Your search keyword '"Aida, Y."' showing total 20 results

1. Convenient method for better preservation of fine structures of cultured macrophages and engulfed yeast cells by freeze-substitution fixation.

Author

Yamaguchi M, Takahashi-Nakaguchi A, Aida Y, Sato-Okamoto M, and Chibana H

Subjects

Animals, Cell Line, Fixatives, Glutaral, Macrophages microbiology, Macrophages physiology, Macrophages ultrastructure, Mice, Microscopy, Electron, Transmission, Phagocytosis, Candida ultrastructure, Cryopreservation methods, Freeze Substitution methods, Macrophages cytology, Saccharomyces cerevisiae ultrastructure, Tissue Fixation methods

Abstract

Rapid freeze-freeze substitution after glutaraldehyde fixation (CF-FS method) obtained the natural and fine structures of macrophages and engulfed yeast cells. Culturing macrophages on single hole molybdenum grids placed in culture dishes made possible the rapid freezing of cells by the 'open sandwich method'. This method may be convenient when rapid-freezing cannot be performed immediately, or when a rapid-freezing device is not available in the lab., (© The Author 2017. Published by Oxford University Press on behalf of The Japanese Society of Microscopy. All rights reserved. For permissions, please e-mail: journals.permissions@oup.com.)

Published

2017

2. The role of macrophage transcription factor MafB in atherosclerotic plaque stability.

Author

Hasegawa H, Watanabe T, Kato S, Toshima T, Yokoyama M, Aida Y, Nishiwaki M, Kadowaki S, Narumi T, Honda Y, Otaki Y, Honda S, Shunsuke N, Funayama A, Nishiyama S, Takahashi H, Arimoto T, Shishido T, Miyamoto T, Abe S, Shibata Y, and Kubota I

Subjects

Animals, Atherosclerosis pathology, Cell Differentiation, Cell Nucleus metabolism, Female, Inflammation, Interleukin-6 metabolism, MafB Transcription Factor genetics, MafB Transcription Factor physiology, Male, Mice, Mice, Inbred C57BL, Mice, Knockout, ApoE, Mice, Transgenic, RAW 264.7 Cells, Tumor Necrosis Factor-alpha metabolism, Apoptosis, Macrophages metabolism, Matrix Metalloproteinase 9 metabolism, Oxidative Stress, Plaque, Atherosclerotic metabolism

Abstract

Background and Aims: Macrophage differentiation is associated with the development of atherosclerosis and plaque vulnerability and is regulated by transcription factor MafB. We previously reported that MafB attenuates macrophage apoptosis, which is associated with atherosclerotic plaque instability. The aim of this study was to elucidate the role of MafB in the progression of atherosclerotic plaque., Methods: We generated macrophage-specific dominant-negative (DN) MafB transgenic mice and intercrossed DN-MafB mice with apolipoprotein E (ApoE) knockout (KO) mice., Results: There was no significant difference in advanced atherosclerotic lesion area between DN-MafB/ApoE KO mice and littermate control ApoE KO mice 9 weeks after high-cholesterol diet. However, DN-MafB/ApoE KO mice showed significantly larger necrotic cores and lower collagen content in atherosclerotic plaques than ApoE KO mice. Although there was no difference in intraplaque macrophage infiltration and efferocytosis, DN-MafB/ApoE KO mice showed significantly more apoptotic macrophages at the plaque edges than did ApoE KO mice. Real-time PCR analysis revealed that peritoneal macrophages of DN-MafB/ApoE KO mice had a greater increase in matrix metalloproteinase-9 and mRNA expression of inflammatory/M1 macrophage markers (tissue necrosis factor-α, interleukin-6, CD11c, and p47phox) after lipopolysaccharide stimulation than those of ApoE KO mice., Conclusion: Macrophage-specific inhibition of MafB may destabilize atherosclerotic plaques in advanced lesions., (Copyright © 2016 Elsevier Ireland Ltd. All rights reserved.)

Published

2016

3. Synthesis of a Vpr-Binding Derivative for Use as a Novel HIV-1 Inhibitor.

Author

Hagiwara K, Ishii H, Murakami T, Takeshima SN, Chutiwitoonchai N, Kodama EN, Kawaji K, Kondoh Y, Honda K, Osada H, Tsunetsugu-Yokota Y, Suzuki M, and Aida Y

Subjects

Anti-HIV Agents pharmacology, Cells, Cultured, HIV Infections virology, Humans, Macrophages virology, Anti-HIV Agents chemical synthesis, HIV Infections prevention & control, HIV-1 drug effects, Hematoxylin chemistry, Macrophages drug effects, Virus Replication drug effects, vpr Gene Products, Human Immunodeficiency Virus metabolism

Abstract

The emergence of multidrug-resistant viruses compromises the efficacy of anti-human immunodeficiency virus type 1 (HIV-1) therapy and limits treatment options. Therefore, new targets that can be used to develop novel antiviral agents need to be identified. We previously identified a potential parent compound, hematoxylin, which suppresses the nuclear import of HIV-1 via the Vpr-importin α interaction and inhibits HIV-1 replication in a Vpr-dependent manner by blocking nuclear import of the pre-integration complex. However, it was unstable. Here, we synthesized a stable derivative of hematoxylin that bound specifically and stably to Vpr and inhibited HIV-1 replication in macrophages. Furthermore, like hematoxylin, the derivative inhibited nuclear import of Vpr in an in vitro nuclear import assay, but had no effect on Vpr-induced G2/M phase cell cycle arrest or caspase activity. Interestingly, this derivative bound strongly to amino acid residues 54-74 within the C-terminal α-helical domain (αH3) of Vpr. These residues are highly conserved among different HIV strains, indicating that this region is a potential target for drug-resistant HIV-1 infection. Thus, we succeeded in developing a stable hematoxylin derivative that bound directly to Vpr, suggesting that specific inhibitors of the interaction between cells and viral accessory proteins may provide a new strategy for the treatment of HIV-1 infection.

Published

2015

4. HIV-1 Vpr induces interferon-stimulated genes in human monocyte-derived macrophages.

Author

Zahoor MA, Xue G, Sato H, Murakami T, Takeshima SN, and Aida Y

Subjects

Cells, Cultured, Dependovirus physiology, HEK293 Cells, HeLa Cells, Humans, Immunity, Innate, Interferon Regulatory Factor-7 genetics, Interferon Regulatory Factor-7 metabolism, Interferons pharmacology, Macrophages drug effects, Macrophages metabolism, Phosphorylation, STAT1 Transcription Factor genetics, STAT1 Transcription Factor metabolism, vpr Gene Products, Human Immunodeficiency Virus genetics, Dependovirus genetics, Gene Expression Profiling methods, Gene Expression Regulation drug effects, Macrophages virology, Oligonucleotide Array Sequence Analysis methods, vpr Gene Products, Human Immunodeficiency Virus metabolism

Abstract

Macrophages act as reservoirs of human immunodeficiency virus type 1 (HIV-1) and play an important role in its transmission to other cells. HIV-1 Vpr is a multi-functional protein involved in HIV-1 replication and pathogenesis; however, its exact role in HIV-1-infected human macrophages remains poorly understood. In this study, we used a microarray approach to explore the effects of HIV-1 Vpr on the transcriptional profile of human monocyte-derived macrophages (MDMs). More than 500 genes, mainly those involved in the innate immune response, the type I interferon pathway, cytokine production, and signal transduction, were differentially regulated (fold change >2.0) after infection with a recombinant adenovirus expressing HIV-1 Vpr protein. The differential expression profiles of select interferon-stimulated genes (ISGs) and genes involved in the innate immune response, including STAT1, IRF7, MX1, MX2, ISG15, ISG20, IFIT1, IFIT2, IFIT3, IFI27, IFI44L, APOBEC3A, DDX58 (RIG-I), TNFSF10 (TRAIL), and RSAD2 (viperin) were confirmed by real-time quantitative PCR and were consistent with the microarray data. In addition, at the post-translational level, HIV-1 Vpr induced the phosphorylation of STAT1 at tyrosine 701 in human MDMs. These results demonstrate that HIV-1 Vpr leads to the induction of ISGs and expand the current understanding of the function of Vpr and its role in HIV-1 immune pathogenesis.

Published

2014

5. Identification of a novel Vpr-binding compound that inhibits HIV-1 multiplication in macrophages by chemical array.

Author

Hagiwara K, Murakami T, Xue G, Shimizu Y, Takeda E, Hashimoto Y, Honda K, Kondoh Y, Osada H, Tsunetsugu-Yokota Y, and Aida Y

Subjects

Animals, Anti-HIV Agents chemistry, Anti-HIV Agents pharmacology, COS Cells, Chlorocebus aethiops, HIV-1 physiology, HeLa Cells, High-Throughput Screening Assays, Humans, vpr Gene Products, Human Immunodeficiency Virus antagonists & inhibitors, Anti-HIV Agents isolation & purification, HIV-1 drug effects, Macrophages virology, Virus Replication drug effects, vpr Gene Products, Human Immunodeficiency Virus chemistry

Abstract

Although HIV-1 replication can be controlled by highly active anti-retroviral therapy (HAART) using protease and reverse transcriptase inhibitors, the development of multidrug-resistant viruses compromises the efficacy of HAART. Thus, it is necessary to develop new drugs with novel targets. To identify new anti-HIV-1 compounds, recombinant Vpr was purified from transfected COS-7 cells and used to screen compounds by chemical array to identify those that bound Vpr. From this screen, 108 compounds were selected as positive for Vpr binding. Among these, one structurally similar group of four compounds showed anti-HIV activity in macrophages. In particular, compound SIP-1 had high inhibition activity and reduced the levels of p24 by more than 98% in macrophages after 8 or 12 days of infection. SIP-1 had no cytotoxic effects and did not disrupt cell cycle progression or induce apoptosis of Molt-4 and HeLa cell lines as measured by MTT assay, flow-cytometry analysis, and a caspase-3 assay. In addition, SIP-1 specifically bound to Vpr as assessed by photo-cross-linked small-molecule affinity beads. These results suggest that Vpr is a good target for the development of compounds that could potentially inhibit HIV-1 replication. Collectively, our results strongly suggest that chemical array is a useful method for screening anti-viral compounds., (Copyright © 2010 Elsevier Inc. All rights reserved.)

Published

2010

6. Novel nuclear import of Vpr promoted by importin alpha is crucial for human immunodeficiency virus type 1 replication in macrophages.

Author

Nitahara-Kasahara Y, Kamata M, Yamamoto T, Zhang X, Miyamoto Y, Muneta K, Iijima S, Yoneda Y, Tsunetsugu-Yokota Y, and Aida Y

Subjects

Animals, COS Cells, Cell Nucleus metabolism, Chlorocebus aethiops, Cytoplasm metabolism, Gene Expression, HeLa Cells, Humans, Immunoblotting, Microscopy, Confocal, Protein Binding, Protein Isoforms biosynthesis, RNA, Messenger biosynthesis, Reverse Transcriptase Polymerase Chain Reaction, alpha Karyopherins biosynthesis, vpr Gene Products, Human Immunodeficiency Virus, Active Transport, Cell Nucleus, Gene Products, vpr metabolism, HIV-1 physiology, Macrophages virology, Virus Replication, alpha Karyopherins metabolism

Abstract

Monocytes/macrophages are major targets of human immunodeficiency virus type 1 (HIV-1) infection. The viral preintegration complex (PIC) of HIV-1 enters the nuclei of monocyte-derived macrophages, but very little PIC migrates into the nuclei of immature monocytes. Vpr, one of the accessory gene products of HIV-1, is essential for the nuclear import of PIC in these cells, although the role of Vpr in the entry mechanism of PIC remains to be clarified. We have shown previously that Vpr is targeted to the nuclear envelope and then transported into the nucleus by importin alpha alone, in an importin beta-independent manner. Here we demonstrate that the nuclear import of Vpr is strongly promoted by the addition of cytoplasmic extract from macrophages but not of that from monocytes and that the nuclear import activity is lost with immunodepletion of importin alpha from the cytoplasmic extract. Immunoblot analysis and real-time PCR demonstrate that immature monocytes express importin alpha at low levels, whereas the expression of three major importin alpha isoforms markedly increases upon their differentiation into macrophages, indicating that the expression of importin alpha is required for nuclear import of Vpr. Furthermore, interaction between importin alpha and the N-terminal alpha-helical domain of Vpr is indispensable, not only for the nuclear import of Vpr but also for HIV-1 replication in macrophages. This study suggests the possibility that the binding of Vpr to importin alpha, preceding a novel nuclear import process, is a potential target for therapeutic intervention.

Published

2007

7. 1-Hydroxyethylidene-1,1-bisphosphonate decreases the postovariectomy enhanced interleukin 1 secretion from peritoneal macrophages in adult rats.

Author

Matsuda T, Matsui K, Shimakoshi Y, Aida Y, and Hukuda S

Subjects

Analysis of Variance, Animals, Cells, Cultured, Female, Lipopolysaccharides, Macrophages metabolism, Peritoneum, Rats, Rats, Inbred Strains, Etidronic Acid pharmacology, Interleukin-1 metabolism, Macrophages drug effects, Ovariectomy

Abstract

Bisphosphonates are potent inhibitors of bone resorption. In previous studies, we have shown that ovariectomy accelerates bone resorption and 1-hydroxyethylidene-1, 1-bisphosphonate (HEBP) inhibits ovariectomy-accelerated bone resorption in female Wistar adult rats. As interleukin 1 (IL-1) stimulates bone resorption in vitro and in vivo, we have investigated the effects of ovariectomy and HEBP administered in vivo on IL-1 secretion from peritoneal macrophages in adult rats. Ovariectomy or sham surgery were performed in female Wistar rats at 40 weeks of age. Ovariectomized and sham-operated rats were administered with HEBP (10 mg) or saline, 10 times in total, from 43 to 46 weeks of age. Paraffin oil-induced peritoneal macrophages at 46 weeks of age were cultured for 24 hours. Lipopolysaccharide (LPS)-stimulated peritoneal macrophages from ovariectomized rats secreted more IL-1 than sham-operated rats. HEBP decreased LPS-stimulated IL-1 secretion from peritoneal macrophages in ovariectomized rats, but not in sham-operated rats. In vivo administration of HEBP decreased IL-1 secretion only in postovariectomy hyperresorptive states. These results suggest that alterations in LPS-stimulated IL-1 secretion from oil-induced peritoneal macrophages may be responsible, at least in part, for the postovariectomy acceleration in bone resorption and its inhibition by HEBP.

Published

1991

8. Down-regulation of Fc receptor expression in guinea pig peritoneal exudate macrophages by muramyl dipeptide or lipopolysaccharide.

Author

Yagawa K, Kaku M, Ichinose Y, Nagao S, Tanaka A, Aida Y, and Tomoda A

Subjects

Animals, Antibodies, Monoclonal, Antigen-Antibody Complex metabolism, Antigen-Antibody Complex physiology, Binding Sites, Antibody drug effects, Guinea Pigs, Immunoglobulin G metabolism, Insulin metabolism, Kinetics, Lectins metabolism, Macrophage Migration-Inhibitory Factors physiology, Mice, Mice, Inbred BALB C, Receptors, Fc analysis, Receptors, IgG, Superoxides metabolism, Wheat Germ Agglutinins, Acetylmuramyl-Alanyl-Isoglutamine pharmacology, Immunosuppressive Agents pharmacology, Lipopolysaccharides pharmacology, Macrophages metabolism, Receptors, Fc drug effects

Abstract

Expression of Fc receptors on the plasma membrane of guinea pig peritoneal exudate macrophages (PEM) was suppressed to almost one-half of that of the controls by long-term exposure to lipopolysaccharide (LPS) or muramyl dipeptide (MDP) in culture. The effect of the reagents was dose and time dependent, and as little as 0.5 ng/ml LPS or 5 ng/ml MDP was effective for the suppression. The expression of the Fc receptors decreased to 60 to 70% of the control level at 48 hr and to 45 to 50% at 72 hr after incubation of the cells in the presence of LPS or MDP. A Scatchard plot of the binding of 125I-soluble immune complexes (I.C.) to the cells revealed that the decrease in the binding of 125I-I.C. is due to a reduction in the number of Fc receptors on the cell membrane and not to a decreased affinity of the receptors. The membrane protein was radio-labeled with 125I, and the Fc receptors were purified by being bound to insoluble I.C. The specific binding of the 125I-labeled Fc receptors, from the LPS-treated macrophages, to the insoluble I.C. was almost one-half of that from the untreated control cells. SDS-PAGE analysis of the purified 125I-labeled Fc receptors revealed that the major peak of the m.w. 44,000 molecule in the LPS-treated cells was almost one-half of that of the control. Contrary to the effect of LPS or MDP, 72-hr incubation of macrophages with MIF-rich supernatant, cultured from lymph node cells, enhanced the expression of Fc receptors. Macrophages were treated with I.C. for 4 hr at 37 degrees C to remove the Fc receptors from the surface membrane. The reappearance of the receptors on the plasma membrane of the cells was significantly suppressed by LPS and MDP. The effect of LPS on the binding of five murine monoclonal antibodies (Ab) raised against PEM to the macrophage membrane and also that of 125I-wheat germ agglutinin (WGA) or 125I-insulin was studied. The monoclonal Ab were selected for their activity to induce superoxide anion generation in the macrophages, as do I.C., although the binding sites for the monoclonal Ab were not related to Fc receptors. The bindings of the five monoclonal Ab were not affected by exposure of the cells to LPS or MDP. Macrophages treated with the reagents bound as much 125I-insulin or WGA as did the untreated control cells.(ABSTRACT TRUNCATED AT 400 WORDS)

Published

1985

9. Triggering of the superoxide generation of macrophages by crosslinking of Fc gamma receptor.

Author

Aida Y and Onoue K

Subjects

Animals, Antigen-Antibody Complex analysis, Cross-Linking Reagents, Guinea Pigs, Kinetics, Receptors, IgG, Immunoglobulin G metabolism, Macrophages immunology, Receptors, Fc metabolism, Superoxides metabolism

Abstract

Crosslinking of monomeric IgG2 molecules bound to the Fc gamma receptors on the cell surface of guinea pig macrophages generated the triggering signal for the superoxide-generating system. A binding experiment indicated that macrophages have saturable binding sites for monomeric IgG2. Scatchard analysis of the binding data showed that macrophages have an average of 4 X 10(5) binding sites per cell and the association constant for the binding was 4.2 X 10(6) M-1. Binding of monomeric IgG2 to macrophages could be detected by subsequent reaction with the 125I-labeled F(ab')2 fragment of rabbit antibody specific for guinea pig Fab. Although binding of IgG2 monomer to Fc receptor did not stimulate superoxide release, further addition of the F(ab')2 fragment of anti-guinea pig Fab antibody did induce generation and release of superoxide, and the amount released was dependent on the dose of cell-bound IgG2. When macrophages were bound with a constant dose of IgG2 monomer in the first step, the superoxide release triggered by the addition of the F(ab')2 of anti-guinea pig Fab was dependent on the dose of the F(ab')2 fragment added. These results show that crosslinking of Fc receptors triggers the superoxide generation.

Published

1984

10. Structural studies of Fc receptors. V. Effect of phospholipase C treatment on the binding activities of the Fc receptor of macrophage or its isolated plasma membrane.

Author

Aida Y, Itonaga M, and Onoue K

Subjects

Animals, Bacillus cereus enzymology, Cell Membrane immunology, Clostridium perfringens enzymology, Guinea Pigs, Kinetics, Macrophages drug effects, Membrane Lipids analysis, Phospholipids analysis, Receptors, Fc drug effects, Macrophages immunology, Phospholipases pharmacology, Receptors, Fc metabolism, Type C Phospholipases pharmacology

Abstract

The effect of phospholipase C treatment on the binding activity of the Fc receptor of guinea pig macrophage was studied to analyze the interaction of the Fc receptor with membrane phospholipids necessary for the activity. It was confirmed by subcellular fractionation that the receptor is localized on the plasma membrane. Treatment of the whole cell or isolated plasma membrane with phospholipase C of Clostridium perfringens diminished the binding of soluble IgG2-immune complex to Fc receptors on the cell or membrane. On the other hand, phospholipase C of Bacillus cereus did not affect the activity when it acted on the whole cell but it did diminish the activity when it acted on the isolated plasma membrane. Analysis of the phospholipids of untreated and treated macrophages or plasma membrane showed that phosphatidylcholine molecules, particularly those located in the membrane (not accessible to attack from the cell surface by phospholipase C of B. cereus), appear to be crucial for efficient interaction of macrophage Fc receptors with immune complex. Ligand-binding experiments with macrophages showed that the diminished binding activity was due to a decrease of the avidity for immune complex, but did not seem to be due to a decrease in the number or affinity of Fc receptors for monomeric IgG2. Taken together with the previous results which demonstrated that Fc receptors which had apparently lost the activity due to delipidation could be reconstituted with phosphatidylcholine but not with most other phospholipids, the results seem to indicate that the diminution of the binding activity to the immune complex of macrophage or its plasma membrane caused by phospholipase C treatment is due to the impairment of multivalent interaction between Fc receptor molecules on the membrane and IgG2 molecules in the immune complex, probably as a result of the loss of interaction of the head groups of phospholipids with Fc receptor molecules and the change in membrane properties resulting from the increase of diglycerides.

Published

1984

11. Muramyl dipeptide induced augmentation of the proliferative response of thymocytes to phytohemagglutinin.

Author

Aida Y, Aono M, and Onoue K

Subjects

Animals, Centrifugation, Density Gradient, Chromatography, Gel, Guinea Pigs, Acetylmuramyl-Alanyl-Isoglutamine pharmacology, Lymphocyte Activation drug effects, Macrophages immunology, Phytohemagglutinins pharmacology, T-Lymphocytes immunology

Abstract

N-Acetylmuramyl-L-alanyl-D-isoglutamine (MDP) augmented the proliferative response of thymocytes to phytohemagglutinin (PHA). The augmenting effect of MDP disappeared by passage of glass-nonadherent thymocytes through Sephadex G-10 (G-10) column or by removal of low density cells by the Ficoll-Conray gradient centrifugation. The diminished augmenting effects of MDP on the proliferative response of glass-nonadherent-G-10 nonadherent thymocytes was restored by the addition of the G-10 adherent cells. When G-10 adherent cell fraction was extensively depleted of macrophages by glass adherence and EA-rosetting, it was found that neither the macrophage-depleted G-10 adherent cell fraction nor the macrophage fraction supported by itself the proliferative response of G-10 nonadherent thymocytes. However, addition of macrophage fraction together with the macrophage-depleted G-10 adherent cells did support the proliferation of G-10 nonadherent thymocytes. It was further shown that peritoneal exudate macrophages could be substituted for thymic macrophage fraction. These results suggested that both the G-10 adherent-glass nonadherent cells and macrophages were essential for the MDP-induced augmentation of the proliferative response of thymocytes to PHA and these cells exerted different accessory roles in this response.

Published

1987

12. Effects of disodium ethane-1-hydroxy-1,1-diphosphonate (EHDP) on interleukin 1 production by macrophages.

Author

Aida Y, Toda Y, Shimakoshi Y, Yamada K, and Aono M

Subjects

Acetylmuramyl-Alanyl-Isoglutamine pharmacology, Animals, Calcimycin pharmacology, Cell Adhesion drug effects, Guinea Pigs, Lipopolysaccharides pharmacology, Macrophages drug effects, Superoxides metabolism, Tetradecanoylphorbol Acetate pharmacology, Etidronic Acid pharmacology, Interleukin-1 biosynthesis, Macrophages metabolism

Abstract

The effects of disodium ethane-1-hydroxy-1,1-diphosphonate (EHDP) on the in vitro functions of guinea pig macrophages were studied. A high dose (1 mg/ml) of EHDP inhibited interleukin 1 (IL 1) production by oil-induced peritoneal macrophages stimulated with muramyl dipeptide (MDP), lipopolysaccharide (LPS), phorbol myristic acetate (PMA), heat-aggregated IgG2 or calcium ionophore A23187. On the other hand, low doses (less than 0.125 mg/ml) of EHDP augmented the MDP induced IL 1 production by macrophages. This biphasic effect was also observed when macrophages were exposed to EHDP at 37 C for 24 hr and then stimulated with IL 1 inducers. Superoxide anion generation induced by formyl peptide or PMA was not affected by preincubation of the macrophages with doses of EHDP up to 1 mg/ml. Adherence and spreading of macrophages was inhibited by EHDP in a dose dependent manner without affecting cell viability. These results demonstrated that EHDP acted on macrophages directly and modulated IL 1 production in vitro.

Published

1986

13. Structural studies of fc receptors. II. The effect of dissociation and reassociation of phospholipids on the activity of Fc gamma receptors of macrophages.

Author

Aida Y and Onoue K

Subjects

Animals, Chemical Phenomena, Chemistry, Chromatography, Gel, Detergents, Guinea Pigs, In Vitro Techniques, Receptors, IgG, Solubility, Macrophages metabolism, Phospholipids pharmacology, Receptors, Fc metabolism, Receptors, Immunologic metabolism

Abstract

The receptor for the Fc portion of immunoglobulin G (Fc receptor) of guinea pig macrophages was solubilized with a detergent and partially delipidated to the point where the ligand binding activity was essentially lost. Delipidation of the Fc receptor was done by fractionating the macrophage lysate by gel filtration in the presence of detergent. The elution behavior of Fc receptor-detergent complex and phospholipid-detergent mixed micelles varied depending on the kind of detergents used for membrane solubilization and for gel filtration. Separation of phospholipids from Fc receptor was best achieved when octylglucoside-solubilized fraction was chromatographed on Sepharose CL-6B in the presence of deoxycholate; the phospholipid peak emerged at Kav = 0.55 and the Fc receptor at Kav = 0.45. The fraction of Kav = 0.45 showed only a marginal activity when the activity was measured after removal of detergents, but activity was clearly shown when phospholipid fraction was added to this fraction prior to removal of the detergents. Reappearance of the Fc receptor activity was shown to be due to association of phospholipids with the Fc receptor. Three kinds of phospholipids with different polar head groups examined, phosphatidylcholine, phosphatidylserine, and phosphatidylethanolamine, were all able to reconstitute active Fc receptor, although phosphatidylethanolamine was somewhat less effective than the others. Thus, our study demonstrated the amphipathic nature of the Fc receptor, the binding of which is dependent on the interaction with phospholipids.

Published

1983

14. Structural studies of Fc receptors. IV. Structure required for phospholipids for reconstitution of the delipidated Fc receptor of macrophages.

Author

Itonaga M, Aida Y, and Onoue K

Subjects

Animals, Cell Fractionation, Cell Membrane immunology, Guinea Pigs, Molecular Weight, Receptors, Fc isolation & purification, Type C Phospholipases pharmacology, Macrophages immunology, Membrane Lipids physiology, Phospholipids physiology, Receptors, Fc metabolism

Abstract

To analyze the interaction of the macrophage Fc receptor with phospholipids, we established an experimental system for delipidation of Fc receptor fraction and reconstitution of the Fc receptor activity in phospholipid vesicles. The separation of FcR from membrane phospholipids was achieved by ion exchange chromatography on DEAE-cellulose of the anionic detergent-lysate of the crude membrane fraction of guinea pig macrophages in the presence of detergent. The separation was based on the difference in charge between the complex of FcR and the anionic detergent and that of phospholipids and the detergent. The FcR fraction free of phospholipids showed no FcR activity as assessed in terms of its ability to inhibit the binding of labeled soluble immune complex of IgG2 antibody to macrophages, but the same fraction showed a definite activity when associated with phospholipids. This fraction was shown to contain a component of 44,000 daltons that is susceptible to surface-labeling and binds to IgG2-Sepharose in the affinity chromatography, indicating this component to be the Fc receptor. Reconstitution experiments with this fraction showed that phosphatidylcholine is the most effective phospholipid to reconstitute the FcR activity among those tested. Phosphatidylserine, phosphatidylinositol, and sphingomyelin were ineffective, while phosphatidylethanolamine showed a moderate effect. The inactivating effect of phospholipase C treatment on the Fc receptor activity of the membrane was shown to be due to the cleavage of phospholipids in the membrane but not due to modification of the Fc receptor molecule itself.

Published

1984

15. Structural studies of Fc receptors. III. Isolation and molecular weight analysis of the component chain of Fc gamma receptor of macrophage.

Author

Aida Y and Onoue K

Subjects

Animals, Chromatography, Affinity methods, Electrophoresis, Polyacrylamide Gel, Guinea Pigs, Immunoglobulin G, Macromolecular Substances, Molecular Weight, Receptors, IgG, Macrophages immunology, Receptors, Fc isolation & purification

Abstract

Surface receptors of guinea pig peritoneal macrophages specific for the Fc region of IgG (Fc gamma receptor) were isolated and identified as a surface-radioiodinated component with a molecular weight of 44,000 that bound in an Fc-specific manner to IgG2 of guinea pig immunoglobulin immobilized in any of the following three different ways: IgG2 antibody in insoluble immune complex, IgG2 antibody bound to antigen-coupled Sepharose, and IgG2 covalently coupled to Sepharose. In order to obtain the Fc gamma receptor retaining the binding activity, the Fc-binding component was isolated by IgG2 affinity chromatography in which mild acidic buffer (pH 5.0-4.0) was chosen to elute the component bound to the affinity column. Forty-five to sixty-two percent of the eluted radioactivity was shown to rebind to the IgG2-affinity column. The bound fraction showed a single radioactive peak of 44,000 daltons in sodium dodecyl sulfate-polyacrylamide gel electrophoresis. The Fc-binding component isolated by the affinity chromatography behaved similarly in gel filtration in the presence of a detergent, as did the detergent-solubilized Fc gamma receptor before isolation by affinity chromatography. These results suggested that the Fc gamma receptor was isolated in a native form. Furthermore, it was confirmed that the isolated Fc gamma receptor is distinct from actin or the actin-like protein (DNase I-binding protein) which had been reported to bind to IgG-affinity column.

Published

1984

16. Fc receptor-mediated desensitization of superoxide (O2-) generation response of guinea-pig macrophages and polymorphonuclear leucocytes.

Author

Yagawa K, Kaku M, Ichinose Y, Aida Y, and Tomoda A

Subjects

Animals, Antigen-Antibody Complex immunology, Dose-Response Relationship, Immunologic, Guinea Pigs, Lectins immunology, Macrophages immunology, Neutrophils immunology, Time Factors, Wheat Germ Agglutinins, Macrophage Activation, Macrophages metabolism, Neutrophils metabolism, Receptors, Fc immunology, Superoxides metabolism

Abstract

Guinea-pig macrophages were pretreated with soluble immune complexes (1 hr, at 37 degrees). By this procedure, the capacity of the cells to produce superoxide anions (O2-) upon stimulation with wheatgerm agglutinin (WGA) was inhibited by as much as 80% (desensitization). However, the receptors for WGA were still available on the cell surfaces as determined by the binding of 125I-labelled WGA to both the pretreated and control cells. This inhibition of O2- generation was also observed when opsonized zymosan (Op-zymosan) was used as the stimulus for O2- generation. In contrast, the inhibition by soluble immune complexes was less than 25% of the control levels when the desensitized cells were stimulated with N-formyl-L-methionyl-L-leucyl-L-phenylalanine (fMLP) or phorbol myristate acetate (PMA). The same procedure was also used to desensitize guinea-pig polymorphonuclear leucocytes (PMN). In this case, the O2- generation of the PMN was suppressed to 50-55% of the control level when WGA or fMLP was used as stimulus. However, the PMA-induced O2- generation was far less affected by this treatment, as was the case with the macrophages. The activity of the desensitized macrophages for O2- generation recovered gradually to a normal level 24 hr after removal of the immune complexes from the medium. These results suggest that (i) some regulatory mechanisms which suppress the activation of NADPH oxidase are accentuated by prolonged exposure of guinea-pig macrophages and PMN with soluble immune complexes; (ii) the mechanism for O2- generation mediated by WGA or Op-zymosan may be different from that for O2- generation mediated by PMA, and (iii) the mechanism for O2- generation mediated by fMLP differs between macrophages and PMN.

Published

1985

17. Characterization of three monoclonal antibodies which induce and modulate superoxide anion generation in guinea pig macrophages.

Author

Yagawa K, Kaku M, Ichinose Y, Aida Y, and Tomoda A

Subjects

Adenylyl Cyclases metabolism, Animals, Antigen-Antibody Complex physiology, Binding Sites, Antibody, Female, Guinea Pigs, Macrophages enzymology, Macrophages immunology, Mice, Mice, Inbred BALB C, Receptors, Fc analysis, Time Factors, Antibodies, Monoclonal physiology, Macrophage Activation, Macrophages metabolism, Superoxides metabolism

Abstract

Three monoclonal antibodies (Ab), termed KY 12, KY 22, and KY 25 and raised against guinea pig macrophages, induced superoxide anion (O2-) generation in the cells. Although each monoclonal Ab bound to macrophages, each had a different pattern of binding to other cell types. In response to each of the Ab, the amount of O2- generated by 5 X 10(5) macrophages was between 0.5 and 0.7 nmol/min and was augmented threefold to fivefold by the addition of F(ab')2 fragments of rabbit Abs to mouse Ig. When macrophages were pretreated with soluble immune complexes (I.C.) prior to stimulation by the monoclonal Ab, the O2- generation stimulated by KY 12 or KY 22 was reduced by more than 70%. In contrast, pretreatment of macrophages with I.C. did not reduce O2- generation in response to KY 25. KY 12 and KY 22 stimulated adenyl cyclase activity in macrophages, but KY 25 did not. Pretreatment of the cells with soluble I.C. did not interfere with the enhancing effect of the monoclonal Ab on adenyl cyclase activity. Pretreatment of macrophages with KY 12 reduced by over 60% of subsequent generation of O2- in response to wheat germ agglutinin, I.C., formyl-methionyl-leucyl-phenylalanine, phorbol myristate acetate, KY 22, or KY 25. KY 22 or KY 25 did not suppress the generation of O2- in response to other stimuli. These results suggest that KY 22 and KY 25 activate O2- generation in a manner that differs from that of KY 12. These monoclonal Ab should prove useful in examining the regulation of O2- production.

Published

1985

18. Structural studies of Fc receptors. I. Binding properties, solubilization, and partial characterization of fc receptors of macrophages.

Author

Yagawa K, Onoue K, and Aida Y

Subjects

Animals, Antigen-Antibody Complex, Chromatography, Gel, Dose-Response Relationship, Immunologic, Guinea Pigs, Hydrogen-Ion Concentration, Macrophages enzymology, Phospholipases pharmacology, Rabbits, Solubility, Sonication, Binding Sites, Antibody, Immunoglobulin Fc Fragments, Macrophages immunology

Published

1979

19. Fc receptor-mediated desensitization of superoxide (O2-) generation response of guinea-pig macrophages and polymorphonuclear leucocytes.

Author

Yagawa, K., Kaku, M., Ichinose, Y., Aida, Y., and Tomoda, A.

Subjects

SUPEROXIDES, NEUTROPHILS, MACROPHAGES, GUINEA pigs, ANTIGEN presenting cells, GRANULOCYTES

Abstract

Guinea-pig macrophages were pretreated with soluble immune complexes (1 hr, at 37°). By this procedure, the capacity of the cells to produce superoxide anions (O2-) upon stimulation with wheatgerm agglutinin (WGA) was inhibited by as much as 80% (desensitization). However, the receptors for WGA were still available on the cell surfaces as determined by the binding of 125I-labelled WGA to both the pretreated and control cells. This inhibition of O2- generation was also observed when opsonized zymosan (Op-zymosan) was used as the stimulus for O2- generation. In contrast, the inhibition by soluble immune complexes was less than 25% of the control levels when the desensitized cells were stimulated with N-formyl-L-methionyl-L-leucyl- L-phenylalanine (fMLP) or phorbol myristate acetate (PMA). The same procedure was also used to desensitize guinea-pig polymorphonuclear leucocytes (PMA). In this case, the O2- generation of the PMN was suppressed to 50-55% of the control level when WGA or fMLP was used as stimulus. However, the PMA- induced O2- generation was far less affected by this treatment, as was the case with the macrophages. The activity of the densensitized macrophages for O2- generation recovered gradually to a normal level 24 hr after removal of the immune complexes from the medium. These results suggest that (i) some regulatory mechanisms which suppress the activation of NADPH oxidase are accentuated by prolonged exposure of guinea-pig macrophages and PMN with soluble immune complexes; (ii) the mechanism for O2- generation mediated by WGA or Op-zymosan may be different from that for O2- generation mediated by PMA, and (iii) the mechanism for Or generation mediated by fMLP differs between macrophages and PMN. [ABSTRACT FROM AUTHOR]

Published

1985

20. Thymic Accessory Cells Required for the Increased Responsiveness of Thymocyte Subpopulations to Interleukin 1--Like Monokine in Guinea Pigs.

Author

Aida, Y., Kakimoto, K., Kawakami, K., Chiba, J., Aono, M., and Onoue, K.

Subjects

ANTIGEN presenting cells, GUINEA pigs, INTERLEUKIN-1, PHYTOHEMAGGLUTININS, MONOKINES, MACROPHAGES

Abstract

The proliferative response of guinea-pig thymocytes to co-mitogenic stimulation with phytohaemagglutinin and the guinea-pig interleukin I (IL-I )-like lymphocyte-activating monokine was lost by removing the cells that adhere to a Sephadex G-10 (G-10) column or the cells of low density in a Ficoll-Conray gradient. The diminished response in the G-10 non-adherent thymocyte or high-density thymocyte fraction was restored by the addition of a macrophage depleted G-10) adherent thymocyte fraction or a low-density. Ia-positive thymocyte fraction but not by the addition of peritoneal macrophages. These results suggest that the accessory cells which mediate the Increased responsiveness of thymocytes to the IL-1-like monokine existed in G-10 adherent cell fractions and the cells with this accessory function were not macrophages. The accessory cells were shown to be of low density, glass-non-adherent, G-l0-adherent, Fc receptor-negative, and Ia-positive. These results also suggest that the G-10-non-adherent and high-density thymocyte subpopulation, which is unresponsive or responds very little to the IL-1-like monokine by itself, acquires responsiveness to the monokine and proliferates by stimulation with the IL-1-like monokine and lectin in the presence of the accessory cells. [ABSTRACT FROM AUTHOR]

Published

1988