Your search keyword '"Tsukasa Ashihara"' showing total 83 results

1. Application of Super High Definition Images in Telemedicine: System Requirements and Technologies for Teleradiology and Telepathology.

Author

Junji Suzuki, Isao Furukawa, Tetsuro Fujii, Sadayasu Ono, Tsukasa Ashihara, Jun-Ichi Hata, and Yutaka Ando

Published

2000

2. Signal Analysis and Compression Performance Evaluation of Pathological Microscopic Images.

Author

A. Okumura, Junji Suzuki, Isao Furukawa, Sadayasu Ono, and Tsukasa Ashihara

Published

1997

3. Abstracts

Author

Akira Matsuno, Tadashi Nagashima, R.Yoshiyuki Osamura, Hiromi IKE, Yoshitaka TAMADA, Norio IIJIMA, Seiji HAYASHI, Masaki TANAKA, Akihiko ISHIHARA, Michinori HASEGAWA, Fumihiko SUWA, Yasuhiko IBATA, Shin-ichi IZUMI, Yuko SENBA, Masashi SHIN, Yoshitaka HISHIKAWA, Takehiko KOJI, Toshiki IWASAKA, Shinobu UMEMURA, Kochi KAKIMOTO, Akemi TAKAHASHI, Haruko KOIZUMI, R.Yoshiyuki OSAMURA, Shuji Yamashita, Atsushi Takayanagi, Nobuyoshi Shimizu, Atsuko ISHIZUYA-OKA, Shuichi UEDA, Akira Komiyama, Ryohei Katoh, Akira Yokoyama, Akira Kawaoi, Shigeko Torihashi, S. Tsuyama, D-H. Yang, F. Murata, Hikaru TAJIMA, Masataka ITOH, Shinichi TAKAHASHI, Hitoshi ISHIDA, Syouzou SAITO, Hayato KAWAKAMI, Hiroshi HIRANO, Tateo DAIMON, Kazuhiro KAWAI, Katsuko KATAOKA, Etsuko SUZAKI, Kinji Ito, Minako Hoshida, Michiko Hayashi, Athuko Ito, Dong-Hua YANG, Shinichiro Tsuyama, Fusayoshi Murata, Kiyokazu MORIOKA, Hiromi Takano-Ohmuro, Noriaki ANDOH, Haruo OHTANI, Hiroshi NAGURA, Norio MIYOSHI, Kazuhiro KARAYA, Masakatsu WATANABE, Masaru FUKUDA, Toshihiro Kobayashi, Teruhiko Okada, Harumichi Seguchi, Tadashi Ueda, Yoshimaro Ishikawa, Keiichi Tsukinoki, Tomoko Imaizumi, Yoshiko Miyoshi, Takayuki Yamamoto, Yoshihisa Watanabe, Kazunari Karakida, M Iwasa, S Noriki, Y Imamura, M Fukuda, Kazuo KOMIYAMA, Masahiro Okaue, Yasuyuki Oda, Junichi SATO, Tadao OKANO, Ram MORO, Atsuko ITO, Michiko HAYASHI, Minako HOSHIDA, Kinji ITO, Kohsuke CHIDA, Yasuhide MITSUMOTO, Michihihsa MORIGUCHI, Tomoki NAKAJIMA, Hiroshi HIKITA, Takeshi OKANOUE, Tsukasa ASHIHARA, Hiroyuki SUGIHARA, Takanori HATTORI, Yohei Hosokawa, Shouichi Arai, Tsukasa Ashihara, Naoki Tani, Hiroki Taniguchi, Masayoshi Nakanishi, Chouhei Sakakura, Takeshi Mazaki, Yasunari Tsuchihashi, Hisakazu Yamagishi, Nobuki Nakamura, Eri Miyagi, Koich Suzuki, Akihiro Hemmi, Yoshika SAKAMOTO, Takaaki ITO, Koji OKUDELA, Hitoshi KITAMURA, Kan-yu NAKANO, Ken-ichi IYAMA, Fumiko Date, Hironobu Sasano, Hiroshi Nagura, Hirokazu FURUTA, Keiichi YOKOYAMA, Shinsuke MASUDA, Tetsuro TAKAMATSU, Y. TAJIMA, M. KAWASAKI, J. OHNO, K. KUSAMA, S. MARUYAMA, and Kenzou UCHIDA

Subjects

Histology, Physiology, Cell Biology, Biochemistry, Pathology and Forensic Medicine

Published

1999

4. Abstracts

Author

Toshiyuki MATSUZAKI, Takeshi SUZUKI, Kuniaki TAKATA, Shin HASHIGUCHI, Masazumi HIRATA, Hiroaki MURATA, Hideyuki TAKESHITA, Katsuyuki KUSUZAKI, Eiichi KONISHI, Yasusuke HIRASAWA, Tsukasa ASHIHARA, T. Suginoshita, K. Kusuzaki, S. Hashiguchi, M. Hirata, J. Fukuroku, Y. Urata, Y. Hirasawa, T. Ashihara, Kanji KAWAI, Kazushige UEDA, Toshiya OCHIAI, Atsuhiro OGINO, Hirosumi ITOI, Hisakazu YAMAGISHI, Yoji URATA, Takahiro OKA, Toshiaki YAMAASHI, Masahiko AKITA, Ken TANOOKA, Kojun SETSU, Yasuhisa Maezawa, Hisatoshi Baba, Nobuaki Furusawa, Kenzou Uchida, Shinichi Imura, Yoshitaka TAMADA, Seiji HAYASHI, Norio IIJIMA, Hiromi IKE, Akihiko ISHIHARA, Masaki TANAKA, Fumihiko SUWA, Yasuhiko IBATA, Masaru Kimura, Hiroyasu SUGA, Norio MIYOSI, Takao NAKAGAWA, Masaru FUKUDA, Vadim S. Zinchuk, Teruhiko Okada, Toshihiro Kobayashi, Eva Garcia del Saz, Harumichi Seguchi, Youyun Zhang, Jibin Dai, Xinhua Zhou, Fong Dong, Akihiro HEMMI, Akira KOMIYAMA, Shinichi OHNO, Ryohei KATOH, Hideyuki Takeshita, Katsuyuki Kusuzaki, Yoshiro Tsuji, Masazumi Hirata, Shin Hashiguchi, Yasusuke Hirasawa, Tsukasa Ashihara, Shigeru MORIKAWA, Ikuko TORII, Makoto NAGASAKI, Satoko MISHIMA, Akira Mizoguchi, Chizuka Ide, Ichiro NAITO, Satoko INOUE, Satimaru SENO, Jun WATANABE, Kazumasa KONDO, Kazuto Mino, Shinsuke KANAMURA, Kohsuke CHIDA, Tetusya GOTO, Teruo TANAKA, Shigeru TAKAMI, Tatsuroh ODA, Fumiaki NISHIYAMA, Tomohiko Wakayama, Shoichi Iseki, AHMED KHALED, S. NORIKI, H. MAEGAWA, M. FUKUDA, Mingsen Jiang, Zujiang Yu, Mingyi Yang, Huifen Dong, Masaki UENO, Yutaka FUTAESAKU, Yoshimichi KOZUKA, Misai YANO, Michiko ONO, Yawara SUMI, Masanori T. Itoh, Minoru YOSHIDA, Atsuko Ito, Michiko Hayashi, Minako Hoshida, Kinji Ito, Kyoumi NAKAZATO, Keiji SUZUKI, Katuyuki NAKAJIMA, Tsuyoshi SAGA, Mitsuaki YOSHIZUKA, Norimichi Nemoto, Wei Lu, Hitomi Nakamura, Satoshi Hayakawa, Fuminao Chishima, Akio WATANABA, Akira KAWAOI, Lidia KRIA, Akihiro OHIRA, Tsugio AMEMIYA, Kazuhiro KARAYA, Takashi KONDO, Shinobu UMEMURA, Masanori YASUDA, Johbu ITOH, Susumu TAKEKOSHI, Yoshiyuki OSAMURA, Keiichi WATANABE, Yukihiro SASAKI, Helen AHMED, Takumi TAKEUCHI, Tetsuo UEKI, Takahiro KAJIWARA, Nobuo MORIYAMA, Kazuki KAWABE, Hiromichi YOKOI, Yoshihiro YAMAMA, Yoshihiro TSURUO, Kazunori ISHIMURA, Yoichiro Kato, Tomoko Yamamoto, Makio Kobayashi, Shin-ichi KOMIYAMA, Daisuke AOKI, Eiichiro TOMINAGA, Nobuyuki SUSUMU, Yasuhiro UDAGAWA, Shiro NOZAWA, Hideaki MURATA, Youzi URATA, Toshihisa Ito, Kohjiro HORITA, Yoshiaki IMAMURA, Sakon NORIKI, Gizo NAKAGAWARA, Yiqun Mo, Qunwei Zhang, Akio Yamaguchi, Kohjiro Horita, Shu Zheng, Chong-Guang Leng, Hideho Ueda, Yasuhisa Fujii, Nobuo Terada, Takeshi Baba, S. Yamazaki, S. Kameyama, R. Fukasawa, N. Moriyama, K. Kawabe, Yasuhiro KOBAYASHI, Hayato KAWAKAMI, Yoshikazu YOSHINO, Hiroshi HIRANO, Yoshihiro AKIMOTO, Lisa K. KREPPEL, Gerald W. HART, Kenji KAWASHIMA, Kyomi NAKAZATO, Katsuya HIRAISHI, Katsuaki UEHARA, Junichi SHIMADA, Shinji FUSHIKI, Nobuyuki Susumu, Ryohachi ARAI, Kazuyoshi SAKAI, Ikuko NAGATSU, Bo-Chul Shin, Yoshihiro ASAKAWA, Masato KOMURO, Lanxian Zhou, Hua Yuan, Jialuo Hu, Wenduo Huang, Xiaoyun Wang, Yohei MIYAMOTO, Mari SHIMBO, Shigeyuki TAHARA, Makoto SUGIYAMA, Ichiro TAKUMI, Naoko SANNO, Akira TERAMOTO, Minoru MATSUDA, Hisaki FUKUSHIMA, Ryota TANAKA, Ikuya SANTO, Tateo HANAOKA, Tomoyuki GOYA, Akihiko KUDO, and Akihiko Kudo

Subjects

Histology, Physiology, Cell Biology, Biochemistry, Pathology and Forensic Medicine

Published

1998

5. Angiogenesis in hepatocellular carcinoma as evaluated by CD34 immunohistochemistry

Author

Hiroyuki Kimura, Masamichi Kakusui, Keizo Kagawa, Tsukasa Ashihara, Tomoki Nakajima, Takeshi Deguchi, Tatsuo Katagishi, Takeshi Okanoue, and Kei Kashima

Subjects

Adenoma, Liver Cirrhosis, Pathology, medicine.medical_specialty, Carcinoma, Hepatocellular, Angiogenesis, CD34, Antigens, CD34, Biology, Neovascularization, Image Processing, Computer-Assisted, medicine, Carcinoma, Humans, neoplasms, Neoplasm Staging, Hyperplasia, Neovascularization, Pathologic, Hepatology, Liver Neoplasms, Antibodies, Monoclonal, Cancer, medicine.disease, Immunohistochemistry, digestive system diseases, Ki-67 Antigen, Hepatocellular carcinoma, Monoclonal, Disease Progression, Endothelium, Vascular, medicine.symptom

Abstract

To clarify the relationship between angiogenesis and hepatocarcinogenesis on progression of hepatocellular carcinoma (HCC), we quantitatively evaluated angiogenesis by CD34 immunohistochemistry in liver cirrhosis (LC), adenomatous hyperplasia (AH), and HCC, and proliferative activity estimated by Ki-67 immunohistochemistry. Angiogenesis was evaluated by CD34 immunohistochemistry using monoclonal antibody HPCA-2, and tumor proliferative activity was evaluated using monoclonal antibody MIB-1. We used an image analysis system to assess the microvessel density as the area percentage of the endothelial area. Angiogenesis was generally observed in HCC and there was no significant difference among all clinical stages and histological grades of HCC. On the other hand, the staining of CD34 was partly observed in sinusoids of AH, although no positive staining was seen in any sinusoids of LC. The proliferative activity was significantly correlated with the clinical stage and histological grade of HCC. Our results indicate that the quantitation of angiogenesis does not provide significant prognostic information in HCC, but that it may have diagnostic value in distinguishing HCC from non-HCC. Meanwhile, AH, which is not morphologically diagnosed as cancer, shows positive staining for CD34, suggesting that some portion of AH contains cancerous characteristics.

Published

2008

6. Detection of underlying characteristics of nuclear chromatin patterns of thyroid tumor cells using texture and factor analyses

Author

Kunio Mochizuki, Nobuki Nakamura, Shin-ichi Murata, Hiroto Yamashita, Tsukasa Ashihara, Yoji Urata, Tetsuo Kondo, Tadao Nakazawa, and Ryohei Katoh

Subjects

Adenoma, Pathology, medicine.medical_specialty, Karyometry, Biophysics, Papanicolaou stain, Biology, Pathology and Forensic Medicine, Endocrinology, Adenocarcinoma, Follicular, Biopsy, Image Processing, Computer-Assisted, medicine, Humans, Thyroid Neoplasms, Cell Nucleus, medicine.diagnostic_test, Goiter, Biopsy, Needle, Thyroid, DNA, Neoplasm, Cell Biology, Hematology, Anatomy, medicine.disease, Chromatin, Adenocarcinoma, Papillary, medicine.anatomical_structure, Adenocarcinoma, Factor Analysis, Statistical, Cytometry

Abstract

Background Aspiration biopsy cytology of thyroid tumors has been used more frequently in recent times to differentiate between malignant and benign lesions. Chromatin patterns of the tumor cell nuclei are one of most important factors for cytologic diagnosis. The interpretation of nuclear chromatin patterns is subjective and more difficult than that of nuclear size or shape. In the present report, we investigated how to detect underlying chromatin characteristics of benign and malignant thyroid tumor cells by means of texture and factor analyses. Methods We employed a computer-aided system in which light microscopy was combined with an image processor and monochrome camera. Using this system, 100 randomly selected cells in a Papanicolaou stained, aspiration biopsy cytologic smear in each case of 39 benign and malignant thyroid tumor cases were digitized. We applied two-dimensional and higher texture analyses with the use of co-occurrence and run-length matrices to analyze the chromatin patterns. Factor analysis was used to determine whether a large number of independent variables actually measured one or more underlying common variables. Results According to parameters with high factor-loading values, the morphologic chromatin characters were classified into three categories according to heterogeneity, contrast, and homogeneity of chromatin patterns. On the basis of analyses with these morphologic categories, nuclei of papillary carcinoma showed higher contrast of chromatin patterns than did those of the benign group. Moreover, there was a variety of contrasting chromatin patterns among cells in each papillary carcinoma case in comparison with the benign group. In contrast, follicular carcinomas showed a significant difference in the standard deviation of factor 3, which indicated more monotonous chromatin patterns among cells in each follicular carcinoma case than in each benign case. Conclusion We believe that this technique, using texture and factor analyses, is useful in the detection of underlying characteristics of nuclear chromatin patterns in aspiration biopsy cytology. Cytometry 49:91–95, 2002. © 2002 Wiley-Liss, Inc.

Published

2002

7. Acridine Orange Excited by Low-Dose Radiation Has a Strong Cytocidal Effect on Mouse Osteosarcoma

Author

Mitsuoki Hashiba, Katsuyuki Kusuzaki, Shin Hashiguchi, Hiroaki Murata, Yasusuke Hirasawa, Tsukasa Ashihara, Tsunehiko Nishimura, and Hideyuki Takeshita

Subjects

Cancer Research, Lung Neoplasms, Time Factors, Combination therapy, Cell Survival, medicine.medical_treatment, Photodynamic therapy, Mice, chemistry.chemical_compound, In vivo, Tumor Cells, Cultured, medicine, Animals, Photosensitizer, Cell Size, Osteosarcoma, Chemistry, business.industry, X-Rays, Acridine orange, Dose-Response Relationship, Radiation, General Medicine, medicine.disease, Acridine Orange, In vitro, Survival Rate, Radiation therapy, Microscopy, Fluorescence, Photochemotherapy, Oncology, Cancer research, Nuclear medicine, business, Neoplasm Transplantation

Abstract

The study was conducted to clarify the cytocidal effect of combination therapy consisting of administration of acridine orange (AO), which is a photosensitizer, and radiation therapy using in vitro and in vivo mouse osteosarcoma models. The results revealed that AO combined with low-dose X-ray irradiation of about 1–5 Gy had a strong cytocidal effect on the cultured mouse osteosarcoma cells regardless of their chemosensitivity, and that this combination therapy inhibited growth of the in vivo mouse osteosarcoma by induction of tumor necrosis. This effect was inhibited by L-histidine, but not by mannitol. These findings suggested that AO might be excited by X-rays and kill osteosarcoma cells through the release of singlet oxygen, which is toxic to living cells. This mechanism is similar to that of photodynamic therapy with AO.

Published

2002

8. Simple tumor profile chart based on cell kinetic parameters and histologic grade is useful for estimating the natural growth rate of hepatocellular carcinoma

Author

Michihisa Moriguchi, Keizo Kagawa, Yasuhide Mitsumoto, Tatsuo Katagishi, Tsukasa Ashihara, Hiroyuki Shintani, Hiroyuki Kimura, Takeshi Deguchi, Takeshi Okanoue, and Tomoki Nakajima

Subjects

Male, medicine.medical_specialty, Pathology, Carcinoma, Hepatocellular, H&E stain, Apoptosis, Biology, Gastroenterology, Pathology and Forensic Medicine, Immunoenzyme Techniques, Internal medicine, In Situ Nick-End Labeling, medicine, Carcinoma, Humans, Doubling time, Growth rate, Aged, Neoplasm Staging, Retrospective Studies, Aged, 80 and over, Large cell, Liver Neoplasms, Middle Aged, HCCS, medicine.disease, Kinetics, Ki-67 Antigen, Hepatocellular carcinoma, Immunohistochemistry, Female, Cell Division

Abstract

Thirty-four untreated hepatocellular carcinomas (HCCs) with known growth rates were classified into 5 groups on a tumor profile chart based on their doubling time (DT), Ki-67-positive index (Ki-67-PI), apoptotic index (Apo-I), and histologic grade. The slow-growing HCCs (DT > 100 days) consisted of well-differentiated tumors with slight cell kinetic imbalance and were divided into groups A and B. Group A had Apo-I values

Published

2002

9. DNA cytofluorometric analysis of chondrocytes in human articular cartilages under normal aging or arthritic conditions

Author

H. Murata, Tsukasa Ashihara, Yasusuke Hirasawa, Shin Hashiguchi, Hideyuki Takeshita, Takako Nozaki, Katsuyuki Kusuzaki, K. Emoto, and S. Sugimoto

Subjects

Adult, Male, Pathology, medicine.medical_specialty, Aging, Adolescent, Cell, Biomedical Engineering, Arthritis, Osteoarthritis, Cell Separation, Arthritis, Rheumatoid, Articular cartilage, Chondrocytes, DNA ploidy, Aging, Arthritis, Chondrocytes, Rheumatology, medicine, Humans, Orthopedics and Sports Medicine, Child, Aged, Aged, 80 and over, Chemistry, Cartilage, Infant, Newborn, Osteonecrosis, Infant, Cell cycle, Middle Aged, medicine.disease, Flow Cytometry, Diploidy, Staining, medicine.anatomical_structure, Child, Preschool, Immunology, Cytogenetic Analysis, Collagenase, Immunohistochemistry, Female, Cell Division, medicine.drug

Abstract

Objective Since most chondrocytes in articular cartilage are in the resting phase (G0) of the cell cycle, it has been difficult to investigate their cell kinetics using 3H-thymidine autoradiography, or immunohistochemistry. In the present study, DNA cytofluorometry, which is useful to analyse the cell kinetics even for such inactive cell populations as in the G0 phase, was applied to human chondrocytes of the articular cartilages under normal aging and pathologic conditions such as osteoarthritis (OA), rheumatoid arthritis (RA), and aseptic necrosis (AN). Design The human articular cartilages for the study were obtained from autopsy and surgical materials. Fifty joints were used for the study of aging, 54 for the study of OA, 20 for studying RA, and 10 for AN study. The isolated chondrocytes were quickly prepared from fresh articular cartilages, using a combination method of enzymatic digestion with papain and collagenase, followed by mechanical cell separation by churning and homogenization. Results The DNA histograms obtained by cytofluorometry with propidium-iodide staining showed that most chondrocytes had diploid DNA content (2c) in all cartilages studied, suggesting that they were in the G0 phase. However, there were a few chondrocytes having tetraploid DNA content (4c) in the normally aged articular cartilages, and there were some cells having DNA content between 2c and 4c in the diseased cartilages. The former cells were considered to be G0-phase cells of the 4c chondrocytes, while the latter cells were considered to be in the DNA synthetic (S) phase or G2-phase of the 2c chondrocytes. The frequency of 4c chondrocytes in aged cartilage was significantly increased, compared to that in the young cartilage. In contrast to the normal cartilage, the frequency of S- and G2-phase cells, which was expressed as the S– G2 index, in diseased cartilages (OA, RA and AN) was significantly high ( P 0.0001). In OA cartilage, the S–G2 index was much higher in the severe or moderate stage than in the mild stage, suggesting that the chondrocytes in clusters may actively proliferate. Conclusion These results showed that in normal articular cartilages most chondrocytes are in the G0 phase, while some became 4c polyploid cells, and that these G0-phase chondrocytes had a potential to proliferate under diseased conditions.

Published

2001

10. A long-term survival case of multiple hepatocellular carcinoma with metachronous lymph node metastasis

Author

Hisakazu Yamagishi, Teruhisa Sonoyama, Toshiya Ochiai, Yoji Urata, Takeshi Yamano, and Tsukasa Ashihara

Subjects

Pathology, medicine.medical_specialty, Hepatology, business.industry, Androgen Receptor Gene, Lymph node metastasis, medicine.disease, Primary tumor, digestive system diseases, Metastasis, Lesion, Infectious Diseases, medicine.anatomical_structure, Hepatocellular carcinoma, medicine, medicine.symptom, Complication, business, Lymph node

Abstract

A long-term survival case of multiple hepatocellular carcinoma (HCC) with metachronous metastasis to a lymph node is reported. The patient, a 66-year-old woman, had two primary HCC nodules, one each in the left and right hepatic lobes, which were resected. She developed a lymph node lesion and a secondary HCC 45 and 62 months after the first operation, respectively. She has been well for the 7 years since the first operation despite undergoing hepatic resection for HCC twice as well as lymph node resection. Clonal analysis, based on the methylation pattern of the X chromosome-linked androgen receptor gene, suggested that the two primary tumors were multicentric and that the lymph node lesion had arisen by metastasis from the primary tumor in the right hepatic lobe.

Published

2000

11. Osteoblastic differentiation and P-glycoprotein multidrug resistance in a murine osteosarcoma model

Author

Takehiko Suginoshita, Hiroaki Murata, Katsuyuki Kusuzaki, Shin Hashiguchi, Yasusuke Hirasawa, Hideyuki Takeshita, Henry J. Mankin, Mark C. Gebhardt, Tsukasa Ashihara, and Masazumi Hirata

Subjects

Cancer Research, Cellular differentiation, Antineoplastic Agents, P-glycoprotein, Mice, multidrug resistance, Tumor Cells, Cultured, medicine, Animals, ATP Binding Cassette Transporter, Subfamily B, Member 1, Osteosarcoma, Osteoblasts, biology, Cell growth, Regular Article, Cell Differentiation, differentiation, Transfection, medicine.disease, Phenotype, Drug Resistance, Multiple, Multiple drug resistance, Disease Models, Animal, Cell Transformation, Neoplastic, Oncology, Doxorubicin, Immunology, Cancer research, biology.protein, Alkaline phosphatase, malignancy

Abstract

A recent study of multidrug resistance (MDR) 1 gene transfected osteosarcoma cells found a cause-effect relationship between increased expression of P-glycoprotein (P-gp) and a low aggressive phenotype. However, several experimental and clinical studies have observed contradictory findings in that P-gp expression has been associated with tumour progression. In the present study, we characterized P-gp-positive and P-gp-negative single-cell clones of a murine osteosarcoma, to further investigate the relationship between P-gp expression and changes in cell phenotype. Although these clones were all selected by doxorubicin (DOX) exposure, they were heterogeneous with respect to MDR1 gene expression. The P-gp-positive clones revealed MDR phenotype, whereas the P-gp-negative clones showed no resistance to drugs. Morphological and functional analysis showed that both the P-gp-positive and P-gp-negative clones were more differentiated than the parent cells in terms of enhanced activity of cellular alkaline phosphatase, an increase in well-organized actin stress fibres and enhanced osteogenic activity. Moreover, these subclones all displayed a decrease in malignant potential such as oncogenic activity, tumour growth rate and metastatic ability, regardless of their P-gp status. These results indicate that the observed osteoblastic differentiation and less aggressive phenotype in DOX-selected osteosarcoma cells may not only be explained by the direct effect of P-gp, and accordingly, consideration of the effect of DOX, as well as P-gp, appears to be important. © 2000 Cancer Research Campaign

Published

2000

12. Clonal expansion in evolution of chronic hepatitis to hepatocellular carcinoma as seen at an X-chromosome locus

Author

Takeshi Yamano, Yoji Urata, Toshiya Ochiai, Tsukasa Ashihara, and Hisakazu Yamagishi

Subjects

Pathology, medicine.medical_specialty, Carcinoma, Hepatocellular, X Chromosome, Clone (cell biology), Locus (genetics), Biology, Polymerase Chain Reaction, medicine, Carcinoma, Humans, X chromosome, Aged, Hepatitis, Chronic, Hepatitis, Hyperplasia, Hepatology, Liver Neoplasms, DNA, Middle Aged, medicine.disease, Clone Cells, Androgen receptor, Liver, Receptors, Androgen, Hepatocellular carcinoma, Monoclonal, Female, Polymorphism, Restriction Fragment Length

Abstract

Clonal analysis has shown that hepatocellular carcinoma arises from a single cell. However, the clonality of precancerous lesions and adjacent nonneoplastic tissues is not clear. We analyzed a human androgen receptor locus to elucidate the clonal state of liver tissues including post-hepatitic lesions associated with hepatocarcinogenesis. The analysis was based on a restriction fragment length polymorphism involving an androgen receptor locus on the X chromosome, taking advantage of physiologic random inactivation by methylation of 1 of 2 X chromosomes in females during embryogenesis. Clonality was assessed in 79 randomly located tissue samples microdissected from noncirrhotic liver, including a total of 40 morphologically normal sites in 4 normal livers and 39 sites from a single HCV-infected liver. In addition, 51 regenerative nodules, 4 areas of adenomatous hyperplasia, and 18 hepatocellular carcinomas were sampled. All samples were obtained from livers involved by various neoplasms. Eight of forty samples (20.0%) from the four normal livers and 20 of the 39 samples (51.3%) from the single HCV-infected liver showed a monoclonal pattern. Moreover, 30 of 51 regenerative nodules (58.9%) showed a monoclonal pattern. No histologic differences were evident between mono- and polyclonal nodules. On the other hand, the 18 carcinomas and 4 areas of adenomatous hyperplasia all were monoclonal. Mean calculated monoclonal areas of normal liver and liver with chronic hepatitis were 1.1 and 3.3 mm(2). Our results suggest that areas representing a single clone of hepatocytes are present in normal liver, and these progressively expand as changes advance from chronic hepatitis to hepatocellular carcinoma.

Published

2000

13. Constrained, Random, and Independent Motion of Texas-Red-labeled Chromatin in Living Interphase PtK2 Cells

Author

Naoko Masuzawa, Katsumi Yagi, Tsukasa Ashihara, and Yoji Urata

Subjects

Histology, Physiology, PTK2, Chromosome, Texas Red, Cell Biology, Biology, Nuclear matrix, Biochemistry, Pathology and Forensic Medicine, Chromatin, Cell biology, chemistry.chemical_compound, Prophase, chemistry, Interphase, DNA

Abstract

In this study, we observed and analyzed the sub-micron motion of interphase chromosomes in living cells, labeled with the fluorescent thymidine analogue, Texas-Red dUTP. Our approach has an advantage in that chromosomes can be analyzed with regard to the nuclear architecture. We calibrated the observed motion of fluorescence-labeled chromatin by eliminating the rotational and translational movement of living nuclei that could significantly affect chromatin motion. Mathematical analyses of chromatin motion showed that: (1) interphase chromatin in living nuclei moves randomly, and the motion is limited within a small sub-region; (2) chromatin near the nuclear envelope moves in a more limited area than does centrally located chromatin; and (3) closely situated chromatin domains move independently of each other. Random and constrained chromatin motion in living nuclei supports the concept that interphase chromatin fibers are loose, flexible and floating in the nuclear matrix, and that chromatin anchors to the backbone of chromosomes. Moreover, that the random motions of DNA domains are independent of each other suggests that interphase chromatin arranges without structurally rigid continuity. This active motion of chromatin is consistent with dynamic biological processes, requiring chromosome motility and interactions. Additionally, the dynamic properties of interphase chromosomes may be significant in the interpretation of acquired chromosomal aberrations.

Published

2000

14. [Untitled]

Author

Isao Furukawa, Junji Suzuki, Tetsurou Fujii, Tsukasa Ashihara, Yutaka Ando, Sadayasu Ono, and Jun-ichi Hata

Subjects

Telemedicine, Multimedia, Computer Networks and Communications, business.industry, Computer science, Teleradiology, computer.software_genre, System requirements, Hardware and Architecture, Media Technology, Computer vision, Artificial intelligence, Computed radiography, Medical diagnosis, business, Telepathology, computer, Software, Digitization, Image compression

Abstract

It was recognized early on that the digitization of medical information would advance the efficiency of diagnostic technology. However, the digitization of image data, which makes up the majority of medical information, is dependent on advances in technologies such as input, processing, transmission, storage, and display. Insufficient advances in such technologies has effectively limited the digitization of image data for medical use. The result of this has been non-networked systems or LANs confined to a single hospital. Such isolated systems integrate only portions of digital medical images such as x-ray computer tomography (CT), magnetic resonance (MR), and computed radiography (CR). Fortunately, recent advances in the areas of super high definition image I/O, high-quality encoding, super high speed transmission, and high-capacity storage has turned the tide in favor of the digitization and networking of all medical information. This paper will focus on the digitization and networking of medical image information used within hospitals and provide a multifaceted study of the technologies necessary for these advances. This will allow us to discuss the present state of related technical developments and the level that has been attained so far. In addition, we have targeted image information that demands the highest level of quality (radiological and pathological images) for application in medical diagnosis using super high definition images, the image technology being developed by the authors of this paper. We will cover the concrete issues and approaches to solutions that must be investigated when building and networking a digital system.

Published

2000

15. Photodynamic Inactivation with Acridine Orange on a Multidrug‐resistant Mouse Osteosarcoma Cell Line

Author

Shin Hashiguchi, Tsukasa Ashihara, Hiroaki Murata, Ginjirou Minami, Takako Nozaki, Hideyuki Takeshita, Katsuyuki Kusuzaki, and Yasusuke Hirasawa

Subjects

musculoskeletal diseases, Male, Cancer Research, Pathology, medicine.medical_specialty, medicine.medical_treatment, Photodynamic therapy, Bone Neoplasms, Biology, Multidrug resistance, Article, chemistry.chemical_compound, Mice, medicine, Tumor Cells, Cultured, Neoplasm, Animals, Humans, Chemotherapy, Osteosarcoma, Mice, Inbred C3H, Ploidies, Acridine orange, medicine.disease, Molecular biology, Drug Resistance, Multiple, Multiple drug resistance, Oncology, chemistry, Photochemotherapy, Cell culture, Drug Resistance, Neoplasm, Acridine

Abstract

Overcoming multidrug resistance (MDR) is an urgent issue to improve the prognosis of osteosarcoma patients. In this study, we undertook to clarify the effect of photodynamic therapy (PDT) with acridine orange (AO) on the MDR mouse osteosarcoma (MOS / ADR1) cell line, by comparing the outcome with the effect on a chemosensitive osteosarcoma (MOS) cell line. Cultured cells of MOS and MOS / ADR1 cell lines were exposed to AO at various concentrations for various times, followed by long- or short-term (10 or 1 min) illumination with blue light (466.5 nm) for excitation. Living cells were counted by means of the trypan blue exclusion test. The results showed that AO rapidly bound to DNA, RNA and lysosomes of living MOS and MOS / ADR1 cells and also that most tumor cells in both cell lines died rapidly (viability ratio to untreated cells: 1/1000) within 48 h under conditions of continuous or 15-min flash exposure to AO at concentrations above 1.0 microg/ml plus 10-min illumination with blue light. Even after flash exposure to AO at concentrations above 1.0 microg/ml plus 1-min illumination, the viability of MOS/ADR1 cells decreased to a viability ratio of less than 1/ 1000 within 72 h. Based on these results, we concluded that AO with photo-excitation has a strong cytocidal effect, not only on chemosensitive mouse osteosarcoma cells, but also on MDR mouse osteosarcoma cells. These results suggested that photodynamic therapy with AO may be a new approach to treating MDR human osteosarcomas.

Published

2000

16. Prognostic value of DNA ploidy response to chemotherapy in human osteosarcomas

Author

Katsuyuki Kusuzaki, Shin Hashiguchi, Hideyuki Takeshita, Yasusuke Hirasawa, Tsukasa Ashihara, Hiroaki Murata, and Masazumi Hirata

Subjects

Adult, Male, Cancer Research, Pathology, medicine.medical_specialty, Adolescent, medicine.medical_treatment, Bone Neoplasms, Biology, Disease-Free Survival, Antineoplastic Combined Chemotherapy Protocols, medicine, Humans, Doxorubicin, Child, Dna ploidy, Aged, Cisplatin, Osteosarcoma, Chemotherapy, Ploidies, Middle Aged, Aneuploidy, Prognosis, medicine.disease, Methotrexate, Microscopy, Fluorescence, Oncology, Chemotherapy, Adjuvant, Aneuploid Cells, Female, Ploidy, medicine.drug

Abstract

We analyzed the DNA ploidy alterations after preoperative chemotherapy in 30 patients with non-metastatic osteosarcomas of the extremities. All of the patients received intensive chemotherapy with doxorubicin, cisplatin and methotrexate as well as wide tumor resection. DNA ploidy was determined by DNA cytofluorometry using isolated and smeared cells from biopsied and resected tumors after preoperative chemotherapy. The results showed that 12 diploid and nine non-diploid osteosarcomas did not change their ploidy pattern, but nine non-diploid tumors changed to a diploid pattern with the disappearance of the aneuploid cells. The nine patients with altered ploidy tumors had a better histologic response to chemotherapy and a better prognosis than the patients with non-altered tumors especially diploid tumors (P = 0.0138). Therefore, we conclude that a decrease in aneuploid cells after chemotherapy is closely correlated with a good prognosis in half of the cases of aneuploid osteosarcoma. These results also suggest that aneuploid cells are more chemosensitive than diploid cells in human osteosarcomas.

Published

1999

17. Relationship between chromosomal aberrations by fluorescence in situ hybridization and DNA ploidy by cytofluorometry in osteosarcoma

Author

Yasusuke Hirasawa, Tatuto Abe, Johji Inazawa, Tsukasa Ashihara, Katsuyuki Kusuzaki, and Hiroaki Murata

Subjects

Adult, Male, Cancer Research, Adolescent, Bone Neoplasms, Locus (genetics), In situ hybridization, Biology, Tumor Cells, Cultured, medicine, Humans, In Situ Hybridization, Fluorescence, Aged, Chromosome Aberrations, Osteosarcoma, Polysomy, Ploidies, medicine.diagnostic_test, Chromosome, DNA, Neoplasm, Middle Aged, Flow Cytometry, medicine.disease, Molecular biology, Chromosome 17 (human), Oncology, Genetic marker, Female, Chromosome Deletion, Ploidy, Fluorescence in situ hybridization

Abstract

An analysis of the chromosomal aberrations and DNA ploidy in the interphase nuclei of seven human osteosacomas was preformed by double-target fluorescence in situ hybridization (FISH) and DNA cytofluorometry. The FISH study of the numerical aberrations in chromosomes 1 and 17 or the structural aberrations in chromosome arm 1p or 17p was carried out by using four locus specific DNA markers, with one pair consisting of 1q12 and 1p36 and the other pair consisting of the 17 cemtromere and 17p13.3. There was no significant differences in the percentage of deletions in chromosome 1 and 17 between osteosarcomas and normal tissues. However, all seven tumors studied had extra copies. Cells with more than three probe signals were regarded as having chromosome polysomy. The percentage of polysomy of chromosome 1 was 20.0-64.0%, and chromosome 17 was 28.0-60.0%. The DNA ploidy patterns of hyperdiploid cells showing a greater DNA content than diploid cells were obtained by DNA cytoflurometry. Five of the seven tumors were non-diploid, and the remaining two were diploid. The percentage of polysomy was correlated with the percentage of hyperdiploid cells in each tumor. Thus, these findings indicated that the DNA ploidy changes were closely correlated with aberrations in the chromosome copy number in osteosarcomas.

Published

1999

18. Cytofluorometric DNA ploidy analysis in giant cell tumor of bone: histologic and prognostic value

Author

Hideyuki Takeshita, Yassusuke Hirasawa, Tsukasa Ashihara, Shin Hashiguchi, Hiroaki Murata, Masazumi Hirata, and Katsuyuki Kusuzaki

Subjects

Adult, Male, Cancer Research, Pathology, medicine.medical_specialty, Adolescent, Cell Proliferative Activity, Bone Neoplasms, Biology, Malignant transformation, chemistry.chemical_compound, Predictive Value of Tests, medicine, Humans, Fluorometry, Grading (tumors), Dna ploidy, Aged, Giant Cell Tumor of Bone, DNA, Middle Aged, Aneuploidy, Prognosis, medicine.disease, Diploidy, Microscopy, Fluorescence, Oncology, chemistry, Female, Ploidy, Cell Division, Giant-cell tumor of bone, DNA ploidy analysis

Abstract

DNA ploidy analysis by DNA cytofluorometry was performed on 41 tumors obtained from 37 patients with primary giant cell tumor of bone (GCT). Histologically, 26 of the tumors from primary or recurrent lesions were evaluated as grade I, and 13 tumors as grade II. Among the 33 primary GCT patients, 4 patients had local recurrence or pulmonary metastasis. The DNA ploidy pattern and the percentage of hyperdiploid cells showing a greater DNA content than diploid cells, were obtained from DNA cytofluorometry. All of the 33 primary tumors were diploid. Of 6 recurrent tumors, 4 were diploid and 2 were euploid-polyploid. One of the two pulmonary metastatic tumors was diploid, but another that demonstrated a malignant transformation to malignant fibrous histiocytoma was aneuploid. The percentage of hyperdiploid cells was significantly different between primary and recurrent tumors (P = 0.0188) and between grade I and grade II tumors (P = 0.0052), while there was no difference between primary tumors in the cases that recurred or metastasized and those that did not. Thus, these data indicate that cell proliferative activity is closely correlated with biological aggressiveness and histological grading, although DNA ploidy is not useful for predicting prognosis.

Published

1999

19. Prognostic significance of DNA ploidy pattern in osteosarcomas in association with chemotherapy

Author

Yasusuke Hirasawa, Hideyuki Takeshita, Masazumi Hirata, Shin Hashiguchi, Hiroaki Murata, Katsuyuki Kusuzaki, and Tsukasa Ashihara

Subjects

Adult, G2 Phase, Male, musculoskeletal diseases, Cancer Research, Pathology, medicine.medical_specialty, Adolescent, medicine.medical_treatment, Aneuploidy, Antineoplastic Agents, Bone Neoplasms, Biology, Disease-Free Survival, S Phase, Biopsy, medicine, Humans, Child, Survival rate, Aged, Cisplatin, Osteosarcoma, Chemotherapy, Ploidies, medicine.diagnostic_test, DNA, Neoplasm, Middle Aged, Prognosis, medicine.disease, Oncology, Female, Methotrexate, Ploidy, medicine.drug

Abstract

In this study, we analysed the DNA ploidy of osteosarcomas at biopsy and attempted to clarify the relationship between DNA ploidy pattern and prognosis. Thirty patients with non-metastatic osteosarcoma of an extremity were studied. All underwent intensive chemotherapy with doxorubicin, cisplatin and methotrexate, in addition to wide tumor resection. DNA ploidy was detected by DNA cytofluorometry, using isolated and smeared cells of biopsied tumor tissue. Twelve tumors showed a diploid ploidy pattern and 18 showed a non-diploid pattern such as aneuploidy (15 tumors) and euploid-polyploidy (3 tumors). The event-free survival rate at 9 years was 63.5% in non-diploid osteosarcoma patients and 13.3% in diploid osteosarcoma patients. There was a statistically significant difference between the two groups (P = 0.0278). These results lead us to conclude that a non-diploid osteosarcoma may be more sensitive to chemotherapy than a diploid tumor.

Published

1999

20. Novel Formula for Cell Kinetics in Xenograft Model of Hepatocellular Carcinoma Using Histologically Calculable Parameters

Author

Tsukasa Ashihara, Tatsuo Katagishi, Takeshi Deguchi, Keizo Kagawa, Yasuhide Mitsumoto, Kei Kashima, Tomoki Nakajima, Masamichi Kakusui, Hiroyuki Kimura, and Takeshi Okanoue

Subjects

Male, Cell kinetics, Carcinoma, Hepatocellular, Necrosis, Transplantation, Heterologous, Tumor cells, Biology, Mice, Idoxuridine, Tumor Cells, Cultured, medicine, Animals, Humans, Stage (cooking), Mice, Inbred BALB C, Liver Neoplasms, Cell Biology, HCCS, medicine.disease, Kinetics, Bromodeoxyuridine, Apoptosis, Hepatocellular carcinoma, Immunology, Cancer research, medicine.symptom, Neoplasm Transplantation

Abstract

The growth rate of tumors should be assessed in terms of both tumor cell proliferation and death. The former is considered to be determined by growth fraction and cell-cycle time, whereas the latter is mainly determined by apoptosis, especially in tumors with a low level of necrosis. While most hepatocellular carcinomas (HCCs) in a relatively early stage contain only a small amount of necrosis, the growth rate supposedly depends mainly on growth fraction, cell-cycle time, and apoptosis. However, their quantitative relationship remains unknown. We have derived a novel theoretical formula for determining this relationship in nonnecrotic HCC, using Ki-67-positive index, apoptotic score, and a correction factor, all calculable by histological assessment without injecting labeling agents. Furthermore, we confirmed the reliability of this formula, using a xenograft model of human HCC with less than 15% necrosis. In this model the values of cell-cycle time calculated from the formula were very close to those estimated by a conventional double-labeling method and showed high correlations. Since our novel formula can clarify the cell kinetics without cumbersome labeling procedures, it is expected to be clinically applicable to HCC with a small portion of necrosis, using the radiographically measured growth rate and the histologically assessed cell kinetic parameters.

Published

1999

21. Abstracts

Author

Takanori Nagaoka, Seiichiro Okajima, Masahito Oyamada, Tetsuro Takamatsu, Yasusuke Hirasawa, Mamoru Sano, Hitoshi Bamba, Yasuo Hisa, Toshiyuki Uno, Kazuhiro Syogaki, Yoshitaka Tamada, Norio Iizima, Yasuhiko Ibata, Akihiko ISHIHARA, Masaki TANAKA, Yoshitaka TAMADA, Norio IIJIMA, Seiji HAYASHI, Yasuhiko IBATA, Seiichiro OKAJIMA, Yasusuke HIRASAWA, Satomi Ebara, Kenzo Kumamoto, Tadao Matsuura, Sumio NISHIKAWA, Fumie SASAKI, Tomoko Imaizumi, Keiichi Tsukinoki, Yoshiko Miyoshi, Takayuki Yamamoto, Yoshihisa Watanabe, Masamoto Murakami, Masao Kasahara, Junko HIRATA, Chizuru OGAWA, Ichiro KUMANO, Masumi SUDA, Hirohiko IWATSUKI, Yoshitaka HISHIKAWA, Naofumi NAGASUE, Takehiko KOJI, Jun Watanabe, Hiroko Mondo, Yasuharu Takamori, Shinsuke Kanamura, V. Zinchuk, T. Okada, T. Kobayashi, H. Seguchi, Toshiya Ochiai, Yoji Urata, Teruhisa Sonoyama, Hisakazu Yamagishi, Tsukasa Ashihara, Masato OHNISHI, Atsuyuki WADA, Kiyoshi KUROKAWA, Hisao YAMADA, Yoshiko TAKAGISHI, Nicholas J. SEVERS, Yoshiharu MURATA, Keiichi YOKOYAMA, Shinsuke MASUDA, Masahito OYAMADA, Tetsuro TAKAMATSU, Shinsuke Masuda, Tsutomu Matsushita, Yumiko Oyamada, Wuxiong Zhou, Tomoyuki Kaneko, Shingo Kamoshida, Naoki Ogane, Masanori Yasuda, Takashi Bessho, Hiroshi Kajiwara, R.Yoshiyuki Osamura, Ryohei KATOH, Eri MIYAGI, Nobuki NAKAMURA, Xin LI, Koichi SUZUKI, Kenichi KAKUDO, Makio KOBAYASHI, Akira KAWAOI, Yoshihiko Kobayashi, Ryohei Katoh, Akira Kawaoi, Yoichiro KATO, Yoshiaki IMAMURA, Masaru FUKUDA, Hiroshi KAJIWARA, Masanori YASUDA, Reiko KUROTANI, Shingo KAMOSHIDA, Hironobu MAEDA, Takeshi HIRASAWA, Toshinari MURAMATSU, Masaru MURAKAMI, Takao SHINOZUKA, Yoshiyuki OSAMURA, Ahmed KHALED, Sakon NORIKI, Hisataka KATOH, Yayoi NISHI, Shuichi Kohri, Yoshio Shiina, Emi INUI, Munekado KOJIMA, Shinji FUSHIKI, Tsuneharu MIKI, Koichi Okada, Keiichi Yokoyama, Koji Okihara, Osamu Ukimura, Munekado Kojima, Tsuneharu Miki, Yoshiko Ueda, Suketaka Kanazawa, Takashi Kitaoka, Akihiro Ohira, A. Meddeb Ouertani, Tsugio Amemiya, Yasuo KOKUBO, Nobuaki FURUSAWA, Yasuhisa MAEZAWA, Kenzou UCHIDA, Takafumi YAYAMA, Hiroshi Tatsuo, Hisatoshi Baba, Masaru Fukuda, KENICHI OYAMA, REIKO KUROTANI, NAOKO SANNO, AKIRA TERAMOTO, R. YOSHIYUKI OSAMURA, Xiu ling LI, Tomokatsu HORI, Kintomo TAKAKURA, Osami KUBO, and Yasuhiko TAJIKA

Subjects

Histology, Physiology, Cell Biology, Biochemistry, Pathology and Forensic Medicine

Published

1999

22. Abstracts

Author

Kohtaro Takei, Naoaki SAITO, Norio SAKAI, Yasuhito SHIRAI, Atsushi MIYAWAKI, Mayumi NISHI, Hiroshi OGAWA, Mitsuhiro KAWATA, Tokuko Haraguchi, Masahito Watanabe, Masahisa Shimada, Shigeru HASEGAWA, Susumu TERAKAWA, Takashi TSUBOI, Yoji URATA, Naoko MASUZAWA, Tsukasa ASHIHARA, Akihiko KUDO, Hiroshi HIRANO, Takehiko KOJI, Shoichi Iseki, Masamoto Murakami, Masao Kasahara, Masanobu MIYAZAKI, Yoshiyuki OZONO, Shigeru KOHNO, Isamu Sugawara, and Yuxiu SHi

Subjects

Histology, Physiology, Cell Biology, Biochemistry, Pathology and Forensic Medicine

Published

1999

23. [Untitled]

Author

Yuhwsuke Sawada, Tsukasa Ashihara, Yoshihiro Takashima, and Isao Nakajima

Subjects

medicine.medical_specialty, Telemedicine, Point (typography), SIMPLE (military communications protocol), Multimedia, business.industry, media_common.quotation_subject, Internet privacy, MEDLINE, Medicine (miscellaneous), Health Informatics, computer.software_genre, Health informatics, Promotion (rank), Health Information Management, Communications satellite, Medicine, business, computer, Information Systems, media_common, Preventive healthcare

Abstract

There are several problems on the practical use of telemedicine, for example, the difficulties involved in promoting communication between medical facilities, uncooperative clinicians, and the absence of high-speed circuits and high-resolution CRT. From the Japanese point of view, we suggest ways to resolve these problems. We will analyze and propose scenarios for realizing successful communications among medical institutions, medical communication and its characteristics, barriers to the promotion of communications among medical institutions, second-opinion centers, and separate satellites and separate circuits. We also mention the World Wide Web for teleconsultation, provision of assistance to people with data handicaps via a communications satellite, and assistance to programs designed for training telemedicine specialists. Using a communication satellite, we offer programs that explain preventive medicine, support activities for nursing at home, explain the risks of fast food, and support activities for the handicapped and women in a simple manner to computer illiterates.

Published

1999

24. Aberrations of Chromosomes 1 and 17 in Six Human Osteosarcoma Cell Lines Using Double-Target Fluorescence In Situ Hybridization

Author

Hiroaki Murata, Katsuyuki Kusuzaki, Johji Inazawa, Tsukasa Ashihara, Tatsuo Abe, Hideyuki Takeshita, and Yasusuke Hirasawa

Subjects

Chromosome Aberrations, Genetic Markers, Osteosarcoma, Cancer Research, medicine.diagnostic_test, Aneuploidy, Chromosome, Bone Neoplasms, Biology, medicine.disease, Molecular biology, Chromosome 17 (human), Chromosomes, Human, Pair 1, Chromosome Arm, Tumor Cells, Cultured, Genetics, medicine, Humans, Interphase, Molecular Biology, Metaphase, In Situ Hybridization, Fluorescence, Chromosomes, Human, Pair 17, Fluorescence in situ hybridization

Abstract

Analysis of six human osteosarcoma cell lines was performed by using double-target fluorescence in situ hybridization (FISH). FISH was applied to interphase nuclei, not to metaphase chromosomes. In this study, numerical aberrations of chromosomes 1 and 17 or structural chromosomal aberrations of chromosome arm 1p or 17p, in which it has been suggested that there are one or more tumor suppressor genes in various malignant tumors, were examined with this technique. All six of the human osteosarcoma cell lines studied had extra copies of chromosomes 1 and 17. A high frequency of deletions (>60%) in chromosome 1 was found in two cell lines and deletions of chromosome 17 were found in one cell line.

Published

1998

25. Relation between cellular doxorubicin binding ability to nuclear DNA and histologic response to preoperative chemotherapy in patients with osteosarcoma

Author

Hideyuki Takeshita, Hiroaki Murata, Tsukasa Ashihara, Shin Hashiguchi, Yasusuke Hirasawa, Katsuyuki Kusuzaki, and Masazumi Hirata

Subjects

Adult, Male, musculoskeletal diseases, Oncology, Cancer Research, medicine.medical_specialty, Pathology, Necrosis, Adolescent, medicine.medical_treatment, Bone Neoplasms, In Vitro Techniques, Immunofluorescence, Internal medicine, Tumor Cells, Cultured, medicine, Humans, Doxorubicin, Child, Aged, Osteosarcoma, Chemotherapy, Antibiotics, Antineoplastic, medicine.diagnostic_test, business.industry, Prognosis, medicine.disease, Drug Resistance, Multiple, DNA-Binding Proteins, Multiple drug resistance, Chemotherapy, Adjuvant, Drug Resistance, Neoplasm, Immunohistochemistry, Female, Tumor necrosis factor alpha, Drug Screening Assays, Antitumor, medicine.symptom, business, medicine.drug

Abstract

BACKGROUND. Although chemosensitivity to antiosteosarcoma agents is the most important prognostic factor in human osteosarcoma, none of the many chemosensitivity tests reported previously are reliable and clinically useful. In this study, the authors investigated the reliability and clinical availability of doxorubicin (Adriamycin; Adria Laboratories, Columbus, OH) binding assay (ABA) as a new chemosensitivity test for osteosarcoma. METHODS. Doxorubicin (adriamycin [ADM]) binding ability (%AB) to nuclear DNA in isolated osteosarcoma cells was assessed by ABA in 14 patients with primary osteosarcoma who were treated with preoperative chemotherapy containing ADM and 6 patients with relapsed osteosarcoma after intensive chemotherapy. Histologic responses to preoperative chemotherapy were evaluated by percentage of tumor necrosis (%necrosis). RESULTS. Four of the 14 patients with primary osteosarcoma had %AB > 80% (97.3 ± 3.7%) and demonstrated good histologic responses (>90% of %necrosis) to preoperative chemotherapy, whereas the remaining 10 patients had %AB < 80% (38.9 ± 21.0%) and demonstrated poor responses. Patients with recurrent osteosarcoma that was clinically evaluated to be resistant to previous chemotherapy also had low %AB (34.2 ± 28.3%). CONCLUSIONS. Because the results of the current study revealed that ABA is useful for predicting chemosensitivity to chemotherapy with ADM as well as chemotherapy without ADM for patients with osteosarcoma, and because ABA technically is simple and results can be assessed rapidly, the authors conclude that ABA is a clinically useful chemosensitivity test for patients with osteosarcoma.

Published

1998

26. Ploidy analysis in paraffin-embedded malignant fibrous histiocytoma by DNA cytofluorometry and fluorescence in situ hybridization

Author

Tatuo Abe, Johji Inazawa, Tsukasa Ashihara, Hiroaki Murata, Yasusuke Hirasawa, and Katsuyuki Kusuzaki

Subjects

Genetic Markers, Cancer Research, Pathology, medicine.medical_specialty, Biopsy, Centromere, Biology, medicine, Humans, In Situ Hybridization, Fluorescence, Chromosome Aberrations, Polysomy, Ploidies, Histiocytoma, Benign Fibrous, medicine.diagnostic_test, Chromosomes, Human, Pair 11, Hybridization probe, Chromosome Mapping, Chromosome, Karyotype, DNA, Neoplasm, Flow Cytometry, medicine.disease, Molecular biology, Oncology, Chromosomes, Human, Pair 1, Paraffin, Genetic marker, Interphase, Ploidy, DNA Probes, Chromosomes, Human, Pair 17, Chromosomes, Human, Pair 8, Fluorescence in situ hybridization

Abstract

To prove the relationship between chromosomal aberration and DNA ploidy in human malignant fibrous histiocytoma (MFH), fluorescence in situ hybridization (FISH) and DNA cytofluorometry were performed in this study. For FISH study, the nucleus of each tumor cell was isolated from paraffin-embedded tissue of nine MFHs. Five chromosome-specific DNA probes (1p36, 1q12, 8q21.3, 11 centromere, and 17 centromere) were hybridized on cell nuclei. Cells with more than three probe signals were regarded as chromosome polysomy. All of the tumors analyzed by FISH had extra copies. The average percentage of polysomy in all tumors was high, ranging from 10.2% to 49.2%. The DNA ploidy patterns, and the percentage of hyperdiploid cells showing a greater DNA content than diploid cells, were obtained from DNA cytofluorometry. Three of nine were diploid patterns and six were non-diploid patterns, and the percentage of hyperdiploid cells in all tumors was high, ranging from 9.1% to 61.9%. The percentage of polysomy could be correlated with the percentage of hyperdiploid cells in each cell. In this study, we found that the DNA ploidy change was closely correlated with aberrations of chromosome copy number in MFH. In addition, the alterations of specific chromosome copy number could be detected in MFH showing diploid cells. Thus, these data indicate that FISH and DNA cytofluorometry are available as a cytogenetic tool for the analysis of interphase nuclei of bone and soft tissue tumors including MFH.

Published

1997

27. Histochemical Expression of Inducible Nitric Oxide Synthase and Inflammatory Cytokines in Alveolar Macrophages in Patients with ARDS

Author

Yoji Urata, Atsuko Kobayashi, Satoru Hashimoto, Tsukasa Ashihara, Yoshifumi Tanaka, Hideki Onodera, and Kunihiko Kooguchi

Subjects

ARDS, Pathology, medicine.medical_specialty, Histology, Physiology, medicine.medical_treatment, Lung injury, Biochemistry, Pathology and Forensic Medicine, Proinflammatory cytokine, law.invention, law, medicine, Macrophage, biology, medicine.diagnostic_test, business.industry, Cell Biology, respiratory system, medicine.disease, Intensive care unit, Nitric oxide synthase, Bronchoalveolar lavage, Cytokine, Immunology, biology.protein, business

Abstract

To evaluate the role of inducible nitric oxide synthase (iNOS) and proinflammatory cytokines in acute respiratory distress syndrome (ARDS), we immunostained alveolar macrophages (AMs) in the bronchoalveolar lavage fluid (BALF) collected from patients with ARDS, patients in the operating room whose lung function were normal, and non-ARDS patients who were intubated and artificially ventilated for one week in the intensive care unit. We observed the significant expression of iNOS, interleukin-6 (IL-6) and interleukin-8 (IL-8), in AMs obtained from BAL in ARDS patients by the immunocytochemical approach. By comparison, statistically significant elevation was detected in IL-8 levels in BALF supernatant from the ARDS patients compared with the control and the non-ARDS patients. These results suggest that the expression of proinflammatory cytokines and iNOS in AMs as determined by immunocytochemical technique may be an important predictor of the early stage of lung injury in ARDS. We suggest that NO and proinflammatory cytokines produced by AMs might play a pivotal role in acute lung injury. The immunocytochemical approach could be the most sensitive predictor for activated AMs in ARDS patients.

Published

1997

28. The Relationship between Numerical Aberrations of Chromosome 17 and Nuclear DNA Content in Colorectal Carcinoma Detected by Fluorescent In Situ Hybridization (FISH) and Cytofluorometry Using Auto-scanning Stage

Author

Yoji Urata, Tsukasa Ashihara, Eiichi Konishi, Atsuhiro Ogino, Toshiya Ochiai, Takahiro Oka, Kawai K, Hirosumi Itoi, Hisakazu Yamagishi, and Shinshichi Hamada

Subjects

Histology, Physiology, Hybridization probe, Cell Biology, In situ hybridization, Cell cycle, Biology, Biochemistry, Molecular biology, Pathology and Forensic Medicine, Nuclear DNA, Chromosome 17 (human), chemistry.chemical_compound, chemistry, Propidium iodide, Ploidy, DNA

Abstract

Recently, interphase cytogenetics using fluorescent in situ hybridization (FISH) was performed on various kinds of solid tumor, and their inherent karyotypic heterogeneities were revealed. Concerning this heterogeneity, we evaluated both the exhibiting number of chromosome 17 and nuclear DNA content on an identical nucleus by means of computer-controlled auto-scanning stage in order to demonstrate the alteration in number of chromosome 17 among cytofluorometrically distinct subpopulations.We investigated 8 lesions of surgically resected colorectal carcinomas, which were classified as aneuploid in quantitative DNA analysis and also exhibited an increase of 17-aneusomy nuclei. We used paraffin-embedded archival blocks. First, we prepared isolated cell specimens, and memorized the position of the cells on a glass slide using computer-controlled auto-scanning stage. Next, the specimens were stained with propidium iodide, and the fluorescent intensity was evaluated as nuclear DNA content in the order of cell position data. And lastly, FISH was performed with (peri) centromerespecific DNA probes for chromosome 17, and we enumerated the number of signals in a nucleus also according to cell position data. Then, we compared the distribution of number of chromosome 17 among cytofluorometrically distinct subpopulations. Three of 8 lesions showed a single GO+G1 peak, and the rest exhibited plural GO+G1 peaks in DNA profile. And 4 of 5 lesions, which showed plural GO+G1 peaks, presented a peak at the DNA value of (near) 2c. We could detect an alteration in the distribution of number of chromosome 17 between diploid peak and aneuploid peaks in 4 of 4 lesions which presented a peak at the DNA value of (near) 2c. However, we could ot find a difference in the distribution of number of chromosome 17 between GO+G1 peak and G2+M peak. These observations indicate that the distribution of number of chromosome 17 reflects an endoreduplication of genome content, yet, it does not alter in accordance with the phase of cell cycle. It is necessary to evaluate nuclear DNA content simultaneously in order to assess an essential cytogenetic change.

Published

1997

29. Investigation on the Surgical Treatment for Multifocal Early Gastric Cancers. Based on the Cell Proliferation Analysis by DNA-cytofluorometry

Author

Hisakazu Yamagishi, Tsukasa Ashihara, Teruhisa Sonoyama, Yuji Ueda, Masashi Nakata, Hirosumi Itoi, and Takahiro Oka

Subjects

chemistry.chemical_compound, chemistry, business.industry, Cell growth, Gastroenterology, Cancer research, Medicine, Surgery, business, Surgical treatment, DNA

Abstract

私たちの教室で治療した胃癌症例中で多発胃癌は5.6%あるが, 早期胃癌の中では多発のものは8.6%を占めて近年増加傾向にある. この多発早期胃癌は単発早期胃癌と比較して高齢者に多く, 隆起型, 分化型 (高分化腺癌) の頻度が高く, 占居部位は大半が胃体部, 幽門部で幽門側切除が可能であった. 私たちは多発早期胃癌の悪性度評価法として, 各病巣の癌細胞増殖動態を顕微測光法で解析してきた. 予後良, 好例では各病巣のDNAプロイディ・パターンはdiploidで増殖動態は類似し, 病巣間で著差を認めなかった. 一方, 予後不良例ではS-G2期細胞の増加, 多倍体化などの進行胃癌で見られる増殖動態を示し, これらの所見は病巣間でばらつきを示した. したがって, DNAプロイディ・パターンは多発早期胃癌の悪性度の指標になりうると考えられた. また, リンパ節転移の頻度は単発例と差がなく, 単発早期胃癌と同様な進行度評価を適用しうると考えられた.

Published

1995

30. Evaluation of hepatic proliferative activity in chronic liver diseases and hepatocellular carcinomas by proliferating cell nuclear antigen (PCNA) immunohistochemical staining of methanol-fixed tissues

Author

Keizo Kagawa, Masamichi Kakusui, Toru Ohkawara, Takeshi Okanoue, Takeshi Deguchi, Kei Kashima, Tomoki Nakajima, Tsukasa Ashihara, Hiroyuki Kimura, and Kazushige Ueda

Subjects

Pathology, medicine.medical_specialty, Carcinoma, Hepatocellular, Tissue Fixation, Cirrhosis, Polymers, Chronic liver disease, Fixatives, Surgical oncology, Formaldehyde, Proliferating Cell Nuclear Antigen, Internal medicine, Humans, Medicine, Hepatitis, Analysis of Variance, biology, business.industry, Liver Diseases, Methanol, Liver Neoplasms, Gastroenterology, Hepatology, medicine.disease, Immunohistochemistry, Proliferating cell nuclear antigen, Liver, Hepatocellular carcinoma, Chronic Disease, biology.protein, business, Cell Division

Abstract

The proliferative activity of chronic liver diseases and hepatocellular carcinomas (HCCs) was studied by PCNA immunohistochemistry. Human liver tissues were obtained by surgical operation or needle biopsy, and PCNA was detected by immunohistochemistry. PCNA-labelling indices (PCNA-LIs) of methanol-fixed tissues corresponded with the incidence of S-phase cells previously reported, whereas paraformaldehyde-fixed tissues showed extremely high PCNA-LIs in all specimens. Therefore, methanol-fixed tissues were used for evaluation. The PCNA-LIs of the methanol-fixed tissues were: normal liver 0.78 +/- 0.38%, chronic persistent hepatitis 1.06 +/- 0.86%, chronic aggressive hepatitis 2A 1.01 +/- 0.50%, chronic aggressive hepatitis 2B 4.20 +/- 1.79%, inactive cirrhosis 0.81 +/- 0.49%, active cirrhosis 1.96 +/- 0.93%, HCC of Edmondson's type I 4.83 +/- 1.98%, type II 6.65 +/- 1.69%, and type III 38.7 +/- 30.6%. PCNA-positive cells showed little specific distribution; in periportal areas in chronic hepatitis, at the margins of pseudolobules in cirrhosis, and throughout the tumor in HCC. These findings indicated that proliferative activity increased during the progression of chronic hepatitis, but that it decreased at the stage of cirrhosis. In chronic liver diseases, the PCNA-LIs reflected hepatitis activity. HCC showed higher proliferative activity than liver cirrhosis, and the histological grade was correlated with the PCNA-LI.

Published

1994

31. Biological Role of Proliferating Cell Nuclear Antigen (PCNA) Expression during Rat Liver Regeneration

Author

Takeshi Okanoue, Kei Kashima, Tsukasa Ashihara, Keizo Kagawa, Takeshi Deguchi, Tomoki Nakajima, Hiroshi Hikita, and Eiichi Konishi

Subjects

Pathology, medicine.medical_specialty, Histology, Nucleoplasm, DNA synthesis, Physiology, Regeneration (biology), Cell Biology, Biology, Biochemistry, Molecular biology, Pathology and Forensic Medicine, Proliferating cell nuclear antigen, chemistry.chemical_compound, chemistry, In vivo, biology.protein, medicine, Immunohistochemistry, Paraformaldehyde, DNA

Abstract

To elucidate the role of proliferating cell nuclear antigen (PCNA) in vivo, PCNA immunohistochemistry combined with 3H-thymidine autoradiography was performed on 2 types of regenerating rat livers. One group of rats underwent 2/3 partial hepatectomy (PH), and the other group 1/3 PH. After 3H-thymidine labeling, the livers were fixed with paraformaldehyde (PFA) and methanol, and paraffin-embedded. In methanol-fixed tissues, the serial changes of the PCNA-positive index (PCNA-PI) corresponded well with those of the 3H-thymidine-labeling index (3H-thymidine-LI) after each PH. In PFA-fixed tissues, however, the PCNA-PI was 26% before PH, when the 3H-thymidine-LI was below 1%. Furthermore, the 1/3 PH group, despite a continued low 3H-thymidine-LI, showed a rise in PCNA-PI to a level comparable to that in the 2/3 PH group. From these results, we propose 3 phases of PCNA expression. In PFA-fixed tissues, PCNA that was detectable before PH was considered pooled in G0-phase nucleoplasm (Phase I), and some or many of the PCNA-positive cells failed to enter the S-phase in the 1/3 PH group, reflecting the increased PCNA not bound to DNA replicons (Phase II). In methanol-fixed tissues, PCNA was detected only in the S-phase, indicating its direct involvement in DNA synthesis (Phase III). Therefore, determining PCNA-PI in methanol-fixed tissues is useful to evaluate proliferative activity, whereas that in PFA-fixed tissues must be assessed with great caution.

Published

1994

32. EGF binding activity of rat hepatocytes in liver regeneration after partial hepatectomyCell cycle analysis by cytofluorometry

Author

Takayuki Takeuchi, Kei Kashima, Keizo Kagawa, Yoji Urata, Tsukasa Ashihara, Hisashi Tada, Takeshi Okanoue, and Hiroshi Hikita

Subjects

medicine.medical_specialty, Hepatology, medicine.medical_treatment, Endogeny, Cell cycle, Partial hepatectomy, Biology, Liver regeneration, Nuclear DNA, Cell biology, chemistry.chemical_compound, Endocrinology, chemistry, Internal medicine, medicine, Hepatectomy, Receptor, hormones, hormone substitutes, and hormone antagonists, DNA

Abstract

To analyze EGF binding activity in liver regeneration at cell cycle level, we performed the double measurement of nuclear DNA content and cellular bound EGF content in freshly isolated rat hepatocytes from normal and regenerating liver after 67% hepatectomy using autostaging cytofluorometry. The data demonstrated that the bound EGF content of resting cells increased in proportion to their DNA content, while cycling cells had significantly consistently lower bound hEGF throughout cell cycle. These changes are supposed to reflect ‘down-regulation’ of EGF receptor at the cell cycle level, and the data suggested a major role of endogenous EGF in cell proliferation during liver regeneration.

Published

1993

33. Usefulness of monitoring of complement fragments in a patient with idiopathic interstitial pneumonia

Author

Hideki Onodera, Masahiro Ueda, Masayuki Okamoto, Masako Deguchi, Kunio Yanagida, Kasamatsu Y, Youhei Hosokawa, Motoharu Kondo, Shigeru Sugino, Risa Narahara, Mitsuo Kishimoto, Shuhei Takemura, Wataru Fukuda, and Tsukasa Ashihara

Subjects

Pathology, medicine.medical_specialty, business.industry, Immunology, medicine, Immunology and Allergy, General Medicine, medicine.disease, business, Idiopathic interstitial pneumonia, Immune complex, Complement (complexity)

Abstract

症例は67歳女性.呼吸困難,乾性咳,発熱にて入院した.現病歴,胸部X線写真, CTなどより特発性間質性肺炎と診断した.抗生物質,ステロイドの投与にていったん症状の改善を認めたが,入院中再び呼吸困難が増悪し,ステロイドの増量にもかかわらず呼吸不全にて死亡した.剖検では肺炎所見を認めず,死因は急速に進行した肺線維化による呼吸不全と右心不全によるものと考えられた.経過中,補体分解産物iC3, Bb, c4dおよびC3a, C5aを経時的に測定できた.剖検所見と補体の動きからその病態に補体の活性化がかかわっていたことが示唆された.

Published

1990

34. Correlation of fixation, HCL hydrolysis and proteolytic digestion in bromodeoxyuridine immunohistochemistry of human stomach labeled by extracorporial perfusion system

Author

Yasunari Tsuchihashi, Shinjo Mitsufuji, Yohei Hosokawa, Kazushi Isetani, Tsukasa Ashihara, Toshio Tani, and Kazuhiko Tokita

Subjects

Pathology, medicine.medical_specialty, Histology, Physiology, Stomach, Proteolytic enzymes, Broxuridine, Cell Biology, Biology, Biochemistry, Molecular biology, Pathology and Forensic Medicine, chemistry.chemical_compound, medicine.anatomical_structure, chemistry, Cancer cell, medicine, Immunohistochemistry, Fixative, Bromodeoxyuridine, Fixation (histology)

Abstract

Bromodeoxyuridine (BrdU) immunohistochemistry has recently been introduced for the visualization of DNA-synthesizing nuclei. To determine the optimal conditions for detecting BrdU-incorporated nuclear DNA in formalin- or ethanol-fixed, paraffin-embedded human gastric tissues, we tested several different pretreatment procedures of hydrolysis with HCl and enzymatic digestion with actinase before the immunohistochemical staining. Three cases of surgically resected stomachs were perfused with artificial blood containing BrdU and fixed in formalin, ethanol or with their combination for different durations. The results of BrdU-immunohistochemical stainings were checked and the labeling indices were compared. As for hydrolysis, treatment with 2N HCl at 25°C for 90min was sufficient to detect the immunoreactivity in the stomach irrespective of fixative conditions tested. However, to obtain the most suitable stainings an additional enzymatic digestion was needed, and the optimal condition with actinase was different according to the fixation time in formalin- and/or ethanol-fixed tissues. There are also a few differences in the demonstrability of nuclear BrdU among various kinds of cells, i.e. normal epithelial cells, immunoblasts in the lymphoid follicle and cancer cells. Our method could extend the range of application of BrdU immunohistochemistry for cell kinetic studies using human surgically resected organs.

Published

1990

35. BETA.-Adrenergic effects on salivary glands: Growth and gene regulation

Author

Tsukasa Ashihara, Setsuya Fujita, and Tibor Barka

Subjects

Regulation of gene expression, medicine.medical_specialty, Histology, Salivary gland, Physiology, Cell growth, β adrenergic, Cell Biology, Biology, Biochemistry, Pathology and Forensic Medicine, Parotid gland, Endocrinology, medicine.anatomical_structure, Internal medicine, Gene expression, medicine, β adrenergic receptor

Published

1990

36. Combined analysis of nuclear morphometry and DNA cytofluorometry on thyroid tumors

Author

Yasunari Tsuchihashi, Hirosumi Itoi, Tsukasa Ashihara, Sin-ichi Murata, Yoji Urata, and Fumio Matsuzuka

Subjects

chemistry.chemical_compound, Pathology, medicine.medical_specialty, chemistry, business.industry, Medicine, business, Thyroid tumors, DNA

Abstract

私達の近年の開発研究に基づく顕微測光と画像解析の結合解析法を応用し, 顕微蛍光測光法による細胞増殖動態の解析単独では鑑別の困難な, 甲状腺の腺腫様過形成5例濾胞腺腫12例および濾胞癌12例を検索した.単離採取した一つひとつの細胞について, 細胞測光による核DNA定量と細胞核の形態解析 (面積, 周囲長, 核DNA濃度, 形状係数など) を対応させて行った.各症例について細胞周期の全ての時期の細胞 (全細胞) 群に対して形態解析を行うとともに, 細胞周期に基づく形状変化の影響を除外して客観的に形態学的特性を評価するために, 2倍体細胞 (G0-G1期細胞) 群に限定した解析も行った.その結果, 検索した腺腫様過形成, 濾胞腺腫および濾胞癌の核DNA量分布パタンは類似していたが, 2倍体細胞の核形態の不規則さは, 腺腫様過形成や腺腫よりも腺癌において有意に高度であることが定量的に示された.以上より, 本法が, 甲状腺腫瘍の良・悪性鑑別に, 細胞測光法や画像解析法単独による解析よりも, 有用であると考えられた.

Published

1990

37. A staining method for bone canaliculi

Author

Hiroaki Murata, Tsukasa Ashihara, Hideyuki Takeshita, Katsuyuki Kusuzaki, Hironari Shinjo, Yasusuke Hirasawa, and Naoto Kageyama

Subjects

Male, Pathology, medicine.medical_specialty, Osteoblasts, Staining and Labeling, business.industry, Histology, Anatomy, Bone canaliculus, digestive system, Bone and Bones, Rats, Staining, Bone cell, Animals, Medicine, Orthopedics and Sports Medicine, Surgery, Rats, Wistar, business

Abstract

The modified Bodian method with protargol (silver protein) is ordinarily used to detect nerve fibers. With this technique, applied to decalcified rat bone sections, the bone canaliculi were clearly stained black with good contrast to the bone matrix in both lamellar and woven bone. In addition, the connections between the bone canaliculi and other canaliculi, osteoblasts, osteoclasts, and chondrocytes were easily detectable. We found that the bone canaliculi of woven bone were fewer in number and ran more irregularly than those of lamellar bone. We believe that this staining method for bone canaliculi in decalcified bone is superior to previously reported methods and may be useful in studies on bone pathology.

Published

1995

38. Acridine orange induces binucleation in chondrocytes

Author

Hideyuki Takeshita, Yasusuke Hirasawa, Takako Nozaki, H. Murata, Katsuyuki Kusuzaki, Shin Hashiguchi, Tsukasa Ashihara, and K. Emoto

Subjects

Cell fusion, Mitotic index, Chondrocytes, Growth plate, Binuclear cells, Acridine orange, Acridine orange, Biomedical Engineering, Mitosis, Cell growth rate, DNA, Biology, Molecular biology, Acridine Orange, chemistry.chemical_compound, Brdu labeling, Chondrocytes, Biochemistry, chemistry, Rheumatology, Cytoplasm, Animals, Orthopedics and Sports Medicine, Cattle, Cell Division

Abstract

Objective Although it is well known that binuclear cells commonly appear among the chondrocytes of normal cartilages as well as among neoplastic chondrocytes of chondrosarcomas, the mechanism of binucleation is still unclear. Therefore, this study was undertaken to clarify the mechanism of binucleation in chondrocytes, using primary culture cells of growth plate cartilage. Design These chondrocytes were exposed to acridine orange (AO) which is a fluorescent dye for differentiating certain DNAs and RNAs in nuclei and cytoplasm, and which inhibits mitosis. After exposure to 0.5μg/ml AO, for 0, 6, 24, 48, and 96h, the following parameters were investigated: (1) cell growth rate (GR); (2) frequency of hyperdiploid cells (%HDC) by DNA cytofluorometry; (3) mitotic index (MI); (4) BrdU labeling index (LI); (5) frequency of binuclear cells (%BNC). Results Compared with the control cells, which were cultured in AO-free medium, the GR was remarkably inhibited at 24h. MI was also decreased from 6 to 24h, and LI decreased at 48h. However, these parameters were recovered at 96h. The %HDC was increased from 6 to 96h, and the %BNC was also increased to a maximum of six times that of the control cells at 96h. Discussion These results suggested that the binuclear cells observed among the cultured chondrocytes may be formed from G2 arrested cells by amitotic nuclear division, but not by mitosis without cytoplasmic division or cell fusion.

Published

2001

39. Development of bone canaliculi during bone repair

Author

Hironari Shinjo, Naoto Kageyama, Hiroaki Murata, Yasusuke Hirasawa, Hideyuki Takeshita, Tsukasa Ashihara, Shin Hashiguchi, and Katsuyuki Kusuzaki

Subjects

Fracture Healing, Histology, Mature Bone, Bone decalcification, Physiology, Chemistry, Osteoid, Endocrinology, Diabetes and Metabolism, Bone healing, Anatomy, Bone canaliculus, Bone and Bones, Rats, medicine.anatomical_structure, Osteocyte, Intramembranous ossification, Bone cell, medicine, Animals, Rats, Wistar

Abstract

We recently found that silver impregnation staining with protargol (silver protein), that is, a modified Bodian method, is useful for histologically identifying the details of bone canaliculi structure, using thin sections of decalcified bone tissues. With this staining method, we conducted the present study to assess the development of bone canaliculi during the process of intramembranous ossification using a fracture-like stimulation model of the rat femur. After making a drill-hole in the cortex of the rat femur, decalcified thin sections were obtained after 3, 5, 7, and 14 days by the standard paraffin-embedding procedure. Silver staining for bone canaliculi was performed using our previously reported technique. The results showed that woven bone covered the fracture surface of the cortex after 5 days, then immature lamellar bone attached to the woven bone after 7 days, and finally the lamellar bone matured and became thick with appositional growth after 14 days. The osteocytes in the woven bone appeared at an early stage of bone repair and developed a few canaliculi that were short and irregularly distributed in the osteoid matrix, while the osteocytes in the lamellar bone at a late stage formed many bone canaliculi that were long and regularly distributed in mature bone matrix. Therefore, we concluded that woven bone osteocytes may be necessary for induction of the lamellar bone osteocytes followed by active appositional growth of the lamellar bone at the early stage of bone repair, and also that both bone tissues could be clearly distinguished from one another based on the pattern of development of bone canaliculi by the osteocytes, as seen with the use of our sensitive staining method.

Published

2000

40. Total tumor cell elimination with minimum damage to normal tissues in musculoskeletal sarcomas following photodynamic therapy with acridine orange

Author

Yasusuke Hirasawa, Takehiko Suginoshita, Hiroaki Murata, Hideyuki Takeshita, Katsuhiro Aomori, Tsukasa Ashihara, Ginjorou Minami, Katsuyuki Kusuzaki, and Shin Hashiguchi

Subjects

Male, Cancer Research, Pathology, medicine.medical_specialty, Ratón, medicine.medical_treatment, Normal tissue, Photodynamic therapy, Antineoplastic Agents, Bone Neoplasms, Curettage, chemistry.chemical_compound, Mice, Medicine, Animals, Musculoskeletal Diseases, Mice, Inbred C3H, Osteosarcoma, business.industry, Acridine orange, General Medicine, medicine.disease, Acridine Orange, Disease Models, Animal, Treatment Outcome, Oncology, chemistry, Photochemotherapy, Acridine, Sarcoma, business, Mutagens

Abstract

Acridine orange (AO) has unique biological actions enabling tumor visualization (fluorovisualization) and a strong cytocidal effect (photodynamic therapy: AO-PDT) under illumination with blue light. Accordingly, in this study, we attempted to develop a new surgical technique for total tumor cell elimination using these photodynamic reactions with AO in a mouse osteosarcoma model. The results showed that local tumor recurrence was significantly inhibited (23%) in the group treated with curettage under fluorovisualization and AO-PDT, compared to that (80%) in the control group treated with curettage alone under ordinary light. Therefore, we concluded that the combination of curettage under fluorovisualization and AO-PDT may be useful for total tumor cell elimination with minimum damage to normal tissue in musculoskeletal sarcomas.

Published

2000

41. Intrinsic resistance to chemotherapeutic agents in murine osteosarcoma cells

Author

Katsuyuki Kusuzaki, Tsukasa Ashihara, Mark C. Gebhardt, Hideyuki Takeshita, Yasusuke Hirasawa, and Henry J. Mankin

Subjects

musculoskeletal diseases, Cytoplasm, Cell Membrane Permeability, Cell, Biological Transport, Active, Antineoplastic Agents, Bone Neoplasms, Drug resistance, Cross Reactions, Mice, Adenosine Triphosphate, medicine, Tumor Cells, Cultured, Cytotoxic T cell, Animals, Humans, Orthopedics and Sports Medicine, Doxorubicin, ATP Binding Cassette Transporter, Subfamily B, Member 1, Cisplatin, Osteosarcoma, Antibiotics, Antineoplastic, urogenital system, business.industry, General Medicine, DNA, Neoplasm, Saponins, medicine.disease, Alkaline Phosphatase, Calcium Channel Blockers, Drug Resistance, Multiple, Clone Cells, Multiple drug resistance, Gene Expression Regulation, Neoplastic, Molecular Weight, medicine.anatomical_structure, Phenotype, Verapamil, Cell culture, Drug Resistance, Neoplasm, Immunology, Cancer research, Surgery, business, Cell Division, medicine.drug

Abstract

Background: There are two general categories of drug resistance: acquired and intrinsic. The mechanisms involved in acquired drug resistance have been extensively studied, and several mechanisms have been described. However, the mechanisms responsible for intrinsic drug resistance have not been elucidated, to our knowledge. The purpose of the present study was to investigate the cytological and biochemical differences between acquired and intrinsic drug resistance in osteosarcoma cells. Methods: We previously isolated a clonal cell line (MOS/ADR1) to study acquired resistance in osteosarcoma by exposure of parental murine osteosarcoma cells (MOS) to doxorubicin. In the present study, we cloned a new, intrinsically resistant cell line (MOS/IR1) by single-cell culture of MOS cells and we investigated the differences in cell phenotype and the mechanisms of resistance in both of these resistant clones. Results: The MOS/ADR1 and MOS/IR1 cells were sevenfold and fivefold more resistant to doxorubicin than the parental murine osteosarcoma cells. Morphologically, the MOS/ADR1 cell line was composed of polygonal cells, whereas the MOS/IR1 cell line consisted of plump spindle cells with long cytoplasmic processes. The MOS/IR1 cells showed a much lower level of alkaline phosphatase activity than did the MOS/ADR1 and MOS cells. There were no substantial differences in the cellular DNA content or the doubling time among these three lines. Overexpression of the P-glycoprotein involved in the function of an energy-dependent drug-efflux pump was detected in the MOS/ADR1 cells but not in the MOS/IR1 cells. After the cells were incubated with doxorubicin for one hour, the two resistant lines had less accumulation of the drug than did the parent line (p < 0.05). The addition of a P-glycoprotein antagonist, verapamil, or the depletion of cellular adenosine triphosphate resulted in a marked increase in the accumulation of doxorubicin in the MOS/ADR1 cells (p < 0.05) but not in the MOS/IR1 cells. The MOS/ADR1 cells were found to exhibit cross-resistance only to substrates for P-glycoprotein (such as doxorubicin, vincristine, and etoposide), whereas the MOS/IR1 cells were resistant to all of the drugs studied (including cisplatin and methotrexate). The degree of drug resistance in the MOS/IR1 cells was found to be associated with the molecular weight of the drugs (p < 0.05). Permeabilization of the plasma membrane by saponin increased both the accumulation of doxorubicin (p < 0.05) and the cytotoxic activity of this drug in all lines, but the effects were most pronounced in the MOS/IR1 cells. Conclusions: Taken together, this data suggests that reduced drug accumulation in the MOS/IR1 cells may be due to the effect of decreased permeability of the plasma membrane on the transport of drugs from the extracellular environment into the cytosol of the cell and that this may be the mechanism responsible for intrinsic resistance to multiple drugs in the MOS/IR1 cell line. Clinical Relevance: Current drug treatment for human osteosarcoma may include multiple chemotherapeutic agents, such as doxorubicin, cisplatin, and methotrexate. These drugs exhibit different cytotoxic actions and, thus, the mechanisms of resistance to individual drugs vary. Clinical resistance to multidrug chemotherapy may be observed in tumors that recur after repetitive chemotherapy and in previously untreated tumors. In the former group, a tumor cell may express multidrug resistance by combining several different mechanisms due to its exposure to various drugs. In the latter group, however, this is not likely. Decreased intracellular drug accumulation due to reduced permeability of the plasma membrane, found in the MOS/IR1 cells, is one possible mechanism and may explain the intrinsic resistance to multidrug chemotherapy for the treatment of osteosarcoma. Further study regarding the resistance mechanism in the MOS/IR1 cells may help to overcome the intrinsic drug resistance in osteosarcoma.

Published

2000

42. Relationship between P-glycoprotein positivity, doxorubicin binding ability and histologic response to chemotherapy in osteosarcomas

Author

Yasusuke Hirasawa, Hiroaki Murata, Tsukasa Ashihara, Masazumi Hirata, Shin Hashiguchi, Katsuyuki Kusuzaki, and Hideyuki Takeshita

Subjects

Adult, Male, Cancer Research, medicine.medical_specialty, Pathology, Adolescent, medicine.medical_treatment, Histological response, Fluorescent Antibody Technique, Bone Neoplasms, Immunofluorescence, Gastroenterology, Internal medicine, medicine, Humans, Doxorubicin, ATP Binding Cassette Transporter, Subfamily B, Member 1, Child, P-glycoprotein, Chemotherapy, Osteosarcoma, Antibiotics, Antineoplastic, biology, medicine.diagnostic_test, business.industry, medicine.disease, Multiple drug resistance, Binding ability, Oncology, biology.protein, Female, sense organs, business, medicine.drug

Abstract

We previously reported that the doxorubicin binding ability detected by the doxorubicin (adriamycin) binding assay was closely correlated with the chemosensitivity of human osteosarcomas. In this study, we undertook to clarify the relationship between P-glycoprotein positivity (%PPG) and doxorubicin binding ability (%DB) in human osteosarcomas in order to determine which is a more sensitive index of histologic response to chemotherapy. Ten primary osteosarcomas were analyzed by the doxorubicin binding assay and by immunofluorescence to detect cellular P-glycoprotein positivity. Three good responders to chemotherapy containing doxorubicin showed a %DB greater than 90% (average: 96.43%), whereas the seven poor responders had values less than 80% (average: 35.31%). The difference between the two groups was statistically significant (P = 0.0167). However, the average %PPG of the three good responders was 6.73%, whereas the %PPG of the seven poor responders was 14.27%. There was no significant difference in %PPG between the two groups (P = 0.3051). No negative correlation between the %DB and the %PPG of all osteosarcomas (r = 0.536, P = 0.1104) was found, although there was a trend that those tumors with a high %PPG showed a low %DB. These results suggest that osteosarcomas showing a low %DB and %PPG with poor response to chemotherapy, may have multidrug resistance mechanisms other than P-glycoprotein. Therefore, we conclude that doxorubicin binding ability, which reflects all of the doxorubicin-resistant mechanisms, was more sensitive than P-glycoprotein positivity in predicting the chemosensitivity of human osteosarcoma.

Published

1999

43. Response of DNA ploidy to chemotherapy in primary and metastatic lesions in human osteosarcomas

Author

Hiroaki Murata, Tsukasa Ashihara, Yasusuke Hirasawa, Masazumi Hirata, Katsuyuki Kusuzaki, Shin Hashiguchi, and Hideyuki Takeshita

Subjects

Male, Cancer Research, Pathology, medicine.medical_specialty, Metastatic lesions, Lung Neoplasms, Adolescent, medicine.medical_treatment, Bone Neoplasms, Biology, Antineoplastic Combined Chemotherapy Protocols, medicine, Humans, Doxorubicin, Child, Dna ploidy, Chemotherapy, Osteosarcoma, Lung, Ploidies, DNA, Neoplasm, medicine.disease, Aneuploidy, medicine.anatomical_structure, Oncology, Tumor necrosis factor alpha, Female, Ploidy, medicine.drug

Abstract

Primary and pulmonary metastatic and pulmonary metastatic tumors (two synchronous and seven metachronous metastases) in nine patients with osteosarcomas were studied by DNA cytofluorometry. All patients were treated with both pre and postoperative chemotherapy. The results showed that all five diploid osteosarcomas and three of the four aneuploid tumors did not markedly change their ploidy pattern after preoperative chemotherapy, and had almost the same ploidy patterns as the pulmonary metastatic lesions. Those eight tumors showed poor histologic response and chemoresistance by the doxorubicin binding assay. Only one aneuploid osteosarcoma showing good histologic response and chemosensitivity changed its ploidy pattern to diploid, with the disappearance of aneuploid tumor cells and its synchronous pulmonary metastatic tumor also showed conversion to a diploid pattern with massive tumor necrosis. It is evident that those tumors showing no change in their ploidy pattern after chemotherapy were resistant to the chemotherapy. Therefore, we conclude that regardless of whether the pulmonary metastatic tumors were synchronous or metachronous, they showed the same change in their ploidy pattern as well as their chemosensitivity as the primary human osteosarcoma from which they were derived.

Published

1999

44. Telepathology system for microscopic images utilizing superhigh-definition imaging system over B-ISDN

Author

Tsukasa Ashihara, Akira Okumura, Sadayasu Ono, Toshikazu Sakano, Fujii Tatsuya, Junji Suzuki, Jun-ichi Hata, Isao Furukawa, and Katsuhiro Ishimaru

Subjects

Engineering, business.industry, Image quality, Real-time computing, Digital data, Integrated Services Digital Network, Digital image, Transmission (telecommunications), Computer vision, Artificial intelligence, Medical diagnosis, business, Telepathology, Image resolution

Abstract

It has been recognized early on that digitizing medical information makes diagnostic technology more advanced and efficient. In order to convert image information, which comprises the majority of all medical information, into digital data, various technologies including those for input, processing, transmission storage, and display need to develop at roughly the same pace. To data, there have been few cases where this has been done. However, recent major advances in high-resolution image input/output, image encoding, super-fast transmission, high-capacity storage, and other technologies have intensified the drive towards digitizing and networking all medical information. This paper will show that the spread of super-high-speed networks capable of transmitting large amounts of data in a short time is indispensable for accurate medical diagnosis, and that this will make it possible to realize an integrated medical information syste. A target application for the medical image diagnosis of the Super High Definition imags being developed by the authors of this paper is telepathology, which particularly demands high-quality images. In this paper, we will study, among other things, the concrete issues crucial to building and networking a digital system and the approach to resolving such issues. We will also report on the building of our experimental system that fulfills such demands as well as discuss a pathological microscopic image transmission system with image quality that will not lower diagnostic accuracy and fast response and good operability that will not make diagnosticians feel impatient. Finally, we will discuss a test in which we remotely operated a microscope over an ATM line to prove that it is possible to capture, transmit, and display a still super-high-definition digital image with a resolution of 2,048 X 2,048 pixels in about 5 seconds.

Published

1999

45. [Predictability of Gleason score and reduction time (tau) of prostatic volume after castration for the prognosis of prostatic cancer]

Author

Tsukasa Ashihara, Akio Iida, Hiroki Watanabe, Koji Okihara, Wataru Inoue, Makoto Watanabe, Fumiya Hongo, Eiichi Konishi, Masahito Saitoh, Yutaro Azuma, Jun Nakamura, and Tsuneyuki Nakanouchi

Subjects

Oncology, Male, medicine.medical_specialty, Multivariate analysis, Time Factors, Wilcoxon signed-rank test, Urology, Statistics, Nonparametric, chemistry.chemical_compound, Prostate, Predictive Value of Tests, Internal medicine, mental disorders, medicine, Humans, Castration, Survival analysis, Aged, Ultrasonography, Aged, 80 and over, medicine.diagnostic_test, business.industry, Cancer, Prostatic Neoplasms, Organ Size, medicine.disease, Prognosis, Survival Analysis, medicine.anatomical_structure, chemistry, Predictive value of tests, Multivariate Analysis, Transrectal ultrasonography, business

Abstract

PURPOSE: The efficacy of the reduction time (tau) after castration as a prognostic factor was examined by comparing to Gleason score. MATERIALS AND METHODS: The change of prostatic volume after castration was observed from the castration to 3 months after in 24 cases of prostatic cancer. Prostatic volume was examined by transrectal ultrasonography of the prostate. Survival curves was calculated by Kaplan-Meier method. Differences among survival curves were analyzed using Cox-Mantel test. RESULTS: tau had a close relationship to the prognosis of each case (Wilcoxon test: p < 0.05, Cox-Mantel test: p < 0.05). Gleason score had a weak relationship to prognosis (Wilcoxon test: N. S., Cox-Mantel test: p < 0.05). CONCLUSIONS: tau was efficient as prognostic factor compared to Gleason score.

Published

1998

46. Expression of inducible nitric oxide synthase and inflammatory cytokines in alveolar macrophages of ARDS following sepsis

Author

Tsukasa Ashihara, Satoru Hashimoto, Yoji Urata, Yoshihiro Kitamura, Atsuko Kobayashi, Kunihiko Kooguchi, and Hideki Onodera

Subjects

Pulmonary and Respiratory Medicine, Adult, Male, ARDS, medicine.medical_treatment, Fluorescent Antibody Technique, Nitric Oxide Synthase Type II, Pulmonary Edema, Lung injury, Critical Care and Intensive Care Medicine, Proinflammatory cytokine, Sepsis, Macrophages, Alveolar, Medicine, Humans, Prospective Studies, Aged, Lung, medicine.diagnostic_test, biology, business.industry, Interleukin-6, Interleukins, Interleukin-8, Proteins, Middle Aged, medicine.disease, Nitric oxide synthase, Bronchoalveolar lavage, Cytokine, medicine.anatomical_structure, Immunology, biology.protein, Female, Inflammation Mediators, Nitric Oxide Synthase, Cardiology and Cardiovascular Medicine, business, Bronchoalveolar Lavage Fluid, Interleukin-1

Abstract

Study objective The objective of this study was to evaluate the role of inducible nitric oxide synthase (iNOS) and proinflammatory cytokines in alveolar macrophages (AMs) in the pathogenesis of ARDS following sepsis. Setting ICU in a university hospital. Design Prospective exploratory, open-labeled study was carried out. Patients A total of 24 patients were investigated: 8 patients diagnosed as having ARDS following sepsis (ARDS group); 8 patients under general anesthesia in the operating room whose lung functions were normal (control group); and 8 patients who were intubated and artificially ventilated for 1 week in the ICU whose lung functions were not deteriorated without fulfilling the ARDS criteria and whose general state fulfilled the sepsis criteria (long-term ventilation group, or LTV group). Measurements and results The expression of iNOS, interleukin-1β (IL-1β), interleukin-6 (IL-6), and interleukin-8 (IL-8) in AMs obtained from RAL fluid (RALF) was determined by the immunofluorescent technique. We observed the significant expression of iNOS, IL-6, and IL-8 only in the ARDS group. Meanwhile, NOx (the sum of NO 2 – + NO 3 – ) was elevated in the BALF supernatant, and IL-6 and IL-8 levels in both the BALF supernatant and the serum were also elevated in the ARDS group. No significant expressions were detected in the control and the LTV group. Conclusions The result that iNOS was detected only in ARDS patients following sepsis suggests that iNOS together with proinflammatory cytokines produced by AMs might play a pivotal role in the pathogenesis of acute lung injury and be useful for monitoring disorders in the lung in such conditions.

Published

1998

47. Actin organization associated with the expression of multidrug resistant phenotype in osteosarcoma cells and the effect of actin depolymerization on drug resistance

Author

Hideyuki Takeshita, Katsuyuki Kusuzaki, Yasusuke Hirasawa, Henry J. Mankin, Tsukasa Ashihara, and Mark C. Gebhardt

Subjects

Cancer Research, Cytochalasin B, Cellular differentiation, macromolecular substances, Microfilament, chemistry.chemical_compound, Mice, polycyclic compounds, Tumor Cells, Cultured, Animals, ATP Binding Cassette Transporter, Subfamily B, Member 1, Cytoskeleton, Actin, P-glycoprotein, Osteosarcoma, biology, Cell Differentiation, Actins, Drug Resistance, Multiple, Cell biology, Multiple drug resistance, Oncology, chemistry, Cytoplasm, Doxorubicin, Immunology, biology.protein

Abstract

We have previously reported that P-glycoprotein (Pgp)-overexpressing multidrug resistant (MDR) osteosarcoma cells were functionally more differentiated than their parent cells. The present study showed that in the parent cells, the actin filaments were sparsely distributed or were diffusely spread throughout the cytoplasm, whereas the MDR osteosarcoma cells exhibited a remarkable increase in well-organized actin stress fibers. Furthermore, dihydrocytochalasin B, a specific inhibitor of actin polymerization, dramatically disrupted this network of stress fibers, increased the intracellular accumulation of doxorubicin (DOX) and modified the resistance against DOX. These results indicate that the organization of actin filaments associated with cellular differentiation may be involved in the expression of Pgp function in the MDR osteosarcoma cells.

Published

1998

48. Signal characteristics and compression performance evaluation of digital pathological microscopic images with up to SHD resolution

Author

Junji Suzuki, Akira Okumura, Sadayasu Ono, Isao Furukawa, and Tsukasa Ashihara

Subjects

Color difference, business.industry, Computer science, Image quality, ComputingMethodologies_IMAGEPROCESSINGANDCOMPUTERVISION, Image processing, computer.file_format, JPEG, Digital image, 2K resolution, Distortion, Chrominance, Computer vision, Artificial intelligence, business, Telepathology, computer

Abstract

Digitizing high-quality microscopic images and developing input/output technology for displaying those results is critical to tele-pathology in which pathological microscopic images are transferred to remote locations where they are diagnosed by specialists. This paper will discuss the results achieved by directly digitizing pathological microscopic images at a 2k by 2k resolution, and then using a super high definition imaging system to analyze their signals and evaluate compression performance. We will start off by digitizing samples that a pathologist will actually use in making a diagnosis, and then analyze their color distribution and spatial frequencies characteristics by comparing them to general images. This will make it apparent that such pathological images characteristically contain high spatial frequency in their chrominance components. We will also discuss the evaluation results of color differences for L.a.b space and compression ratios achieved when using JPEG to encode pathological images. We will also present a subjective evaluation of the influence sub- sampling of chrominance components has on image quality.© (1997) COPYRIGHT SPIE--The International Society for Optical Engineering. Downloading of the abstract is permitted for personal use only.

Published

1997

49. Medical tele-education system with superhigh-definition (SHD) image viewer

Author

Tsukasa Ashihara, Hiroshi Tsumura, Yoji Urata, Jun-ichi Hata, Yoshimi Fukuhara, and Sadayasu Ono

Subjects

Multimedia, Computer science, Image quality, Hypermedia, Image processing, Client-side, computer.software_genre, Expert system, law.invention, law, Adaptation (computer science), computer, Server-side, Image compression

Abstract

We have been studying a medical tele-education support system by an individual tutoring system, called CALAT, and a super high definition (SHD) image processing system, called SuperFM-III.Now, we are in a trial operation to use the SuperFM-III for a super high definition image controlviewer on the CALAT client side, and have created the courseware of the pathological images. Inthis paper, we show the concept and the implementation of this system.KEY WORDS: Super High Definition image, Tele-education, Medical-education 1. INTRODUCTION Recently, the research on the tele-education support system which uses the characteristic ofthedistributed hypermedia environment of WWW (World-Wide Web) is becoming active. However,there have been few systems where the individual adaptation mechanism operates to select the appropriate content that the system can actively present according to the student's levelof understanding.In NTT (Nippon Telegraph and Telephone Corporation), an individual tutoring system CAIAT(Computer Aided Learning and Authoring environment for Tele-education)1 which uses WWW isbeing investigated. In CALAT, the individual adaptation mechanism is achieved by using anintelligent education support system CAIRNEY (CAl expeRt system for NEw technologY)2 for theWWW server side. CAIRNEY, which has been developed in NTf, is an intelligent CAl system ofa standalone type. The system has the courseware more than 200 titles.Also, NTT is researching on the SuperFM-III (Super Frame Memories III system)3' 4) The

Published

1996

50. Cytogenetic analyses of hepatocellular carcinoma by in situ hybridization with a chromosome-specific DNA probe

Author

Tomoki Nakajima, Tsukasa Ashihara, Hiroyuki Kimura, Kei Kashima, Takeshi Deguchi, Tatsuo Katagishi, Keizo Kagawa, Toru Ohkawara, Masamichi Kakusui, and Takeshi Okanoue

Subjects

Adult, Male, Cancer Research, Pathology, medicine.medical_specialty, Carcinoma, Hepatocellular, Centromere, In situ hybridization, Biology, Malignancy, medicine, Humans, neoplasms, In Situ Hybridization, Aged, Ploidies, Hybridization probe, Liver Neoplasms, Cytogenetics, Chromosome, Nuclear Proteins, Cell Differentiation, HCCS, Middle Aged, medicine.disease, Neoplasm Proteins, Chromosome 17 (human), Ki-67 Antigen, Oncology, Cancer research, Female, Ploidy, Tumor Suppressor Protein p53, Cell Division, Chromosomes, Human, Pair 17

Abstract

BACKGROUND Numerical chromosome analysis has been established in solid tumors by using in situ hybridization (ISH) with a chromosome-specific probe. We analyzed human hepatocellular carcinoma (HCC) by ISH for chromosome 17 and investigated the correlation of its copy number with histologic malignancy, proliferative activity, p53 mutation, and DNA ploidy. METHODS Chromosome 17 was hybridized with a pericentromere-specific DNA probe directly on the tumor cells isolated from paraffin blocks of 25 surgically resected HCCs. Proliferative activity was measured by Ki-67 immunohistochemistry, p53 mutation was analyzed by p53 immunohistochemistry, and DNA ploidy was estimated by cytofluorometry. RESULTS Forty-four percent of the 25 HCCs showed numerical abnormality of chromosome 17. Many disomic cases had a less malignant histology, whereas many polysomic cases had a more malignant histology. The Ki-67 positive index of polysomic cases was higher than that of disomic cases. In 22 cases (88.0%), the copy number of chromosome 17 was well matched with DNA ploidy. However, the numerical abnormality of chromosome 17 did not show a significant correlation with p53 mutation. Two of four HCCs that showed histologic heterogeneity were also heterogenous on ploidy pattern and the copy number of chromosome 17. Conversely, there was one case in which only ISH could demonstrate heterogeneity, although the other features exhibited homogeneity. CONCLUSIONS Numerical chromosome abnormalities correlated with the increase of histologic malignancy proliferative activity, and DNA ploidy. Moreover, ISH analysis was useful in assessing the intratumoral heterogeneity in HCC, especially when current methods failed to detect it. Thus, ISH provides information on important biologic features, such as malignant potential and intratumoral heterogeneity, in HCC. Cancer 1996;77:271-7.

Published

1996