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Dive into the research topics where Tadaaki Nakajima is active.

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Featured researches published by Tadaaki Nakajima.


Proceedings of the National Academy of Sciences of the United States of America | 2016

Retinoic acid signaling determines the fate of uterine stroma in the mouse Müllerian duct.

Tadaaki Nakajima; Taisen Iguchi; Tomomi Sato

Significance Oviduct, uterus, and vagina are all derived from the Müllerian duct. Epithelial fate of these female reproductive organs in developing mice is determined by factors secreted from the stroma; however, how the preceding stromal differentiation of female reproductive tracts from the Müllerian duct occurs is still unclear. This study showed that retinoic acid (RA) signaling was activated in the proximal Müllerian duct, which develops into oviduct and uterus. Furthermore, RA treatment induced uterine stromal differentiation, whereas inhibition of RA receptor signaling induced vaginal stromal differentiation. Therefore, we concluded that RA establishes a border between the stroma of uterus and vagina. The Müllerian duct develops into the oviduct, uterus, and vagina, all of which are quite distinct in their morphology and function. The epithelial fate of these female reproductive organs in developing mice is determined by factors secreted from the stroma; however, how stromal differentiation occurs in the female reproductive organs derived from the Müllerian duct is still unclear. In the present study, roles of retinoic acid (RA) signaling in developing female reproductive tracts were investigated. Retinol dehydrogenase 10 (RDH10) and aldehyde dehydrogenase family 1 subfamily A2 (ALDH1A2) mRNAs and proteins and transactivation activity of endogenous RA were found in the stroma of proximal Müllerian ducts and gradually decreased from the proximal to caudal regions in fetal mice. In organ-cultured Müllerian ducts, retinaldehyde or RA treatment induced uterine epithelial differentiation, defined as a layer of columnar epithelial cells negative for oviductal and vaginal epithelial markers. In contrast, inhibition of RA receptor (RAR) signaling induced vaginal epithelial differentiation, characterized as vaginal epithelial marker genes–positive stratified epithelium. Grafting experiments of the organ-cultured Müllerian duct revealed irreversible epithelial fate determination. Although RAR did not directly bind to the homeobox A10 (Hoxa10) promoter region, RA–RAR signaling stimulated Hoxa10 expression. Thus, RA–RAR signaling in the Müllerian duct determines the fate of stroma to form the future uterus and vagina.


Endocrinology | 2015

Neonatal Estrogen Receptor β Is Important in the Permanent Inhibition of Epithelial Cell Proliferation in the Mouse Uterus

Tadaaki Nakajima; Yuki Tanimoto; Masami Tanaka; Pierre Chambon; Hajime Watanabe; Taisen Iguchi; Tomomi Sato

Estrogen receptor α (ERα) plays a pivotal role in the mouse uterine and vaginal epithelial cell proliferation stimulated by estrogen, whereas ERβ inhibits cell proliferation. ERβ mRNA is expressed in neonatal uteri and vaginae; however, its functions in neonatal tissues have not been ascertained. In this study, we investigated the ontogenic mRNA expression and localization of ERβ, and its roles in cell proliferation in neonatal uteri and vaginae of ERβ knockout (βERKO) mice. ERβ mRNA and protein were abundant in the uterine and vaginal epithelia of 2-day-old mice and decreased with age. In uterine and vaginal epithelia of 2-day-old βERKO mice, cell proliferation was greater than that in wild-type animals and in uterine epithelia of 90- and 365-day-old βERKO mice. In addition, p27 protein, known as a cyclin-dependent kinase inhibitor, was decreased in the uteri of 90- and 365-day-old βERKO mice. Inhibition of neonatal ERs by ICI 182780 (an ER antagonist) treatment stimulated cell proliferation and decreased p27 protein in the uterine luminal epithelium of 90-day-old mice but not in the vaginal epithelium. These results suggest that neonatal ERβ is important in the persistent inhibition of epithelial cell proliferation with accumulation of p27 protein in the mouse uterus. Thus, suppression of ERβ function in the uterine epithelium during the neonatal period may be responsible for a risk for proliferative disease in adults.


Zoological Science | 2017

Sex Reversal and Analyses of Possible Involvement of Sex Steroids in Scallop Gonadal Development in Newly Established Organ-Culture Systems

Ayano Otani; Tadaaki Nakajima; Tomomi Okumura; Shiro Fujii; Yasuhiro Tomooka

Many molluscs perform sex reversal, and sex hormones may be involved in the process. In adult scallops, Patinopecten yessoensis, gonadotropin releasing hormone and 17β-estradiol (E2) are involved in male sexual maturation, however, little is known about the effects of E2 and testosterone (T) on the gonadal differentiation in young scallops. In the present study, scallop gonadal development was analyzed to determine the sex reversal stage in Funka bay, and effects of E2 and T were examined. In Funka bay, almost all scallops were male at month 12. Scallops equipped with ambiguous gonads were 61.1% at month 16 and disappeared at month 18. Therefore, sex reversal in Funka bay occurs at around month 16. For establishment of organ culture systems for bivalves, Manila clam gonads were cultured in 15% L-15 medium diluted with HBSS containing 10% KSR on agarose gel at 10°C, and the gonads survived for 14 days. Scallop gonads were also able to be cultured in 30% L15 medium diluted with ASW containing 10% KSR on agarose gel for seven days. At mature stage, Foxl2 and Tesk were predominantly expressed in ovary and testis, respectively. When scallop gonads at sex reversal stage were organ-cultured, sex steroid treatment decreased Tesk expression in the majority of scallop gonads at sex reversal stage. However, no obvious change in Foxl2 and Tesk expression was detected in mature gonads in response to either E2 or T in culture, suggesting sex steroid treatment might affect gonadal development at sex reversal stage.


Journal of Agricultural and Food Chemistry | 2018

Intestinal Anti-Inflammatory Activity of Perillaldehyde

Takuya Uemura; Takuya Yashiro; Rei Oda; Naoki Shioya; Tadaaki Nakajima; Masakazu Hachisu; Shoko Kobayashi; Chiharu Nishiyama; Gen-ichiro Arimura

Monoterpenoid perillaldehyde (PA) is the major component in Perilla frutescens leaf essential oil, but its function regarding anti-inflammatory effect is unclear. We explored the anti-inflammatory activity of PA in a dextran sulfate sodium (DSS)-induced colitis mouse model using relief of bodyweight loss (avg. 49.2% mitigation; P = 0.094) and colon damage (avg. 35.3% mitigation; P < 0.05) by administration of PA at a 100 mg/kg dosage. The PA administration resulted in suppression of DSS-induced expression of pro-inflammatory cytokine genes and matrix metalloproteinase-9 in the colon (e.g., avg. 60.6% mitigation for TNF-α mRNA levels; P < 0.05). These effects were confirmed in macrophage RAW264.7 cells stimulated with lipopolysaccharide (LPS). Application of PA induced cell suppression of LPS-induced expressions of genes and proteins of pro-inflammatory cytokines and induced activation of c-Jun N-terminal kinases (JNKs, p54 and p46; P < 0.05) but not nuclear factor-κB p65. The half maximal inhibitory concentration for decreased expression levels of TNF-α mRNA was 171.7 μM. We discuss the in vivo function of PA in amelioration of intestinal inflammation via JNK-mediated cytokine regulation.


Biology of Reproduction | 2018

Stratification of mouse vaginal epithelium. 1. Development of 3 dimensional models in vitro with clonal cell lines

Minako Ogawa-Tominaga; Tomohiro Umezu; Tadaaki Nakajima; Yasuhiro Tomooka

Abstract The mouse vagina consists of stratified squamous epithelium and stroma and is regulated by ovarian hormones. Vaginal epithelial cells do not stratify, but rather form a monolayer and show an inconsistent responsiveness to ovarian hormones when cultured on plastic dish or matrix. To address the discrepancy between in vivo and in vitro observations, three-dimensional (3D) coculture models are developed with clonal vaginal epithelial and stromal cell lines; stromal cells are embedded in collagen gel and epithelial cells are seeded on the gel. In the 3D models, epithelial cells express Transformation related protein 63 (Trp63) and begin to stratify when they are cocultured with two out of three stromal cell lines, but not with the other stromal cell line. Stroma may consist of various types of cells with distinct functions. Summary Sentence Stratification of vaginal epithelium was induced in three-dimensional models with clonal mouse vaginal epithelial and stromal cell lines.


Biology of Reproduction | 2018

Stratification of mouse vaginal epithelium 2. Identification of factors inducing stratification

Rikako Takashina; Tadaaki Nakajima; Tomohiro Umezu; Kiyohiko Komatsu; Tatsuro Banba; Taichi Asada; Kensuke Ohse; Yasufumi Murakami; Yasuhiro Tomooka

Abstract Stratification of the vaginal epithelium is regulated by stromal factors. To analyze the mechanisms of stratification in vitro, 3 dimensional (3D) co-culture models were established with clonal cell lines. In the models, stromal cells were embedded in collagen gel and epithelial cells were seeded on the gel. In the 3D co-culture, stromal SV-6c4a1b cells induced epithelial stratification but stromal MV-1e6g1a cells did not, suggesting that SV-6c4a1b cells secretemolecules to induce stratification. Microarray analyses of these stromal cell lines identified chordin-like 1 (Chrd1) andWNT1 inducible signaling pathway protein 2 (Wisp2) as candidate genes inducing stratification. Chrdl1 variant1 and variant2 mRNAs were expressed not only in stromal SV-6c4a1b and MV-1e6g1a cells but also in epithelial SV-4b6b cells. Wisp2-overexpressing MV-1e6g1a cells, secreting WISP2 as much as SV-6c4a1b cells, induced stratification of epithelial cells. In addition, Wisp2-knockdowned SV-6c4a1b cells were unable to induce epithelial stratification. These results suggest that WISP2 is one of the stromal factors inducing stratification of the mouse vaginal epithelium. Summary Sentence WISP2 secreted by vaginal stroma and regulated by estrogen induced stratification in vaginal epithelium.


Biochemical and Biophysical Research Communications | 2017

Accumulation of immunoglobulin G against Dermatophagoides farinae tropomyosin in dorsal root ganglia of NC/Nga mice with atopic dermatitis-like symptoms

Ayaka Otsu; Hiroaki Kawasaki; Mitsutoshi Tominaga; Ayako Shigenaga; Hironori Matsuda; Nobuaki Takahashi; Tadaaki Nakajima; Hisashi Naito; Takeshi Baba; Hideoki Ogawa; Yasuhiro Tomooka; Fumiyuki Yamakura; Kenji Takamori

Atopic dermatitis (AD), a chronic inflammatory skin disease, manifests as intractable itch, but its underlying mechanisms are poorly understood. This study assessed the relationship between immunoglobulin G (IgG) and dorsal root ganglia (DRG) in NC/Nga mice, a model of AD that manifests AD-like symptoms including itch. Immunohistochemical analysis showed large amounts of IgG in DRG extracts of NC/Nga mice with AD-like dermatitis, with a large fraction of the IgG distributed in satellite glial cells of the DRG. Proteomic analysis showed that this IgG was reactive against tropomyosin of Dermatophagoides farinae. These findings indicate that the accumulation of anti-tropomyosin IgG in DRG of atopic NC/Nga mice may be associated with the pathogenesis of AD-like symptoms, including itch.


ACS Omega | 2017

Rapid and Easy Extracellular Vesicle Detection on a Surface-Functionalized Power-Free Microchip toward Point-of-Care Diagnostics

Ryo Ishihara; Tadaaki Nakajima; Yoshitaka Uchino; Asuka Katagiri; Kazuo Hosokawa; Mizuo Maeda; Yasuhiro Tomooka; Akihiko Kikuchi

Extracellular vesicles (EVs) are promising novel cancer biomarkers. However, rapid and easy analysis of EVs is challenging because conventional detection methods require large sample volumes and long detection times. Microchip-based analytical systems have particularly attracted attention for development of point-of-care (POC) diagnostics. Previously, various biomarker detection methods on a portable power-free poly(dimethylsiloxane) (PDMS) microchip using laminar flow-assisted dendritic amplification have been developed. Recently, for easy functionalization, we proposed a microchannel inner surface-functionalized power-free PDMS microchip (SF-PF microchip) utilizing electron beam-induced graft polymerization. In this study, we apply the technique and prepare a novel SF-PF microchip. On the microchip, EVs were successfully detected. The required sample volume was 1.0 μL, and the total analysis time was 20 min. The microchip can contribute to EV-based POC cancer diagnosis.


Biochemical and Biophysical Research Communications | 2017

Role of extracellular vesicles in the interaction between epithelial and mesenchymal cells during oviductal ciliogenesis.

Shota Nakano; Shohei Yamamoto; Atsumasa Okada; Tadaaki Nakajima; Mamiko Sato; Tomoko Takagi; Yasuhiro Tomooka


Journal of Pediatric and Adolescent Gynecology | 2017

Efficacy of Fibroblast Growth Factor on Epithelialization of the Neovagina in Patients with Mayer-Rokitansky-Küster-Hauser Syndrome Who Underwent Vaginoplasty

Tomoko Nagata; Aiko Kawano; Makiko Koyama; Tomomi Nakamura; Fumiki Hirahara; Tadaaki Nakajima; Tomomi Sato; Hideya Sakakibara

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Yasuhiro Tomooka

Tokyo University of Science

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Tomomi Sato

Yokohama City University

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