Your search keyword '"Mie Kobayashi-Ishihara"' showing total 7 results

1. Introduction of Human Flt3-L and GM-CSF into Humanized Mice Enhances the Reconstitution and Maturation of Myeloid Dendritic Cells and the Development of Foxp3+CD4+ T Cells

Author

Ryutaro Iwabuchi, Shota Ikeno, Mie Kobayashi-Ishihara, Haruko Takeyama, Manabu Ato, Yasuko Tsunetsugu-Yokota, and Kazutaka Terahara

Subjects

lcsh:Immunologic diseases. Allergy, 0301 basic medicine, Myeloid, Immunology, T cells, 03 medical and health sciences, 0302 clinical medicine, medicine, Immunology and Allergy, dendritic cells, Flt3-L, CD86, CD40, biology, Chemistry, GM-CSF, hemic and immune systems, Dendritic cell, Molecular biology, cytokines, Haematopoiesis, humanized mice, 030104 developmental biology, medicine.anatomical_structure, Humanized mouse, biology.protein, Stem cell, lcsh:RC581-607, CD80, 030215 immunology

Abstract

Two cytokines, fms-related tyrosine kinase 3 ligand (Flt3-L) and granulocyte-macrophage colony-stimulating factor (GM-CSF) are considered to be the essential regulators of dendritic cell (DC) development in vivo. However, the combined effect of Flt3-L and GM-CSF on human DCs has not been evaluated in vivo. In this study, we, therefore, aimed at evaluating this using a humanized mouse model. Humanized non-obese diabetic/SCID/Jak3null (hNOJ) mice were constructed by transplanting hematopoietic stem cells from human umbilical cord blood into newborn NOJ mice, and in vivo transfection (IVT) was performed by hydrodynamic injection-mediated gene delivery using plasmids encoding human Flt3-L and GM-CSF. Following IVT, Flt3-L and GM-CSF were successfully induced in hNOJ mice. At 10 days post-IVT, we found, in the spleen, that treatment with both Flt3-L and GM-CSF enhanced the reconstitution of two myeloid DC subsets, CD14−CD1c+ conventional DCs (cDCs) and CD14−CD141+ cDCs, in addition to CD14+ monocyte-like cells expressing CD1c and/or CD141. GM-CSF alone had less effect on the reconstitution of these myeloid cell populations. By contrast, none of the cytokine treatments enhanced CD123+ plasmacytoid DC (pDC) reconstitution. Regardless of the reconstitution levels, three cell populations (CD1c+ myeloid cells, CD141+ myeloid cells, and pDCs) could be matured by treatment with cytokines, in terms of upregulation of CD40, CD80, CD86, and CD184/CXCR4 and downregulation of CD195/CCR5. In particular, GM-CSF contributed to upregulation of CD80 in all these cell populations. Interestingly, we further observed that Foxp3+ cells within splenic CD4+ T cells were significantly increased in the presence of GM-CSF. Foxp3+ T cells could be subdivided into two subpopulations, CD45RA−Foxp3hi and CD45RA−Foxp3lo T cells. Whereas CD45RA−Foxp3hi T cells were increased only after treatment with GM-CSF alone, CD45RA−Foxp3lo T cells were increased only after treatment with both Flt3-L and GM-CSF. Treatment with Flt3-L alone had no effect on the number of Foxp3+ T cells. The correlation analysis demonstrated that the development of these Foxp3+ subpopulations was associated with the maturation status of DC(-like) cells. Taken together, this study provides a platform for studying the in vivo effect of Flt3-L and GM-CSF on human DCs and regulatory T cells.

Published

2018

2. HIV LTR-Driven Antisense RNA by Itself Has Regulatory Function and May Curtail Virus Reactivation From Latency

Author

Mie Kobayashi-Ishihara, Kazutaka Terahara, Javier P. Martinez, Makoto Yamagishi, Ryutaro Iwabuchi, Christian Brander, Manabu Ato, Toshiki Watanabe, Andreas Meyerhans, and Yasuko Tsunetsugu-Yokota

Subjects

0301 basic medicine, Microbiology (medical), reactivation, latency reversing agents, lcsh:QR1-502, Biology, Microbiology, lcsh:Microbiology, Virus, law.invention, 03 medical and health sciences, Transcription (biology), law, Sense (molecular biology), latency, Original Research, Reporter gene, Wild type, virus diseases, HIV, Provirus, Virology, Antisense RNA, 030104 developmental biology, Suppressor, viral antisense RNA

Abstract

Latently infected T lymphocytes are an important barrier toward eliminating a persistent HIV infection. Here we describe an HIV-based recombinant fluorescent-lentivirus referred to as “rfl-HIV” that enables to analyze sense and antisense transcription by means of fluorescence reporter genes. This model virus exhibited similar transcriptional and functional properties of the antisense transcript as observed with a wild type HIV, and largely facilitated the generation of latently-infected T cells clones. We show that latently-infected cells can be divided into two types, those with and those without antisense transcription. Upon addition of latency reversal agents, only the cells that lack antisense transcripts are readily reactivated to transcribe HIV. Thus, antisense transcripts may exhibit a dominant suppressor activity and can lock an integrated provirus into a non-reactivatable state. These findings could have important implications for the development of strategies to eradicate HIV from infected individuals. This work was supported by grants from Japan Society for the Promotion of Science (JSPS KAKENHI #15H06877 for MK-I, #JP17K08800 for KT), ViiV Healthcare Japan Research Grant 2015 (MK-I), Grants-in-Aid from the Ministry of Health, Labour and Welfare (H24-AIDS-008 to YT-Y) and Japan Agency for Medical Research and Development (AMED #JP17fk0410305h0103 to YT-Y and #JP18fk0410003 to KT). MK-I received Fellowships from Japan Foundation for AIDS Prevention and JSPS Oversea Research Fellow Program. AM and JM were supported by a grant from the Spanish Ministry of Economy, Industry and Competitiveness and FEDER grant no. SAF2016-75505-R (AEI/MINEICO/FEDER, UE) and through the “María de Maeztu” Program for Units of Excellence in R&D (MDM-2014-0370).

Published

2018

3. Humanized mice dually challenged with R5 and X4 HIV-1 show preferential R5 viremia and restricted X4 infection of CCR5+CD4+ T cells

Author

Seiji Okada, Manabu Ato, Yasuko Tsunetsugu-Yokota, Mie Kobayashi-Ishihara, Shota Ikeno, Kazutaka Terahara, and Masayuki Ishige

Subjects

CD4-Positive T-Lymphocytes, Receptors, CXCR4, Receptors, CCR5, Immunology, Cell, Human immunodeficiency virus (HIV), Viremia, Biology, Virus Replication, medicine.disease_cause, Microbiology, Immunodeficiency virus, Green fluorescent protein, Mice, In vivo, medicine, Animals, virus diseases, Persistent viremia, medicine.disease, Virology, Infectious Diseases, medicine.anatomical_structure, HIV-1, Early phase

Abstract

CCR5-tropic (R5) immunodeficiency virus type 1 (HIV-1) strains are highly transmissible during the early stage of infection in humans, whereas CXCR4-tropic (X4) strains are less transmissible. This study aimed to explore the basis for early phase R5 and X4 HIV-1 infection in vivo by using humanized mice dually challenged with R5 HIV-1NLAD8-D harboring DsRed and X4 HIV-1(NL-E) harboring EGFP. Whereas R5 HIV-1 replicated well, X4 HIV-1 caused only transient viremia with variable kinetics; however, this was distinct from the low level but persistent viremia observed in mice challenged with X4 HIV-1 alone. Flow cytometric analysis of HIV-1-infected cells revealed that X4 HIV-1 infection of CCR5(+)CD4(+) T cells was significantly suppressed in the presence of R5 HIV-1. X4 HIV-1 was more cytopathic than R5 HIV-1; however, this was not the cause of restricted X4 HIV-1 infection because there were no significant differences in the mortality rates of CCR5(+) and CCR5(-) cells within the X4 HIV-1-infected cell populations. Taken together, these results suggest that restricted infection of CCR5(+)CD4(+) T cells by X4 HIV-1 (occurring via a still-to-be-identified mechanism) might contribute to the preferential transmission of R5 HIV-1 during the early phase of infection.

Published

2015

4. Development of a sensitive novel diagnostic kit for the highly pathogenic avian influenza A (H5N1) virus

Author

Yasuko Tsunetsugu-Yokota, Hang L.K. Nguyen, Kazuo Ohnishi, Mai T.Q. Le, Giang T. Dang, Kengo Nishimura, Long T. Nguyen, Shigeyuki Itamura, Mie Kobayashi-Ishihara, Shuhei Misawa, Hitoshi Takahashi, Ikuyo Takayama, Tsutomu Kageyama, and Masato Tashiro

Subjects

Monoclonal antibody, medicine.medical_specialty, medicine.drug_class, viruses, Hemagglutinin (influenza), Clinical specimens, medicine.disease_cause, Sensitivity and Specificity, Virus, Rapid influenza diagnosis, Immunoenzyme Techniques, Medical microbiology, Influenza, Human, Pandemic, medicine, Humans, H5 hemagglutinin, Influenza A Virus, H5N1 Subtype, medicine.diagnostic_test, biology, business.industry, Highly pathogenic avian influenza virus, virus diseases, Virology, Influenza A virus subtype H5N1, Infectious Diseases, Vietnam, Parasitology, Immunoassay, biology.protein, Pharynx, Reagent Kits, Diagnostic, business, Research Article

Abstract

Background Sporadic emergence of the highly pathogenic avian influenza (HPAI) H5N1 virus infection in humans is a serious concern because of the potential for a pandemic. Conventional or quantitative RT-PCR is the standard laboratory test to detect viral influenza infections. However, this technology requires well-equipped laboratories and highly trained personnel. A rapid, sensitive, and specific alternative screening method is needed. Methods By a luminescence-linked enzyme immunoassay, we have developed a H5N1 HPAI virus detection kit using anti-H5 hemagglutinin monoclonal antibodies in combination with the detection of a universal NP antigen of the type A influenza virus. The process takes 15 minutes by use of the fully automated luminescence analyzer, POCube. Resutls We tested this H5/A kit using 19 clinical specimens from 13 patients stored in Vietnam who were infected with clade 1.1 or clade 2.3.4 H5N1 HPAI virus. Approximately 80% of clinical specimens were H5-positive using the POCube system, whereas only 10% of the H5-positive samples were detected as influenza A-positive by an immunochromatography-based rapid diagnostic kit. Conclusions This novel H5/A kit using POCube is served as a rapid and sensitive screening test for H5N1 HPAI virus infection in humans.

Published

2014

5. Broad Cross-Reactive Epitopes of the H5N1 Influenza Virus Identified by Murine Antibodies against the A/Vietnam/1194/2004 Hemagglutinin

Author

Tsutomu Kageyama, Kazuo Ohnishi, Hitoshi Takahashi, Yasuko Tsunetsugu-Yokota, Mie Kobayashi-Ishihara, Kengo Nishimura, Shigeyuki Itamura, Kazutaka Terahara, and Manabu Ato

Subjects

Viral Diseases, medicine.drug_class, Immunology, Hemagglutinin (influenza), lcsh:Medicine, Enzyme-Linked Immunosorbent Assay, Hemagglutinin Glycoproteins, Influenza Virus, Cross Reactions, Monoclonal antibody, medicine.disease_cause, Microbiology, Epitope, Virus, Epitopes, Mice, Diagnostic Medicine, Virology, Emerging Viral Diseases, Influenza, Human, medicine, Influenza A virus, Medicine and Health Sciences, Animals, Humans, lcsh:Science, Multidisciplinary, biology, Influenza A Virus, H5N1 Subtype, lcsh:R, Biology and Life Sciences, Antibodies, Monoclonal, Influenza A virus subtype H5N1, Clinical Laboratory Sciences, Influenza, Viral Disease Diagnosis, Epitope mapping, Infectious Diseases, biology.protein, lcsh:Q, Clinical Immunology, Antibody, Epitope Mapping, Research Article

Abstract

There is an urgent need for a rapid diagnostic system to detect the H5 subtype of the influenza A virus. We previously developed monoclonal antibodies (mAbs) against the H5 hemagglutinin (HA) for use in a rapid diagnostic kit. In this study, we determined the epitopes of the anti-H5 HA murine mAbs OM-b, AY-2C2, and YH-1A1. Binding assays of the mAbs to different strains of H5 HAs indicated that OM-b and AY-2C2 cross-reacted with HAs from clades 1, 2.1.3.2, 2.2, and 2.3.4, whereas YH-1A1 failed to bind to those of clades 2.1.3.2 and 2.3.4. HA chimeras revealed that the epitopes for each of the mAbs were in the HA1 region. Analysis of escape mutants revealed that OM-b and AY-2C2 mAbs interacted mainly with amino acid residues D43 and G46, and the YH-1A1 mAb interacted with G139 and K or R140 of H5 HA. Multiple alignments of H5 HA protein sequences showed that D43 and G46 were very conserved among H5N1 HAs, except those in clade 2.2.1 and clade 7 (88.7%). The epitope for YH-1A1 mAb was highly variable in the HAs of H5N1, although it was well conserved in those of H5N2-N9. The OM-b and AY-2C2 mAbs could bind to the HAs of clades 1.1 and 2.3.2.1 that are currently epidemic in Asia, and we conclude that these would be effective for the detection of H5N1 infections in this region.

Published

2014

6. Epigenetic heterogeneity in HIV-1 latency establishment

Author

Mie Kobayashi-Ishihara, Yuka Matsuda, Takaomi Ishida, Makoto Yamagishi, Toshiki Watanabe, and Dai Fujikawa

Subjects

Chromatin Immunoprecipitation, Methylation, Hiv 1 latency, Virus, Article, Epigenesis, Genetic, Histones, Jurkat Cells, Transcription (biology), Genes, Reporter, Gene silencing, Humans, Epigenetics, RNA, Small Interfering, Genetics, Multidisciplinary, biology, Polycomb Repressive Complex 2, Virus Latency, Histone, HEK293 Cells, biology.protein, HIV-1, RNA Interference, Early phase, PRC2

Abstract

Despite prolonged antiretroviral therapy, HIV-1 persists as transcriptionally inactive proviruses. The HIV-1 latency remains a principal obstacle in curing AIDS. It is important to understand mechanisms by which HIV-1 latency is established to make the latent reservoir smaller. We present a molecular characterization of distinct populations at an early phase of infection. We developed an original dual-color reporter virus to monitor LTR kinetics from establishment to maintenance stage. We found that there are two ways of latency establishment i.e., by immediate silencing and slow inactivation from active infection. Histone covalent modifications, particularly polycomb repressive complex 2 (PRC2)-mediated H3K27 trimethylation, appeared to dominate viral transcription at the early phase. PRC2 also contributes to time-dependent LTR dormancy in the chronic phase of the infection. Significant differences in sensitivity against several stimuli were observed between these two distinct populations. These results will expand our understanding of heterogeneous establishment of HIV-1 latency populations.

Published

2014

7. HIV-1-encoded antisense RNA suppresses viral replication for a prolonged period

Author

Tadanori Yamochi, Mie Kobayashi-Ishihara, Yuka Matsuda, Takaomi Ishida, Ryutaro Takahashi, Kazumi Nakano, Toshiki Watanabe, Takuma Hara, Ariko Miyake, and Makoto Yamagishi

Subjects

Gene Expression Regulation, Viral, lcsh:Immunologic diseases. Allergy, Time Factors, HIV Infections, Biology, Transfection, Virus Replication, Proviruses, Genes, Reporter, Transcription (biology), RNA interference, Virology, Gene expression, Sense (molecular biology), Humans, RNA, Antisense, RNA, Messenger, Promoter Regions, Genetic, HIV Long Terminal Repeat, Cell Nucleus, Research, NF-kappa B, RNA, Reverse Transcription, Molecular biology, Antisense RNA, Antisense Orientation, HEK293 Cells, Infectious Diseases, Viral replication, Mutation, HIV-1, Leukocytes, Mononuclear, Nucleic Acid Conformation, RNA, Viral, RNA Interference, lcsh:RC581-607, Plasmids

Abstract

Background Recent evidence proposes a novel concept that mammalian natural antisense RNAs play important roles in cellular homeostasis by regulating the expression of several genes. Identification and characterization of retroviral antisense RNA would provide new insights into mechanisms of replication and pathogenesis. HIV-1 encoded-antisense RNAs have been reported, although their structures and functions remain to be studied. We have tried to identify and characterize antisense RNAs of HIV-1 and their function in viral infection. Results Characterization of transcripts of HEK293T cells that were transiently transfected with an expression plasmid with HIV-1NL4–3 DNA in the antisense orientation showed that various antisense transcripts can be expressed. By screening and characterizing antisense RNAs in HIV-1NL4–3-infected cells, we defined the primary structure of a major form of HIV-1 antisense RNAs, which corresponds to a variant of previously reported ASP mRNA. This 2.6 kb RNA was transcribed from the U3 region of the 3′ LTR and terminated at the env region in acutely or chronically infected cell lines and acutely infected human peripheral blood mononuclear cells. Reporter assays clearly demonstrated that the HIV-1 LTR harbours promoter activity in the reverse orientation. Mutation analyses suggested the involvement of NF-κΒ binding sites in the regulation of antisense transcription. The antisense RNA was localized in the nuclei of the infected cells. The expression of this antisense RNA suppressed HIV-1 replication for more than one month. Furthermore, the specific knockdown of this antisense RNA enhanced HIV-1 gene expression and replication. Conclusions The results of the present study identified an accurate structure of the major form of antisense RNAs expressed from the HIV-1NL4–3 provirus and demonstrated its nuclear localization. Functional studies collectively demonstrated a new role of the antisense RNA in viral replication. Thus, we suggest a novel viral mechanism that self-limits HIV-1 replication and provides new insight into the viral life cycle.

Published

2012