Your search keyword '"Hideyo Ugai"' showing total 39 results

1. Characterization of a recombinant Bacteroides fragilis sialidase expressed in Escherichia coli

Author

Haruyuki Nakayama-Imaohji, Miad Elahi, Tomomi Kuwahara, Ayano Tada, Hitoshi Houchi, Hideyo Ugai, and Takaaki Yamamoto

Subjects

0301 basic medicine, Glycosylation, Gene Expression, Neuraminidase, Sialidase, medicine.disease_cause, Microbiology, Protein Refolding, law.invention, Bacteroides fragilis, 03 medical and health sciences, chemistry.chemical_compound, law, Neuraminic acid, Escherichia coli, medicine, Ions, biology, Hydrolysis, Mucins, biology.organism_classification, Fetuin, N-Acetylneuraminic Acid, Recombinant Proteins, Sialic acid, Enzyme Activation, 030104 developmental biology, Infectious Diseases, chemistry, Biochemistry, Recombinant DNA

Abstract

The human gut commensal Bacteroides fragilis produces sialidases that remove a terminal sialic acid from host-derived polysaccharides. Sialidase is considered to be involved in B. fragilis infection pathology. A native B. fragilis sialidase has been purified and characterized, and was shown to be post-translationally modified by glycosylation. However, the biochemical properties of recombinant B. fragilis sialidase expressed in a heterologous host remain uncharacterized. In this study, we examined the enzymatic properties of the 60-kDa sialidase NanH1 of B. fragilis YCH46, which was prepared as a recombinant protein (rNanH1) in Escherichia coli. In E. coli rNanH1 was expressed as inclusion bodies, which were separated from soluble proteins to allow solubilization of insoluble rNanH1 in a buffer containing 8 M urea and renaturation in refolding buffer containing 100 mM CaCl2 and 50 mM L-arginine. The specific activity of renatured rNanH1 measured using 4-methylumberiferyl-α-D-N-acetyl neuraminic acid as a substrate was 6.16 μmol/min/mg. The optimal pH of rNanH1 ranged from 5.0 to 5.5. The specific activity of rNanH1 was enhanced in the presence of calcium ions. rNanH1 preferentially hydrolyzed the sialyl α2,8 linkage and cleaved sialic acids from mucin and serum proteins (e.g., fetuin and transferrin) but not from α1-acid glycoprotein, which is similar to the previously observed biochemical properties for a native sialidase purified from B. fragilis SBT3182. The results and methods described in this study will be useful for preparing and characterizing recombinant proteins for other B. fragilis sialidase isoenzymes.

Published

2018

2. Adenoviral Vectors for RNAi Delivery

Author

Hideyo Ugai

Subjects

Small hairpin RNA, RNA interference, virus diseases, Gene silencing, Vector (molecular biology), Gene delivery, Biology, Non-coding RNA, Gene, Virology, eye diseases, Viral vector

Abstract

Human adenoviruses (HAdVs) are nonenveloped viruses containing double-stranded deoxyribonucleic acid and the biology of species C HAdV serotype 5 (HAdV-C5) is relatively well-characterized. Because HAdV vector effectively transduces cells, it has been widely used as gene delivery vectors of transgenes in the research fields of gene therapy and basic science. Therefore, HAdV vector is a feasible vehicle to deliver noncoding ribonucleic acids (ncRNAs) in mammalian cells. In vitro and in vivo analyses of ncRNAs using HAdV vectors have been reported. However, studies of viral biology including HAdV have shown that viral genomes encode the gene(s) for RNA interference (RNAi) inhibitor(s) and that the gene products interfere with the key molecules in the RNAi machinery during productive infection. In this chapter, we provide an overview of RNAi in adenoviral biology, adenoviral vectors for RNAi-mediated gene silencing delivery, and the advantages and disadvantages of conventional HAdV vectors.

Published

2016

3. Adenoviral protein V promotes a process of viral assembly through nucleophosmin 1

Author

David A. Matthews, David T. Curiel, Hideyo Ugai, Minghui Wang, Long P. Le, and George C. Dobbins

Subjects

Nucleolus, Immunoelectron microscopy, Biology, Virus Replication, medicine.disease_cause, Article, Adenoviridae, Cell Line, 03 medical and health sciences, Protein V, 0302 clinical medicine, Virology, medicine, Adenovirus, 030304 developmental biology, Nucleophosmin 1, Adenoviral assembly, 0303 health sciences, Nucleophosmin, Nucleoplasm, Cancer gene therapy, Viral Core Proteins, Virus Assembly, Nuclear Proteins, Molecular biology, Viral replication, Cell culture, 030220 oncology & carcinogenesis, Cancer cell, Cell Nucleolus

Abstract

Adenoviral infection induces nucleoplasmic redistribution of a nucleolar nucleophosmin 1/NPM1/B23.1. NPM1 is preferentially localized in the nucleoli of normal cells, whereas it is also present at the nuclear matrix in cancer cells. However, the biological roles of NPM1 during infection are unknown. Here, by analyzing a pV-deletion mutant, Ad5-dV/TSB, we demonstrate that pV promotes the NPM1 translocation from the nucleoli to the nucleoplasm in normal cells, and the NPM1 translocation is correlated with adenoviral replication. Lack of pV causes a dramatic reduction of adenoviral replication in normal cells, but not cancer cells, and Ad5-dV/TSB was defective in viral assembly in normal cells. NPM1 knockdown inhibits adenoviral replication, suggesting an involvement of NPM1 in adenoviral biology. Further, we show that NPM1 interacts with empty adenovirus particles which are an intermediate during virion maturation by immunoelectron microscopy. Collectively, these data implicate that pV participates in a process of viral assembly through NPM1.

Published

2012

4. Chimeric adenoviral vectors incorporating a fiber of human adenovirus 3 efficiently mediate gene transfer into prostate cancer cells

Author

Hideyo Ugai, Natalya Belousova, Paul Dent, Miho Murakami, David T. Curiel, Alexander Pereboev, Paul B. Fisher, and Maaike Everts

Subjects

Reporter gene, Urology, Genetic enhancement, Cancer, Biology, medicine.disease, medicine.disease_cause, Virology, Adenoviridae, Prostate cancer, Oncology, DU145, Cancer cell, Cancer research, medicine, Vector (molecular biology)

Abstract

BACKGROUND—We have developed a range of adenoviral (Ad) vectors based on human adenovirus serotype 5 (HAdV-5) displaying the fiber shaft and knob domains of species B viruses (HAdV-3, HAdV-11, or HAdV-35). These species B Ads utilize different cellular receptors than HAdV-5 for infection. We evaluated whether Ad vectors displaying species B fiber shaft and knob domains (Ad5F3Luc1, Ad5F11Luc1, and Ad5F35Luc1) would efficiently infect cancer cells of distinct origins, including prostate cancer. METHODS—The fiber chimeric Ad vectors were genetically generated and compared with the original Ad vector (Ad5Luc1) for transductional efficiency in a variety of cancer cell lines, including prostate cancer cells and primary prostate epithelial cells (PrEC), using luciferase as a reporter gene. RESULTS—Prostate cancer cell lines infected with Ad5F3Luc1 expressed higher levels of luciferase than Ad5Luc1, as well as the other chimeric Ad vectors. We also analyzed the transductional efficiency via monitoring of luciferase activity in prostate cancer cells when expressed as a fraction of the gene transfer in PrEC cells. In the PC-3 and DU145 cell lines, the gene transfer ratio of cancer cells versus PrEC was once again highest for Ad5F3Luc1. CONCLUSION—Of the investigated chimeric HAdV-5/species B vectors, Ad5F3Luc1 was judged to be the most suitable for targeting prostate cancer cells as it showed the highest transductional efficiency in these cells. It is foreseeable that an Ad vector incorporating the HAdV-3 fiber could potentially be used for prostate cancer gene therapy.

Published

2009

5. JDP2 suppresses adipocyte differentiation by regulating histone acetylation

Author

Hideyo Ugai, Kazunari K. Yokoyama, Takehide Murata, Mizuho Iwama, Koji Nakade, H Li, Jianzhi Pan, S Itohara, Atsushi Yoshiki, B Liu, Makoto Kimura, and Yuichi Obata

Subjects

CCAAT-Enhancer-Binding Protein-delta, Male, Cellular differentiation, In Vitro Techniques, SAP30, Histones, Mice, chemistry.chemical_compound, Histone H3, Pregnancy, 3T3-L1 Cells, Adipocyte, Adipocytes, Animals, Promoter Regions, Genetic, Molecular Biology, DNA Primers, Mice, Knockout, Adipogenesis, Base Sequence, biology, Acetylation, Cell Differentiation, Cell Biology, Fibroblasts, Molecular biology, Chromatin, Mice, Inbred C57BL, Repressor Proteins, Histone, chemistry, Gene Targeting, Mutation, biology.protein, Jun dimerization protein, Female

Abstract

Among the events that control cellular differentiation, the acetylation of histones plays a critical role in the regulation of transcription and the modification of chromatin. Jun dimerization protein 2 (JDP2), a member of the AP-1 family, is an inhibitor of such acetylation and contributes to the maintenance of chromatin structure. In an examination of Jdp2 'knock-out' (KO) mice, we observed elevated numbers of white adipocytes and significant accumulation of lipid in the adipose tissue in sections of scapulae. In addition, mouse embryo fibroblasts (MEFs) from Jdp2 KO mice were more susceptible to adipocyte differentiation in response to hormonal induction and members of the CCAAT/enhancer-binding proteins (C/EBP) gene family were expressed at levels higher than MEFs from wild-type mice. Furthermore, JDP2 inhibited both the acetylation of histone H3 in the promoter of the gene for C/EBPdelta and transcription from this promoter. Our data indicate that JDP2 plays a key role as a repressor of adipocyte differentiation by regulating the expression of the gene for C/EBPdelta via inhibition of histone acetylation.

Published

2007

6. Thermostability/Infectivity Defect Caused by Deletion of the Core Protein V Gene in Human Adenovirus Type 5 Is Rescued by Thermo-selectable Mutations in the Core Protein X Precursor

Author

Anton V. Borovjagin, David T. Curiel, Hideyo Ugai, Minghui Wang, and Long P. Le

Subjects

Genes, Viral, viruses, Molecular Sequence Data, Mutant, Mutation, Missense, Virus Replication, medicine.disease_cause, Genome, Article, Microscopy, Electron, Transmission, Structural Biology, medicine, Humans, Point Mutation, Amino Acid Sequence, Protein Precursors, Molecular Biology, Gene, Genetics, Mutation, Base Sequence, Sequence Homology, Amino Acid, biology, Adenoviruses, Human, Viral Core Proteins, Point mutation, Temperature, Chromosome Mapping, biology.organism_classification, Mastadenovirus, Adenoviridae, Viral replication, Gene Deletion

Abstract

Mastadenoviruses represent one of the four major genera of the Adenoviridae family comprising a variety of mammalian pathogens including human adenovirus (Ad), whose genomes encode a gene for minor core protein V (pV), not found in other genera of Adenoviridae. Deletion of other genus-specific genes (gene IX and E3 genes) from the Ad type 5 (Ad5) genome has been studied experimentally in vitro and the results on biological characterization of the mutants support the phylogenetic evidence of those genes being non-essential for Ad viability. On this basis it seemed logical to suggest that a deletion of gene V from the Ad5 genome could also be tolerated. To test this hypothesis we constructed and rescued the first pV-deletion mutant of human Ad5. As compared to Ad5, this mutant formed small plaques, had dramatically reduced thermostability and lower infectivity. A subsequent thermoselection screen of the pV-deleted Ad5 allowed isolation of a suppressor mutant Ad5-dV/TSB with restored biological characteristics. Since replication and viral assembly of Ad5-dV/TSB could still occur in the absence of pV, we conclude that pV is a non-essential component of the virion. The observed rescue of the biological defects appears to be associated with a cluster of point mutations in the gene encoding the precursor for the other core protein, X/Mu. This finding, thus, suggests possible roles of pV and protein X/Mu precursor in viral assembly. It also provides an interesting insight into genetic events that mediate molecular adaptation of viruses to possible changes in the genetic background in the course of their evolutionary divergence. The possible mechanism of the observed genetic suppression is discussed.

Published

2007

7. A database of recombinant viruses and recombinant viral vectors available from the RIKEN DNA bank

Author

Takehide Murata, Bingbing Liu, Hatsumi Nakata, Jianzhi Pan, Megumi Hirose, Izumu Saito, Sanae Inamoto, Hideyo Ugai, Kazunari K. Yokoyama, Yukari Kujime, Koji Nakade, Erika Suzuki, Makoto Kimura, Yoshinori Nagamura, Kumiko Inabe, Yoshihiro Ugawa, Takahito Yamasaki, Hirofumi Hamada, Yuichi Obata, and Miho Terashima

Subjects

DNA, Complementary, Genetic Vectors, DNA, Recombinant, Information Storage and Retrieval, Biology, computer.software_genre, Recombinant virus, Adenoviridae, Viral vector, law.invention, chemistry.chemical_compound, Japan, Shuttle vector, law, Research community, Drug Discovery, Genetics, Humans, Genomic library, Molecular Biology, Gene, Genetics (clinical), Gene Library, Internet, Database, Genetic Therapy, Virology, chemistry, Recombinant DNA, Molecular Medicine, Databases, Nucleic Acid, computer, DNA

Abstract

Background Viral vectors are required as gene-delivery systems for gene therapy and basic research. Recombinant adenoviruses (rAds) expressing genes of interest are being developed as research tools and many studies in vitro and in vivo have already been performed with such rAds. Methods Shuttle vectors for rAds were constructed with full-length cDNAs and rAds were generated in HEK293 cells by the COS-TPC method. The rAds and shuttle vectors were developed by the Japanese research community and deposited in the RIKEN DNA Bank (RDB; http://www.brc.riken.jp/lab/dna/en/) for distribution to the scientific community. The Recombinant Virus Database (RVD; http://www.brc.riken.jp/lab/dna/rvd/) was established at the RIKEN BioResource Center (BRC) in Japan as the source of information about and distribution of the various resources. Results The RIKEN BRC is releasing more than 300 recombinant viruses (RVs) and 500 shuttle vectors, as well as all related information, which is included in a newly established database, the RVD. The RVD consists of (i) information about the RVs, the inserted cDNAs and the shuttle vectors; (ii) data about sequence-tagged sites (STSs) that are markers of viral DNAs; and (iii) experimental protocols for the use of RVs. Conclusions The new database and available resources should be very useful to scientists who are studying human gene therapy and performing related basic research. It is a web-interfaced flat-file database that can be accessed through the internet. Moreover, all of the resources deposited in the RDB, which is a public facility in Japan, are available to researchers around the world. Copyright © 2005 John Wiley & Sons, Ltd.

Published

2005

8. Purification of infectious adenovirus in two hours by ultracentrifugation and tangential flow filtration

Author

Hong Tang, Yuichi Obata, Miho Terashima, Hideyo Ugai, Makoto Kimura, Takehide Murata, Jianzhi Pan, Kazunari K. Yokoyama, Megumi Hirose, Yukari Kujime, Bingbing Liu, Mujun Zhao, Kumiko Inabe, Takahito Yamasaki, and Hirofumi Hamada

Subjects

viruses, Blotting, Western, Biophysics, Gene transfer, Recombinant adenoviruses, Cell Biology, Biology, Virus Replication, Biochemistry, Virology, Molecular biology, In vitro, Adenoviridae, Cross-flow filtration, Titer, In vivo, Humans, Electrophoresis, Polyacrylamide Gel, Ultracentrifuge, Ultracentrifugation, Molecular Biology, Filtration, HeLa Cells

Abstract

Adenoviruses are excellent vectors for gene transfer and are used extensively for high-level expression of the products of transgenes in living cells. The development of simple and rapid methods for the purification of stable infectious recombinant adenoviruses (rAds) remains a challenge. We report here a method for the purification of infectious adenovirus type 5 (Ad5) that involves ultracentrifugation on a cesium chloride gradient at 604,000g for 15 min at 4 degrees C and tangential flow filtration. The entire procedure requires less than two hours and infectious Ad5 can be recovered at levels higher than 64% of the number of plaque-forming units (pfu) in the initial crude preparation of viruses. We have obtained titers of infectious purified Ad5 of 1.35 x 10(10) pfu/ml and a ratio of particle titer to infectious titer of seven. The method described here allows the rapid purification of rAds for studies of gene function in vivo and in vitro, as well as the rapid purification of Ad5. (c) 2005 Elsevier Inc. All rights reserved.

Published

2005

9. Spontaneous mutations in the human gene for p53 in recombinant adenovirus during multiple passages in human embryonic kidney 293 cells

Author

Kumiko Inabe, Erika Suzuki, Takehide Murata, Hirofumi Hamada, Hideyo Ugai, and Kazunari K. Yokoyama

Subjects

Viral Plaque Assay, Mutation rate, Genetic enhancement, Genetic Vectors, DNA, Recombinant, Biophysics, Biology, Molecular cloning, Kidney, medicine.disease_cause, Biochemistry, Adenoviridae, Cell Line, Gene Frequency, medicine, Humans, Cloning, Molecular, Molecular Biology, Gene, Cloning, Genetics, Mutation, HEK 293 cells, Cell Biology, Genes, p53, Molecular biology

Abstract

Infectious recombinant adenovirus (rAd) is usually produced in human embryonic kidney 293 cells that harbor the E1 gene and rAd has been shown to be an efficient tool for gene transfer both in vivo and in vitro. It also has considerable potential in human gene therapy. However, rates of spontaneous mutations in genes introduced into host cells after multiple passages remain to be clarified. We have characterized the spontaneous mutation of genomes derived from human adenovirus type 5 (Ad5) and of human p53-rAd during multiple passages by two different methods, namely, a plaque assay and a molecular cloning assay, with subsequent direct nucleotide sequencing. Using the plaque assay, we found no mutations in the E1A and p53 genes derived from infectious Ad5 and p53-rAd, respectively. By contrast, we found spontaneous mutations in the E1A gene of Ad5, with a mutation rate of 9.28 x 10(-8) per base pair per plaque, in the molecular cloning assay. The rate of mutation of the p53 gene of p53-rAd, as determined by the molecular cloning assay, ranged from 1.50 x 10(-7) to 3.25 x 10(-7) per base pair per passage. The mutations in the p53 gene of p53-rAd were localized mainly in the transcriptional activation domain, the SH3 domain, and the regulation domain and they were rarely found in the DNA-binding domain, which is a major site for mutations in human cancers. Our results indicate that multiple passages can generate a heterogeneous population of p53-rAd and that the molecular cloning assay is an efficient technique with which to search for mutations in the genome of p53-rAd that cannot be detected by a plaque assay.

Published

2003

10. Isolation of embryonic stem-like cells from equine blastocysts and their differentiation in vitro1

Author

Hideyo Ugai, Takehide Murata, Kazunari K. Yokoyama, Akira Minamihashi, Yuichi Obata, Kahori Kurosaka, Shigeo Saito, Ken Sawai, Yusuke Yamamoto, and Yoshiro Kobayashi

Subjects

KOSR, Cellular differentiation, Biophysics, Cell Biology, Embryoid body, Oct-4, Biology, Biochemistry, Molecular biology, Structural Biology, Neurosphere, Genetics, Stem cell, Induced pluripotent stem cell, Molecular Biology, Adult stem cell

Abstract

Embryonic stem (ES) cells are pluripotent cells with the potential capacity to generate any type of cell. We describe here the isolation of pluripotent ES-like cells from equine blastocysts that have been frozen and thawed. Our two lines of ES-like cells (E-1 and E-2) appear to maintain a normal diploid karyotype indefinitely in culture in vitro and to express markers that are characteristic of ES cells from mice, namely, alkaline phosphatase, stage-specific embryonic antigen-1, STAT-3 and Oct 4. After culture of equine ES-like cells in vitro for more than 17 passages, some ES-like cells differentiated to neural precursor cells in the presence of basic fibroblast growth factor (bFGF), epidermal growth factor and platelet-derived growth factor. We also developed a protocol that resulted in the differentiation of ES-like cells in vitro to hematopoietic and endothelial cell lineages in response to bFGF, stem cell factor and oncostatin M. Our observations set the stage for future developments that may allow the use of equine ES-like cells for the treatment of neurological and hematopoietic disorders.

Published

2002

11. Species D human adenovirus type 9 exhibits better virus-spread ability for antitumor efficacy among alternative serotypes

Author

Hideyo Ugai, David T. Curiel, and Junji Uchino

Subjects

Serotype, Cancer Treatment, lcsh:Medicine, medicine.disease_cause, Adenovirus Infections, Human, 0302 clinical medicine, Viral classification, Coxsackie B virus, Vector (molecular biology), lcsh:Science, 0303 health sciences, Multidisciplinary, Cell Death, virus diseases, Gene Therapy, Viral Load, 3. Good health, Oncology, 030220 oncology & carcinogenesis, Medicine, Viral Vectors, Research Article, Coxsackie and Adenovirus Receptor-Like Membrane Protein, Antineoplastic Agents, Biology, Microbiology, Vector Biology, Virus, Cell Line, 03 medical and health sciences, Species Specificity, Spheroids, Cellular, Virology, Genetics, medicine, Animals, Humans, Serotyping, Tropism, 030304 developmental biology, Clinical Genetics, Adenoviruses, Human, lcsh:R, Cancer, Human Genetics, medicine.disease, eye diseases, Culture Media, Viral replication, Cancer cell, lcsh:Q, DNA viruses, Viral Transmission and Infection

Abstract

Species C human adenovirus serotype 5 (HAdV-C5) is widely used as a vector for cancer gene therapy, because it efficiently transduces target cells. A variety of HAdV-C5 vectors have been developed and tested in vitro and in vivo for cancer gene therapy. While clinical trials with HAdV-C5 vectors resulted in effective responses in many cancer patients, administration of HAdV-C5 vectors to solid tumors showed responses in a limited area. A biological barrier in tumor mass is considered to hinder viral spread of HAdV-C5 vectors from infected cells. Therefore, efficient virus-spread from an infected tumor cell to surrounding tumor cells is required for successful cancer gene therapy. In this study, we compared HAdV-C5 to sixteen other HAdV serotypes selected from species A to G for virus-spread ability in vitro. HAdV-D9 showed better virus-spread ability than other serotypes, and its viral progeny were efficiently released from infected cells during viral replication. Although the HAdV-D9 fiber protein contains a binding site for coxsackie B virus and adenovirus receptor (CAR), HAdV-D9 showed expanded tropism for infection due to human CAR (hCAR)-independent attachment to target cells. HAdV-D9 infection effectively killed hCAR-negative cancer cells as well as hCAR-positive cancer cells. These results suggest that HADV-D9, with its better virus-spread ability, could have improved therapeutic efficacy in solid tumors compared to HAdV-C5.

Published

2014

12. Structural organization and expression of the mouse gene for Pur-1, a highly conserved homolog of the human MAZ gene

Author

Takehide Murata, Ichirou Kanazawa, Kailai Sun, Hideyo Ugai, Keiichi Itakura, Kazunari K. Yokoyama, Jun Song, Christian Geltinger, Hiroo Murakami, Masatoshi Matsumura, and Hatsumi Tsutsui

Subjects

Untranslated region, Genetics, General transcription factor, Transcription (biology), Gene expression, Promoter, Biology, Biochemistry, Molecular biology, Gene, Genomic organization, Housekeeping gene

Abstract

We have characterized the genomic structure and expression of the mouse gene for Pur-1. The cloned Pur-1 gene spans a 5-kb region encompassing the promoter, five exons, four introns and the 3'-untranslated region. All exon-intron junction sequences conform to the GT/AG rule. The promoter region has typical features of a housekeeping gene: a high G + C content (77.5%); a high frequency of CpG dinucleotides, in particular within the region 0.5 kb upstream of the site of initiation of translation; and the absence of canonical TATA and CAAT boxes. S1 nuclease protection assay demonstrated the presence of multiple sites for initiation of transcription around a site 108 nucleotides upstream of the ATG codon. Comparison of Pur-1 with the human gene for MAZ (Myc-associated zinc finger protein) revealed a striking homology of both their nucleotide and deduced protein sequences, an identical genomic organization and high similarity in promoter architecture and mRNA expression pattern. Sequence analysis of the 5'-flanking region of Pur-1 revealed numerous potential binding sites for transcription factors Sp1, AP-2 and Pur-1/MAZ itself. An element required for basal Pur-1 expression was mapped from nucleotide -258 to +43. This region also mediated stimulation of basal transcription by ectopically expressed MAZ protein. We conclude that the Pur-1 gene is the murine homolog of human MAZ and, like it, belongs to the family of housekeeping genes.

Published

2001

13. Interaction of Myc-Associated Zinc Finger Protein with DCC, the Product of a Tumor-Suppressor Gene, during the Neural Differentiation of P19 EC Cells

Author

Kazunari K. Yokoyama, Hatsumi Tsutsui, Takehide Murata, Hideyo Ugai, Takashi Shiga, Masaaki Komatsu, Jun Song, Eric R. Fearon, and Hai-Ou Li

Subjects

Cytoplasm, Time Factors, Transcription, Genetic, Deleted in Colorectal Cancer, Xenopus, Cellular differentiation, Genes, myc, Biochemistry, Promoter Regions, Genetic, Neurons, Zinc finger, Reverse Transcriptase Polymerase Chain Reaction, Cell Differentiation, Zinc Fingers, Transfection, DCC Receptor, Immunohistochemistry, DNA-Binding Proteins, Signal transduction, Plasmids, Protein Binding, Signal Transduction, Recombinant Fusion Proteins, Blotting, Western, Molecular Sequence Data, Active Transport, Cell Nucleus, Biophysics, Receptors, Cell Surface, Tretinoin, Biology, Models, Biological, DNA-binding protein, Cell Line, Two-Hybrid System Techniques, Animals, Humans, Amino Acid Sequence, RNA, Messenger, Molecular Biology, Transcription factor, Cell Nucleus, Binding Sites, Sequence Homology, Amino Acid, Activator (genetics), Tumor Suppressor Proteins, Cell Biology, Blotting, Northern, Precipitin Tests, Molecular biology, Protein Structure, Tertiary, Microscopy, Fluorescence, RNA, Cell Adhesion Molecules, Transcription Factors

Abstract

Expression of the DCC (deleted in colorectal cancer) protein is strongly induced during the neural differentiation of mouse P19 embryonal carcinoma (EC) cells that occurs when these cells are treated with retinoic acid (RA). Myc-associated zinc finger protein (MAZ) is a DNA-binding protein that is widely expressed and functions in human, mouse and hamster cells as an activator, an initiator or a terminator of transcription. However, the biological functions of MAZ remain elusive. We report here that MAZ associates with the cytoplasmic domain of the DCC protein in vivo and in vitro. Yeast two-hybrid assays confirmed this association. An immunofluorescence study demonstrated that DCC protein is expressed at elevated levels in neuron-like P19 EC cells, in particular in axons, in which the MAZ protein is also expressed. We found that MAZ was translocated from the nucleus to the cytoplasm during the RA-induced terminal differentiation of P19 EC cells with resultant loss of the ability of MAZ to bind to the ME1a1 site of the c-myc promoter. Taken together, our observations imply that the DCC protein might play a critical role as a signaling molecule in the regulation of the transcriptional activity of MAZ during the neural differentiation of P19 EC cells.

Published

2001

14. Independent Repression of a GC-rich Housekeeping Gene by Sp1 and MAZ Involves the Same cis-Elements

Author

Kailai Sun, Kazunari K. Yokoyama, Hideyo Ugai, Jun Song, and Ichiro Kanazawa

Subjects

Sp1 Transcription Factor, Molecular Sequence Data, Biochemistry, DNA-binding protein, Histone Deacetylases, Cell Line, Proto-Oncogene Proteins c-myc, Gene expression, Animals, Humans, Promoter Regions, Genetic, Molecular Biology, Transcription factor, Gene, Zinc finger, Base Sequence, biology, Chemistry, Zinc Fingers, Promoter, DNA, Cell Biology, Precipitin Tests, Molecular biology, Housekeeping gene, DNA-Binding Proteins, Histone, Gene Expression Regulation, biology.protein, Transcription Factors

Abstract

The transcription factors Sp1 and MAZ (Myc-associated zinc finger protein) contain several zinc finger motifs, and each functions as both a positive and a negative regulator of gene expression. In this study, we characterized the extremely GC-rich promoter of the human gene for MAZ, which is known as a housekeeping gene. Unique symmetrical motifs in the promoter region (nucleotides -383 to -334) were essential for the expression of the gene for MAZ, whereas an upstream silencer element (nucleotides -784 to -612) was found to act in a position-dependent but orientation-independent manner. Sp1 and MAZ bound to the same cis-elements in the GC-rich promoter, apparently sharing DNA-binding sites. The relative extent of binding of Sp1 and MAZ to these cis-elements corresponded to the extent of negative regulation of the expression of the gene for MAZ in various lines of cells. Furthermore, novel repressive domains in both Sp1 (amino acids 622-788) and MAZ (amino acids 127-292) were identified. Suppression by Sp1 and suppression by MAZ were independent phenomena; histone deacetylases were involved in the autorepression by MAZ itself, whereas DNA methyltransferase 1 was associated with suppression by Sp1. Our results indicate that both deacetylation and methylation might be involved in the regulation of expression of a single gene via the actions of different zinc finger proteins that bind to the same cis-elements.

Published

2001

15. TOK-1, a Novel p21Cip1-binding Protein That Cooperatively Enhances p21-dependent Inhibitory Activity toward CDK2 Kinase

Author

Kazunari K. Yokoyama, Hideyo Ugai, Takashi Ono, Sanae M.M. Iguchi-Ariga, Hirotake Kitaura, Hiroyoshi Ariga, and Takehide Murata

Subjects

Time Factors, Cell Cycle Proteins, Mitogen-activated protein kinase kinase, Biochemistry, MAP2K7, CDC2-CDC28 Kinases, Protein Isoforms, Tissue Distribution, Cloning, Molecular, Fluorescent Antibody Technique, Indirect, Glutathione Transferase, Cell Cycle, Nuclear Proteins, Cyclin-Dependent Kinases, Recombinant Proteins, COS Cells, Codon, Terminator, Plasmids, Protein Binding, Cyclin-Dependent Kinase Inhibitor p21, DNA, Complementary, Molecular Sequence Data, Protein Serine-Threonine Kinases, Biology, Cell Line, Cyclins, Proliferating Cell Nuclear Antigen, Two-Hybrid System Techniques, Animals, Humans, Amino Acid Sequence, c-Raf, Kinase activity, Molecular Biology, Cell Nucleus, Base Sequence, Models, Genetic, MAP kinase kinase kinase, Cyclin-dependent kinase 4, Calcium-Binding Proteins, Cyclin-Dependent Kinase 2, Phosphotransferases, Cyclin-dependent kinase 2, Cell Biology, Blotting, Northern, Protein Structure, Tertiary, Mutagenesis, Site-Directed, biology.protein, Cyclin-dependent kinase 9, Carrier Proteins, HeLa Cells

Abstract

A p21(Cip1/Waf1/Sdi1) is known to act as a negative cell-cycle regulator by inhibiting kinase activity of a variety of cyclin-dependent kinases. In addition to binding of the cyclin-dependent kinase to the N-terminal region of p21, p21 is also bound at its C-terminal region by proliferating cell nuclear antigen (PCNA), SET/TAF1, and calmodulin, indicating the versatile function of p21. In this study, we cloned cDNA encoding a novel protein named TOK-1 as a p21 C-terminal-binding protein by a two-hybrid system. Two splicing isoforms of TOK-1, TOK-1alpha and TOK-1beta, comprising 322 and 314 amino acids, respectively, were co-localized with p21 in nuclei and showed a similar expression profile to that of p21 in human tissues. TOK-1alpha, but not TOK-1beta, directly bound to the C-terminal proximal region of p21, and both were expressed at the G(1)/S boundary of the cell cycle. TOK-1alpha also preferentially bound to an active form of cyclin-dependent kinase 2 (CDK2) via p21, and these made a ternary complex in human cells. Furthermore, the results of three different types of experiments showed that TOK-1alpha enhanced the inhibitory activity of p21 toward histone H1 kinase activity of CDK2. TOK-1alpha is thus thought to be a new type of CDK2 modulator.

Published

2000

16. Assignment of the human gene for KBF2/RBP-Jk to chromosome 9p12-13 and 9q13 by fluorescencein situ hybridization

Author

Chie Koga, Hiroo Murakami, Fumiko Saito-Ohara, Jun Song, Tatsuro Ikeuchi, Xiaoren Tang, Kazunari K. Yokoyama, and Hideyo Ugai

Subjects

clone (Java method), Genetics, biology, medicine.diagnostic_test, Pseudogene, Nuclear Proteins, In situ hybridization, Cosmids, Major histocompatibility complex, Molecular biology, DNA-Binding Proteins, Mice, Immunoglobulin J Recombination Signal Sequence-Binding Protein, Cosmid, biology.protein, medicine, Animals, Humans, Chromosomes, Human, Pair 9, Gene, Peptide sequence, In Situ Hybridization, Fluorescence, Genetics (clinical), Transcription Factors, Fluorescence in situ hybridization

Abstract

The transcription factor KBF2 has been characterized as a factor that binds to the NFkB site of mouse major histocompatibility complex (MHC) class I genes and its amino acid sequence has been shwn to be identical to those of members of the recombination signal-sequence binding protein (RBP-Jk) family. Previous studies by Amakawa et al. (Genomics 17, 306-315, 1993) demonstrated that the functional gene is localized at human chromosome 3q25. However, in the present study we showed by in situ hybridization with the functional KBF2/RBPJk cosmid clone that the gene is localized at 9p12-13 and 9q13, namely, at the same loci as pseudogenes that were reported previously (Zhang et al, Jpn J Human Genet 39, 391-401, 1994).

Published

1997

17. An Adenovirus Vector Incorporating Carbohydrate Binding Domains Utilizes Glycans for Gene Transfer

Author

Hideyo Ugai, Ferhat Ak, David T. Curiel, Masaharu Nakayama, Julius W. Kim, Joel N. Glasgow, and Groningen Research Institute of Pharmacy

Subjects

Glycobiology, Cancer Treatment, Adenoviruses, Porcine, lcsh:Medicine, CELLULAR RECEPTORS, Biochemistry, THERAPY, chemistry.chemical_compound, Viral classification, Cricetinae, Neoplasms, Molecular Cell Biology, Pathology, Vector (molecular biology), lcsh:Science, IN-VIVO, Genetics, Multidisciplinary, biology, Gene Transfer Techniques, Gene targeting, Gene Therapy, Extracellular Matrix, EX-VIVO, Oncology, Gene Targeting, Medicine, Viral Vectors, Research Article, Plasmids, Glycan, Glycosylation, Protein domain, Blotting, Western, Genetic Vectors, Computational biology, CHO Cells, Gene delivery, FIBER PROTEIN, Microbiology, Vector Biology, Viral vector, Cricetulus, Diagnostic Medicine, Polysaccharides, Virology, Cell Line, Tumor, Animals, Humans, BREAST-CANCER, CANCER-CELLS, Biology, Glycoproteins, DNA Primers, POLY-N-ACETYLLACTOSAMINE, UDP-GALACTOSE, Adenoviruses, Human, GLYCOSYLATION, lcsh:R, Genetic Therapy, chemistry, Cancer cell, biology.protein, lcsh:Q, Glycolipids, DNA viruses, Biomarkers, General Pathology

Abstract

Background: Vectors based on human adenovirus serotype 5 (HAdV-5) continue to show promise as delivery vehicles for cancer gene therapy. Nevertheless, it has become clear that therapeutic benefit is directly linked to tumor-specific vector localization, highlighting the need for tumor-targeted gene delivery. Aberrant glycosylation of cell surface glycoproteins and glycolipids is a central feature of malignant transformation, and tumor-associated glycoforms are recognized as cancer biomarkers. On this basis, we hypothesized that cancer-specific cell-surface glycans could be the basis of a novel paradigm in HAdV-5-based vector targeting.Methodology/Principal Findings: As a first step toward this goal, we constructed a novel HAdV-5 vector encoding a unique chimeric fiber protein that contains the tandem carbohydrate binding domains of the fiber protein of the NADC-1 strain of porcine adenovirus type 4 (PAdV-4). This glycan-targeted vector displays augmented CAR-independent gene transfer in cells with low CAR expression. Further, we show that gene transfer is markedly decreased in cells with genetic glycosylation defects and by inhibitors of glycosylation in normal cells.Conclusions/Significance: These data provide the initial proof-of-concept for HAdV-5 vector-mediated gene delivery based on the presence of cell-surface carbohydrates. Further development of this new targeting paradigm could provide targeted gene delivery based on vector recognition of disease-specific glycan biomarkers.

Published

2013

18. Nucleotide Sequence of the Gene Encoding β-Isopropylmalate Dehydrogenase (leuB) fromBacteroides fragilis

Author

Shigeru Akimoto, Mahfuzur R. Sarker, Tomomi Kuwahara, Hideyo Ugai, and Yoshinari Ohnishi

Subjects

3-Isopropylmalate Dehydrogenase, Molecular Sequence Data, Immunology, Dehydrogenase, Microbiology, Bacteroides fragilis, Open Reading Frames, Virology, Nucleotide, Amino Acid Sequence, Gene, Peptide sequence, chemistry.chemical_classification, Base Sequence, Sequence Homology, Amino Acid, biology, Nucleic acid sequence, biology.organism_classification, Molecular biology, Molecular Weight, Alcohol Oxidoreductases, Open reading frame, chemistry, Biochemistry, Genes, Bacterial

Abstract

The complete nucleotide sequence of the gene (leuB) coding for beta-isopropylmalate dehydrogenase of Bacteroides fragilis was determined. An open reading frame of 1,061 nucleotides was detected that could encode a polypeptide of 353 amino acid residues with a calculated molecular mass of 39,179 Da. The deduced amino acid sequence of the beta-isopropylmalate dehydrogenase from B. fragilis showed substantial sequence similarity with the beta-isopropylmalate dehydrogenases from other bacteria.

Published

1995

19. Genetic materials at the gene engineering division, RIKEN BioResource Center

Author

Akiko Yoshikawa, Shotaro Kishikawa, Kazuko Ueno, Makoto Kimura, Koji Nakade, Kumiko Inabe, Satoko Masuzaki, Kazunari K. Yokoyama, Chitose Kurihara, Yukari Kujime, Takehide Murata, Yuri Nakano, Jianzhi Pan, Megumi Hirose, Takahito Yamasaki, Masato Okubo, Yuka Kusa, Hideyo Ugai, and Yuichi Obata

Subjects

Genetics, Microbial, Genetic Research, International Cooperation, Biology, Information Centers, Genome, General Biochemistry, Genetics and Molecular Biology, Viral vector, chemistry.chemical_compound, Mice, Japan, Complementary DNA, Animals, Laboratory, Animals, Humans, Gene, Genetics, General Veterinary, General Medicine, Restriction Enzyme Mapping, Government Programs, genomic DNA, Disease Models, Animal, chemistry, Cosmid, Animal Science and Zoology, Databases, Nucleic Acid, Genetic Engineering, DNA

Abstract

Genetic materials are one of the most important and fundamental research resources for studying biological phenomena. Scientific need for genetic materials has been increasing and will never cease. Ever since it was established as RIKEN DNA Bank in 1987, the Gene Engineering Division of RIKEN BioResource Center (BRC) has been engaged in the collection, maintenance, storage, propagation, quality control, and distribution of genetic resources developed mainly by the Japanese research community. When RIKEN BRC was inaugurated in 2001, RIKEN DNA Bank was incorporated as one of its six Divisions, the Gene Engineering Division. The Gene Engineering Division was selected as a core facility for the genetic resources of mammalian and microbe origin by the National BioResource Project (NBRP) of the Ministry of Education, Culture, Sports, Science and Technology (MEXT), Japan in 2002. With support from the scientific community, the Division now holds over 3 million clones of genetic materials for distribution. The genetic resources include cloned DNAs, gene libraries (e.g., cDNA and genomic DNA cloned into phage, cosmid, BAC, phosmid, and YAC), vectors, hosts, recombinant viruses, and ordered library sets derived from animal cells, including human and mouse cells, microorganisms, and viruses. Recently genetic materials produced by a few MEXT national research projects were transferred to the Gene Engineering Division for further dissemination. The Gene Engineering Division performs rigorous quality control of reproducibility, restriction enzyme mapping and nucleotide sequences of clones to ensure the reproducibility of in vivo and in vitro experiments. Users can easily access our genetic materials through the internet and obtain the DNA resources for a minimal fee. Not only the materials, but also information of features and technology related to the materials are provided via the web site of RIKEN BRC. Training courses are also given to transfer the technology for handling viral vectors. RIKEN BRC supports scientists around the world in the use of valuable genetic materials.

Published

2010

20. Derivation of a triple mosaic adenovirus for cancer gene therapy

Author

Hideyo Ugai, David T. Curiel, Hongju Wu, Qiana L. Matthews, and Yizhe Tang

Subjects

Genetic enhancement, Adenoviridae Infections, lcsh:Medicine, medicine.disease_cause, 0302 clinical medicine, Neoplasms, Biotechnology/Applied Microbiology, Polylysine, Vector (molecular biology), lcsh:Science, 0303 health sciences, education.field_of_study, Multidisciplinary, Cell Death, 3. Good health, 030220 oncology & carcinogenesis, Genetic Engineering, Research Article, Radiology and Medical Imaging, Surface Properties, Population, Blotting, Western, Genetic Vectors, DNA, Recombinant, Virus Attachment, Biology, Thymidine Kinase, Adenoviridae, Cell Line, 03 medical and health sciences, Capsid, Virology, medicine, Humans, education, 030304 developmental biology, Genetics and Genomics/Gene Therapy, lcsh:R, Virion, Cancer, Genetic Therapy, medicine.disease, Luminescent Proteins, Herpes simplex virus, Microscopy, Fluorescence, Thymidine kinase, Cancer cell, Cancer research, lcsh:Q, Capsid Proteins

Abstract

A safe and efficacious cancer medicine is necessary due to the increasing population of cancer patients whose particular diseases cannot be cured by the currently available treatment. Adenoviral (Ad) vectors represent a promising therapeutic medicine for human cancer therapy. However, several improvements are needed in order for Ad vectors to be effective cancer therapeutics, which include, but are not limited to, improvement of cellular uptake, enhanced cancer cell killing activity, and the capability of vector visualization and tracking once injected into the patients. To this end, we attempted to develop an Ad as a multifunctional platform incorporating targeting, imaging, and therapeutic motifs. In this study, we explored the utility of this proposed platform by generating an Ad vector containing the poly-lysine (pK), the herpes simplex virus type 1 (HSV-1) thymidine kinase (TK), and the monomeric red fluorescent protein (mRFP1) as targeting, tumor cell killing, and imaging motifs, respectively. Our study herein demonstrates the generation of the triple mosaic Ad vector with pK, HSV-1 TK, and mRFP1 at the carboxyl termini of Ad minor capsid protein IX (pIX). In addition, the functionalities of pK, HSV-1 TK, and mRFP1 proteins on the Ad vector were retained as confirmed by corresponding functional assays, indicating the potential multifunctional application of this new Ad vector for cancer gene therapy. The validation of the triple mosaic Ad vectors also argues for the ability of pIX modification as a base for the development of multifunctional Ad vectors.

Published

2009

21. In vitro dynamic visualization analysis of fluorescently labeled minor capsid protein IX and core protein V by simultaneous detection

Author

Hideyo Ugai, Minghui Wang, David T. Curiel, Masato Yamamoto, Long P. Le, and David A. Matthews

Subjects

viruses, Green Fluorescent Proteins, Biology, medicine.disease_cause, Virus Replication, Article, Green fluorescent protein, Adenoviridae, Cell Line, Structural Biology, medicine, Humans, Adenovirus infection, Molecular Biology, Fluorescent Dyes, Staining and Labeling, Viral Core Proteins, Virion, medicine.disease, Molecular biology, Transport protein, Oncolytic virus, Kinetics, Luminescent Proteins, Protein Transport, Capsid, Viral replication, Cell culture, Capsid Proteins, Subcellular Fractions

Abstract

Oncolytic adenoviruses represent a promising therapeutic medicine for human cancer therapy, but successful translation into human clinical trials requires careful evaluation of their viral characteristics. While the function of adenovirus proteins has been analyzed in detail, the dynamics of adenovirus infection remain largely unknown due to technological constraints that prevent adequate tracking of adenovirus particles after infection. Fluorescence labeling of adenoviral particles is one new strategy designed to directly analyze the dynamic processes of viral infection in virus-host cell interactions. We hypothesized that the double labeling of an adenovirus with fluorescent proteins would allow us to properly analyze intracellular viruses and the fate of viral proteins in a live analysis of an adenovirus as compared to single labeling. Thus, we generated a fluorescently labeled adenovirus with both a red fluorescent minor capsid protein IX (pIX) [pIX monomeric red fluorescent protein 1 (mRFP1)] and a green fluorescent minor core protein V (pV) [pV enhanced green fluorescent protein (EGFP)], resulting in Ad5-IX-mRFP1-E3-V-EGFP. The fluorescent signals for pIX-mRFP1 and pV-EGFP were detected within 10 min in living cells. However, a growth curve analysis of Ad5-IX-mRFP1-E3-V-EGFP showed an approximately 150-fold reduced production of the viral progeny at 48 h postinfection as compared to adenovirus type 5. Interestingly, pIX-mRFP1 and pV-EGFP were initially localized in the cytoplasm and nucleolus, respectively, at 18 h postinfection. These proteins were observed in the nucleus during the late stage of infection, and relocalization of the proteins was observed in an adenoviral-replication-dependent manner. These results indicate that simultaneous detection of adenoviruses using dual-fluorescent proteins is suitable for real-time analysis, including identification of infected cells and monitoring of viral spread, which will be required for a complete evaluation of oncolytic adenoviruses.

Published

2009

22. Genetic incorporation of the protein transduction domain of Tat into Ad5 fiber enhances gene transfer efficacy

Author

Juan L. Contreras, Tie Han, Leslie Perry, Hongju Wu, Yizhe Tang, Gene P. Siegal, and Hideyo Ugai

Subjects

Coxsackie and Adenovirus Receptor-Like Membrane Protein, viruses, Amino Acid Motifs, Mice, Nude, Biology, Gene delivery, Cell Line, lcsh:Infectious and parasitic diseases, Viral vector, Retinoblastoma-like protein 1, Mice, 03 medical and health sciences, Transduction (genetics), 0302 clinical medicine, Transduction, Genetic, Virology, Animals, Humans, lcsh:RC109-216, 5-HT5A receptor, 030304 developmental biology, 0303 health sciences, Adenoviruses, Human, Research, Genetic Therapy, Glioma, biochemical phenomena, metabolism, and nutrition, Molecular biology, Protein Structure, Tertiary, 3. Good health, Infectious Diseases, Organ Specificity, Cell culture, GATAD2B, 030220 oncology & carcinogenesis, Gene Products, tat, biology.protein, Receptors, Virus, Capsid Proteins, GRB2, Neoplasm Transplantation

Abstract

Background Human adenovirus serotype 5 (Ad5) has been widely explored as a gene delivery vector for a variety of diseases. Many target cells, however, express low levels of Ad5 native receptor, the Coxsackie-Adenovirus Receptor (CAR), and thus are resistant to Ad5 infection. The Protein Transduction Domain of the HIV Tat protein, namely PTDtat, has been shown to mediate protein transduction in a wide range of cells. We hypothesize that re-targeting Ad5 vector via the PTDtat motif would improve the efficacy of Ad5-mediated gene delivery. Results In this study, we genetically incorporated the PTDtat motif into the knob domain of Ad5 fiber, and rescued the resultant viral vector, Ad5.PTDtat. Our data showed the modification did not interfere with Ad5 binding to its native receptor CAR, suggesting Ad5 infection via the CAR pathway is retained. In addition, we found that Ad5.PTDtat exhibited enhanced gene transfer efficacy in all of the cell lines that we have tested, which included both low-CAR and high-CAR decorated cells. Competitive inhibition assays suggested the enhanced infectivity of Ad5.PTDtat was mediated by binding of the positively charged PTDtat peptide to the negatively charged epitopes on the cells' surface. Furthermore, we investigated in vivo gene delivery efficacy of Ad5.PTDtat using subcutaneous tumor models established with U118MG glioma cells, and found that Ad5.PTDtat exhibited enhanced gene transfer efficacy compared to unmodified Ad5 vector as analyzed by a non-invasive fluorescence imaging technique. Conclusion Genetic incorporation of the PTDtat motif into Ad5 fiber allowed Ad5 vectors to infect cells via an alternative PTDtat targeting motif while retaining the native CAR-mediated infection pathway. The enhanced infectivity was demonstrated in both cultured cells and in in vivo tumor models. Taken together, our study identifies a novel tropism expanded Ad5 vector that may be useful for clinical gene therapy applications.

Published

2007

23. A Multi Targeting Conditionally Replicating Adenovirus Displays Enhanced Oncolysis while Maintaining Expression of Immunotherapeutic Agents

Author

Hideyo Ugai, David T. Curiel, G. Yancey Gillespie, and G. Clement Dobbins

Subjects

viruses, medicine.medical_treatment, lcsh:Medicine, Biology, Virus Replication, medicine.disease_cause, Virus, Adenoviridae, 03 medical and health sciences, 0302 clinical medicine, Cell Line, Tumor, Neoplasms, medicine, Humans, lcsh:Science, Cytotoxicity, Sequence Deletion, 030304 developmental biology, Cytopathic effect, Oncolytic Virotherapy, 0303 health sciences, Multidisciplinary, Base Sequence, lcsh:R, Immunotherapy, Virology, 3. Good health, Oncolytic virus, Oncolytic Viruses, Viral replication, Cell culture, 030220 oncology & carcinogenesis, lcsh:Q, Adenovirus E1A Proteins, Oligopeptides, Research Article

Abstract

Studies have demonstrated that oncolytic adenoviruses based on a 24 base pair deletion in the viral E1A gene (D24) may be promising therapeutics for treating a number of cancer types. In order to increase the therapeutic potential of these oncolytic viruses, a novel conditionally replicating adenovirus targeting multiple receptors upregulated on tumors was generated by incorporating an Ad5/3 fiber with a carboxyl terminus RGD ligand. The virus displayed full cytopathic effect in all tumor lines assayed at low titers with improved cytotoxicity over Ad5-RGD D24, Ad5/3 D24 and an HSV oncolytic virus. The virus was then engineered to deliver immunotherapeutic agents such as GM-CSF while maintaining enhanced heterogenic oncolysis.

Published

2015

24. Derivation, Maintenance, and Induction of the Differentiation In Vitro of Equine Embryonic Stem Cells

Author

Shigeo Saito, Kazunari K. Yokoyama, Arika Minamihashi, Takehide Murata, Ken Sawai, and Hideyo Ugai

Subjects

KOSR, Cellular differentiation, Growth factor, medicine.medical_treatment, Basic fibroblast growth factor, Stem cell factor, Biology, Embryonic stem cell, Cell biology, Endothelial stem cell, chemistry.chemical_compound, chemistry, medicine, Stem cell

Abstract

We describe here the isolation and maintenance of pluripotent embryonic stem (ES) cells from equine blastocysts that have been frozen and thawed. Equine ES cells appear to maintain a normal diploid karyotype in culture. These cells express markers that are characteristic of mouse ES cells, namely, alkaline phosphatase, stage-specific-embryonic antigen 1, STAT3, and Oct4. We also describe protocols for the induction of differentiation in vitro to neural precursor cells in the presence of basic fibroblast growth factor (bFGF), epidermal growth factor, and platelet-derived growth factor and to hematopoietic and endothelial cell lineages in the presence of bFGF, stem cell factor, and oncostatin M. Equine ES cells provide a powerful tool for gene targeting and the generation of transgenic clonal offspring.

Published

2006

25. Accumulation of infectious mutants in stocks during the propagation of fiber-modified recombinant adenoviruses

Author

Hideyo Ugai, Yuichi Obata, Takehide Murata, Kumiko Inabe, Takahito Yamasaki, Hirofumi Hamada, and Kazunari K. Yokoyama

Subjects

viruses, Mutant, DNA Mutational Analysis, Genetic Vectors, Molecular Sequence Data, Biophysics, Genome, Viral, Biology, medicine.disease_cause, Kidney, Transfection, Virus Replication, Biochemistry, law.invention, Adenoviridae, Cell Line, law, medicine, Humans, Amino Acid Sequence, Molecular Biology, Gene, Recombination, Genetic, Mutation, Base Sequence, Genetic Variation, Cell Biology, Virology, Viral replication, Cell culture, Recombinant DNA, Capsid Proteins

Abstract

In infected cells, replication errors during viral proliferation generate mutations in adenoviruses (Ads), and the mutant Ads proliferate and evolve in the intracellular environment. Genetically fiber-modified recombinant Ads (rAd variants) were generated, by modification of the fiber gene, for therapeutic applications in host cells that lack or express reduced levels of the Coxsackievirus and adenovirus receptor. To assess the genetic modifications of rAd variants that might induce the instability of Ad virions, we examined the frequencies of mutants that accumulated in propagated stocks. Seven of 41 lines of Ad variants generated mutants in the stocks and all mutants were infectious. Moreover, all the mutations occurred in the modified region that had been added at the 3' end of the fiber gene. Our results show that some genetic modifications at the carboxyl terminus of Ad fiber protein lead to the instability of Ad virions.

Published

2005

26. A simple method for the simultaneous detection of E1A and E1B in adenovirus stocks

Author

Sanae Watanabe, Takahito Yamazaki, Hideyo Ugai, Erika Suzuki, Jianzhi Pan, Takehide Murata, Megumi Hirose, Yukari Kujime, and Kazunari K. Yokoyama

Subjects

Cancer Research, viruses, Biology, medicine.disease_cause, Virus Replication, Polymerase Chain Reaction, Virus, law.invention, Adenoviridae, Cell Line, chemistry.chemical_compound, law, medicine, Humans, Adenovirus E1B Proteins, Polymerase chain reaction, DNA Primers, Electrophoresis, Agar Gel, Recombination, Genetic, General Medicine, Virology, Molecular biology, Staining, Oncology, chemistry, DNA, Viral, Recombinant DNA, Agarose, Adenovirus E1A Proteins, Ethidium bromide, HeLa Cells

Abstract

Recombinant adenoviral vectors have been developed for use as therapeutic agents and for the introduction of exogenous genes into living cells. However, the occurrence of replication-competent adenoviruses (RCA) in adenovirus stocks produced in 293 cells remains a major problem in terms of the safe use of such vectors. To overcome the problems associated with the occurrence of RCA, we have established a simple method for the simultaneous detection of amplified E1A and E1B from RCA that might contaminate adenoviral stocks. The products amplified by polymerase chain reaction (PCR) were fractionated by regular electrophoresis on agarose gels and visualized by staining with ethidium bromide. This method is rapid and inexpensive for detection of RCA in the preparation of adenoviruses.

Published

2003

27. Generation of cloned calves and transgenic chimeric embryos from bovine embryonic stem-like cells

Author

Ken Sawai, Akira Minamihashi, Takehide Murata, Hideyo Ugai, Shigeo Saito, Yoshiro Kobayashi, Yusuke Yamamoto, Hiroki Hirayama, Yuichi Obata, Kazunari K. Yokoyama, Satoru Moriyasu, Soichi Kageyama, and Jianzhi Pan

Subjects

KOSR, Cellular differentiation, medicine.medical_treatment, Cloning, Organism, Basic fibroblast growth factor, Green Fluorescent Proteins, Molecular Sequence Data, Biophysics, Biology, Oct-4, Biochemistry, Animals, Genetically Modified, chemistry.chemical_compound, Epidermal growth factor, medicine, Animals, Transgenes, Molecular Biology, Cell Nucleus, Platelet-Derived Growth Factor, Epidermal Growth Factor, Reverse Transcriptase Polymerase Chain Reaction, Growth factor, Stem Cells, Cell Differentiation, Cell Biology, Embryo, Mammalian, Embryonic stem cell, Molecular biology, Luminescent Proteins, Blastocyst, chemistry, Gene Expression Regulation, Cattle, Fibroblast Growth Factor 2, Stem cell, Cell Division, Signal Transduction

Abstract

Bovine embryonic stem-like cells (ES-like cells) appear to maintain a normal diploid karyotype indefinitely during culture in vitro and to express marker proteins that are characteristic of ES cells from mice, namely, alkaline phosphatase (AP), stage-specific embryonic antigen-1 (SSEA-1), STAT-3, and Oct 4. After proliferation of undifferentiated ES-like cells in vitro, some bovine ES-like cells differentiated to neural precursor cells, which were cultured in the presence of basic fibroblast growth factor (bFGF), epidermal growth factor (EGF), and platelet-derived growth factor (PDGF). In addition, calves were successfully cloned using ES-like cells and the frequency of term pregnancies for blastocysts derived from ES-like cells was higher than those of early pregnancies and maintained pregnancies after nuclear transplantation (NT) with bovine somatic cells. Successful cloning from bovine ES-like cells should allow the introduction into cattle of specific genetic characteristics of biomedical and/or agricultural importance.

Published

2003

28. K-562 cells lack MHC class II expression due to an alternatively spliced CIITA transcript with a truncated coding region

Author

Hideyo Ugai, Noel E. Day, Kazunari K. Yokoyama, and A. T. Ichiki

Subjects

Cancer Research, Genes, MHC Class II, Molecular Sequence Data, chemical and pharmacologic phenomena, Major histocompatibility complex, Interferon-gamma, CIITA, Coding region, Humans, Amino Acid Sequence, RNA, Messenger, Promoter Regions, Genetic, Gene, Genetics, MHC class II, Messenger RNA, biology, Alternative splicing, Histocompatibility Antigens Class II, Nuclear Proteins, Hematology, Stop codon, Cell biology, Alternative Splicing, Oncology, biology.protein, Codon, Terminator, DNA Transposable Elements, Trans-Activators, K562 Cells

Abstract

The focus of this study was to determine the functional capacity of class II transactivator (CIITA), a regulatory factor of major histocompatibility complex (MHC) class II genes, in K-562 cells. We show that CIITA mRNA is present in K-562 cells and the interferon-gamma (IFN-gamma)-inducible CIITA promoter-IV exhibits low levels of basal activity, which is greatly enhanced upon treatment with IFN-gamma. Further study revealed that the CIITA cDNA contains an insertion of genomic sequence, which introduces a stop codon. The truncated coding region of the CIITA transcript in K-562 cells provides a possible explanation for the absence of MHC class II molecules.

Published

2003

29. Transcriptional regulation by zinc-finger proteins Sp1 and MAZ involves interactions with the same cis-elements (Review)

Author

Hideyo Ugai, Hatsumi Nakata-Tsutsui, Shotaro Kishikawa, Erika Suzuki, Takehide Murata, Kazunari K. Yokoyama, and Jun Song

Subjects

Regulation of gene expression, Zinc finger, Histone, biology, Regulatory sequence, Genetics, biology.protein, Transcriptional regulation, Promoter, General Medicine, DNA-binding protein, Molecular biology, Transcription factor

Abstract

Various transcription factors, such as Sp1 and MAZ, include C2H2-type zinc-finger motifs and are able to bind to GC-rich cis-elements that are distributed in the promoter regions of numerous mammalian genes. The consensus sequence of Sp1-binding sites is very similar to that of MAZ-binding sites. In fact, Sp1 and MAZ bind to the same cis-elements in the promoters of the genes for the receptor for serotonin 1A (HT1Ar), endothelial nitric-oxide synthase (eNOS), phenylethanolamine N-methyltransferase (PNMT), the receptor for parathyroid hormone (PTHr), MAZ and the major late promoter of adenovirus (AdMLP). It appears that two consecutive zinc-finger motifs of Sp1 and MAZ might be essential for the interaction of each protein with DNA. Sp1 and MAZ activated the expression of the genes for HT1Ar and PTHr, as well as AdMLP. Both Sp1 and MAZ inhibited the expression of the gene for MAZ, while expression of the gene for eNOS was enhanced by Sp1 and repressed by MAZ. These observations suggest that both Sp1 and MAZ might have dual functions in the regulation of gene expression. Our results suggest, furthermore, that histone deacetylases are involved in autorepression of the gene for MAZ, while expression of DNA methyltransferase I is associated with suppression of the expression of the gene for MAZ by Sp1. Thus, both deacetylation and methylation might be involved in the regulation of expression of individual genes, with different zinc-finger proteins binding to the same cis-elements but recruiting different proteins, such as methylases and acetylases, to the transcriptional complex.

Published

2003

30. Physical and genetic map of the Bacteroides fragilis YCH46 chromosome

Author

Tomomi Kuwahara, Haruyuki Nakayama, Syed Mohammed Shaheduzzaman, Mahfuzur R. Sarker, Hideyo Ugai, Yoshinari Ohnishi, Tsuyoshi Miki, and Shigeru Akimoto

Subjects

Genetics, Gel electrophoresis, Chromosome, Biology, Chromosomes, Bacterial, biology.organism_classification, Physical Chromosome Mapping, Microbiology, Molecular biology, Genome, Bacteroides fragilis, Pulsed-field gel electrophoresis, Humans, Restriction digest, RRNA Operon, Deoxyribonucleases, Type II Site-Specific, Molecular Biology, Gene

Abstract

The chromosome of Bacteroides fragilis strain YCH46 was shown to be a single circular DNA molecule of about 5.3 Mb having 16 NotI, seven AscI, and six I-CeuI sites. A physical map of the chromosome was constructed by four independent experimental approaches: linking clone analysis, cross-Southern hybridization, partial restriction digestion, and two-dimensional pulsed-field gel electrophoresis. Six rRNA operons and 10 known genes were localized on the physical map.

Published

2002

31. The coactivators p300 and CBP have different functions during the differentiation of F9 cells

Author

Hiroaki Kawasaki, Kiyoshi Uchida, Hideyo Ugai, and Kazunari K. Yokoyama

Subjects

Cellular differentiation, Response element, Molecular Sequence Data, Biology, environment and public health, Transactivation, Mice, Transcription (biology), Drug Discovery, Gene expression, Tumor Cells, Cultured, Animals, CREB-binding protein, Phosphorylation, Genetics (clinical), Regulation of gene expression, Base Sequence, Nuclear Proteins, Promoter, Cell Differentiation, Molecular biology, CREB-Binding Protein, Gene Expression Regulation, biology.protein, Trans-Activators, Molecular Medicine, E1A-Associated p300 Protein, Cell Division

Abstract

We have characterized an element (differentiation response element, DRE) in the promoter region of the c-jun gene that is both necessary and sufficient for retinoic acid (RA) and adenovirus early region (E1A) mediated up-regulation of c-jun gene expression during the differentiation of F9 cells. The DRF complex, which binds specifically to DRE, is composed of the E1A-associated protein p300 and the activation transcription factor-2 (ATF-2) as a DNA-binding subunit of the DRF. The molecular association of p300 and ATF-2 enhances the transcription of the c-jun gene, which requires protein kinase C alpha mediated phosphorylation of Ser-121 of ATF-2 within its p300 interaction domain. We used antisense oligodeoxynucleotides (AS-ODNs) capable of binding specifically to the mRNA for either p300 or CBP to examine the individual roles of p300 and CBP during the RA-induced differentiation, exit from the cell cycle, and apoptosis of F9 cells. F9 cells treated with AS-ODNs specific for p300 mRNA became resistant to RA-induced differentiation, while cells incubated with AS-ODNs specific for CBP mRNA were still able to differentiate. Despite their similarities p300 and CBP appear to have distinct functions during the differentiation of F9 cells. These results suggest that ATF-2 and p300 cooperate in the control of transcription by forming a protein complex in response to RA or E1A, and that the phosphorylation of ATF-2 and p300 is probably a signaling event in the pathway that leads to the transactivation of the c-jun gene in F9 cell differentiation.

Published

1999

32. p300 and ATF-2 are components of the DRF complex, which regulates retinoic acid- and E1A-mediated transcription of the c-jun gene in F9 cells

Author

Kazunari K. Yokoyama, Hiroaki Kawasaki, Jun Song, Hideyo Ugai, Robert Chiu, Nic Jones, Yang Shi, Kazunari Taira, and Richard Eckner

Subjects

Transcriptional Activation, Protein Kinase C-alpha, Genes, Viral, Transcription, Genetic, Cellular differentiation, viruses, Recombinant Fusion Proteins, Response element, Retinoic acid, Tretinoin, Transfection, environment and public health, Cell Line, Transactivation, chemistry.chemical_compound, Mice, Genes, jun, Genetics, Animals, Phosphorylation, Cyclic AMP Response Element-Binding Protein, Promoter Regions, Genetic, Transcription factor, Protein Kinase C, Regulation of gene expression, biology, Activating Transcription Factor 2, c-jun, Nuclear Proteins, Cell Differentiation, Molecular biology, Activating transcription factor 2, Isoenzymes, chemistry, Gene Expression Regulation, biology.protein, Trans-Activators, E1A-Associated p300 Protein, Developmental Biology, Transcription Factors, Research Paper

Abstract

Transcriptional activation of the c-jun gene is a critical event in the differentiation of F9 cells. In our previous studies we characterized an element [differentiation response element (DRE)] in the c-jun promoter that is both necessary and sufficient to confer the capacity for differentiation-dependent up-regulation. This element binds the differentiation regulatory factor (DRF) complex, of which one component is the adenovirus E1A-associated protein p300. We have now identified activation transcription factor-2 (ATF-2) as a DNA-binding subunit of the DRF complex. p300 and ATF-2 interact with each other in vivo and in vitro. The bromodomain and the C/H2 domain of p300 mediate the binding to ATF-2, which in turn requires a proline-rich region between amino acids 112 and 350 for its interaction with p300. The phosphorylation of the serine residue at position 121 of ATF-2 appears to be induced by protein kinase Cα (PKCα) after treatment of cells with retinoic acid (RA) or induction with E1A. In cotransfection assays, wild-type ATF-2 enhanced the transcription of an E2/tk–luciferase construct, in conjunction with p300–E2. However, a mutant form of ATF-2 with a mutation at position 121 (pCMVATF–2Ser121–Ala) did not. These results suggest that ATF-2 and p300 cooperate in the control of transcription by forming a protein complex that is responsive to differentiation-inducing signals, such as RA or E1A, and moreover, that the phosphorylation of ATF-2 by PKCα is probably a signaling event in the pathway that leads to the transactivation of the c-jun gene in F9 cells.

Published

1998

33. Detection of Bacteroides fragilis by PCR assay targeting the neuraminidase-encoding gene

Author

Shigeru Akimoto, Tomomi Kuwahara, Yoshinari Ohnishi, Hideyo Ugai, Takemi Kinouchi, and T. Kamogashira

Subjects

DNA, Bacterial, Molecular Sequence Data, Neuraminidase, Applied Microbiology and Biotechnology, Polymerase Chain Reaction, Sensitivity and Specificity, Microbiology, law.invention, Bacteroides fragilis, chemistry.chemical_compound, Species Specificity, law, Gene, Bacteroidaceae, Polymerase chain reaction, DNA Primers, biology, Base Sequence, biology.organism_classification, Molecular biology, chemistry, Genes, Bacterial, biology.protein, Nested polymerase chain reaction, Bacteria, DNA

Abstract

Oligonucleotide primers were designed on the basis of the sequence of the neuraminidase-encoding gene (nanH) of Bacteroides fragilis and used for the specific detection of this anaerobe by the nested PCR assay. Fifty-nine of 60 representative strains of Bact. fragilis were detected, while none of 45 strains of other species generated visible PCR products. The detection limits of Bact. fragilis cells and DNA by the nested PCR were 10 colony-forming units and 10 fg of chromosomal DNA, respectively. The PCR assay targeting the nanH gene has the potential for the detection of Bact. fragilis.

Published

1996

34. Control elements of Dnmt1 gene are regulated in cell-cycle dependent manner

Author

Takehide Murata, Hideyo Ugai, Takahito Yamazaki, Kazunari K. Yokoyama, and Shotaro Kishikawa

Subjects

DNA (Cytosine-5-)-Methyltransferase 1, DNA Replication, Sp1 Transcription Factor, Blotting, Western, DNMT3A Gene, Hydroxamic Acids, environment and public health, Histones, Sp3 transcription factor, DNA (Cytosine-5-)-Methyltransferases, Promoter Regions, Genetic, Gene, biology, urogenital system, Cell Cycle, Nuclear Proteins, Acetylation, General Medicine, DNA Methylation, Precipitin Tests, Molecular biology, Chromatin, DNA-Binding Proteins, Sp3 Transcription Factor, Histone, Gene Expression Regulation, embryonic structures, DNA methylation, Trans-Activators, biology.protein, Histone deacetylase, Chromatin immunoprecipitation, Transcription Factors

Abstract

The Dnmt1 gene is constitutively expressed and is required for the maintenance of global methylation after DNA replication. We investigated here the effects of histone deacetylase (HDAC) inhibitor and DNA demetylation agent on promoter activity of mouse Dnmt1 gene in somatic cells. The promoter activity of Dnmt1 gene was increased approximately 2-fold in the treatment of cells by Tricostatin A (TSA) at 1 x 10(-8) M, as compared with that without treatment of TSA. By contrast, treatment with 5-azacytidne (5aza-C) did not affect the promoter activity of the Dnmt1 gene. This result indicates the Dnmt1 gene is possibly regulated by histone acetylation. We also examined the expression levels of Dnmt1 gene and of its control elements like Sp1, Sp3 and p300 by the chromatin immunoprecipitation and Western blot analysis. The expression of Dnmt1 gene is observed at early S phase. Sp1 is recruited mainly at the G1 phase and Sp3 is recruited at the early S phase. p300 is also obviously recruited at the second S phase. These data indicated that the regulators of Dnmt1 gene were controlled in cell-cycle dependent manner.

Published

2003

35. Transcriptional regulation of the c-jun gene by AP-1 repressor protein JDP2 during the differentiation of F9 cells

Author

Takehide Murata, Hongjie Li, Hideyo Ugai, Chunyuan Jin, and Kazunari K. Yokoyama

Subjects

Regulation of gene expression, Transcription, Genetic, biology, YY1, Chemistry, Cellular differentiation, Response element, Cell Differentiation, Electrophoretic Mobility Shift Assay, General Medicine, Cell biology, Repressor Proteins, Transcription Factor AP-1, Mice, Transactivation, Gene Expression Regulation, Genes, jun, GATAD2B, Tumor Cells, Cultured, Jun dimerization protein, biology.protein, Animals, Regulator gene

Abstract

ATF-2 and p300 cooperate in the activation of transcription of the c-jun gene during the differentiation of F9 cells. We show here that a repressor of AP-1, JDP2 (Jun dimerization protein 2), inhibits the transactivation of the c-jun gene by ATF-2 and p300, by recruitment of a histone deacetylase complex, thereby repressing the retinoic acid (RA)-induced transcription of the c-jun gene and inhibiting the RA-mediated differentiation of F9 cells. Furthermore, JDP2/HDAC complex was replaced by p300 complex on the DRE (differentiation response element) of the c-jun promoter within 24 h after the start of exposure of cells to RA, with an accompanying change in the histone-acetylation status of the chromatin, indicating that the initiation of transcription of the c-jun gene was controled by sequential action of HDAC(s) and HAT(s) on c-jun promoter.

Published

2002

36. Roles of histone acetylation in the Dnmtl gene expression

Author

Shotaro Kishikawa, Kazunari K. Yokoyama, Takehide Murata, and Hideyo Ugai

Subjects

Regulation of gene expression, Trichostatin A, Epigenetics of physical exercise, Histone methyltransferase, DNA methylation, Histone methylation, medicine, General Medicine, Cancer epigenetics, Biology, Molecular biology, Epigenomics, medicine.drug

Abstract

The DNA methylation plays a key role in the regulation of gene expression, genotnic imprinting and X chromosome inactivation and has been shown to be essential for mammalian development. The Dnmtl is one of the DNA methyltransferases that catalyzed DNA methylation on CpG dinucleotides. The Dnmtl is constitutively expressed and is required for the maintenance of global methylation after DNA replication. In this study, we investigated the effects of histone deacetylase (HDAC) inhibitor and DNA demethylation agent on promoter activity of mouse Dnmtl gene in somatic cells. The promoter activity of Dnmtl gene was increased approximately 2-fold in the treatment of cells by Trichostatin A (TSA) at lx 10"* M, as compared with that without of treatment of TSA. By contrast, treatment with 5-azacytidine (5aza-C) did not affect the promoter activity of the Dnmtl gene. These results indicate that the Dnmtl gene is possibly to regulated by histone acetylation.

Published

2002

37. Recombinant Virus Bank for Gene Delivery

Author

Kazunari K. Yokoyama, Takehide Murata, Yukari Kujime, Kumiko Inabe, Sanae Inamoto, Megumi Hirose, Erika Suzuki, Takahito Yamasaki, Miho Terashima, and Hideyo Ugai

Subjects

Recombination, Genetic, Multidisciplinary, Japan, Genetic enhancement, Genetic Vectors, Viruses, Gene delivery, Biology, Recombinant virus, Virology, Gene, Biological Specimen Banks, Viral vector

Abstract

Viral vectors have been developed as therapeutic agents for the introduction of exogenous genes into living cells ([1][1]), and clinical trials of gene therapy and the use of viral vectors in the laboratory have been reported with increasing frequency during the past decade ([2][2]–[4][3]). We

Published

2005

38. An adenoviral vector expressing human adenovirus 5 and 3 fiber proteins for targeting heterogeneous cell populations

Author

Miho Murakami, Paul B. Fisher, Hideyo Ugai, Natalya Belousova, Minghui Wang, Maaike Everts, Joel N. Glasgow, Paul Dent, and David T. Curiel

Subjects

Recombinant Fusion Proteins, Cell, Population, Genetic Vectors, CHO Cells, Biology, Viral vector, 03 medical and health sciences, Transduction (genetics), 0302 clinical medicine, Cricetulus, Transduction, Genetic, Virology, Cell Line, Tumor, Cricetinae, medicine, Animals, Humans, Adenovirus, Fiber, education, Receptor, Tropism, 030304 developmental biology, 0303 health sciences, education.field_of_study, Tumor, Chinese hamster ovary cell, Adenoviruses, Human, virus diseases, Tropism expansion, eye diseases, 3. Good health, Viral Tropism, medicine.anatomical_structure, Cell culture, 030220 oncology & carcinogenesis, Receptors, Virus, Capsid Proteins, Mosaic

Abstract

Human adenovirus serotype 5 (HAdV-5) attaches to its primary receptor, the coxsackie and adenovirus receptor (CAR) as the first step of infection. However, CAR expression decreases as tumors progress, thereby diminishing the utility of HAdV-5-based vectors for cancer therapy. In contrast, many aggressive tumor cells highly express CD46, a cellular receptor for HAdV-3. We hypothesized that a mosaic HAdV vector, containing two kinds of fiber proteins, would provide extensive transduction in a heterogeneous population of tumor cells with varying expression levels of HAdV receptors. We therefore generated a fiber-mosaic HAdV vector displaying both a chimeric HAdV-3 fiber and the HAdV-5 fiber protein. We verified the structural integrity of purified viral particles and confirmed that the fiber-mosaic HAdV vector has expanded tropism. We conclude that the use of fiber-mosaic HAdV vectors is a promising approach for transducing a heterogeneous cell population with different expression levels of adenovirus receptors.

39. Evaluation of adenovirus capsid labeling versus transgene expression

Author

Robert A. Oster, Jing Li, Priyanka Uprety, Aiman Fatima, Justin C. Roth, Svetlana Komarova, Qiana L. Matthews, Hideyo Ugai, Minghui Wang, and David T. Curiel

Subjects

Recombinant Fusion Proteins, Transgene, Genetic enhancement, viruses, Short Report, Biology, medicine.disease_cause, Adenoviridae, lcsh:Infectious and parasitic diseases, law.invention, 03 medical and health sciences, 0302 clinical medicine, Genes, Reporter, law, Virology, medicine, Humans, lcsh:RC109-216, Luciferase, Transgenes, Luciferases, Molecular Biology, 030304 developmental biology, 0303 health sciences, Staining and Labeling, Adenovirus genome, Suicide gene, Recombinant Proteins, Infectious Diseases, Capsid, 030220 oncology & carcinogenesis, Recombinant DNA, Capsid Proteins

Abstract

Adenoviral vectors have been utilized for a variety of gene therapy applications. Our group has incorporated bioluminescent, fluorographic reporters, and/or suicide genes within the adenovirus genome for analytical and/or therapeutic purposes. These molecules have also been incorporated as capsid components. Recognizing that incorporations at either locale yield potential advantages and disadvantages, our report evaluates the benefits of transgene incorporation versus capsid incorporation. To this end, we have genetically incorporated firefly luciferase within the early region 3 or at minor capsid protein IX and compared vector functionality by means of reporter readout.