility complex molecules to the cell surface. The similar but distinct functional activity of the Ad19 E3/19K protein, combined with the new sequence which differs from those of subgroup B and C proteins, allows a more precise definition of amino acids essential for HLA binding.

Published

1996

21. Potential salmon sperm origin of the E3 region insert of the adenovirus 5 dl309 mutant.

Author

Gingras MC, Arevalo P, and Aguilar-Cordova E

Subjects

Adenovirus E3 Proteins biosynthesis, Animals, Avian Sarcoma Viruses enzymology, Avian Sarcoma Viruses genetics, Base Sequence, DNA Primers, HeLa Cells, Humans, Male, Molecular Sequence Data, Plasmids, Polymerase Chain Reaction, Prolactin genetics, Proton-Translocating ATPases genetics, Repetitive Sequences, Nucleic Acid, Salmon, Sequence Homology, Nucleic Acid, Thymidine Kinase biosynthesis, Transfection, Adenovirus E3 Proteins genetics, Adenoviruses, Human, DNA metabolism, Genetic Vectors, Spermatozoa physiology

Abstract

The plasmid pJM17 is a commonly used adenoviral backbone derived from the dl309 mutant virus. It contains unknown sequences inserted in the E3 region during construction of the dl309 mutant. Complete description of the backbone sequence is required for interpretation of potential vector effects and for regulatory approval of a vector to be used in clinical trials. The anonymous E3 insert was sequenced and analyzed. The insert fragment is 646 base pairs (bp) long and is 100 bp shorter than the vector sequences it replaces. It interrupts the expression of the E3B 10.4K, 14.6K, and 14.7K genes, but not the E3A glycoprotein (gp) 19K gene. Sequence analysis and Southern blotting suggest that the insert might originate from salmon sperm DNA used as carrier during the construction of dl309. Transcription from the insert was not detected by Northern blot analysis of vector-transduced cells but was detected by reverse transcriptase polymerase chain reaction.

Published

1996

22. Tumor necrosis factor alpha increases expression of adenovirus E3 proteins.

Author

Deryckere F, Ebenau-Jehle C, Wold WS, and Burgert HG

Subjects

Animals, Humans, Up-Regulation immunology, Adenovirus E3 Proteins biosynthesis, Adenovirus E3 Proteins drug effects, Tumor Necrosis Factor-alpha physiology

Abstract

Human adenovirus can cause persistent infections in man. Implicated in this phenomenon is the early transcription unit 3 (E3) of the virus which encodes proteins that are primarily devoted to counteract the lytic attack by the host immune system: Several E3 proteins (14.7K, 10.4K and 14.5K) protect infected cells from the lytic activity of tumor necrosis factor alpha (TNF) while the most abundant E3 protein, E3/19K, inhibits lysis by cytotoxic T cells. E3/19K interacts with class I histocompatibility (MHC) antigens in the rough endoplasmic reticulum, thereby preventing transport of MHC molecules to the cell surface and, consequently, MHC-restricted T cell recognition. In addition, the 10.4K and 14.5K proteins downregulate cell surface expression of the epidermal growth factor receptor. Interestingly, adenovirus-mediated pneumonia in mice is accompanied by induction of TNF, a cytokine known to enhance MHC expression. We previously showed that TNF is unable to restore MHC class I expression in E3/19K transfected cells but rather leads to a further reduction of MHC antigens. This effect correlated with an increased production of E3/19K mRNA and protein. We now find in addition an upregulation of other E3 proteins in transfected as well as in infected cells. This coordinated upregulation of E3 proteins indicates that TNF stimulates the E3 promoter, probably by activating the transcription factor NF-kappa B. Thus, a novel interaction between the immune system and adenovirus is described in which the virus takes advantage of an immune mediator to promote expression of several immunosubversive proteins supporting its escape from immunosurveillance.

Published

1995

23. Characterization of an 11K protein produced by early region 3 of mouse adenovirus type 1.

Author

Beard CW and Spindler KR

Subjects

Adenoviridae chemistry, Adenoviridae metabolism, Adenovirus E3 Proteins analysis, Adenovirus E3 Proteins biosynthesis, Amino Acid Sequence, Animals, Antibodies, Viral, Base Sequence, Cell Line, Endoplasmic Reticulum chemistry, Glycosylation, Hexosaminidases metabolism, Membrane Proteins analysis, Membrane Proteins biosynthesis, Mice, Molecular Sequence Data, Molecular Weight, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins immunology, Adenovirus E3 Proteins chemistry, Membrane Proteins chemistry

Abstract

Early region 3 (E3) of mouse adenovirus type 1 produces three mRNAs that can encode three proteins with unique carboxy-terminal exons. A bacterial fusion protein encoding the unique terminus of one the three predicted proteins was used to generate antiserum in rabbits. This antiserum detected a 14K protein on a Western blot of infected cell lysates. Immunoprecipitation and endoglycosidase H digestion revealed that the 14K protein was a glycoprotein with a core molecular weight of 11K, and we are designating this protein E3 gp 11K. Through in vitro translation experiments we determined that the previously predicted signal sequence of gp11K was cleaved when the protein was expressed during an infection. Biochemical and immunofluorescence microscopy data indicated that E3 gp11K was localized to the endoplasmic reticulum of infected cells. Biochemical experiments further indicated that gp11K is a peripheral membrane protein.

Published

1995

24. Down-regulation of human adenovirus E1a by E3 gene products: evidence for translational control of E1a by E3 14.5K and/or E3 10.4K products.

Author

Zhang X, Bellett AJ, Hla RT, Voss T, Müllbacher A, and Braithwaite AW

Subjects

Adenovirus E1A Proteins genetics, Adenovirus E3 Proteins genetics, Animals, Cells, Cultured, Gene Expression Regulation, Viral, Half-Life, Humans, Mice, RNA, Messenger metabolism, Species Specificity, Adenovirus E1A Proteins biosynthesis, Adenovirus E3 Proteins biosynthesis, Adenoviruses, Human genetics, Down-Regulation, Protein Biosynthesis

Abstract

The mechanism for down-regulation of E1a expression by products encoded in the E3 transcription unit of human adenovirus types 2 and 5, that occurs in infected L929 cells, has been investigated further. We show that the phenomenon occurs in different mouse cells and also in some human cells suggesting that the observations have relevance to natural human infections. We also provide evidence that probably all viral proteins are down-regulated by E3 products, although to different extents, but that host proteins are unaffected. Whereas E1a protein levels and synthesis are reduced in the presence of E3 products, E1a protein half-life and polysomal E1a RNA levels and size distribution are not. These data suggest that E3 products down-regulate E1a protein levels by interfering with the translation of E1a-specific mRNA. Studies were additionally carried out with mutant adenoviruses containing different defects in the E3 transcription unit. Based on these studies it seems likely that the E3 14.5K and 10.4K proteins are crucially involved in E1a down-regulation. Our data are discussed in terms of strategies for immune evasion by group C human adenoviruses.

Published

1994

25. The adenovirus E3 14.7-kilodalton protein which inhibits cytolysis by tumor necrosis factor increases the virulence of vaccinia virus in a murine pneumonia model.

Author

Tufariello J, Cho S, and Horwitz MS

Subjects

Adenovirus E3 Proteins antagonists & inhibitors, Adenovirus E3 Proteins biosynthesis, Administration, Intranasal, Animals, Disease Models, Animal, Female, Humans, Lung microbiology, Lung pathology, Mice, Mice, Inbred BALB C, Recombinant Proteins biosynthesis, Recombinant Proteins pharmacology, Survival Analysis, Tumor Cells, Cultured, Tumor Necrosis Factor-alpha antagonists & inhibitors, Tumor Necrosis Factor-alpha biosynthesis, Vaccinia microbiology, Virulence drug effects, Virus Replication drug effects, Adenovirus E3 Proteins pharmacology, Pneumonia, Viral microbiology, Tumor Necrosis Factor-alpha pharmacology, Vaccinia virus drug effects, Vaccinia virus pathogenicity

Abstract

The 14.7-kilodalton protein (14.7K protein) encoded by the adenovirus (Ad) E3 region inhibits tumor necrosis factor alpha (TNF-alpha)-mediated lysis of cells in tissue culture experiments, but the relevance of this effect in vivo is incompletely understood. To examine the effect of the ability of the Ad 14.7K protein to block TNF lysis upon viral pathogenesis in a murine model, we cloned the 14.7K protein-encoding gene into vaccinia virus (VV), permitting its study in isolation from other Ad E3 immunomodulatory proteins. The gene for murine TNF-alpha was inserted into the same VV containing the 14.7K gene to ensure that each cell infected with the VV recombinant would express both the agonist (TNF) and its antagonist (14.7K). VV was utilized as the vector because it accommodates large and multiple inserts of foreign DNA with faithful, high-level expression of the protein products. In addition, infection of mice with VV induces disease with quantifiable morbidity, mortality, and virus replication. The results of intranasal infections of BALB/c mice with these VV recombinants indicate that the Ad 14.7K protein increases the virulence of VV carrying the TNF-alpha gene by reversing the attenuating effect of TNF-alpha on VV pathogenicity. This was demonstrated by increased mortality, pulmonary pathology, and viral titers in lung tissue following infection with VV coexpressing the 14.7K protein and TNF-alpha, compared with the control virus expressing TNF-alpha alone. These results suggest that the 14.7K protein, which is nonessential for Ad replication in tissue culture, is an immunoregulatory protein which functions in vivo to help counteract the antiviral effects of TNF-alpha.

Published

1994

26. Endogenous expression of E1A in human cells enhances the effect of adenovirus E3 on class I major histocompatibility complex antigen expression.

Author

Routes JM, Metz BA, and Cook JL

Subjects

Adenovirus E1A Proteins biosynthesis, Adenovirus E3 Proteins biosynthesis, Adenoviruses, Human growth & development, Cell Line, Transformed, Cytotoxicity, Immunologic, Down-Regulation, Humans, Adenovirus E1A Proteins immunology, Adenovirus E3 Proteins immunology, Adenoviruses, Human immunology, Genes, MHC Class I immunology

Abstract

Group C human adenovirus (Ad) serotypes (e.g., Ad type 2 [Ad2] and Ad5) cause persistent infections in humans. One explanation for Ad persistence is an ineffective cytotoxic T-lymphocyte response due to diminished cell surface expression of class I major histocompatibility antigen (MHC Ag) on Ad-infected cells, an effect mediated by the Ad E3 19-kDa glycoprotein (E3 effect). However, we previously reported that, except for the Ad5 E1-transformed human cell line 293, a variety of human lymphoid, epithelial, and fibroblastic cells are resistant to the E3 effect during Ad5 infection (J. M. Routes and J. L. Cook, J. Immunol. 144:2763-2770, 1990). The present study tested the hypothesis that endogenous expression of E1A proteins in 293 cells sensitizes cells to this E3 effect, resulting in an enhanced downregulation of surface class I MHC Ag expression following Ad5 infection. Human epithelial and fibroblastic cells expressing E1A gene products for at least 72 h exhibited an enhanced E3 effect following Ad5 infection that was independent of baseline levels of surface class I MHC Ag expression and of E1A induction of E3 19-kDa glycoprotein expression. There was a direct correlation between the level of endogenous E1A expressed and the magnitude of the E3 effect. We postulate that the in vivo existence of cells stably expressing either E1A proteins or E1A-like activities in the microenvironment of Ad5 infection provides a reservoir of Ad-infected cells that is relatively protected from the virus-specific cytotoxic T-lymphocyte response, thereby favoring Ad persistence in humans.

Published

1993