Your search keyword '"Wakashin H"' showing total 22 results

1. Liver changes in experimental nitroglycol poisoning

Author

Kawai, K., primary, Wakashin, H., additional, and Yoshikawa, H., additional

Published

1970

2. Microbial ligand-independent regulation of lymphopoiesis by NOD1.

Author

Iwamura C, Ohnuki H, Flomerfelt FA, Zheng L, Carletti A, Wakashin H, Mikami Y, Brooks SR, Kanno Y, Gress RE, Tosato G, Nakayama T, O'Shea JJ, Sher A, and Jankovic D

Subjects

Animals, Mice, Colitis, Ligands, Signal Transduction, Immunity, Innate, Lymphopoiesis

Abstract

Aberrant differentiation of progenitor cells in the hematopoietic system is known to severely impact host immune responsiveness. Here we demonstrate that NOD1, a cytosolic innate sensor of bacterial peptidoglycan, also functions in murine hematopoietic cells as a major regulator of both the generation and differentiation of lymphoid progenitors as well as peripheral T lymphocyte homeostasis. We further show that NOD1 mediates these functions by facilitating STAT5 signaling downstream of hematopoietic cytokines. In steady-state, loss of NOD1 resulted in a modest but significant decrease in numbers of mature T, B and natural killer cells. During systemic protozoan infection this defect was markedly enhanced, leading to host mortality. Lack of functional NOD1 also impaired T cell-dependent anti-tumor immunity while preventing colitis. These findings reveal that, in addition to its classical role as a bacterial ligand receptor, NOD1 plays an important function in regulating adaptive immunity through interaction with a major host cytokine signaling pathway., (© 2023. This is a U.S. Government work and not under copyright protection in the US; foreign copyright protection may apply.)

Published

2023

3. Central administered xenin induced Fos expression in nesfatin-1 neurons in rats.

Author

Saito S, Hashimoto H, Wakashin H, Ishibane M, Pae S, Saito S, Reien Y, Hirayama Y, Seo Y, Mizushima T, and Anzai N

Subjects

Humans, Rats, Animals, Nucleobindins metabolism, Nucleobindins pharmacology, Neurons metabolism, DNA-Binding Proteins metabolism, Calcium-Binding Proteins metabolism

Abstract

Xenin is a 25-amino acid peptide identified in human gastric mucosa, which is widely expressed in peripheral and central tissues. It is known that the central or peripheral administration of xenin decreases food intake in rodents. Nesfatin-1/NUCB2 (nesfatin-1) has been identified as an anorexic neuropeptide, it is often found co-localized with many peptides in the central nervous system. After the intracerebroventricular administration of xenin on nesfain-1-like immunoreactivity (LI) neurons, we examined its effects on food intake and water intake in rats. As a result, Fos-LI neurons were observed in the organum vasculosum of the laminae terminalis (OVLT), the median preoptic nucleus (MnPO), the subfornical organ (SFO), the supraoptic nucleus (SON), the paraventricular nucleus (PVN), the arcuate nucleus (Arc), the lateral hypothalamic area (LHA), the central amygdaloid nucleus (CAN), the dorsal raphe nucleus (DR), the locus coeruleus (LC), the area postrema (AP) and the nucleus of the solitary tract (NTS). After the administration, the number of Fos-LI neurons was significantly increased in the LC and the OVLT, the MnPO, the SFO, the SON, the PVN, the Arc, the LHA, the CAN, the DR, the AP and the NTS, compared with the control group. After the administration of xenin, we conducted double immunohistochemistry for Fos and nesfatin-1, and found that the number of nesfatin-1-LI neurons expressing Fos were significantly increased in the SON, the PVN, the Arc, the LHA, the CAN, the DR, the AP and the NTS, compared with the control group. The pretreatment of nesfatin-1 antisense significantly attenuated this xenin-induced feeding suppression, while that of nesfatin-1 missense showed no improvement. These results indicate that central administered xenin may have anorexia effects associated with activated central nesfatin-1 neurons., Competing Interests: Declaration of Competing Interest The authors hereby declare no conflicts of interest associated with this study.., (Copyright © 2023 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2023

4. HIV-1 Vpr suppresses expression of the thiazide-sensitive sodium chloride co-transporter in the distal convoluted tubule.

Author

Shrivastav S, Lee H, Okamoto K, Lu H, Yoshida T, Latt KZ, Wakashin H, Dalgleish JLT, Koritzinsky EH, Xu P, Asico LD, Chung JY, Hewitt S, Gildea JJ, Felder RA, Jose PA, Rosenberg AZ, Knepper MA, Kino T, and Kopp JB

Subjects

Aldosterone metabolism, Aldosterone pharmacology, Animals, Chlorocebus aethiops, Kidney Tubules, Distal metabolism, Mice, Mice, Transgenic, Phosphoenolpyruvate, RNA, Messenger metabolism, Receptors, Mineralocorticoid genetics, Receptors, Mineralocorticoid metabolism, Renin metabolism, Sodium metabolism, Sodium Chloride metabolism, Sodium Chloride Symporters metabolism, Solute Carrier Family 12, Member 3 genetics, Solute Carrier Family 12, Member 3 metabolism, Thiazides, Gene Products, vpr metabolism, HIV-1 genetics

Abstract

HIV-associated nephropathy (HIVAN) impairs functions of both glomeruli and tubules. Attention has been previously focused on the HIVAN glomerulopathy. Tubular injury has drawn increased attention because sodium wasting is common in hospitalized HIV/AIDS patients. We used viral protein R (Vpr)-transgenic mice to investigate the mechanisms whereby Vpr contributes to urinary sodium wasting. In phosphoenolpyruvate carboxykinase promoter-driven Vpr-transgenic mice, in situ hybridization showed that Vpr mRNA was expressed in all nephron segments, including the distal convoluted tubule. Vpr-transgenic mice, compared with wild-type littermates, markedly increased urinary sodium excretion, despite similar plasma renin activity and aldosterone levels. Kidneys from Vpr-transgenic mice also markedly reduced protein abundance of the Na+-Cl- cotransporter (NCC), while mineralocorticoid receptor (MR) protein expression level was unchanged. In African green monkey kidney cells, Vpr abrogated the aldosterone-mediated stimulation of MR transcriptional activity. Gene expression of Slc12a3 (NCC) in Vpr-transgenic mice was significantly lower compared with wild-type mice, assessed by both qRT-PCR and RNAScope in situ hybridization analysis. Chromatin immunoprecipitation assays identified multiple MR response elements (MRE), located from 5 kb upstream of the transcription start site and extending to the third exon of the SLC12A3 gene. Mutation of MRE and SP1 sites in the SLC12A3 promoter region abrogated the transcriptional responses to aldosterone and Vpr, indicating that functional MRE and SP1 are required for the SLC12A3 gene suppression in response to Vpr. Thus, Vpr attenuates MR transcriptional activity and inhibits Slc12a3 transcription in the distal convoluted tubule and contributes to salt wasting in Vpr-transgenic mice., Competing Interests: Author JBK holds a patent relating to monoclonal antibodies to HIV-1 Vpr and methods of using same. United States Patent 7,993,647 (2015). No other conflicts of interest, financial or otherwise, are declared by the authors. This does not alter our adherence to PLOS ONE policies on sharing data and materials.

Published

2022

5. The Effects of Trypsin Inhibitor on Insulin Secretion Using Rat Pancreas in an Organ Bath.

Author

Morita A, Ouchi M, Satoh K, Kobayashi S, Terada M, Wakashin H, Kon H, Hayashi K, Anzai N, Shimizu A, Sugihara H, Oba K, and Fujita T

Subjects

Animals, Insulin metabolism, Insulin Secretion, Male, Pancreas metabolism, Rats, Rats, Wistar, Amylases, Trypsin Inhibitors metabolism, Trypsin Inhibitors pharmacology

Abstract

Background/aim: We developed an experimental method to reproduce insulin secretion from isolated rat pancreas preparations using an organ bath system. However, secretion of trypsin, another pancreatic enzyme, interferes with insulin production in such systems. We aimed to ascertain the minimum trypsin inhibitor (TI), dose for obtaining a sustained, stable rate of insulin secretion., Materials and Methods: The action of TI (1-10 μg/ml) on pancreatic preparations of male Wistar-Imamichi rats in organ bath experiments was assessed by measuring insulin, amylase, and trypsin activity., Results: The level of insulin outflow remained steady in the TI-treated samples, in contrast to that in the untreated control, where insulin secretion decreased over time. The level of amylase outflow did not change significantly. Trypsin activity was significantly lower in the TI-treated samples than in the control., Conclusion: Even low concentrations of TI can maintain insulin secretion by inhibiting trypsin activity in organ bath experiments., (Copyright © 2021 International Institute of Anticancer Research (Dr. George J. Delinasios), All rights reserved.)

Published

2021

6. The kidney of the Nodularia freshwater mussel has a larger filtration-size and counter-current system with improved water excretion compared with the seawater mussel Mytilus.

Author

Seo E, Wakashin H, and Seo Y

Subjects

Animals, Contrast Media, Fresh Water, Glomerular Filtration Rate, Immunohistochemistry, Kidney cytology, Kidney diagnostic imaging, Kidney Function Tests, Magnetic Resonance Imaging, Seawater, Kidney physiology, Mytilus physiology, Unionidae physiology

Abstract

Histological studies and magnetic resonance imaging were employed to analyze the kidney structure and function of the freshwater mussel, Nodularia douglasiae. The Nodularia kidney consists of proximal, intermediate and distal tubules. The epithelia of the renal tubules were composed of a single layer of cuboidal cells. The proximal and distal tubules run in opposite directions underneath the pericardial cavity. Molecular weight cut-off (MWCO) values for the kidney filtration were detected by MR tracer injections: gadolinium-diethylenetriaminepentaacetic acid (GdDTPA) at 0.55 kDa, an oligomer-based contrast agent (CH3-DTPA-Gd) at 2.2 kDa, as well as Gd-DTPA-polylysine at 10, 22, and 110 kDa. The T1w-MRI intensity and T1 relaxation rate (R1) of the pericardial cavity and renal tubules increased with tracers smaller than 10 kDa. The other tracers showed only minimal or no increase. Thus, we concluded that the MWCO of the kidney is 22 kDa, 50 times larger than that for the Mytilus living in seawater. Since the R1 values of the renal tubules were similar to those of the pericardial cavity, the kidney did not concentrate filtrated tracers. The slow decay of the magnetic resonance (MR) tracers from the renal tubules indicated a low filtration rate, suggesting that the counter-current system reabsorbs useful solutes without reabsorption of water. The higher MWCO may be beneficial to maintain the tubular oncotic pressure and allow excretion of excess water. In conclusion, a main renal function of the freshwater mussel is the excretion of water, opposite to that of the seawater mussel and vertebrates, which preserve water., Competing Interests: Competing interests The authors declare no competing or financial interests., (© 2021. Published by The Company of Biologists Ltd.)

Published

2021

7. Suppressor of cytokine signalling 3 (SOCS3) expressed in podocytes attenuates glomerulonephritis and suppresses autoantibody production in an imiquimod-induced lupus model.

Author

Fukuta M, Suzuki K, Kojima S, Yabe Y, Suzuki K, Iida K, Yamada H, Makino S, Iwata A, Tanaka S, Iwamoto T, Suto A, Nakagomi D, Wakashin H, Maezawa Y, Maezawa Y, Takemoto M, Asanuma K, and Nakajima H

Subjects

Animals, Cytokines metabolism, Imiquimod, Mice, Mice, Inbred BALB C, Suppressor of Cytokine Signaling 3 Protein genetics, Glomerulonephritis chemically induced, Podocytes metabolism, Suppressor of Cytokine Signaling 3 Protein metabolism

Abstract

Objective: Recently, podocytes have been recognised not only as a physical barrier to prevent urinary protein loss but also as producers of proinflammatory cytokines. However, the roles of podocytes in the pathogenesis of lupus nephritis (LN) remain largely unknown. This study aims to determine the roles of suppressor of cytokine signalling (SOCS) family members expressed in glomeruli in the regulation of LN., Methods: We investigated the expression of SOCS family members in glomeruli in murine lupus model induced by repeated epicutaneous administration of the TLR7/8 agonist imiquimod. We also investigated the roles of SOCS3 expressed in podocytes in the imiquimod-induced glomerulonephritis and systemic autoimmunity by using podocyte-specific SOCS3-deficient mice (podocin-Cre x SOCS3 fl/fl mice (SOCS3-cKO mice)). Finally, we investigated the expression of proinflammatory cytokines and chemokines in SOCS3-deficient podocyte cell lines., Results: qPCR analysis revealed that among SOCS family members, SOCS3 was preferentially induced in glomeruli on epicutaneous administration of imiquimod and that interleukin 6 (IL-6) induced SOCS3 expression in podocyte cell lines. SOCS3-cKO mice exhibited severe glomerulonephritis, high levels of serum creatinine and urine albumin and decreased survival rate compared with control SOCS3-WT mice. Levels of anti-double-strand DNA antibody, SOCS (GC) formation and the numbers of follicular helper T (Tfh) cells and GC B cells in the spleen were higher in SOCS3-cKO mice than those in SOCS3-WT mice. Serum IL-6 levels and expression of IL-6 mRNA in glomeruli were also elevated in SOCS3-cKO mice. IL-6-induced IL-6 expression was enhanced in SOCS3-deficient podocyte cell lines compared with that in SOCS3-sufficient podocyte cell lines., Conclusion: SOCS3 expressed in podocytes plays protective roles for the development of glomerulonephritis and inhibits autoantibody production in the imiquimod-induced lupus model presumably by suppressing IL-6 production of podocytes., Competing Interests: Competing interests: None declared., (© Author(s) (or their employer(s)) 2021. Re-use permitted under CC BY-NC. No commercial re-use. See rights and permissions. Published by BMJ.)

Published

2021

8. JPH203, a newly developed anti-cancer drug, shows a preincubation inhibitory effect on L-type amino acid transporter 1 function.

Author

Okunushi K, Furihata T, Morio H, Muto Y, Higuchi K, Kaneko M, Otsuka Y, Ohno Y, Watanabe Y, Reien Y, Nakagawa K, Sakamoto S, Wakashin H, Shimojo N, and Anzai N

Subjects

Dose-Response Relationship, Drug, HT29 Cells, Humans, Large Neutral Amino Acid-Transporter 1 physiology, Leucine metabolism, Time Factors, Tyrosine pharmacology, Adenocarcinoma genetics, Adenocarcinoma metabolism, Antineoplastic Agents pharmacology, Benzoxazoles pharmacology, Colonic Neoplasms genetics, Colonic Neoplasms metabolism, Drug Screening Assays, Antitumor methods, Large Neutral Amino Acid-Transporter 1 metabolism, Tyrosine analogs & derivatives

Abstract

JPH203 is a novel anti-cancer drug targeting L-type amino acid transporter 1 (LAT1), which plays a primary role in the uptake of essential amino acids in tumor cells. Although a co-incubation inhibitory effect of JPH203 has been shown in a conventional uptake assay, its preincubation inhibitory effects have remained undetermined. Therefore, we aimed to characterize the preincubation inhibitory effects of JPH203 on LAT1 function using leucine uptake assays in LAT1-positive human colon cancer HT-29 cells. Preincubation of the cells with JPH203 (0.3 μM for 120 min) decreased the activity level to 30% of that in dimethylsulfoxide-treated cells. Similarly, in time-dependency analysis, preincubation of HT-29 cells with 10 μM JPH203 for 30, 60, and 120 min decreased the leucine uptake activity (42%, 32%, and 28% of that in control cells, respectively). Furthermore, the IC 50 value of the combination of preincubation and co-incubation effects was lower than that of co-incubation inhibition alone (34.2 ± 3.6 nM vs. 99.2 ± 11.0 nM). In conclusion, we revealed that JPH203 has the capability to inhibit LAT1 function through preincubation effects. Moreover, preincubation synergistically enhances the co-incubation inhibitory effects. These findings provide a novel insight into the anti-cancer effects of JPH203 in cancer therapy., Competing Interests: Declaration of Competing Interest The authors indicated no potential conflicts of interest., (Copyright © 2020 The Authors. Production and hosting by Elsevier B.V. All rights reserved.)

Published

2020

9. APOL1 renal risk variants exacerbate podocyte injury by increasing inflammatory stress.

Author

Wakashin H, Heymann J, Roshanravan H, Daneshpajouhnejad P, Rosenberg A, Shin MK, Hoek M, and Kopp JB

Subjects

Animals, Apolipoprotein L1 metabolism, Humans, In Vitro Techniques, Inflammation metabolism, Interleukin-1beta metabolism, Intracellular Signaling Peptides and Proteins metabolism, Kidney Glomerulus pathology, Mice, Mice, Transgenic, Podocytes pathology, Protein Isoforms, Apolipoprotein L1 genetics, Inflammation genetics, Kidney Glomerulus metabolism, Nephrectomy, Podocytes metabolism, RNA, Messenger metabolism, Stress, Physiological genetics

Abstract

Background: Apolipoprotein L1, APOL1, is a trypanosome lytic factor present in human and certain other primates. APOL1 gene variants, present in individuals of recent sub-Saharan African descent, increase risk for glomerular disease and associate with the disease progression, but the molecular mechanisms have not been defined., Objectives: We focus on the mechanism how APOL1 variant proteins enhance podocyte injury in the stressed kidney., Methods: First, we investigated the expression of APOL1 protein isoform and the localization of APOL1 protein in the kidney. Next, we examined the role of APOL1 in the podocyte stress and the inflammatory signaling in the kidney after hemi-nephrectomy., Results: We identified a novel RNA variant that lacks a secretory pathway signal sequence and we found that the predicted APOL1-B3 protein isoform was expressed in human podocytes in vivo and by BAC-APOL1 transgenic mice. APOL1-B3-G2 transgenic mice, carrying a renal risk variant, manifested podocyte injury and increased pro-IL-1β mRNA in isolated glomeruli and increased IL-1β production in the remnant kidney after uninephrectomy. APOL1-B3 interacted with NLRP12, a key regulator of Toll-like receptor signaling., Conclusions: These results suggest a possible mechanism for podocyte injury by which one of the APOL1 protein isoforms, APOL1-B3 and its renal risk variants, enhances inflammatory signaling.

Published

2020

10. Development of an organ bath technique for isolated rat pancreas preparations to assess the effect of 1,5-AG on insulin secretion.

Author

Morita A, Ouchi M, Satoh K, Terada M, Kon H, Wakashin H, Hayashi K, Anzai N, Oba K, Shimizu A, and Fujita T

Subjects

Animals, Rats, Deoxyglucose blood, Insulin Secretion, Pancreas metabolism, Tissue Culture Techniques methods

Abstract

To investigate substances related to insulin secretion, we reported a convenient experimental method to reproduce insulin secretion from isolated rat pancreas preparations using an organ bath. While the method has experimental utility for investigating insulin secretion, optimization of the experimental design is still needed. The level of insulin outflow in the control decreased over time in our previous study. Decreasing serum 1,5-anhydroglucitol (1,5-AG) levels is also known to be shown in patients with worsening glycemic control. There is one in vitro report demonstrated that 1,5-AG induced insulin release. It appears that discussion needs to be deepened further on it. In this study, we investigated the effect of 1,5-AG on insulin secretion through to optimize the condition of endocrine function using the ex vivo organ bath technique. The level of insulin outflow in the control and 1,5-AG groups decreased over time in the organ bath experiment. To analyze the effect of trypsin on reduced insulin secretion, pancreas preparation was treated with soybean trypsin inhibitor (TI). Insulin outflow levels of the TI group were significantly higher than the control group. An enzyme indicator of tissue damage tended to be lower in the TI group. There was no significant enhancement of insulin secretion by 1,5-AG. The present study demonstrated the utility of TI application for the organ bath technique. This finding supported the development of an organ bath technique for the assessment of the effects of novel therapeutics on insulin secretion.

Published

2020

11. Size-selective filtration of the atrial wall estimated from the accumulation of tracers in the kidney of the mussel Mytilus galloprovincialis .

Author

Wakashin H, Seo E, and Seo Y

Subjects

Animals, Extremities physiology, Filtration, Kidney diagnostic imaging, Magnetic Resonance Imaging, Manganese, Seawater, Atrial Function physiology, Kidney physiology, Mytilus physiology

Abstract

In order to determine the molecular weight cut-off (MWCO) for the atrial wall filtration into kidneys of the Mytilus galloprovincialis , we employed five magnetic resonance (MR) tracers: manganese chloride (Mn 2+ ), gadolinium chloride (Gd 3+ ), manganese-ethylenediaminetetraacetic acid (MnEDTA), gadolinium-diethylenetriamine pentaacetic acid (GdDTPA) and oligomer-based contrast agent (CH3-DTPA-Gd). After injection of the MR tracers (1 or 2 mmol l -1 ×0.1 ml) into the visceral mass, T 1 -weighted MR imaging ( T 1w ) were measured at 20°C. The MR tracers were distributed uniformly in the visceral mass within 1 h after injection. The T 1 = R 1 ) were measured at 20°C. The MR tracers were distributed uniformly in the visceral mass within 1 h after injection. The T 1w -MRI intensity and R 1 of the kidney ( R 1K ) were increased by Mn 2+ and MnEDTA, with urine concentrations estimated at 210 and 65 µmol l -1 , respectively. The rest of the tracers showed only minimal or no increase. When the mussels were additionally incubated in seawater with 10 µmol l -1 MnCl 2 , R 1K was increased in the GdDTPA group, but not in the GdCl 3 group. Therefore, Gd 3+ might have inhibited renal accumulation of Mn 2+ and Gd 3+ Incubation in seawater with 10 µmol l -1 MnEDTA showed no increase in the R 1K , but additional incubation with 10 µmol l -1 MnCl 2 caused an increase in R 1K It is suggested that injected MnEDTA was filtrated as MnEDTA per se, and not likely separated into free Mn 2+ Thus, we concluded that the MWCO of the atrial wall of the M. galloprovincialis is around 0.5 kDa, which is almost 1/100 of that for vertebrate animals, and suggests a reduction in efforts to reabsorb metabolites and osmolytes from the urine., Competing Interests: Competing interestsThe authors declare no competing or financial interests., (© 2019. Published by The Company of Biologists Ltd.)

Published

2019

12. T 2 Distribution in the Forearm Muscles and the T 2 Threshold for Defining Activated Muscle.

Author

Takamori M, Akiyama S, Yoshida K, Wakashin H, and Seo Y

Subjects

Adult, Female, Healthy Volunteers, Humans, Male, Reference Values, Sensitivity and Specificity, Exercise physiology, Forearm diagnostic imaging, Magnetic Resonance Imaging methods, Muscle, Skeletal diagnostic imaging, Muscle, Skeletal physiology

Abstract

Purpose: In order to detect exercised muscles by the increase in T 2 , we have defined a Gaussian T 2 distribution and reference values (T 2r and SD r ) in resting state muscles, and a threshold for detecting exercised muscles., Methods: The subjects were healthy adult volunteers (14 males and 12 females). Multiple-spin-echo (MSE) MR images were obtained with 10 TE values from 10 to 100 ms using a 0.2T MRI system. T 2 values for 10 forearm muscles were obtained in the resting state and after isometric wrist flexion exercise with 5%, 15%, and 25% of the maximum voluntary contraction (MVC). Z values were obtained by (T 2e - T 2r )/SD r , where T 2e was T 2 after exercise. Based on sample size calculations, three thresholds (Z T = 1.00, 2.56, and 3.07) were applied to agonist and antagonist muscles., Results: A normal distribution of T 2 was detected in resting muscles at 34 ± 3 ms (mean ± standard deviation [SD]) in 26 subjects using the Kolmogorov-Smirnov test, the Shapiro-Wilk test, and the Jarque-Bera test (P > 0.05). No gender differences were shown between the T 2 or SD, and a similar result was obtained in 12 measurements on a single subject (P < 0.01). The T 2r and SD r were used for reference values. The threshold Z T = 1.00 showed the highest sensitivity (0.86) even with 5% MVC, but it showed a lower specificity (0.85) than the other thresholds. Z T = 3.07 showed the highest specificity (1.0), but it showed a lower sensitivity (0.36) with the 5% MVC, compared with Z T = 2.56 (0.50). The receiver operating characteristics analysis also supported these results., Conclusion: We found that the T 2 distribution in muscles was Gaussian, suggesting that a one-sample t-test can be applied, and that Z T = 2.56 could cover low-intensity exercise with high specificity and a low false-positive rate.

Published

2019

13. Sodium-coupled monocarboxylate transporter 1 interacts with the RING finger- and PDZ domain-containing protein PDZRN3.

Author

Otsuka Y, Furihata T, Nakagawa K, Ohno Y, Reien Y, Ouchi M, Wakashin H, Tsuruoka S, and Anzai N

Subjects

Biological Transport physiology, Cell Line, HEK293 Cells, Humans, Protein Interaction Domains and Motifs physiology, Sodium, Ubiquitin-Protein Ligases, Carrier Proteins metabolism, Monocarboxylic Acid Transporters metabolism

Abstract

Sodium-coupled monocarboxylate transporter SMCT1 (SLC5A8) mediates monocarboxylate transport in the proximal tubule of the kidney. We have identified PDZK1 and PDZ domain-containing RING finger 3 (PDZRN3) as potent binding partners of SMCT1, which has a PDZ motif (Thr-Arg-Leu), by yeast two-hybrid screening and revealed that PDZK1 enhances the transport activity of SMCT1. In this study, we aimed to characterize the interaction between SMCT1 and PDZRN3 as well as to examine how PDZRN3 regulates SMCT1 function. An interaction between SMCT1 and PDZRN3 through the PDZ motif was observed in a co-immunoprecipitation assay and yeast two-hybrid assay. A transport assay showed that PDZRN3 abolished the enhancing effect of PDZK1 on nicotinate uptake via SMCT1. Our results suggest that SMCT1 interacts with PDZRN3 and that PDZRN3 may regulate SMCT1 function by interfering with the interaction between SMCT1 and PDZK1.

Published

2019

14. APOL1 risk allele RNA contributes to renal toxicity by activating protein kinase R.

Author

Okamoto K, Rausch JW, Wakashin H, Fu Y, Chung JY, Dummer PD, Shin MK, Chandra P, Suzuki K, Shrivastav S, Rosenberg AZ, Hewitt SM, Ray PE, Noiri E, Le Grice SFJ, Hoek M, Han Z, Winkler CA, and Kopp JB

Abstract

APOL1 risk alleles associate with chronic kidney disease in African Americans, but the mechanisms remain to be fully understood. We show that APOL1 risk alleles activate protein kinase R (PKR) in cultured cells and transgenic mice. This effect is preserved when a premature stop codon is introduced to APOL1 risk alleles, suggesting that APOL1 RNA but not protein is required for the effect. Podocyte expression of APOL1 risk allele RNA, but not protein, in transgenic mice induces glomerular injury and proteinuria. Structural analysis of the APOL1 RNA shows that the risk variants possess secondary structure serving as a scaffold for tandem PKR binding and activation. These findings provide a mechanism by which APOL1 variants damage podocytes and suggest novel therapeutic strategies., Competing Interests: The authors declare no competing interests.

Published

2018

15. Accumulation and excretion of manganese ion in the kidney of M ytilus galloprovincialis .

Author

Wakashin H, Seo E, and Seo Y

Subjects

Animals, Kidney metabolism, Magnetic Resonance Imaging, Renal Elimination physiology, Manganese metabolism, Mytilus metabolism

Abstract

T 1 -weighted magnetic resonance imaging ( T 1w -MRI) was employed to detect the accumulation of manganese ion (Mn 2+ ) in urine in the kidney of the mussel Mytilus galloprovincialis , and the longitudinal relaxation rates (1/ T 1 = R 1 ) were measured. When the mussel was exposed to seawater containing 10 µmol l -1 Mn 2+ , the T 1w -MRI intensity and R 1 of the kidney, stomach and digestive glands were increased. Mn 2+ might be taken into the hemolymph via the gastrointestinal tract, and then filtrated into the pericardium via the auricles. Although the image intensity in the pericardium was not affected by manganese, an image intensity enhancement was observed in the distal part of the renopericardial communication canals between the pericardium and the kidneys, indicating Mn 2+ was concentrated in the excretion pathway. As the seawater Mn 2+ concentration ([Mn 2+ ] SW for 24 h, the Mn -1 , R 1 of the kidney ( R 1K ) was elevated. When the mussels were immersed in 3-10 µmol l -1 [Mn 2+ ] SW for 24 h, the Mn 2+ concentration in the kidney ([Mn 2+ ] K ) showed a 15-fold increase compared with the ambient [Mn 2+ ] SW In the range of [Mn 2+ ] SW from 10 to 50 µmol l -1 , R 1K reached a plateau level that corresponded to 200 µmol l -1 [Mn 2+ ] K As [Mn 2+ ] K fell transiently, voluntary excretion of urine from the kidney was assumed. The decreases in intensity were not synchronized between the right and left kidneys, and the closure of the shells might not be essential for urinary excretion. The voluntary excretion suggested an additional explanation for the large range in metal concentratons in the kidneys of the mussel., Competing Interests: Competing interestsThe authors declare no competing or financial interests., (© 2018. Published by The Company of Biologists Ltd.)

Published

2018

16. Podocytes degrade endocytosed albumin primarily in lysosomes.

Author

Carson JM, Okamura K, Wakashin H, McFann K, Dobrinskikh E, Kopp JB, and Blaine J

Subjects

Animals, Cells, Cultured, Denys-Drash Syndrome genetics, Denys-Drash Syndrome pathology, Disease Models, Animal, Endocytosis, Fluorescein-5-isothiocyanate analogs & derivatives, Fluorescein-5-isothiocyanate metabolism, Fluorescein-5-isothiocyanate pharmacokinetics, Humans, Mice, Mice, Transgenic, Proteolysis, Repressor Proteins genetics, Repressor Proteins metabolism, Serum Albumin metabolism, Serum Albumin pharmacokinetics, WT1 Proteins, Albumins metabolism, Lysosomes metabolism, Podocytes metabolism

Abstract

Albuminuria is a strong, independent predictor of chronic kidney disease progression. We hypothesize that podocyte processing of albumin via the lysosome may be an important determinant of podocyte injury and loss. A human urine derived podocyte-like epithelial cell (HUPEC) line was used for in vitro experiments. Albumin uptake was quantified by Western blot after loading HUPECs with fluorescein-labeled (FITC) albumin. Co-localization of albumin with lysosomes was determined by confocal microscopy. Albumin degradation was measured by quantifying FITC-albumin abundance in HUPEC lysates by Western blot. Degradation experiments were repeated using HUPECs treated with chloroquine, a lysosome inhibitor, or MG-132, a proteasome inhibitor. Lysosome activity was measured by fluorescence recovery after photo bleaching (FRAP). Cytokine production was measured by ELISA. Cell death was determined by trypan blue staining. In vivo, staining with lysosome-associated membrane protein-1 (LAMP-1) was performed on tissue from a Denys-Drash trangenic mouse model of nephrotic syndrome. HUPECs endocytosed albumin, which co-localized with lysosomes. Choloroquine, but not MG-132, inhibited albumin degradation, indicating that degradation occurs in lysosomes. Cathepsin B activity, measured by FRAP, significantly decreased in HUPECs exposed to albumin (12.5% of activity in controls) and chloroquine (12.8%), and declined further with exposure to albumin plus chloroquine (8.2%, p<0.05). Cytokine production and cell death were significantly increased in HUPECs exposed to albumin and chloroquine alone, and these effects were potentiated by exposure to albumin plus chloroquine. Compared to wild-type mice, glomerular staining of LAMP-1 was significantly increased in Denys-Drash mice and appeared to be most prominent in podocytes. These data suggest lysosomes are involved in the processing of endocytosed albumin in podocytes, and lysosomal dysfunction may contribute to podocyte injury and glomerulosclerosis in albuminuric diseases. Modifiers of lysosomal activity may have therapeutic potential in slowing the progression of glomerulosclerosis by enhancing the ability of podocytes to process and degrade albumin.

Published

2014

17. IL-22 attenuates IL-25 production by lung epithelial cells and inhibits antigen-induced eosinophilic airway inflammation.

Author

Takahashi K, Hirose K, Kawashima S, Niwa Y, Wakashin H, Iwata A, Tokoyoda K, Renauld JC, Iwamoto I, Nakayama T, and Nakajima H

Subjects

Animals, Asthma metabolism, Blotting, Western, Bronchoalveolar Lavage Fluid immunology, Disease Models, Animal, Eosinophilia metabolism, Epithelial Cells metabolism, Immunohistochemistry, Interleukins biosynthesis, Interleukins metabolism, Mice, Mice, Inbred BALB C, Pneumonia metabolism, Real-Time Polymerase Chain Reaction, Respiratory Mucosa metabolism, Interleukin-22, Asthma immunology, Eosinophilia immunology, Epithelial Cells immunology, Interleukins immunology, Pneumonia immunology, Respiratory Mucosa immunology

Abstract

Background: IL-22 functions as both a proinflammatory cytokine and an anti-inflammatory cytokine in various inflammations, depending on the cellular and cytokine milieu. However, the roles of IL-22 in the regulation of allergic airway inflammation are still largely unknown., Objective: We sought to determine whether IL-22 is involved in the regulation of allergic airway inflammation., Methods: We examined IL-22 production and its cellular source at the site of antigen-induced airway inflammation in mice. We also examined the effect of IL-22 neutralization, as well as IL-22 administration, on antigen-induced airway inflammation. We finally examined the effect of IL-22 on IL-25 production from a lung epithelial cell line (MLE-15 cells)., Results: Antigen inhalation induced IL-22 production in the airways of sensitized mice. CD4(+) T cells, but not other lymphocytes or innate cells, infiltrating in the airways produced IL-22, and one third of IL-22-producing CD4(+) T cells also produced IL-17A. The neutralization of IL-22 by anti-IL-22 antibody enhanced antigen-induced IL-13 production, eosinophil recruitment, and goblet cell hyperplasia in the airways. On the other hand, intranasal administration of recombinant IL-22 attenuated antigen-induced eosinophil recruitment into the airways. Moreover, anti-IL-22 antibody enhanced antigen-induced IL-25 production in the airways, and anti-IL-25 antibody reversed the enhancing effect of anti-IL-22 antibody on antigen-induced eosinophil recruitment into the airways. Finally, IL-22 inhibited IL-13-mediated enhancement of IL-25 expression in IL-1β- or LPS-stimulated MLE-15 cells., Conclusion: IL-22 attenuates antigen-induced airway inflammation, possibly by inhibiting IL-25 production by lung epithelial cells., (Copyright © 2011 American Academy of Allergy, Asthma & Immunology. Published by Mosby, Inc. All rights reserved.)

Published

2011

18. STAT4 is required for IFN-β-induced MCP-1 mRNA expression in murine mast cells.

Author

Iida K, Suzuki K, Yokota M, Nakagomi D, Wakashin H, Iwata A, Kawashima H, Takatori H, and Nakajima H

Subjects

Animals, Cell Degranulation immunology, Cell Proliferation drug effects, Gene Expression drug effects, Interleukin-3 pharmacology, Mast Cells cytology, Mast Cells drug effects, Mast Cells immunology, Mast Cells metabolism, Mice, Mice, Inbred C57BL, Mice, Knockout, Phosphorylation drug effects, Proto-Oncogene Proteins c-kit metabolism, Receptors, IgE agonists, Receptors, IgE metabolism, STAT1 Transcription Factor metabolism, STAT4 Transcription Factor genetics, beta-N-Acetylhexosaminidases metabolism, Chemokine CCL2 genetics, Gene Expression genetics, Gene Expression Regulation immunology, Interferon-beta pharmacology, STAT4 Transcription Factor metabolism

Abstract

Background: Mast cells are immunocompetent cells that are found in almost all tissues and function as sentinels of immune responses. Recently, it has been shown that mast cells play significant roles in innate immune responses. However, it is still largely unknown whether signal transducers and activators of transcription 4 (STAT4), one of the STAT proteins under type I IFN signaling, is involved in type I IFN-mediated gene expression in mast cells., Methods: We investigated the role of STAT4 in IFN-β-induced gene expression in mast cells by using STAT4-deficient (STAT4(-/-)) bone marrow-derived mast cells (BMMCs)., Results: STAT4 was expressed in BMMCs and activated in response to IFN-β but not to IL-12 or IL-23. The development of BMMCs as well as IgE-induced degranulation of BMMCs was normal in STAT4(-/-) mice. On the other hand, while IFN-β-induced mRNA expression of interferon-induced protein with tetratricopeptide repeats 1 (IFIT-1), protein kinase interferon-inducible double stranded RNA dependent (PKR), and myxovirus resistance 1 (Mx1) was similar between STAT4(-/-) BMMCs and wild-type (WT) BMMCs, IFN-β-induced MCP-1 mRNA expression was severely diminished in STAT4(-/-) BMMCs as compared with WT BMMCs., Conclusions: STAT4 plays an essential role in IFN-β-induced MCP-1 mRNA expression in mast cells., (Copyright © 2011 S. Karger AG, Basel.)

Published

2011

19. Role of IL-23-Th17 cell axis in allergic airway inflammation.

Author

Wakashin H, Hirose K, Iwamoto I, and Nakajima H

Subjects

Animals, Eosinophils immunology, Humans, Inflammation immunology, Neutrophils immunology, Asthma immunology, Interleukin-17 metabolism, Interleukin-23 metabolism, T-Lymphocyte Subsets immunology, T-Lymphocytes, Helper-Inducer immunology

Abstract

Asthma is characterized by chronic airway inflammation with intense eosinophil and lymphocyte infiltration, mucus hyperproduction, and airway hyperresponsiveness to a variety of stimuli. It is now generally accepted that antigen-specific Th2 cells and their cytokines orchestrate these pathognomonic features of asthma. On the other hand, Th17 cells and IL-23, a cytokine that preferentially expands Th17 cells, play a significant role in the development of chronic inflammatory diseases, including autoimmune diseases. Recently, we have shown that IL-23 and Th17 cells enhance not only neutrophilic airway inflammation but also Th2 cell-mediated eosinophilic airway inflammation in a murine asthma model. In this review, we will discuss the roles of IL-23 and Th17 cells in airway inflammation in asthma., (Copyright 2009 S. Karger AG, Basel.)

Published

2009

20. IL-23 and Th17 cells enhance Th2-cell-mediated eosinophilic airway inflammation in mice.

Author

Wakashin H, Hirose K, Maezawa Y, Kagami S, Suto A, Watanabe N, Saito Y, Hatano M, Tokuhisa T, Iwakura Y, Puccetti P, Iwamoto I, and Nakajima H

Subjects

Animals, Asthma chemically induced, Disease Models, Animal, Eosinophils immunology, Interleukin-23 immunology, Mice, Mice, Knockout, Mice, Transgenic, Up-Regulation, Asthma immunology, Interleukin-17 immunology, Interleukin-23 metabolism, Pneumonia immunology, T-Lymphocyte Subsets immunology, Th2 Cells immunology

Abstract

Rationale: The IL-23-IL-17A-producing CD4(+) T-cell (Th17 cell) axis plays an important role in the development of chronic inflammatory diseases, including autoimmune diseases. However, the role of the IL-23-Th17 cell axis in the regulation of allergic airway inflammation is still largely unknown., Objectives: To determine the role of IL-23 and Th17 cells in allergic airway inflammation., Methods: We examined the effect of anti-IL-23 antibody on antigen-induced airway inflammation. We also investigated the effect of enforced expression of IL-23 on allergic airway inflammation by generating lung-specific IL-23 transgenic mice. Moreover, we examined the effect of adoptive transfer of antigen-specific Th17 cells on allergic airway inflammation., Measurements and Main Results: IL-23 mRNA was expressed in the lung of sensitized mice upon antigen inhalation, and the neutralization of IL-23 decreased antigen-induced eosinophil recruitment and Th2 cytokine production in the airways. The enforced expression of IL-23 in the airways significantly enhanced antigen-induced eosinophil and neutrophil recruitment into the airways; Th2 cytokine, IL-17A, and tumor necrosis factor (TNF)-alpha production in the airways; goblet cell hyperplasia; and airway hyperresponsiveness. Moreover, IL-23-mediated enhancement of antigen-induced Th2 cytokine production and eosinophil recruitment in the airways was still observed in the mice lacking IL-17A. Furthermore, although adoptive transfer of antigen-specific Th17 cells alone induced neutrophil but not eosinophil recruitment into the airways upon antigen inhalation, cotransfer of Th17 cells with Th2 cells significantly enhanced antigen-induced Th2-cell-mediated eosinophil recruitment into the airways and airway hyperresponsiveness., Conclusions: IL-23 and Th17 cells not only induce Th17-cell-mediated neutrophilic airway inflammation but also up-regulate Th2-cell-mediated eosinophilic airway inflammation.

Published

2008

21. GS143, an IkappaB ubiquitination inhibitor, inhibits allergic airway inflammation in mice.

Author

Hirose K, Wakashin H, Oki M, Kagami S, Suto A, Ikeda K, Watanabe N, Iwamoto I, Furuichi Y, and Nakajima H

Subjects

Administration, Intranasal, Animals, Antigens immunology, Antigens pharmacology, Asthma immunology, Benzoates administration & dosage, Cell Differentiation drug effects, Lung drug effects, Lung immunology, Lung metabolism, Mice, Mice, Inbred BALB C, Mucus drug effects, Mucus immunology, Mucus metabolism, NF-kappa B metabolism, Pyrazoles administration & dosage, Th1 Cells cytology, Th1 Cells drug effects, Th1 Cells immunology, Th2 Cells cytology, Th2 Cells drug effects, Th2 Cells immunology, Asthma prevention & control, Benzoates therapeutic use, I-kappa B Proteins metabolism, NF-kappa B antagonists & inhibitors, Pyrazoles therapeutic use, Ubiquitination drug effects

Abstract

Asthma is characterized by airway inflammation with intense eosinophil infiltration and mucus hyper-production, in which antigen-specific Th2 cells play critical roles. Nuclear factor-kappaB (NF-kappaB) pathway has been demonstrated to be essential for the production of Th2 cytokines and chemokines in the airways in murine asthma models. In the present study, we examined the effect of GS143, a novel small-molecule inhibitor of IkappaB ubiquitination, on antigen-induced airway inflammation and Th2 cytokine production in mice. Intranasal administration of GS143 prior to antigen challenge suppressed antigen-induced NF-kappaB activation in the lung of sensitized mice. Intranasal administration of GS143 also inhibited antigen-induced eosinophil and lymphocyte recruitment into the airways as well as the expression of Th2 cytokines and eotaxin in the airways. Moreover, GS143 inhibited antigen-induced differentiation of Th2 cells but not of Th1 cells in vitro. Taken together, these results suggest that IkappaB ubiquitination inhibitor may have therapeutic potential against asthma.

Published

2008

22. T-bet inhibits both TH2 cell-mediated eosinophil recruitment and TH17 cell-mediated neutrophil recruitment into the airways.

Author

Fujiwara M, Hirose K, Kagami S, Takatori H, Wakashin H, Tamachi T, Watanabe N, Saito Y, Iwamoto I, and Nakajima H

Subjects

Adoptive Transfer, Animals, Asthma genetics, Cell Differentiation, DNA-Binding Proteins genetics, Interleukin-13 metabolism, Interleukin-17 metabolism, Lung immunology, Mice, Mice, Mutant Strains, Neutrophils immunology, STAT6 Transcription Factor metabolism, T-Box Domain Proteins genetics, Th2 Cells cytology, Trachea immunology, Asthma immunology, Eosinophils immunology, T-Box Domain Proteins physiology, Th2 Cells immunology

Abstract

Background: Previous studies have shown that mice lacking T-bet, a critical transcription factor for T(H)1 cell differentiation, spontaneously develop airway inflammation with intense eosinophil infiltrates. However, the mechanism underlying T-bet-mediated inhibition of allergic airway inflammation is still unknown., Objective: To determine the regulatory role of T-bet in antigen-induced allergic airway inflammation., Methods: We examined the role of T-bet in antigen-induced allergic airway inflammation using T-bet(-/-) mice on a BALB/c background that did not develop spontaneous airway inflammation. We also examined the role of T-bet expression of CD4(+) T cells in airway inflammation by adoptive transfer experiments., Results: We found that antigen-induced eosinophil recruitment, goblet cell hyperplasia, and T(H)2 cytokine production in the airways were enhanced in T-bet(-/-) mice. However, in the absence of signal transducer and activator of transcription 6 (STAT6), T-bet deficiency could not induce the antigen-induced eosinophilic airway inflammation. Adoptive transfer of T-bet(-/-) or T-bet(+/+) CD4(+) T cells to T-bet(-/-)Rag-2(-/-) mice revealed that the expression of T-bet in CD4(+) T cells was vital for the inhibition of antigen-induced eosinophilic airway inflammation. Interestingly, antigen-induced neutrophil recruitment in the airways was also enhanced in T-bet(-/-) mice. Moreover, T-bet(-/-) CD4(+) T cells preferentially differentiated into IL-17-producing cells that mediated neutrophilic airway inflammation., Conclusion: T-bet inhibits both T(H)2 cell-mediated eosinophilic inflammation and T(H)17 cell-mediated neutrophilic inflammation in the airways., Clinical Implications: The dysfunction of T-bet may be involved in the pathogenesis of severe asthma, in which accumulation of neutrophils as well as eosinophils in the airways is a hallmark of disease.

Published

2007