Your search keyword '"William S. M. Wold"' showing total 208 results

201. Adenovirus type 2 coded single-stranded DNA binding protein: in vivo phosphorylation and modification

Author

Zvee Gilead, K Sugawara, Maurice Green, Yun-Hua Jeng, and William S. M. Wold

Subjects

Immunology, DNA, Single-Stranded, Biology, Microbiology, Cell Line, Phosphates, chemistry.chemical_compound, Viral Proteins, Virology, Amino Acids, Polyacrylamide gel electrophoresis, Antiserum, chemistry.chemical_classification, Gel electrophoresis, Adenoviruses, Human, Phosphoproteins, Molecular biology, Amino acid, chemistry, Biochemistry, Insect Science, Phosphoserine, Phosphoprotein, Nucleic acid, Phosphothreonine, Electrophoresis, Polyacrylamide Gel, circulatory and respiratory physiology, Protein Binding, Research Article

Abstract

The adenovirus type 2-coded single-stranded DNA binding protein (DBP) was shown to be a phosphoprotein and to exist in at least two forms that differ in mobility by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. After a 30-min pulse with [35S]methionine or 32PO4, 35S- or 32P-labeled DBP had a nominal molecular weight of 74,000 whereas after a 30-min label followed by a 20-h chase, 35S- and 32P-labeled DBP had a nominal molecular weight of 77,000. Both large and small forms of 35S- and 32P-labeled DBP bound to single-stranded DNA-cellulose columns and were eluted by 0.4 to 0.6 M NaCl; both forms also were immunoprecipitated by antiserum against adenovirus type 1-simian virus 40-induced tumor cells (this antiserum contains antibodies against DBP) and by monospecific antiserum against 95 to 99% purified DBP. With highly purified 32P-DBP labeled 7 to 10 h postinfection, it was shown that the 32P radioactivity was firmly associated with protein material (i.e., not contaminating nucleic acids or phospholipids) and had properties expected of a phosphoester of an amino acid; paper electrophoresis of acid hydrolysates of this preparation identified phosphoserine but not phosphothreonine. Phosphoserine but not phosphothreonine was also identified in acid hydrolysates of another preparation of 32P-DBP labeled for 30 min, chased for 20 h, and then immunoprecipitated by adenovirus type 1-simian virus 40 antiserum.

Published

1977

202. Adenovirus mutants with splice-enhancing mutations in the E3 complex transcription unit are also defective in E3A RNA 3'-end formation

Author

Bheem M. Bhat and William S. M. Wold

Subjects

Genetics, Splice site mutation, Transcription, Genetic, RNA Splicing, Immunology, Intron, RNA, RNA-dependent RNA polymerase, Biology, Microbiology, Post-transcriptional modification, Adenoviridae, RNA silencing, Polypyrimidine tract, Virology, Insect Science, RNA splicing, Mutation, RNA, Viral, RNA, Messenger, Research Article

Abstract

Region E3 of adenovirus encodes about 10 overlapping mRNAs with different spliced structures. The mRNAs are 5' coterminal and form two major 3'-coterminal families termed E3A and E3B. As a group, the mRNAs have two 5' splice sites and four or five 3' splice sites. We previously described a novel class of virus mutants with deletions that enhance distant upstream and downstream 5' and 3' splice sites in region E3 (S. L. Deutscher, B. M. Bhat, M. H. Pursley, C. Cladaras, and W. S. M. Wold, Nucleic Acids Res. 13:5771-5788, 1985). We now report that two of these mutants, dl710 and dl712, are defective in RNA 3'-end formation at the E3A site. This result was surprising because the deletions in dl710 and dl712 are upstream of the putative signal for E3A RNA 3'-end formation. The explanation that we favor for this result is that the enhanced splicing activity in these mutants results in the splicing out of the E3A 3'-end site from the RNA precursor before the E3A 3' ends have a chance to form.

Published

1986

203. A short sequence in the COOH-terminus makes an adenovirus membrane glycoprotein a resident of the endoplasmic reticulum

Author

Per A. Peterson, Bheem M. Bhat, William S. M. Wold, and Svante Pääbo

Subjects

Vesicle-associated membrane protein 8, Viral protein, Mutant, Fluorescent Antibody Technique, Biology, medicine.disease_cause, Endoplasmic Reticulum, General Biochemistry, Genetics and Molecular Biology, Article, medicine, Humans, Antigens, Viral, Tumor, chemistry.chemical_classification, Endoplasmic reticulum, Adenoviruses, Human, Adenovirus Early Proteins, Oncogene Proteins, Viral, Flow Cytometry, Transmembrane protein, Amino acid, Biochemistry, chemistry, Cytoplasm, Mutation, Intracellular, HeLa Cells

Abstract

The E19 protein of adenoviruses is a transmembrane protein that abrogates the intracellular transport of class I antigens by forming complexes with them in the ER. We show here that the E19 protein is retained in the ER even in the absence of class I antigens. To define the region conferring residency in the ER, we examined two mutant forms of the viral protein. A 5 amino acid extension of the 15-membered cytoplasmic tail of the protein reduces its interaction with class I antigens but does not change its intracellular distribution. Shortening the tail to 7 amino acids also diminishes the affinity for class I antigens; however, this mutant E19 protein becomes transported to the cell surface. Thus, we concluded that a small stretch of amino acids exposed on the cytoplasmic side of the ER membrane is responsible for the retention of the E19 protein in the ER.

Published

1987

204. Identification of a novel sequence that governs both polyadenylation and alternative splicing in region E3 of adenovirus

Author

Helen A. Brady and William S. M. Wold

Subjects

Genetics, Messenger RNA, Polyadenylation, Base Sequence, Genes, Viral, Adenoviruses, Human, RNA Splicing, Alternative splicing, Mutant, Adenovirus Early Proteins, Nucleic acid sequence, DNA Restriction Enzymes, Oncogene Proteins, Viral, Biology, Genes, RNA splicing, Mutation, splice, RNA, Messenger, Chromosome Deletion, Antigens, Viral, Tumor, Poly A, Gene

Abstract

Region E3 encodes four major overlapping mRNAs with different splicing patterns. There are two poly(A) sites, an upstream site called E3A and a downstream site called E3B. We have analyzed virus mutants with deletions or insertions in E3 in order to identify sequences that function in the alternative processing of E3 pre-mRNAs, and to understand what determines which poly(A) sites and which splice sites are used. In previous studies we established that the 5' boundary of the E3A poly(A) signal is at an ATTAAA sequence. We now show, using viable virus mutants, that the 3' boundary of the E3A signal is located within 47-62 nucleotides (nt) downstream of the ATTAAA (17-32 nt downstream of the last microheterogenous poly(A) addition site). Our data further suggest that the spacing between the ATTAAA, the cleavage sites, and the essential downstream sequences may be important in E3A 3' end formation. Of particular interest, these mutants suggest a novel mechanism for the control of alternative pre-mRNA processing. Mutants which are almost completely defective in E3A 3' end formation display greatly increased use of a 3' splice site located 4 nt upstream of the ATTAAA. The mRNA that uses this 3' splice site is polyadenylated at the E3B poly(A) site. We suggest, for this particular case, that alternative pre-mRNA processing could be determined by a competition between trans-acting factors that function in E3A 3' end formation or in splicing. These factors could compete for overlapping sequences in pre-mRNA.

Published

1987

205. Cyclic AMP and citric acid accumulation by Aspergillus niger

Author

Isamu Suzuki and William S. M. Wold

Subjects

Sucrose, Adenosine, Time Factors, Biophysics, Guanosine, Biochemistry, Cyclic gmp, chemistry.chemical_compound, Theophylline, medicine, Cyclic AMP, Citrates, Molecular Biology, Cyclic GMP, biology, Chemistry, Adenine Nucleotides, fungi, Aspergillus niger, Cell Biology, biology.organism_classification, Guanine Nucleotides, Aspergillus, Cyclic AMP metabolism, Citric acid, medicine.drug

Abstract

Aspergillus niger accumulated citric acid in the medium under certain conditions. Cyclic AMP concentrations of the order of 10−6M and higher caused an increase in the rate of citrate synthesis. Adenosine, ATP, and cyclic GMP at 10−3M also stimulated, but were ineffective at 10−4M. 5′-AMP had no effect while 5′-GMP and guanosine inhibited slightly. ADP showed a 42% inhibition. Theophylline enhanced the cyclic AMP effect. It is proposed that citric acid accumulation by Aspergillus niger may result from abnormal cyclic AMP metabolism.

Published

1973

206. Deletion mutation analysis of the adenovirus type 2 E3-gp19K protein: Identification of sequences within the endoplasmic reticulum lumenal domain that are required for class I antigen binding and protection from adenovirus-specific cytotoxic T lymphocytes

Author

Ralph A. Tripp, Terry W. Hermiston, Linda R. Gooding, William S. M. Wold, and Tim E. Sparer

Subjects

Genes, Viral, Molecular Sequence Data, Immunology, Protein domain, Fluorescent Antibody Technique, Protein Sorting Signals, Biology, Endoplasmic Reticulum, Major histocompatibility complex, Polymerase Chain Reaction, Microbiology, Epitope, Adenoviridae, Cell Line, Virology, Adenovirus E3 Proteins, Humans, Amino Acid Sequence, Peptide sequence, Sequence Deletion, Genetics, Base Sequence, Sequence Homology, Amino Acid, Adenoviruses, Human, Endoplasmic reticulum, Histocompatibility Antigens Class I, ER retention, Protein tertiary structure, Transmembrane protein, Cell biology, Oligodeoxyribonucleotides, Mutagenesis, Insect Science, biology.protein, Research Article, T-Lymphocytes, Cytotoxic

Abstract

Adenovirus E3-gp19K is a transmembrane glycoprotein, localized in the endoplasmic reticulum (ER), which forms a complex with major histocompatibility complex (MHC) class I antigens and retains them in the ER, thereby preventing cytolysis by cytotoxic T lymphocytes (CTL). The ER lumenal domain of gp19K, residues 1 to 107, is known to be sufficient for binding to class I antigens; the transmembrane and cytoplasmic ER retention domains are located at residues ca. 108 to 127 and 128 to 142, respectively. To identify more precisely which gp19K regions are involved in binding to class I antigens, we constructed 13 in-frame virus deletion mutants (4 to 12 amino acids deleted) in the ER lumenal domain of gp19K, and we analyzed the ability of the mutant proteins to form a complex with class I antigens, retain them in the ER, and prevent cytolysis by adenovirus-specific CTL. All mutant proteins except one (residues 102 to 107 deleted) were defective for these properties, indicating that the ability of gp19K to bind to class I antigens is highly sensitive to mutation. All mutant proteins were stable and were retained in the ER. Sequence comparisons among adenovirus serotypes reveal that the ER lumenal domain of gp19K consists of a variable region (residues 1 to 76) and a conserved region (residues 77 to 98). We show, using the mutant proteins, that the gp19K-specific monoclonal antibody Tw1.3 recognizes a noncontiguous epitope in the variable region and that disruption of the variable region by deletion destroys the epitope. The monoclonal antibody and class I antigen binding results, together with the serotype sequence comparisons, are consistent with the idea that the ER lumenal domain of gp19K has three subdomains that we have termed the ER lumenal variable domain (residues 1 to ca. 77 to 83), the ER lumenal conserved domain (residues ca. 84 to 98), and the ER lumenal spacer domain (residues 99 to 107). We suggest that the ER lumenal variable domain of gp19K has a specific tertiary structure that is important for binding to the polymorphic alpha 1 and alpha 2 domains of class I heavy (alpha) chains. We suggest that the ER lumenal conserved domain of gp19K may interact with some conserved protein, perhaps the highly conserved alpha 3 domain of class I heavy chains. Finally, the ER lumenal spacer domain may allow the ER lumenal variable and conserved domains to extend out from the ER membrane so that they can interact with class I heavy chains.

207. Correction: STAT2 Knockout Syrian Hamsters Support Enhanced Replication and Pathogenicity of Human Adenovirus, Revealing an Important Role of Type I Interferon Response in Viral Control.

Author

Karoly Toth, Sang R Lee, Baoling Ying, Jacqueline F Spencer, Ann E Tollefson, John E Sagartz, Il-Keun Kong, Zhongde Wang, and William S M Wold

Subjects

Immunologic diseases. Allergy, RC581-607, Biology (General), QH301-705.5

Abstract

[This corrects the article DOI: 10.1371/journal.ppat.1005084.].

Published

2016

208. STAT2 Knockout Syrian Hamsters Support Enhanced Replication and Pathogenicity of Human Adenovirus, Revealing an Important Role of Type I Interferon Response in Viral Control.

Author

Karoly Toth, Sang R Lee, Baoling Ying, Jacqueline F Spencer, Ann E Tollefson, John E Sagartz, Il-Keun Kong, Zhongde Wang, and William S M Wold

Subjects

Immunologic diseases. Allergy, RC581-607, Biology (General), QH301-705.5

Abstract

Human adenoviruses have been studied extensively in cell culture and have been a model for studies in molecular, cellular, and medical biology. However, much less is known about adenovirus replication and pathogenesis in vivo in a permissive host because of the lack of an adequate animal model. Presently, the most frequently used permissive immunocompetent animal model for human adenovirus infection is the Syrian hamster. Species C human adenoviruses replicate in these animals and cause pathology that is similar to that seen with humans. Here, we report findings with a new Syrian hamster strain in which the STAT2 gene was functionally knocked out by site-specific gene targeting. Adenovirus-infected STAT2 knockout hamsters demonstrated an accentuated pathology compared to the wild-type control animals, and the virus load in the organs of STAT2 knockout animals was 100- to 1000-fold higher than that in wild-type hamsters. Notably, the adaptive immune response to adenovirus is not adversely affected in STAT2 knockout hamsters, and surviving hamsters cleared the infection by 7 to 10 days post challenge. We show that the Type I interferon pathway is disrupted in these hamsters, revealing the critical role of interferon-stimulated genes in controlling adenovirus infection. This is the first study to report findings with a genetically modified Syrian hamster infected with a virus. Further, this is the first study to show that the Type I interferon pathway plays a role in inhibiting human adenovirus replication in a permissive animal model. Besides providing an insight into adenovirus infection in humans, our results are also interesting from the perspective of the animal model: STAT2 knockout Syrian hamster may also be an important animal model for studying other viral infections, including Ebola-, hanta-, and dengue viruses, where Type I interferon-mediated innate immunity prevents wild type hamsters from being effectively infected to be used as animal models.

Published

2015