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6. Blut- und Harnbestandteile

Author

Luszczak, A., Grassberger, R., Hüfner, G., Loewy, A., Zuntz, N., Fischinger, O., May, J., Seydel, F., Oettel, H., Schmidt, O., Frederick, R. C., Kohn-Abrest, E., Froman, J., Leinzinger, Maria, Häusler, H., Rappaport, F., Gottdenker, F., Kanitz, H. R., Apitzsch, J., Hecht, G., Hayes, F. R., Mansfeld, G., Scheff-Pfeifer, Irene, Lugg, J. W. H., Robbins, B. H., Orcutt, F. S., Waters, R. M., Seevers, M. H., Gutschmidt, J., Hinsberg, K., Breutel, E., Friedemann, Theodore E., Klaas, Rosalind, Hallén-Paulsen, L., Gershenfeld, L., Pojurowski, S. D., Looney, J. M., Walsh, Anna I., Florkin, M., Gomez, J., Bing, J., Guyader, G., Campbell, W. R., Hanna, Marion I., Reifer, J., Schalm, L., Danielson, I. S., d'Alessio, Rosa C., Fromageot, Cl., Heitz, P., Jones, D. B., Moeller, O., Desnuelle, P., Sullivan, M. X., Hess, W. C., Popovici, N., Radulescu, A., Hunter, A., Pettigrew, J. B., Jansen, B. C. P., Dauphinee, J. A., Krebs, H. A., Henseleit, K., van Slyke, D. D., Rapoport, S., Eichinger, W., Voisenet, E., Rosenthal, H. G., Binet, L., Weller, G., Hartner, F., Sehleiß, E., Code, C. F., Eggerth, A. H., Littwin, R. J., Deutsch, Joyce V., Koessler, K. K., Hanke, M. T., Kahane, E., Levy, Jeanne, Claudatus, I., Botezatu, M., Kisch, B., Beattie, Florence, Yoshimatsu, S. I., Andes, J. E., Myers, V. C., Greenwald, I., Eucker, H., Böhm, F., Grüner, G., Ludwig, H., Salkowski, E., Euler, H. v., Raekallio, T., Cattelain, E., Chabrier, P., Tchitchibabine, A., Hoffmann, Ch., Schulemann, W., Schönhöfer, F., Wingler, A., Brundage, J. T., Gruber, Ch. M., Reimers, F., Marshall, Jr., E. K., Emerson, Jr., K., Cutting, W. C., Frehden, O., Huang, Chen-Hua, Nosaka, K., Genkin, A. M., Simonovits, S., Wierzuchowski, M., Dzisiów, F., Sysa, J., Borkowski, Z., Colutta, A., and Herbert, Freda Katharine

Published
1941
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9. Nomenclatural note on a Thecadinium species (Dinophyceae, Gonyaulacales), which was described as new independently three times within two months

Author

Hoppenrath, M., Bolch, C. J. S., Yoshimatsu, S., Saldariaga, J. F., Schweikert, M., Campell, C. N., Toriumi, S., Dodge, J. D., Elbrächter, Malte, Taylor, F. J. R., Hoppenrath, M., Bolch, C. J. S., Yoshimatsu, S., Saldariaga, J. F., Schweikert, M., Campell, C. N., Toriumi, S., Dodge, J. D., Elbrächter, Malte, and Taylor, F. J. R.

Published
2005

10. Hypophosphataemia among severely-malnourished children: case series.

Author

Yoshimatsu S, Chisti MJ, Hossain MI, Islam MM, Fukushima T, Wagatsuma Y, Smith JH, Sumazaki R, Ahmed T, Yoshimatsu, Shoji, Chisti, Mohammod Jobayer, Hossain, Md Iqbal, Islam, Md Munirul, Fukushima, Takashi, Wagatsuma, Yukiko, Smith, Jonathan Harvey, Sumazaki, Ryo, and Ahmed, Tahmeed

Abstract

Phosphorus is an essential substance in our body, and hypophosphataemia (HP) is well-described in rickets, refeeding syndrome, diabetic ketoacidosis (DKA), and in chronic alcohol-abuse. However, to our knowledge, HP among severely-malnourished children has not been studied in detail, and information on prevalence, severity, and treatment is scarce. Currently, there are only a few published case reports of HP. This case series describes three cases of HP that presented to Dhaka Hospital of the International Centre for Diarrhoeal Disease Research, Bangladesh (icddr,b). Our first case required mechanical ventilation for respiratory distress associated with severe hypokalaemia (K 1.1 mmol/L) and moderate hypophosphataemia (P 2.1 mg/dL). The second case presented with severe sepsis which was associated with symptomatic hypocalcaemia (Ca 1.68 mmol/L), hypokalaemia (K 1.82 mmol/L), and severe hypophosphataemia (P 0.9 mg/dL). The third case presented with pneumonia and sepsis which were complicated by hypokalaemia (K 2.05 mmol/L) and severe hypophosphataemia (P 1.1 mg/dL). Marked lethargy and severe hypotonia were associated with HP in all of these cases. Manifestations of HP are diverse and can occur in association with other electrolyte imbalances, especially among malnourished children. Malnutrition, combined with sepsis, is one of the major killers of children younger than 5 years of age, and both malnutrition and sepsis can cause HP. It is concluded that the underlying causes of morbidity, including HP, should be actively sought and treated to reduce the mortality of children aged below five years. [ABSTRACT FROM AUTHOR]

Published
2012

11. Endoscopic and pathological manifestations of the gastrointestinal tract in familial amyloidotic polyneuropathy type I (Met30).

Author

Yoshimatsu, Shin-ichi, ando, Yukio, terazaki, Hisayasu, sakashita, Naomi, Tada, Shuji, Yamashita, Taro, Suga, Moritaka, Uchino, Makoto, Ando, Yukio, Yoshimatsu, S, Ando, Y, Terazaki, H, Sakashita, N, Tada, S, Yamashita, T, Suga, M, Uchino, M, and Ando, M

Subjects
GASTROINTESTINAL diseases, AMYLOIDOSIS, PROTEIN analysis, AMYLOID, AUTOPSY, BIOPSY, COLONOSCOPY, COMPARATIVE studies, DIGESTIVE organs, ESOPHAGUS, GASTROSCOPY, INTESTINES, RESEARCH methodology, MEDICAL cooperation, GENETIC mutation, PERIPHERAL neuropathy, RESEARCH, STOMACH, EVALUATION research
Abstract

Yoshimatsu S, Ando Y, Terazaki H, Sakashita N, Tada S, Yamashita T, Suga M, Uchino M, Ando M (Kumamoto University School of Medicine; and Saiseikai Hospital, Kumamoto, Japan). Endoscopic and pathological manifestations of the gastrointestinal tract in familial amyloidotic polyneuropathy type I (Met30). J Intern Med 1998; 243: 65–72. ObjectivesTo evaluate the characteristic changes in the gastrointestinal tract in familial amyloidotic polyneuropathy (FAP) (Met30), both fibre gastroscopy and colonoscopy studies were performed in FAP (Met30) patients. Microscopic changes were also examined in autopsied and biopsied materials from patients with FAP, and compared with data from autopsied samples from patients with AL amyloidosis, and secondary amyloidosis patients. DesignEndoscopic and histopathological study. SettingKumamoto University Hospital, Kumamoto, Japan. SubjectsNine patients with FAP (Met30) underwent fibre gastroscopy and colonoscopy. Six autopsied and 23 biopsied gastrointestinal samples from FAP patients, four from autopsied amyloidosis (including two myeloma associated form), and two from autopsied secondary amyloidosis patients were examined for histopathological study. Main outcome measuresFibre gastroscopy and colonoscopy were employed for macroscopic study. Congo red and H-E staining were performed for histopathological study. Macroscopic changes in the gastrointestinal tract and microscopic differences in the amyloid distribution pattern were compared between the different types of amyloidosis. ResultsFibre gastroscopy and colonoscopy for nine FAP patients revealed that four showed a fine granular appearance in the duodenum, three showed lack of lustre, and two showed mucosal friability in the gastrointestinal tract; however, no macroscopic abnormality was observed in four other FAP patients. Histopathological examination of tissue from FAP patients revealed that, although a small amount of amyloid was recognized in the submucosa perivascular layer, a significant amount of amyloid was seen in and around the nerves of the gastrointestinal tract, but very little in Auerbach's nerve plexus. In total, the amount of deposited amyloid in the tissues was small compared with that in other types of systemic amyloidosis, such as AL and secondary amyloidosis. ConclusionThese results suggest that the major reason why FAP patients show such severe gastrointestinal symptoms, compared with other types of systemic amyloidosis, may be because of the deposition of a significant amount of amyloid in the nerves in the gastrointestinal tract. [ABSTRACT FROM AUTHOR]

Published
1998
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12. Idiopathic myointimal hyperplasia of mesenteric veins: radiological evaluation using CT angiography.

Author

Morimura F, Edo H, Niwa T, Sugiura H, Suyama Y, Okazaki S, Narimatsu K, Ohno H, Okamoto K, Ueno H, Yoshimatsu S, Miyai K, Hamamoto K, and Shinmoto H

Abstract

A 44-year-old man presented with a chief complaint of constipation. Initial contrast-enhanced CT showed extensive bowel wall thickening, mainly in the left colon, with a thin cord-like inferior mesenteric vein (IMV), in contrast to ectatic mesenteric venous branches, suggesting bowel ischaemia owing to venous stasis. One month later, at the time of symptom exacerbation, CT angiography showed a cord-like IMV and ectatic mesenteric venous branches with early enhancement, suggesting the presence of an arteriovenous fistula (AVF). Owing to the progression of bowel ischaemia and necrosis with peritonitis, emergency surgery was performed. Surgical specimens showed focal myointimal hyperplasia of the proximal mesenteric veins in both ischaemic and non-ischaemic lesions of the resected colon, thus leading to the diagnosis of idiopathic myointimal hyperplasia of mesenteric veins (IMHMV) when combined with the clinical and imaging findings. IMHMV is a bowel ischaemic disease caused by non-thrombotic venous obstruction that requires bowel resection and has been suggested to be associated with AVF. Cord-like IMV and AVF in the mesentery are important CT findings that characterize IMHMV. CT angiography is useful in diagnosing IMHMV., Competing Interests: None declared., (© The Author(s) 2023. Published by Oxford University Press on behalf of the British Institute of Radiology.)

Published
2023
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13. Generation of a tyrosine hydroxylase-2A-Cre knockin non-human primate model by homology-directed-repair-biased CRISPR genome editing.

Author

Yoshimatsu S, Okahara J, Yoshie J, Igarashi Y, Nakajima R, Sanosaka T, Qian E, Sato T, Kobayashi H, Morimoto S, Kishi N, Pillis DM, Malik P, Noce T, and Okano H

Subjects
Animals, Tyrosine 3-Monooxygenase genetics, Primates genetics, Mammals genetics, Gene Editing, CRISPR-Cas Systems genetics
Abstract

Non-human primates (NHPs) are the closest animal model to humans; thus, gene engineering technology in these species holds great promise for the elucidation of higher brain functions and human disease models. Knockin (KI) gene targeting is a versatile approach to modify gene(s) of interest; however, it generally suffers from the low efficiency of homology-directed repair (HDR) in mammalian cells, especially in non-expressed gene loci. In the current study, we generated a tyrosine hydroxylase (TH)-2A-Cre KI model of the common marmoset monkey (marmoset; Callithrix jacchus) using an HDR-biased CRISPR-Cas9 genome editing approach using Cas9-DN1S and RAD51. This model should enable labeling and modification of a specific neuronal lineage using the Cre-loxP system. Collectively, the current study paves the way for versatile gene engineering in NHPs, which may be a significant step toward further biomedical and preclinical applications., Competing Interests: Declaration of interests H.O. has been a paid scientific advisory board member of San Bio Co. Ltd., Regenerative Medicine iPS Gateway Center Co. Ltd., and K Pharma, Inc. S.Y. has been a paid associate researcher of Daiichi-Sankyo RD Novare Co. Ltd. However, there was no effect of these companies on the interpretation, writing, or publication of this study. H.O. and S.Y. declare that there are no non-financial conflicts of interest with this work. In addition, the other authors declare that there are neither financial nor non-financial conflicts of interest., (Copyright © 2023 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published
2023
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14. A human induced pluripotent stem cell model from a patient with hereditary cerebral small vessel disease carrying a heterozygous R302Q mutation in HTRA1.

Author

Qian E, Uemura M, Kobayashi H, Nakamura S, Ozawa F, Yoshimatsu S, Ishikawa M, Onodera O, Morimoto S, and Okano H

Abstract

Cerebral autosomal recessive arteriopathy with subcortical infarcts and leukoencephalopathy (CARASIL) is an inherited cerebral small vessel disease (CSVD) caused by biallelic mutations in the high-temperature requirement serine peptidase A1 (HTRA1) gene. Even heterozygous mutations in HTRA1 are recently revealed to cause cardinal clinical features of CSVD. Here, we report the first establishment of a human induced pluripotent stem cell (hiPSC) line from a patient with heterozygous HTRA1-related CSVD. Peripheral blood mononuclear cells (PBMCs) were reprogrammed by the transfection of episomal vectors encoding human OCT3/4 (POU5F1), SOX2, KLF4, L-MYC, LIN28, and a murine dominant-negative mutant of p53 (mp53DD). The established iPSCs had normal morphology as human pluripotent stem cells and normal karyotype (46XX). Moreover, we found that the HTRA1 missense mutation (c.905G>A, p.R302Q) was heterozygous. These iPSCs expressed pluripotency-related markers and had the potential to differentiate into all three germ layers in vitro. HTRA1 and the supposed disease-associated gene NOG were differentially expressed in the patient iPSCs at mRNA levels compared to those of control lines. The iPSC line would facilitate in vitro research for understanding the cellular pathomechanisms caused by the HTRA1 mutation including its dominant-negative effect., (© 2023. The Author(s).)

Published
2023
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15. Attempts for deriving extended pluripotent stem cells from common marmoset embryonic stem cells.

Author

Yoshimatsu S, Nakajima M, Sonn I, Natsume R, Sakimura K, Nakatsukasa E, Sasaoka T, Nakamura M, Serizawa T, Sato T, Sasaki E, Deng H, and Okano H

Subjects
Animals, Humans, Mice, Cell Differentiation, Gene Expression Profiling, Transcriptome, Callithrix, Embryonic Stem Cells metabolism
Abstract

Extended pluripotent stem cells (EPSCs) derived from mice and humans showed an enhanced potential for chimeric formation. By exploiting transcriptomic approaches, we assessed the differences in gene expression profile between extended EPSCs derived from mice and humans, and those newly derived from the common marmoset (marmoset; Callithrix jacchus). Although the marmoset EPSC-like cells displayed a unique colony morphology distinct from murine and human EPSCs, they displayed a pluripotent state akin to embryonic stem cells (ESCs), as confirmed by gene expression and immunocytochemical analyses of pluripotency markers and three-germ-layer differentiation assay. Importantly, the marmoset EPSC-like cells showed interspecies chimeric contribution to mouse embryos, such as E6.5 blastocysts in vitro and E6.5 epiblasts in vivo in mouse development. Also, we discovered that the perturbation of gene expression of the marmoset EPSC-like cells from the original ESCs resembled that of human EPSCs. Taken together, our multiple analyses evaluated the efficacy of the method for the derivation of marmoset EPSCs., (© 2022 Molecular Biology Society of Japan and John Wiley & Sons Australia, Ltd.)

Published
2023
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16. Comparison of endoscopic submucosal resection with ligation and endoscopic submucosal dissection for small rectal neuroendocrine tumors: A multicenter retrospective study.

Author

Matsuno K, Miyamoto H, Kitada H, Yoshimatsu S, Tamura F, Sakurai K, Fukubayashi K, Shono T, Setoyama H, Matsuyama T, Suko S, Narita R, Honda M, Tateyama M, Naoe H, Morinaga J, Tanaka Y, and Gushima R

Abstract

Objectives: Endoscopic submucosal resection with band ligation (ESMR-L) and endoscopic submucosal dissection (ESD) are both standard endoscopic resection methods for rectal neuroendocrine tumors (NETs) <10 mm in size. However, there is no definitive consensus on which is better. Here, we compared the efficacy of ESMR-L and ESD for small rectal NETs., Methods: This was a multicenter retrospective cohort study including 205 patients with rectal NETs who underwent ESMR-L or ESD. Treatment outcomes were compared by univariate analysis, multivariate analysis, and inverse probability treatment weighting (IPTW) using propensity scores. Subgroup analysis evaluated the impact of the endoscopist's experience on the technical outcome., Results: Eighty-nine patients were treated by ESMR-L and 116 by ESD. The R0 resection rate was not significantly different between the two (90% vs. 92%, p = 0.73). The procedure time of ESMR-L was significantly shorter than for ESD (17 min vs. 52 min, p < 0.01) and the hospitalization period was also significantly shorter (3 days vs. 5 days, p < 0.01). These results were confirmed by multivariate analysis and also after IPTW adjustment. The procedure time of ESD was significantly prolonged by a less-experienced endoscopist (49 min vs. 70 min, p = 0.02), but that of ESMR-L was not affected (17 min vs. 17 min, p = 0.27)., Conclusions: For small rectal NETs, both ESMR-L and ESD showed similar high complete resection rates. However, considering the shorter procedure time and shorter hospitalization period, ESMR-L is the more efficient treatment method, especially for less-experienced endoscopists., Competing Interests: None., (© 2022 The Authors. DEN Open published by John Wiley & Sons Australia, Ltd on behalf of Japan Gastroenterological Endoscopy Society.)

Published
2022
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17. Accelerated neuronal aging in vitro ∼melting watch ∼.

Author

Inagaki E, Yoshimatsu S, and Okano H

Abstract

In developed countries, the aging of the population and the associated increase in age-related diseases are causing major unresolved medical, social, and environmental matters. Therefore, research on aging has become one of the most important and urgent issues in life sciences. If the molecular mechanisms of the onset and progression of neurodegenerative diseases are elucidated, we can expect to develop disease-modifying methods to prevent neurodegeneration itself. Since the discovery of induced pluripotent stem cells (iPSCs), there has been an explosion of disease models using disease-specific iPSCs derived from patient-derived somatic cells. By inducing the differentiation of iPSCs into neurons, disease models that reflect the patient-derived pathology can be reproduced in culture dishes, and are playing an active role in elucidating new pathological mechanisms and as a platform for new drug discovery. At the same time, however, we are faced with a new problem: how to recapitulate aging in culture dishes. It has been pointed out that cells differentiated from pluripotent stem cells are juvenile, retain embryonic traits, and may not be fully mature. Therefore, attempts are being made to induce cell maturation, senescence, and stress signals through culture conditions. It has also been reported that direct conversion of fibroblasts into neurons can reproduce human neurons with an aged phenotype. Here, we outline some state-of-the-art insights into models of neuronal aging in vitro . New frontiers in which stem cells and methods for inducing differentiation of tissue regeneration can be applied to aging research are just now approaching, and we need to keep a close eye on them. These models are forefront and intended to advance our knowledge of the molecular mechanisms of aging and contribute to the development of novel therapies for human neurodegenerative diseases associated with aging., Competing Interests: HO was a founder scientist and a Scientific Advisory Board member for SanBio Co., Ltd., and K Pharma Inc. The remaining authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2022 Inagaki, Yoshimatsu and Okano.)

Published
2022
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18. Clinically undetected plasmacytoid urothelial carcinoma of the urinary bladder with non-mass-forming metastases in multiple organs: an autopsy case.

Author

Asano Y, Miyai K, Yoshimatsu S, Sasaki M, Ikewaki K, and Matsukuma S

Abstract

This case report outlines a clinically undetected urinary bladder plasmacytoid urothelial carcinoma (PUC) with multiple metastases detected at autopsy. An 89-year-old man presented with edema in the lower limbs. Pleural fluid cytology revealed discohesive carcinomatous cells, although imaging studies failed to identify the primary site of tumor. The patient died of respiratory failure. Autopsy disclosed a prostate tumor and diffusely thickened urinary bladder and rectum without distinct tumorous lesions. Histologically, the tumor consisted of acinar-type prostate adenocarcinoma with no signs of metastasis. Additionally, small, plasmacytoid tumor cells were observed in the urinary bladder/rectum as isolated or small clustering fashions. These metastasized to the lungs, intestine, generalized lymph nodes in a non-mass-forming manner. Combined with immunohistochemical studies, these tumor cells were diagnosed PUC derived from the urinary bladder. Both clinicians and pathologists should recognize PUC as an aggressive histological variant, which can represent a rapid systemic progression without mass-forming lesions.

Published
2022
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19. Single transcription factor efficiently leads human induced pluripotent stem cells to functional microglia.

Author

Sonn I, Honda-Ozaki F, Yoshimatsu S, Morimoto S, Watanabe H, and Okano H

Abstract

Background: Microglia are innate immune cells that are the only residential macrophages in the central nervous system. They play vital physiological roles in the adult brain and during development. Microglia are particularly in the spotlight because many genetic risk factors recently identified for neurodegenerative diseases are largely expressed in microglia. Rare polymorphisms in these risk alleles lead to abnormal activity of microglia under traumatic or disease conditions., Methods: In the present study, to investigate the multifaceted functions of human microglia, we established a novel robust protocol to generate microglia from human induced pluripotent stem cells (hiPSCs) using a combination of cytokines and small chemicals essential for microglia ontogeny. Moreover, we highly enhanced the microglial differentiation efficiency by forcing the expression of PU.1, a crucial transcription factor for microglial development, during posterior mesoderm differentiation., Results: By our novel method, we demonstrated the generation of a greater number of hiPSC-derived microglia (hiMGLs, approximately 120-folds) than the prior methods (at most 40-folds). Over 90% of the hiMGLs expressed microglia-specific markers, such as CX3CR1 and IBA-1. Whole-transcriptome analysis revealed that these hiMGLs are similar to human primary microglia but differ from monocytes/macrophages. Furthermore, the specific physiological functions of microglia were confirmed through indices of lipopolysaccharide responsiveness, phagocytotic ability, and inflammasome formation. By co-culturing these hiMGLs with mouse primary neurons, we demonstrated that hiMGLs can regulate the activity and maturation of neurons., Conclusions: In this study, our new simple, rapid, and highly efficient method for generating microglia from hiPSCs will prove useful for future investigations on microglia in both physiological and disease conditions, as well as for drug discovery., (© 2022. The Author(s).)

Published
2022
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20. A New Horizon in Reproductive Research with Pluripotent Stem Cells: Successful In Vitro Gametogenesis in Rodents, Its Application to Large Animals, and Future In Vitro Reconstitution of Reproductive Organs Such as "Uteroid" and "Oviductoid".

Author

Yoshimatsu S, Kisu I, Qian E, and Noce T

Abstract

Recent success in derivation of functional gametes (oocytes and spermatozoa) from pluripotent stem cells (PSCs) of rodents has made it feasible for future application to large animals including endangered species and to ultimately humans. Here, we summarize backgrounds and recent studies on in vitro gametogenesis from rodent PSCs, and similar approaches using PSCs from large animals, including livestock, nonhuman primates (NHPs), and humans. We also describe additional developing approaches for in vitro reconstitution of reproductive organs, such as the ovary (ovarioid), testis (testisoid), and future challenges in the uterus (uteroid) and oviduct (oviductoid), all of which may be derived from PSCs. Once established, these in vitro systems may serve as a robust platform for elucidating the pathology of infertility-related disorders and ectopic pregnancy, principle of reproduction, and artificial biogenesis. Therefore, these possibilities, especially when using human cells, require consideration of ethical issues, and international agreements and guidelines need to be raised before opening "Pandora's Box".

Published
2022
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21. Critical roles of FGF, RA, and WNT signalling in the development of the human otic placode and subsequent lineages in a dish.

Author

Saeki T, Yoshimatsu S, Ishikawa M, Hon CC, Koya I, Shibata S, Hosoya M, Saegusa C, Ogawa K, Shin JW, Fujioka M, and Okano H

Abstract

Introduction: Efficient induction of the otic placode, the developmental origin of the inner ear from human pluripotent stem cells (hPSCs), provides a robust platform for otic development and sensorineural hearing loss modelling. Nevertheless, there remains a limited capacity of otic lineage specification from hPSCs by stepwise differentiation methods, since the critical factors for successful otic cell differentiation have not been thoroughly investigated. In this study, we developed a novel differentiation system involving the use of a three-dimensional (3D) floating culture with signalling factors for generating otic cell lineages via stepwise differentiation of hPSCs., Methods: We differentiated hPSCs into preplacodal cells under a two-dimensional (2D) monolayer culture. Then, we transferred the induced preplacodal cells into a 3D floating culture under the control of the fibroblast growth factor (FGF), bone morphogenetic protein (BMP), retinoic acid (RA) and WNT signalling pathways. We evaluated the characteristics of the induced cells using immunocytochemistry, quantitative PCR (qPCR), population averaging, and single-cell RNA-seq (RNA-seq) analysis. We further investigated the methods for differentiating otic progenitors towards hair cells by overexpression of defined transcription factors., Results: We demonstrated that hPSC-derived preplacodal cells acquired the potential to differentiate into posterior placodal cells in 3D floating culture with FGF2 and RA. Subsequent activation of WNT signalling induced otic placodal cell formation. By single-cell RNA-seq (scRNA-seq) analysis, we identified multiple clusters of otic placode- and otocyst marker-positive cells in the induced spheres. Moreover, the induced otic cells showed the potential to generate hair cell-like cells by overexpression of the transcription factors ATOH1, POU4F3 and GFI1 ., Conclusions: We demonstrated the critical role of FGF2, RA and WNT signalling in a 3D environment for the in vitro differentiation of otic lineage cells from hPSCs. The induced otic cells had the capacity to differentiate into inner ear hair cells with stereociliary bundles and tip link-like structures. The protocol will be useful for in vitro disease modelling of sensorineural hearing loss and human inner ear development and thus contribute to drug screening and stem cell-based regenerative medicine., Competing Interests: H.O. is a founding scientist and scientific advisor of SanBio Co. Ltd. and K Pharma Inc. M.H., K.O. and M.F. are co-founders of Otolink Inc. The other authors indicate no potential conflicts of interest., (© 2022 The Japanese Society for Regenerative Medicine. Production and hosting by Elsevier B.V.)

Published
2022
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22. Early development of the cochlea of the common marmoset, a non-human primate model.

Author

Hosoya M, Fujioka M, Okahara J, Yoshimatsu S, Okano H, and Ozawa H

Subjects
Animals, Cell Differentiation, Humans, Callithrix genetics, Cochlea
Abstract

Background: Fine-tuned cochlear development is essential for hearing. Owing to the difficulty in using early human fetal samples, most of our knowledge regarding cochlear development has been obtained from rodents. However, several inter-species differences in cochlear development between rodents and humans have been reported. To bridge these differences, we investigated early otic development of a non-human primate model animal, the common marmoset (Callithrix jacchus)., Methods: We examined 20 genes involved in early cochlear development and described the critical developmental steps for morphogenesis, which have been reported to vary between rodents and marmosets., Results: The results revealed that several critical genes involved in prosensory epithelium specifications showed higher inter-species differences, suggesting that the molecular process for hair cell lineage acquisition in primates differs considerably from that of rodents. We also observed that the tempo of cochlear development was three times slower in the primate than in rodents., Conclusions: Our data provide new insights into early cochlear development in primates and humans and imply that the procedures used for manipulating rodent cochlear sensory cells cannot be directly used for the research of primate cells due to the intrinsic inter-species differences in the cell fate determination program., (© 2022. The Author(s).)

Published
2022
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23. Homologous Recombination-Enhancing Factors Identified by Comparative Transcriptomic Analyses of Pluripotent Stem Cell of Human and Common Marmoset.

Author

Yoshimatsu S, Nakajima M, Qian E, Sanosaka T, Sato T, and Okano H

Subjects
Animals, Embryonic Stem Cells metabolism, Gene Editing, Homologous Recombination, Humans, Callithrix, Transcriptome genetics
Abstract

A previous study assessing the efficiency of the genome editing technology CRISPR-Cas9 for knock-in gene targeting in common marmoset (marmoset; Callithrix jacchus) embryonic stem cells (ESCs) unexpectedly identified innately enhanced homologous recombination activity in marmoset ESCs. Here, we compared gene expression in marmoset and human pluripotent stem cells using transcriptomic and quantitative PCR analyses and found that five HR-related genes (BRCA1, BRCA2, RAD51C, RAD51D, and RAD51) were upregulated in marmoset cells. A total of four of these upregulated genes enhanced HR efficiency with CRISPR-Cas9 in human pluripotent stem cells. Thus, the present study provides a novel insight into species-specific mechanisms for the choice of DNA repair pathways.

Published
2022
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24. Immunoglobulin G4-related disease accompanying a small intestinal ulcer: A case.

Author

Yoshidome Y, Mizoguchi A, Narimatsu K, Takahashi S, Hirata D, Ono S, Onoyama Y, Suzuki S, Horiuchi T, Chiya N, Ikeyama K, Tahara H, Tomioka A, Ito S, Tanemoto R, Nishii S, Inaba K, Sugihara N, Hanawa Y, Horiuchi K, Wada A, Akita Y, Higashiyama M, Komoto S, Tomita K, Yoshimatsu S, Matsukuma S, and Hokari R

Abstract

Immunoglobulin (Ig)G4-related disease (IgG4-RD) is a systemic condition associated with fibroinflammatory lesions and is characterized by elevated serum IgG4 levels and IgG4-positive cell infiltration into the affected tissues. It has been reported that IgG4-RD affects a variety of organs but uncommonly affects the gastrointestinal tract. In particular, there are few cases of lesions in the small intestine, except for sclerosing mesenteritis, which were mostly diagnosed from surgical specimens. Herein, we describe the case of a 70-year-old man who initially presented with abdominal pain, headache, later cognitive decline, and gait disturbance caused by IgG4-RD. Colonoscopy revealed irregular ulcers in the terminal ileum, and computed tomography of the head showed hypertrophic pachymeningitis. Numerous IgG4-positive cells were detected in the ileal and dural biopsies. We diagnosed the patient with IgG4-RD and started steroid pulse therapy. After initiation of treatment, the symptoms quickly improved. The patient was discharged from the hospital after starting oral prednisolone treatment (30 mg). The dosage was gradually reduced to 10 mg. A follow-up colonoscopy revealed scarring of the ileal ulcers. This case may provide valuable information regarding the endoscopic findings of small intestinal lesions in IgG4-RD., Competing Interests: The authors declare that they have no conflict of interest., (© 2021 The Authors. DEN Open published by John Wiley & Sons Australia, Ltd on behalf of Japan Gastroenterological Endoscopy Society.)

Published
2021
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25. Generation of a control human induced pluripotent stem cell line using the defective and persistent Sendai virus vector system.

Author

Zhou Z, Yoshimatsu S, Qian E, Ishikawa M, Sato T, Ohtaka M, Nakanishi M, and Okano H

Subjects
Cell Differentiation, Cellular Reprogramming, Female, Fibroblasts, Genetic Vectors genetics, Humans, Sendai virus genetics, Transgenes, Induced Pluripotent Stem Cells
Abstract

The defective and persistent Sendai virus (SeVdp) vector system allows efficient generation of transgene-free induced pluripotent stem cells (iPSCs) from human somatic cells. By leveraging the system, here we report the generation of an iPSC line from somatic fibroblasts of a healthy control donner (female), named KEIOi002-A (also named YG-iPS). The control iPSC line would be a useful resource for stem cell research and regenerative medicine., (Copyright © 2021 The Authors. Published by Elsevier B.V. All rights reserved.)

Published
2021
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26. Establishing an induced pluripotent stem cell line from neonatal common marmoset fibroblasts by an all-in-one episomal vector approach.

Author

Yoshimatsu S, Qian E, Sato T, Yamamoto M, Ishikawa M, and Okano H

Subjects
Animals, Callithrix, Cell Differentiation, Fibroblasts, Herpesvirus 4, Human, Epstein-Barr Virus Infections, Induced Pluripotent Stem Cells
Abstract

Epstein-Barr virus (EBV)-based episomal vector system enables persistent transgene expression, which is advantageous for efficient derivation of transgene-free induced pluripotent stem cells (iPSCs) without viral transduction. Here, we report establishment of an iPSC line from somatic fibroblasts of a neonatal common marmoset monkey (marmoset; Callithrix jacchus) using an all-in-one episomal vector that we newly developed. The established iPSC line, named NM-iPS, showed standard characteristics of pluripotency such as pluripotency-related marker expression, three germ layer differentiation, and normal karyotype (2n = 46). The novel iPSC line would be a useful resource for stem cell research using non-human primates., (Published by Elsevier B.V.)

Published
2021
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27. Establishment of an induced pluripotent stem cell line from a female domestic ferret (Mustela putorius furo) with an X chromosome instability.

Author

Yoshimatsu S, Murakami R, Nakajima M, Sato T, Kawasaki H, and Okano H

Subjects
Animals, Chromosomal Instability, Disease Models, Animal, Female, X Chromosome, Ferrets genetics, Induced Pluripotent Stem Cells
Abstract

The domestic ferret (ferret; Mustela putorius furo) is an important animal model for neuroscience and preclinical/veterinary medicine owing to its highly developed cerebral cortex and susceptibility to avian influenza and corona viruses. Nevertheless, there is a lack of in vitro ferret models, since immortal cell lines including induced pluripotent stem cells (iPSCs) of ferrets have been scarce. In this study, we established an iPSC line from ferret skin fibroblasts. The established iPSC line, fiPS-1, showed standard characteristics of pluripotency, but its X chromosome was unstable. Collectively, the present study provides a useful resource for in vitro model using the ferret., (Copyright © 2021 The Author(s). Published by Elsevier B.V. All rights reserved.)

Published
2021
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28. Non-viral derivation of a transgene-free induced pluripotent stem cell line from a male beagle dog.

Author

Yoshimatsu S, Edamura K, Yoshii Y, Iguchi A, Kondo H, Shibuya H, Sato T, Shiozawa S, and Okano H

Subjects
Animals, Cell Differentiation, Dogs, Female, Fibroblasts, Male, Stem Cell Research, Transgenes, Induced Pluripotent Stem Cells
Abstract

We previously reported the non-viral derivation of transgene-free induced pluripotent stem cells (iPSCs) from somatic fibroblasts of a female beagle dog using an optimized induction medium and integration-free episomal vectors. Here, we report novel derivation of a male canine iPSC line OF35Y-iPS, which showed standard characteristics of pluripotency such as a strong gene expression profile of pluripotency markers, differentiation potential into all three germ layers, and normal karyotype (78XY). Furthermore, we demonstrated targeted integration of 2A-EGFP into the canine NANOS3 locus. The novel iPSC line would be a useful resource for stem cell research and regenerative veterinary medicine., (Copyright © 2021 The Author(s). Published by Elsevier B.V. All rights reserved.)

Published
2021
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29. Generation of a common marmoset embryonic stem cell line CMES40-OC harboring a POU5F1 (OCT4)-2A-mCerulean3 knock-in reporter allele.

Author

Yoshimatsu S, Murakami R, Sato T, Saeki T, Yamamoto M, Sasaki E, Noce T, and Okano H

Subjects
Alleles, Animals, Cell Differentiation, Cell Line, Embryonic Stem Cells, Octamer Transcription Factor-3 genetics, Callithrix, Genes, Homeobox
Abstract

POU class 5 homeobox 1 (POU5F1, also known as OCT4) is critical for maintenance of pluripotency, germ cell fate, reprogramming into a pluripotent state, and early embryogenesis. We generated an embryonic stem cell (ESC) line of the common marmoset (Callithrix jacchus) harboring a heterozygous knock-in allele of OCT4-P2A-mCerulean-T2A-pac. The ESC line (CMES40-OC) will be valuable for investigation of primed/naïve pluripotency and germ cell fate. Homozygous OCT4 knock-in clones were generated but could not be sustained in an undifferentiated state in long-term culture. The OCT4 knock-in system facilitated simultaneous knock-in of a reporter construct at another locus, DDX4 (VASA)., (Copyright © 2021 The Authors. Published by Elsevier B.V. All rights reserved.)

Published
2021
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30. Non-viral Induction of Transgene-free iPSCs from Somatic Fibroblasts of Multiple Mammalian Species.

Author

Yoshimatsu S, Nakajima M, Iguchi A, Sanosaka T, Sato T, Nakamura M, Nakajima R, Arai E, Ishikawa M, Imaizumi K, Watanabe H, Okahara J, Noce T, Takeda Y, Sasaki E, Behr R, Edamura K, Shiozawa S, and Okano H

Subjects
Animals, Callithrix, Dogs, Gene Expression Profiling, Genetic Vectors metabolism, Germ Layers metabolism, Neural Stem Cells metabolism, Plasmids genetics, RNA, Messenger genetics, RNA, Messenger metabolism, RNA-Seq, Species Specificity, Swine, Viruses, Fibroblasts cytology, Induced Pluripotent Stem Cells cytology, Induced Pluripotent Stem Cells metabolism, Mammals metabolism, Transgenes
Abstract

Induced pluripotent stem cells (iPSCs) are capable of providing an unlimited source of cells from all three germ layers and germ cells. The derivation and usage of iPSCs from various animal models may facilitate stem cell-based therapy, gene-modified animal production, and evolutionary studies assessing interspecies differences. However, there is a lack of species-wide methods for deriving iPSCs, in particular by means of non-viral and non-transgene-integrating (NTI) approaches. Here, we demonstrate the iPSC derivation from somatic fibroblasts of multiple mammalian species from three different taxonomic orders, including the common marmoset (Callithrix jacchus) in Primates, the dog (Canis lupus familiaris) in Carnivora, and the pig (Sus scrofa) in Cetartiodactyla, by combinatorial usage of chemical compounds and NTI episomal vectors. Interestingly, the fibroblasts temporarily acquired a neural stem cell-like state during the reprogramming. Collectively, our method, robustly applicable to various species, holds a great potential for facilitating stem cell-based research using various animals in Mammalia., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2021
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31. Generation and validation of a common marmoset embryonic stem cell line ActiCre-B1 that ubiquitously expresses a tamoxifen-inducible Cre-driver.

Author

Yoshimatsu S, Ohtsu K, Sato T, Yamamoto M, Sasaki E, Shiozawa S, and Okano H

Subjects
Animals, Cell Differentiation, Embryonic Stem Cells, Integrases, Callithrix, Tamoxifen pharmacology
Abstract

We previously reported the efficient targeted introduction of transgenes into the genomic DNA of the common marmoset (Callithrix jacchus) using CRISPR-Cas9. In this study, we generated a marmoset embryonic stem cell (ESC) line that ubiquitously expresses the tamoxifen-inducible Cre-driver ERT2CreERT2. We validated the pluripotency of the ESC line and also successfully demonstrated the temporal control of the Cre-driver in a tamoxifen-dependent manner in the ESCs. This ESC line, named ActiCre-B1, will be a valuable resource for in vitro investigation of phenotypes related to embryonic lethality by targeted knockout of functionally important genes., (Copyright © 2021 The Author(s). Published by Elsevier B.V. All rights reserved.)

Published
2021
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32. Direct Neuronal Reprogramming of Common Marmoset Fibroblasts by ASCL1, microRNA-9/9*, and microRNA-124 Overexpression.

Author

Nemoto A, Kobayashi R, Yoshimatsu S, Sato Y, Kondo T, Yoo AS, Shiozawa S, and Okano H

Subjects
Animals, Callithrix, Cells, Cultured, Fibroblasts, Basic Helix-Loop-Helix Transcription Factors metabolism, Cellular Reprogramming, Disease Models, Animal, MicroRNAs, Nervous System Diseases metabolism, Neurons metabolism
Abstract

The common marmoset ( Callithrix jacchus ) has attracted considerable attention, especially in the biomedical science and neuroscience research fields, because of its potential to recapitulate the complex and multidimensional phenotypes of human diseases, and several neurodegenerative transgenic models have been reported. However, there remain several issues as (i) it takes years to generate late-onset disease models, and (ii) the onset age and severity of phenotypes can vary among individuals due to differences in genetic background. In the present study, we established an efficient and rapid direct neuronal induction method (induced neurons; iNs) from embryonic and adult marmoset fibroblasts to investigate cellular-level phenotypes in the marmoset brain in vitro. We overexpressed reprogramming effectors, i.e., microRNA-9/9*, microRNA-124, and Achaete-Scute family bHLH transcription factor 1, in fibroblasts with a small molecule cocktail that facilitates neuronal induction. The resultant iNs from embryonic and adult marmoset fibroblasts showed neuronal characteristics within two weeks, including neuron-specific gene expression and spontaneous neuronal activity. As directly reprogrammed neurons have been shown to model neurodegenerative disorders, the neuronal reprogramming of marmoset fibroblasts may offer new tools for investigating neurological phenotypes associated with disease progression in non-human primate neurological disease models.

Published
2020
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33. Generation of a male common marmoset embryonic stem cell line DSY127-BV8VT1 carrying double reporters specific for the germ cell linage using the CRISPR-Cas9 and PiggyBac transposase systems.

Author

Yoshimatsu S, Sato T, Yamamoto M, Sasaki E, Nakajima M, Nakamura M, Shiozawa S, Noce T, and Okano H

Subjects
Animals, CRISPR-Cas Systems genetics, Cell Differentiation, Germ Cells, Male, Callithrix, Cell Line, Embryonic Stem Cells, Transposases
Abstract

BLIMP1 (PRDM1) and VASA (DDX4) play pivotal roles in the development of the germ cell linage. Importantly, these genes are specifically expressed in germ cells; BLIMP1 in primordial germ cells (PGCs) to early-stage gonocytes, and VASA in migration-stage PGCs to mature gametes. The high reproductive efficiency of common marmosets (marmosets; Callithrix jacchus) makes them advantageous for use in germ cell research. We herein report the generation of a male marmoset embryonic stem cell (ESC) line harboring BLIMP1 and DDX4 double reporters. This ESC line will be a useful tool for investigating male gametogenesis in non-human primates., Competing Interests: Declaration of competing Interest H.O. serves as a paid scientific advisor at SanBio Co. Ltd. and K Pharma Inc. Rest of the authors declare there are no financial or non-financial competing interests with regard to this work., (Copyright © 2020 The Author(s). Published by Elsevier B.V. All rights reserved.)

Published
2020
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34. Low-Voltage Irreversible Electroporation Using a Comb-Shaped Contact Electrode.

Author

Kurata K, Yoshimatsu S, and Takamatsu H

Subjects
Ablation Techniques, Animals, Equipment Design, Mice, Microelectrodes, NIH 3T3 Cells, Phantoms, Imaging, Electroporation instrumentation, Electroporation methods
Abstract

Objective: Irreversible electroporation (IRE) is a less invasive therapy to ablate tumor cells by delivering short intensive electric pulses more than a few kV via needle-like electrodes. For reducing the required voltage for the IRE, a durable comb-shaped miniature electrode was designed to use in contact with the lesion surface for a new method named contact IRE., Methods: A miniature electrode was newly fabricated by a fine inkjet patterning and the subsequent etching of a copper-clad polyimide film. A train of 10-μs or 100-μs long electric pulses were applied 90 times at the interval of 1 s to a tissue phantom, and its cross section was observed to measure the necrotized area., Results: Cell experiments showed that the maximum ablation depth increased as a function of the applied voltage and reached 400 μm at 20 V. Furthermore, insulation of the lateral space between electrode teeth with a resin and administration of adjuvants to reduce the IRE threshold of the cell membrane did increase the ablation depth by 26% and the ablation area by 40%., Conclusion: The miniature electrode developed in this study successfully necrotized cells in a tissue phantom 400 μm deep from the surface with the electric pulses of only 20 V., Significance: The contact IRE for the surface of skin and gastrointestinal tract will ablate cutaneous and subcutaneous tumors by applying only several tens of volts.

Published
2020
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35. Pathological Progression Induced by the Frontotemporal Dementia-Associated R406W Tau Mutation in Patient-Derived iPSCs.

Author

Nakamura M, Shiozawa S, Tsuboi D, Amano M, Watanabe H, Maeda S, Kimura T, Yoshimatsu S, Kisa F, Karch CM, Miyasaka T, Takashima A, Sahara N, Hisanaga SI, Ikeuchi T, Kaibuchi K, and Okano H

Subjects
Calpain metabolism, Disease Progression, Disease Susceptibility, Frontotemporal Dementia metabolism, Frontotemporal Dementia physiopathology, Humans, Induced Pluripotent Stem Cells cytology, Mitochondria metabolism, Neurons metabolism, Phosphorylation, Phosphotransferases metabolism, tau Proteins metabolism, Alleles, Amino Acid Substitution, Frontotemporal Dementia etiology, Induced Pluripotent Stem Cells metabolism, Mutation, tau Proteins genetics
Abstract

Mutations in the microtubule-associated protein tau (MAPT) gene are known to cause familial frontotemporal dementia (FTD). The R406W tau mutation is a unique missense mutation whose patients have been reported to exhibit Alzheimer's disease (AD)-like phenotypes rather than the more typical FTD phenotypes. In this study, we established patient-derived induced pluripotent stem cell (iPSC) models to investigate the disease pathology induced by the R406W mutation. We generated iPSCs from patients and established isogenic lines using CRISPR/Cas9. The iPSCs were induced into cerebral organoids, which were dissociated into cortical neurons with high purity. In this neuronal culture, the mutant tau protein exhibited reduced phosphorylation levels and was increasingly fragmented by calpain. Furthermore, the mutant tau protein was mislocalized and the axons of the patient-derived neurons displayed morphological and functional abnormalities, which were rescued by microtubule stabilization. The findings of our study provide mechanistic insight into tau pathology and a potential for therapeutic intervention., (Copyright © 2019 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published
2019
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36. A versatile toolbox for knock-in gene targeting based on the Multisite Gateway technology.

Author

Yoshimatsu S, Sone T, Nakajima M, Sato T, Okochi R, Ishikawa M, Nakamura M, Sasaki E, Shiozawa S, and Okano H

Subjects
Animals, Callithrix genetics, Cloning, Molecular methods, Deoxyribonucleases genetics, Genes, Reporter genetics, Green Fluorescent Proteins genetics, Humans, Stem Cell Research, DNA, Recombinant genetics, Gene Knock-In Techniques methods, Gene Targeting methods, Genetic Vectors genetics
Abstract

Knock-in (KI) gene targeting can be employed for a wide range of applications in stem cell research. However, vectors for KI require multiple complicated processes for construction, including multiple times of digestion/ligation steps and extensive restriction mapping, which has imposed limitations for the robust applicability of KI gene targeting. To circumvent this issue, here we introduce versatile and systematic methods for generating KI vectors by molecular cloning. In this approach, we employed the Multisite Gateway technology, an efficient in vitro DNA recombination system using proprietary sequences and enzymes. KI vector construction exploiting these methods requires only efficient steps, such as PCR and recombination, enabling robust KI gene targeting. We show that combinatorial usage of the KI vectors generated using this method and site-specific nucleases enabled the precise integration of fluorescent protein genes in multiple loci of human and common marmoset (marmoset; Callithrix jacchus) pluripotent stem cells. The methods described here will facilitate the usage of KI technology and ultimately help to accelerate stem cell research., Competing Interests: T.S. is currently a paid employee of Takara Bio Inc., but all the experiments in this study were performed while he was in Keio University, where he had no conflicts of interest with the company. H.O. serves as a paid scientific advisor at SanBio Co. Ltd. and K Pharma Inc. The other authors declare neither financial nor non-financial competing interests. This does not alter the authors' adherence to PLOS ONE policies on sharing data and materials.

Published
2019
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37. Robust and efficient knock-in in embryonic stem cells and early-stage embryos of the common marmoset using the CRISPR-Cas9 system.

Author

Yoshimatsu S, Okahara J, Sone T, Takeda Y, Nakamura M, Sasaki E, Kishi N, Shiozawa S, and Okano H

Subjects
Animals, Callithrix, Embryo, Mammalian metabolism, Embryonic Stem Cells metabolism, Female, Forkhead Transcription Factors antagonists & inhibitors, Forkhead Transcription Factors genetics, Gene Targeting, Homologous Recombination, Humans, Male, Models, Animal, Myelin Proteolipid Protein antagonists & inhibitors, Myelin Proteolipid Protein genetics, Neural Stem Cells metabolism, CRISPR-Cas Systems, DNA Breaks, Double-Stranded, Embryo, Mammalian cytology, Embryonic Stem Cells cytology, Gene Editing, Gene Knock-In Techniques methods, Neural Stem Cells cytology
Abstract

Genome editing technology greatly facilitates the genetic modification of various cells and animals. The common marmoset (Callithrix jacchus), a small non-human primate which exhibits high reproductive efficiency, is a widely used animal model in biomedical research. Developing genome editing techniques in the common marmoset will further enhance its utility. Here, we report the successful establishment of a knock-in (KI) method for marmoset embryonic stem cells (ESCs), which is based on the CRISPR-Cas9 system. The use of CRISPR-Cas9, mediated by homologous recombination (HR), enhanced the KI efficiency in marmoset ESCs. Furthermore, we succeeded in performing KI in early-stage marmoset embryos. In the course of the experiments, we found that HR in the marmoset ESCs is innately highly efficient. This suggested that the marmoset possesses a repair mechanism for DNA double-strand breaks. The current study will facilitate the generation of genetically modified marmosets and gene function analysis in the marmoset.

Published
2019
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38. Silylative Kinetic Resolution of Racemic 1-Indanol Derivatives Catalyzed by Chiral Guanidine.

Author

Yoshimatsu S, Yamada A, and Nakata K

Abstract

Efficient kinetic resolution of racemic 1-indanol derivatives was achieved using triphenylchlorosilane by asymmetric silylation in the presence of chiral guanidine catalysts. The chiral guanidine catalyst (R,R)-N-(1-(β-naphthyl)ethyl)benzoguanidine was found to be highly efficient as only 0.5 mol % catalyst loading was sufficient to catalyze the reaction of various substrates with appropriate conversion and high s-values (up to 89). This catalyst system was successfully applied to the gram-scale silylative kinetic resolution of racemic 1-indanol with high selectivity.

Published
2018
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39. Naive-like ESRRB + iPSCs with the Capacity for Rapid Neural Differentiation.

Author

Kisa F, Shiozawa S, Oda K, Yoshimatsu S, Nakamura M, Koya I, Kawai K, Suzuki S, and Okano H

Subjects
Animals, Cell Differentiation genetics, Cell Self Renewal genetics, Cells, Cultured, Cellular Reprogramming genetics, Gene Expression Regulation, Developmental, Humans, Mice, Mouse Embryonic Stem Cells cytology, Neural Stem Cells cytology, Pluripotent Stem Cells cytology, Mouse Embryonic Stem Cells metabolism, Neural Stem Cells metabolism, Pluripotent Stem Cells metabolism, Receptors, Estrogen genetics
Abstract

Several groups have reported the existence of a form of pluripotency that resembles that of mouse embryonic stem cells (mESCs), i.e., a naive state, in human pluripotent stem cells; however, the characteristics vary between reports. The nuclear receptor ESRRB is expressed in mESCs and plays a significant role in their self-renewal, but its expression has not been observed in most naive-like human induced pluripotent stem cells (hiPSCs). In this study, we modified several methods for converting hiPSCs into a naive state through the transgenic expression of several reprogramming factors. The resulting cells express the components of the core transcriptional network of mESCs, including ESRRB, at high levels, which suggests the existence of naive-state hiPSCs that are similar to mESCs. We also demonstrate that these cells differentiate more readily into neural cells than do conventional hiPSCs. These features may be beneficial for their use in disease modeling and regenerative medicine., (Copyright © 2017 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2017
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40. Identification of Essential Containers for Aedes Larval Breeding to Control Dengue in Dhaka, Bangladesh.

Author

Ferdousi F, Yoshimatsu S, Ma E, Sohel N, and Wagatsuma Y

Abstract

Dengue fever (DF), one of the most important emerging arboviral diseases, is transmitted through the bite of container breeding mosquitoes Aedes aegypti and Aedes albopictus. A household entomological survey was conducted in Dhaka from August through October 2000 to inspect water-holding containers in indoor, outdoor, and rooftop locations for Aedes larvae. The objective of this study was to determine mosquito productivity of each container type and to identify some risk factors of households infested with Aedes larvae. Of 9,222 households inspected, 1,306 (14.2%) were positive for Aedes larvae. Of 38,777 wet containers examined, 2,272 (5.8%) were infested with Aedes larvae. Containers used to hold water, such as earthen jars, tanks, and drums were the most common containers for larval breeding. Tires in outdoor and rooftop locations of the households were also important for larval breeding. Although present in abundance, buckets were of less importance. Factors such as independent household, presence of a water storage system in the house, and fully/partly shaded outdoors were found to be significantly associated with household infestation of Aedes larvae. Identification and subsequent elimination of the most productive containers in a given area may potentially reduce mosquito density to below a level at which dengue transmission may be halted.

Published
2015
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41. Factors contribute to efficiency of specimen concentration of Mycobacterium tuberculosis by centrifugation and magnetic beads.

Author

Yoshimatsu S, Kato-Matsumaru T, Aono A, Chikamatsu K, Yamada H, and Mitarai S

Subjects
Analysis of Variance, Bacteriological Techniques methods, Centrifugation, Humans, Japan, Sensitivity and Specificity, Bacteriological Techniques instrumentation, Immunomagnetic Separation methods, Mycobacterium tuberculosis isolation & purification, Specimen Handling methods, Sputum microbiology, Tuberculosis, Pulmonary microbiology
Abstract

Background: A concentration of specimen is recommended for the effective recovery of Mycobacterium tuberculosis (MTB), but the bacteriological efficiency is not well evaluated. The present study evaluated the factors contributing to concentration efficiency of centrifugation and bead-based technique (TB-Beads; Microsens, UK) to recover MTB by using simple in vitro specimens., Methods: Four specimens were prepared (6.5×10(3); 8.1×10(4); 7.9×10(5); and 6.4×10(6)cfu/mL) of different concentrations with or without 5×10(4) of THP-1 cells (RIKEN BRC, Japan). Specimens were subjected to centrifugation at 2000, 3000, and 4000g for 15min, and to TB-Beads. The concentration and recovery rate were calculated to evaluate the efficiency of each method., Results: The specimens containing a higher number of bacteria and THP-1 cells had a tendency to yield a higher concentration and recovery rate (p=0.001-0.083). MTB was recovered more efficiently with THP-1 cells from the 6.5×10(3)cfu/mL specimen by centrifugation (p⩽0.001) than without them; 24.7-54.4% of MTB were recovered with THP-1 cells by centrifugation at 3000g for 15min, while the recovery using TB-Beads was a maximum of 12.7%., Conclusions: The efficiency of centrifugation depends on the bacterial density and the co-existence of THP-1 cells. The efficiency of TB-Beads was not as high as centrifugation., (Copyright © 2015 Asian-African Society for Mycobacteriology. Published by Elsevier Ltd. All rights reserved.)

Published
2015
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42. Detection of Mycobacterium tuberculosis (MTB) in Fecal Specimens From Adults Diagnosed With Pulmonary Tuberculosis Using the Xpert MTB/Rifampicin Test.

Author

Kokuto H, Sasaki Y, Yoshimatsu S, Mizuno K, Yi L, and Mitarai S

Abstract

Background.  The Xpert Mycobacterium tuberculosis (MTB)/rifampicin (RIF) is a fully automated diagnostic test that allows for the detection of MTB including its RIF resistance. Although the test is used for the diagnosis of tuberculosis (TB) in sputum samples worldwide, studies using fecal specimens are scarce. We therefore evaluated the efficacy of the Xpert MTB/RIF test for detection of MTB in fecal specimens obtained from adult pulmonary TB patients, confirmed by culture and/or molecular diagnostic methods. Methods.  We conducted a retrospective case-control study to provide proof-of-concept regarding the efficacy of the Xpert MTB/RIF test using fecal samples for diagnosing pulmonary TB via detection of MTB in adult patients (≥20 years) at the Fukujuji Hospital in Tokyo, Japan. Results.  Fecal specimens were obtained from 56 active pulmonary TB patients (including 48 sputum smear-positive and 8 sputum smear-negative patients), 10 non-TB patients (including 4 Myocobacterium avium complex infections), and 27 healthy individuals who were exposed to active pulmonary TB patients. The sensitivity of the fecal Xpert MTB/RIF was 100% (81.7%-100%) for detection of MTB in specimens from sputum smear-positive (1+ to 3+) patients, 81.0% (58.1%-94.6%) in specimens from sputum smear scanty positive patients, and 50.0% (15.7%-84.3%) in specimens from sputum smear-negative patients. Meanwhile, each of the fecal specimens from the non-TB group was negative for MTB (specificity 100%; 95% confidence interval, 86.2-100). Conclusions.  The fecal Xpert MTB/RIF test could detect MTB in a large proportion of smear-positive pulmonary TB patients, without frequent false-positive results at a TB referral hospital in Japan.

Published
2015
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43. Identification of potential prognostic markers for knee osteoarthritis by serum proteomic analysis.

Author

Takinami Y, Yoshimatsu S, Uchiumi T, Toyosaki-Maeda T, Morita A, Ishihara T, Yamane S, Fukuda I, Okamoto H, Numata Y, and Fukui N

Abstract

Background: As osteoarthritis (OA) is a highly heterogeneous disease in terms of progression, establishment of prognostic biomarkers would be highly beneficial for treatment. The present study was performed to identify novel biomarkers capable of predicting the progression of knee OA., Methods: A total of 69 plasma samples (OA patients undergoing radiographic progression, n = 25; nonprogression, n = 33; healthy donors, n = 11) were analyzed by surface-enhanced laser desorption/ionization time-of-flight mass spectrometry (SELDI-TOF MS), and ion peaks of interest were identified by liquid chromatography and matrix-assisted laser desorption/ionization (MALDI)-TOF MS. The identities of these proteins were further validated by immunoprecipitation combined with SELDI-TOF MS analysis., Results: SELDI-TOF MS analysis indicated that the intensities of 3 ion peaks differed significantly between progressors and nonprogressors. Subsequent analyses indicated that these peaks corresponded to apolipoprotein C-I, C-III, and an N-terminal truncated form of transthyretin, respectively. The identities of these proteins were confirmed by the loss of ion peaks in SELDI-TOF MS spectra by immunoprecipitation using specific antibodies for the respective proteins., Conclusions: Three potential biomarkers were identified whose serum levels differed significantly between OA progressors and nonprogressors. These biomarkers are expected to be prognostic biomarkers for knee OA and to facilitate the development of novel disease-modifying treatments for OA.

Published
2013
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44. Systemic lupus erythematosus complicated by cytomegalovirus-induced hemophagocytic syndrome and colitis.

Author

Sakamoto O, Ando M, Yoshimatsu S, Kohrogi H, Suga M, and Ando M

Subjects
Adult, Agammaglobulinemia etiology, Autoimmune Diseases drug therapy, Colitis virology, Cyclophosphamide adverse effects, Cyclophosphamide therapeutic use, Cytomegalovirus isolation & purification, Fatal Outcome, Female, Gastrointestinal Hemorrhage etiology, Humans, Immunocompromised Host, Immunosuppressive Agents adverse effects, Intestinal Perforation etiology, Leukocytes virology, Lupus Erythematosus, Systemic drug therapy, Lupus Nephritis complications, Multiple Organ Failure etiology, Prednisolone adverse effects, Prednisolone therapeutic use, Autoimmune Diseases complications, Colitis complications, Cytomegalovirus Infections complications, Histiocytosis, Non-Langerhans-Cell complications, Lupus Erythematosus, Systemic complications
Abstract

Here, we report a case of systemic lupus erythematosus (SLE) complicated by cytomegalovirus (CMV)-induced hemophagocytic syndrome (HPS) and colitis. A 44-year-old woman with SLE was treated with corticosteroid and cyclophosphamide for lupus nephritis. Although her lupus nephritis improved, fever, progressive pancytopenia and intestinal bleeding were observed. A bone marrow aspiration showed an increase in mature histiocytes with hemophagocytosis. In addition, a colonoscopy showed hemorrhagic colitis with ulcer and the biopsy specimen from the colon revealed typical CMV cells with CMV inclusions confirmed by immunohistochemistry. Furthermore, a large number of CMV antigen-positive leukocytes was detected, suggesting an active CMV infection. CMV infection is serious in compromised hosts. Therefore clinicians should be aware of the clinical settings in which this infection can arise and the target organs potentially affected in order to initiate the appropriate intervention.

Published
2002
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45. Dynamic MR imaging of hepatic adenomas with pathologic correlation.

Author

Miyazaki T, Yamashita Y, Yamamoto H, Yoshimatsu S, Takahashi M, Ogawa M, and Ishimaru Y

Subjects
Adult, Carcinoma, Hepatocellular diagnosis, Carcinoma, Hepatocellular pathology, Contrast Media, Diagnosis, Differential, Female, Gadolinium, Gadolinium DTPA, Glycogen Storage Disease Type I, Hemangioma diagnosis, Hemangioma pathology, Humans, Hyperplasia, Image Enhancement methods, Liver pathology, Liver Cirrhosis diagnosis, Liver Cirrhosis pathology, Organometallic Compounds, Pentetic Acid analogs & derivatives, Adenoma, Liver Cell diagnosis, Adenoma, Liver Cell pathology, Liver Neoplasms diagnosis, Liver Neoplasms pathology, Magnetic Resonance Imaging methods
Abstract

Two patients with hepatic adenomas (HAs) were evaluated using dynamic magnetic resonance (MR) imaging. Findings of conventional MR imaging of HAs have varied according to reports in the literature, and dynamic MR imaging of HAs has not been previously reported. Dynamic MR imaging using Gd-DTPA showed homogeneous enhancement in the early dynamic phase and prolonged enhancement in the late phase in the typical HA of Case 2. The HA of Case 1 contained fibrosis and exhibited delayed enhancement. The opacification of contrast enhancement was homogeneous and did not occur from the peripheral region as is observed in typical hemangiomas. In addition, washout of contrast material was not as rapid as with typical hepatocellular carcinomas (HCCs).

Published
1994
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46. Fungal metabolites. IV. Synthesis of an antibiotic peptide, trichosporin B-V, from Trichoderma polysporum.

Author

Iida A, Yoshimatsu S, Sanekata M, and Fujita T

Subjects
Amino Acid Sequence, Intercellular Signaling Peptides and Proteins, Molecular Sequence Data, Peptides chemical synthesis, Trichoderma, Anti-Bacterial Agents chemical synthesis, Fungal Proteins chemical synthesis
Abstract

The antibiotic icosapeptide trichosporin B-V, which was isolated from Trichoderma polysporum, was synthesized by assembling five peptide fragments via the N,N'-dicyclohexylcarbodiimide method. The synthesized peptide was identical with the natural one.

Published
1990
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47. Percutaneous histopathologic evaluation of liver in treatment of non-Hodgkin's lymphoma.

Author

Yoshimatsu S

Subjects
Adult, Aged, Aged, 80 and over, Biopsy, Needle methods, Humans, Liver Neoplasms diagnosis, Liver Neoplasms pathology, Liver Neoplasms secondary, Lymphoma, Non-Hodgkin diagnosis, Middle Aged, Neoplasm Staging, Ultrasonography, Liver pathology, Lymphoma, Non-Hodgkin pathology
Abstract

The results of 25 percutaneous biopsies of the liver from 24 patients with non-Hodgkin's lymphoma are reported. In all cases, the value of their serum biochemistry (LDH, GOT, GPT and/or alkaline phosphatase) was abnormal and sufficient tissue material was biopsied to obtain a histopathological evaluation. Specimens from five ultrasonically suspected lymphoma of the liver showed tumor involvement histopathologically. Diffuse tumor involvement was also histologically found in three ultrasonically unsuspected livers. Six liver specimens showed degenerative and/or fibrotic change in the new and previously treated patients.

Published
1988

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