Your search keyword '"Yanagita, Emmy"' showing total 12 results

1. The DNA integrity number and concentration are useful parameters for successful comprehensive genomic profiling test for cancer using formalin‐fixed paraffin embedded tissue.

Author

Yanagita, Emmy, Yamada, Hiroshi, Kobayashi, Tetsuro, Aimono, Eriko, Nakamura, Kohei, Hirasawa, Akira, and Nishihara, Hiroshi

Subjects

*PARAFFIN wax, *MATERIALS handling, *CANCER genes, *ALKANES, *TISSUES

Abstract

The acquisition of high‐quality biospecimens and the appropriate handling of these materials are indispensable for successful clinical sequencing. We developed a cancer clinical sequencing system targeting 160 cancer genes: PleSSision‐Rapid. Through the PleSSision‐Rapid system, we have analyzed DNA quality evaluated by DIN (DNA integrity number) with 1329 formalin‐fixed paraffin embedded (FFPE) samples including 477 prospectively collected tissues for genomic test (P) and 852 archival samples after routine pathological diagnosis (A1/A2). As a result, the samples with more than DIN 2.1 was 92.0% (439/477) in prospectively collected sample (P), while it was 85.6% (332/388) and 76.7% (356/464) in two types of archival samples (A1/A2). We performed the PleSSision‐Rapid sequence using the samples with over DIN 2.1 and DNA concentration >10 ng/μL with which we were able to construct a DNA library, and the probability of sequence success was almost equivalent during all types of specimen processing, at 90.7% (398/439) in (P), 92.5% (307/332) in (A1) and 90.2% (321/356) in (A2), respectively. Our result indicated the clinical benefit to prepare the prospective collection of FFPE materials for indisputable clinical sequence, and that DIN ≥ 2.1 would be a solid parameter for sample preparation of comprehensive genomic profiling tests. [ABSTRACT FROM AUTHOR]

Published

2023

2. Diagnostic meaning of immunohistochemistry-based Cell Cycle Detection on human cutaneous tumors derived from keratinocyte

Author

Bito, Toshinori, Yanagita, Emmy, Matsuoka, Ryosuke, Itoh, Tomoo, and Nishigori, Chikako

Published

2013

3. Cultures derived from pancreatic cancer xenografts with long-term gemcitabine treatment produce chemoresistant secondary xenografts: Establishment of isogenic gemcitabine-sensitive and -resistant models.

Author

Kobayashi-Ooka, Yasuyo, Akagi, Tsuyoshi, Sukezane, Taiko, Yanagita, Emmy, Itoh, Tomoo, and Sasai, Ken

Subjects

*TRANSCRIPTION factors, *PANCREATIC duct, *PANCREATIC cancer, *DRUG target, *DRUG resistance

Abstract

In attempts to establish sophisticated models to reproduce the process of acquired drug resistance, we transformed normal human pancreatic ductal epithelial cells by introducing genes for multiple cellular factors. We also created isogenic gemcitabine-sensitive and -resistant models by short- and long-term gemcitabine treatment, respectively. These models demonstrated differences in drug resistance in vivo , but not in vitro. Gemcitabine treatment also induced squamous transdifferentiation in xenografts in mice. The transcription factor p63 was identified as a possible resistance-determining factor but was unlikely to be solely responsible for the resistance to gemcitabine. This system would prove useful to discover novel molecular targets to overcome chemotherapy resistance, by allowing the evaluation of molecules of interest in xenograft models after in vitro genetic ablation. [ABSTRACT FROM AUTHOR]

Published

2024

4. Evaluation of the usability of various rapid antibody tests in the diagnostic application for COVID-19.

Author

Uwamino, Yoshifumi, Wakui, Masatoshi, Aoki, Wataru, Kurafuji, Toshinobu, Yanagita, Emmy, Morita, Maasa, Nagata, Mika, Inose, Rika, Noguchi, Masayo, Yokota, Hiromitsu, Hasegawa, Naoki, Saya, Hideyuki, and Murata, Mitsuru

Subjects

*COVID-19 pandemic, *REVERSE transcriptase polymerase chain reaction, *SARS-CoV-2, *IMMUNOGLOBULIN G, *IMMUNE response, *ANTIBODY titer

Abstract

Background: The usability of laboratory tests related to severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) is critically important for the world undergoing the COVID-19 pandemic. The present study aimed to assess the diagnostic usability of rapid tests for the detection of antibody against SARS-CoV-2 through comparison of their results with the results of reverse transcription polymerase chain reaction (RT-PCR) test for the detection of SARS-CoV-2 genomic RNA and with the results of a quantitative test for antibody detection. Methods: Serum samples were collected from 18 patients undergoing RT-PCR testing for SARS-CoV-2. Twelve patients were RT-PCR positive while six were negative. A quantitative test based on chemiluminescent immunoassay and three rapid tests based on immunochromatography were performed to detect anti-SARS-CoV-2 IgG and IgM. Results: All the antibody tests exhibited poor sensitivity at the timing of initial RT-PCR diagnosis. IgG responses occurring prior to or simultaneously with IgM responses were observed through not only the quantitative test but also the three rapid tests. Based on concordance with the quantitative test results, the large variance among the three rapid tests was revealed. Conclusions: All antibody tests were unsatisfactory to replace RT-PCR for the early diagnosis of COVID-19. Rapid antibody tests as well as a quantitative antibody test were useful in the assessment of immune responses in COVID-19. The obvious variance among the three rapid tests suggested limited accuracy and difficult standardization. Diagnostic usability of rapid antibody tests for COVID-19 should be investigated rigorously. [ABSTRACT FROM AUTHOR]

Published

2021

5. Engineering cancer stem-like cells from normal human lung epithelial cells.

Author

Sasai, Ken, Takao-Rikitsu, Etsuko, Sukezane, Taiko, Nakagawa, Harumi, Itoh-Yagi, Machiko, Izumi, Yukina, Akagi, Tsuyoshi, Yanagita, Emmy, and Itoh, Tomoo

Subjects

*CANCER stem cells, *METASTASIS, *DRUG resistance in cancer cells, *LUNG cancer diagnosis, *EPITHELIAL cell culture

Abstract

It has been proposed that a subpopulation of tumour cells with stem cell-like characteristics, known as cancer stem cells (CSCs), drives tumour initiation and generates tumour heterogeneity, thus leading to cancer metastasis, recurrence, and drug resistance. Although there has been substantial progress in CSC research into many solid tumour types, an understanding of the biology of CSCs in lung cancer remains elusive, mainly because of their heterogeneous origins and high plasticity. Here, we demonstrate that engineered lung cancer cells derived from normal human airway basal epithelial cells possessed CSC-like characteristics in terms of multilineage differentiation potential and strong tumour-initiating ability. Moreover, we established an in vitro 3D culture system that allowed the in vivo differentiation process of the CSC-like cells to be recapitulated. This engineered CSC model provides valuable opportunities for studying the biology of CSCs and for exploring and evaluating novel therapeutic approaches and targets in lung CSCs. [ABSTRACT FROM AUTHOR]

Published

2017

6. O19-2 Comparison of clinical utility between whole-exome sequencing and targeted sequencing (PleSSision-WET study).

Author

Hayashi, Hideyuki, Tanishima, Shigeki, Mochida, Kaori, Fujikura, Tomoka, Hagiwara, Sachiko, Yanagita, Emmy, Yamada, Hiroshi, Kawano, Ryutaro, Nakamura, Kohei, Ishikawa, Marin, Kato, Yasutaka, Aimono, Eriko, Imai, Mitsuho, Ueki, Arisa, and Nishihara, Hiroshi

Published

2022

7. Immunohistochemical expression profiles of solute carrier transporters in alpha-fetoprotein-producing gastric cancer.

Author

Shimakata, Takaaki, Kamoshida, Shingo, Kawamura, Jumpei, Ogane, Naoki, Kameda, Yoichi, Yanagita, Emmy, Itoh, Tomoo, Takeda, Risa, Naka, Ayano, Sakamaki, Kuniko, Hayashi, Yurie, and Kuwao, Sadahito

Subjects

*STOMACH cancer, *STOMACH cancer treatment, *NUCLEOSIDE transport proteins, *ALPHA fetoproteins, *IMMUNOHISTOCHEMISTRY, *GENE expression profiling, *GENETICS

Abstract

Aims Alpha-fetoprotein ( AFP)-producing gastric cancer ( GC) is an aggressive tumour with high rates of liver metastasis and poor prognosis, and for which a validated chemotherapy regimen has not been established. Drug uptake by solute carrier ( SLC) transporters is proposed as one of the mechanisms involved in sensitivity to chemotherapy. In this study, we aimed to develop important insights into effective chemotherapeutic regimens for AFP-producing GC. Methods and results We evaluated immunohistochemically the expression levels of a panel of SLC transporters in 20 AFP-producing GCs and 130 conventional GCs. SLC transporters examined were human equilibrative nucleoside transporter 1 ( hENT1), organic anion transporter 2 ( OAT2), organic cation transporter ( OCT) 2, OCT6 and organic anion-transporting polypeptide 1B3 ( OATP1B3). The rates of high expression levels of hENT1 ( hENT1high) and OAT2 ( OAT2high) were statistically higher in AFP-producing GC, compared with conventional GC. When analysing hENT1 and OAT2 in combination, hENT1high/ OAT2high was the most particular expression profile for AFP-producing GC, with a greater significance than hENT1 or OAT2 alone. However, no significant differences in OCT2, OCT6 or OATP1B3 levels were detected between AFP-producing and conventional GCs. However, immunoreactivity for hENT1, OAT2 and OCT6 tended to be increased in GC tissues compared with non-neoplastic epithelia. Conclusions Because hENT1 and OAT2 are crucial for the uptake of gemcitabine and 5-fluorouracil, respectively, our results suggest that patients with AFP-producing GC could potentially benefit from gemcitabine/fluoropyrimidine combination chemotherapy. Increased expression of hENT1, OAT2 and OCT6 may also be associated with the progression of GC. [ABSTRACT FROM AUTHOR]

Published

2016

8. Psf3 is a prognostic biomarker in lung adenocarcinoma: a larger trial using tissue microarrays of 864 consecutive resections.

Author

Shunsuke Tauchi, Yasuhiro Sakai, Shuntaro Fujimoto, Hiroyuki Ogawa, Shinya Tane, Daisuke Hokka, Yugo Tanaka, Wataru Nishio, Masahiro Yoshimura, Yanagita, Emmy, Tomoo Itoh, Yoshitake Hayashi, and Yoshimasa Maniwa

Subjects

*BIOMARKERS, *ADENOCARCINOMA, *LUNG cancer, *EPITOPES, *PROGNOSIS

Abstract

OBJECTIVES: Partner of Sld five (Psf ) 3 is a member of the evolutionarily conserved heterotetrameric complex GINS (Go-Ichi-Ni-San). We previously reported that Psf3 could serve as a biomarker of poor prognosis in lung adenocarcinoma. Here, we used tissue microarrays to analyse Psf3 expression in lung adenocarcinoma and investigated whether its expression is associated with survival outcomes. METHODS: The study included 864 consecutive patients with lung adenocarcinoma who underwent complete resection at Hyogo Cancer Center between January 2002 and December 2009. Tissue microarrays were prepared, and Psf3 was detected using mouse antihuman Psf3 primary monoclonal antibodies. The status of Psf3 expression was determined using these microarrays. RESULTS: Of the 864 patients, 375 had high-positive Psf3 expression and 489 had low-positive expression. Psf3 expression was significantly associated with age, sex, T factor, lymph node metastasis, stage and P factor. The 5-year disease-free survival (DFS) rate was significantly lower in patients with high-positive Psf3 expression than in those with low-positive expression, and Psf3 expression, sex, age, T factor and lymph node metastasis were identified as independent and significant prognostic determinants. Among patients with Stage I adenocarcinoma, the 5-year DFS rate was significantly lower in those with high-positive Psf3 expression than in those with low-positive expression, and Psf3 expression was the most powerful survival predictor. CONCLUSIONS: The present findings strengthened our previous data demonstrating that high Psf3 expression in primary lung adenocarcinoma plays an important role in disease progression and is a prognostic indicator, particularly in early-stage adenocarcinoma. [ABSTRACT FROM AUTHOR]

Published

2016

9. Immunohistochemical Profiling of ALK Fusion Gene–Positive Adenocarcinomas of the Lung.

Author

Sakai, Yasuhiro, Nakai, Tokiko, Ohbayashi, Chiho, Imagawa, Naoko, Yanagita, Emmy, Satake, Rumiko, Nitta, Atsushi, Kajimoto, Kazuyoshi, Sakuma, Toshiko, and Itoh, Tomoo

Subjects

*LUNG cancer, *SQUAMOUS cell carcinoma, *THERAPEUTICS, *ADENOCARCINOMA, *ANAPLASTIC lymphoma kinase, *MICROARRAY technology

Abstract

Our aim was to determine whether or not non-small-cell lung cancer is squamous cell carcinoma (SQCC); even in small samples, it is essential in view of the side effects attendant on new therapeutics. Lung adenocarcinoma (ADC) with the EML4-ALK fusion gene has been described as demonstrating mucinous cribriform/acinar growth and signet-ring cells, sometimes partially simulating SQCC. We investigated the relation among morphology, anaplastic lymphoma kinase (ALK) rearrangement, and immunophenotype in 321 ADCs by tissue microarray using SQCC markers cytokeratin (CK)5/6, CK14, desmocollin-3, desmoglein-3, p40, p63 versus ADC markers thyroid transcription factor (TTF)-1 and napsin A. Unlike 312 ALK-negative ADCs, 9 ALK-positive cases were negative for 4 SQCC markers. Only 1 ALK-positive ADC showing assertive morphology was positive for CK5/6 and p63 as well as for TTF-1 and napsin A. Coexpression of TTF-1/p40 was not observed, unlike that of TTF-1/p63 reported previously. There was no statistically significant difference between ALK-negative and ALK-positive ADC by immunohistochemical profiling. [ABSTRACT FROM AUTHOR]

Published

2013

10. Stage-specific embryonic antigen-4 identifies human dental pulp stem cells

Author

Kawanabe, Noriaki, Murata, Satoko, Fukushima, Hiroaki, Ishihara, Yoshihito, Yanagita, Takeshi, Yanagita, Emmy, Ono, Mitsuaki, Kurosaka, Hiroshi, Kamioka, Hiroshi, Itoh, Tomoo, Kuboki, Takuo, and Yamashiro, Takashi

Subjects

*DENTAL pulp, *EMBRYONIC stem cells, *CELL surface antigens, *GENE expression, *FLOW cytometry, *GENETIC regulation

Abstract

Abstract: Embryonic stem cell-associated antigens are expressed in a variety of adult stem cells as well as embryonic stem cells. In the present study, we investigated whether stage-specific embryonic antigen (SSEA)-4 can be used to isolate dental pulp (DP) stem cells. DP cells showed plastic adherence, specific surface antigen expression, and multipotent differentiation potential, similar to mesenchymal stem cells (MSC). SSEA-4+ cells were found in cultured DP cells in vitro as well as in DP tissue in vivo. Flow cytometric analysis demonstrated that 45.5% of the DP cells were SSEA-4+. When the DP cells were cultured in the presence of all-trans-retinoic acid, marked downregulation of SSEA-3 and SSEA-4 and the upregulation of SSEA-1 were observed. SSEA-4+ DP cells showed a greater telomere length and a higher growth rate compared to ungated and SSEA-4− cells. A clonal assay demonstrated that 65.5% of the SSEA-4+ DP cells had osteogenic potential, and the SSEA-4+ clonal DP cells showed multilineage differentiation potential toward osteoblasts, chondrocytes, and neurons in vitro. In addition, the SSEA-4+ DP cells had the capacity to form ectopic bone in vivo. Thus, our results suggest that SSEA-4 is a specific cell surface antigen that can be used to identify DP stem cells. [Copyright &y& Elsevier]

Published

2012

11. Preventive effect of chemical peeling on ultraviolet induced skin tumor formation

Author

Abdel-Daim, Mohamed, Funasaka, Yoko, Kamo, Tsuneyoshi, Ooe, Masahiko, Matsunaka, Hiroshi, Yanagita, Emmy, Itoh, Tomoo, and Nishigori, Chikako

Subjects

*CHEMICAL peel, *SKIN cancer, *ULTRAVIOLET radiation, *RADIATION carcinogenesis, *GENE expression, *LABORATORY mice, *CYCLOOXYGENASE 2

Abstract

Abstract: Background: Chemical peeling is one of the dermatological treatments available for certain cutaneous diseases and conditions or improvement of cosmetic appearance of photoaged skin. Objectives: We assessed the photochemopreventive effect of several clinically used chemical peeling agents on the ultraviolet (UV)-irradiated skin of hairless mice. Methods: Chemical peeling was done using 35% glycolic acid dissolved in distilled water, 30% salicylic acid in ethanol, 10% or 35% trichloroacetic acid (TCA) in distilled water at the right back of UV-irradiated hairless mice every 2 weeks in case of glycolic acid, salicylic acid, and 10% TCA and every 4 weeks in case of 35% TCA for totally 18 weeks after the establishment of photoaged mice by irradiation with UVA+B range light three times a week for 10 weeks at a total dose of 420J/cm2 at UVA and 9.6J/cm2 at UVB. Tumor formation was assessed every week. Skin specimens were taken from treated and non-treated area for evaluation under microscopy, evaluation of P53 expression, and mRNA expression of cyclooxygenase (COX)-2. Serum level of prostaglandin E2 was also evaluated. Results: All types of chemical peeling reduced tumor formation in treated mice, mostly in the treated area but also non-treated area. Peeling suppressed clonal retention of p53 positive abnormal cells and reduced mRNA expression of COX-2 in treated skin. Further, serum prostaglandin E2 level was decreased in chemical peeling treated mice. Conclusions: These results indicate that chemical peeling with glycolic acid, salicylic acid, and TCA could serve tumor prevention by removing photodamaged cells. [ABSTRACT FROM AUTHOR]

Published

2010

12. Successful treatment of Cronkhite-Canada syndrome using anti-tumor necrosis factor antibody therapy.

Author

Watanabe, Daisuke, Ooi, Makoto, Hoshi, Namiko, Kohashi, Michitaka, Yoshie, Tomoo, Ikehara, Nobunao, Yoshida, Masaru, Yanagita, Emmy, Yamasaki, Takashi, Itoh, Tomoo, and Azuma, Takeshi

Published

2014