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2. P1127: WATCHFUL WAITING IS AN ACCEPTABLE TREATMENT OPTION FOR PRIMARY OCULAR ADNEXAL MUCOSA-ASSOCIATED LYMPHOID TISSUE LYMPHOMA: A RETROSPECTIVE STUDY

Author

K. Mizuhara, T. Kobayashi, M. Nakao, R. Takahashi, H. Kaneko, K. Shimura, K. Hirakawa, N. Uoshima, Y. Kamitsuji, K. Wada, E. Kawata, R. Isa, T. Fujino, Y. Matsumura-Kimoto, T. Tsukamoto, S. Mizutani, Y. Shimura, M. Taniwaki, and J. Kuroda

Subjects
Diseases of the blood and blood-forming organs, RC633-647.5
Published
2022
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5. PS1354 MYELOMA-INDUCED MYELOID-DERIVED SUPPRESSOR CELLS ARE TARGETED BY IMMUNOMODULATORY DRUGS THAT REGULATE THE CCL5/CCR5 AXIS AND MIF AND IRF8 EXPRESSION

Author

Y. Mizuno, S. Horiike, J. Kuroda, Y. Fujibayashi, Reiko Isa, T. Kobayashi, T. Takimoto-Shimomura, T. Tsukamoto, Y. Chinen, Y. Matsumura-Kimoto, J. Yamaguchi, Yuji Shimura, S. Kuwahara-Ota, M. Taniwaki, and D. Nishiyama

Subjects
Cancer research, Myeloid-derived Suppressor Cell, Hematology, IRF8, Biology, CCL5
Published
2019
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6. Effect of laser fluence on the deposition and hardnessof boron carbide thin films

Author

Yoshinori Koga, M. Taniwaki, F. Kokai, and Masatou Ishihara

Subjects
Materials science, Analytical chemistry, Mineralogy, General Chemistry, Boron carbide, Nanoindentation, Fluence, Amorphous solid, Pulsed laser deposition, chemistry.chemical_compound, Carbon film, chemistry, General Materials Science, Atomic ratio, Thin film
Abstract

We deposited amorphous thin films of boron carbide by pulsed laser deposition using a B4C target at room temperature. As the laser fluence increased from 1 to 3 J/cm2, the number of 0.25–5 μm particulates embedded in the films decreased, and the B/C atomic ratio of the films increased from 1.8 to 3.2. The arrival of melt droplets, atoms, and small molecular species depending on laser fluence appeared to be involved in the film formation. In addition, with increasing fluence the nanoindentation hardness of the films increased from 14 to 32 GPa. We believe that the dominant factor in the observed increase in the films’ hardness is the arrival of highly energetic ions and atoms that results in the formation of denser films.

Published
2002
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7. Laser ablation of boron carbide: thin-film deposition and plume analysis

Author

A. Goto, Fumio Kokai, Yoshinori Koga, Kazuhiro Yamamoto, K Takahashi, M. Taniwaki, and Masatou Ishihara

Subjects
Materials science, Laser ablation, Mechanical Engineering, Analytical chemistry, General Chemistry, Boron carbide, Fluence, Electronic, Optical and Magnetic Materials, Pulsed laser deposition, Carbide, Amorphous solid, chemistry.chemical_compound, Carbon film, chemistry, Materials Chemistry, Electrical and Electronic Engineering, Thin film
Abstract

Thin films of boron carbide were formed by pulsed laser deposition at room temperature using a sintered B 4 C target. The nature of the particulates embedded in the films and the composition and bonding states of the films varied depending on the laser fluence. The formation of non-stoichiometric amorphous films appeared to be dominated by the arrival of energetic B and C atomic species with expansion velocities of 1–30 km/s and the stability of chemical bonds.

Published
2001
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8. The quality factor of niobium flexure pendulums

Author

Li Ju, M. Taniwaki, R. Andrew, and David Blair

Subjects
Factor (chord), Physics, Quality (physics), Volume (thermodynamics), chemistry, Niobium, General Physics and Astronomy, chemistry.chemical_element, Atomic physics
Abstract

The quality factor of niobium is shown to be dependent on both geometry and treatment, but is roughly independent of frequency. The Q -factor is given by Q ≈ 10 7 ( V S ) 1 2 , where V S is the volume to surface ratio (in SI units). The geometry effects lead to a lower Q -factor than previously expected for test masses suspended by membrane flexures.

Published
1999
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9. The Ig Heavy Chain Gene Is Frequently Involved in Chromosomal Translocations in Multiple Myeloma and Plasma Cell Leukemia as Detected by In Situ Hybridization

Author

K, Nishida, A, Tamura, N, Nakazawa, Y, Ueda, T, Abe, F, Matsuda, K, Kashima, and M, Taniwaki

Subjects
Adult, Male, congenital, hereditary, and neonatal diseases and abnormalities, education, Immunology, Immunoglobulin Variable Region, Paraproteinemias, Chromosome Disorders, Biochemistry, Translocation, Genetic, Leukemia, Plasma Cell, Bone Marrow, immune system diseases, hemic and lymphatic diseases, Humans, Chromosomes, Artificial, Yeast, In Situ Hybridization, Fluorescence, Aged, Aged, 80 and over, Chromosome Aberrations, Chromosomes, Human, Pair 14, Gene Rearrangement, Genes, Immunoglobulin, Chromosomes, Human, Pair 11, Chromosome Mapping, Cell Biology, Hematology, Middle Aged, Chromosome Banding, Karyotyping, Female, Chromosomes, Human, Pair 18, Immunoglobulin Heavy Chains, Multiple Myeloma
Abstract

Chromosome rearrangement of 14q32.33 has recurrently occurred with variable partner sites, including 11q13.3, 8q24.1, 18q21.3, and 6p21.1 in multiple myeloma (MM). To assess the actual incidence of 14q32.33 translocation and to elucidate its implication in the pathogenesis of MM, we studied 42 patients with MM, plasma cell leukemia, or plasmacytoma and 5 with monoclonal gammopathy with undetermined significance (MGUS) by G-banding and molecular cytogenetic methods. Using double-color fluorescence in situ hybridization (DCFISH) with 2 Ig heavy chain (IgH) gene probes, a yeast artificial chromosome (YAC) clone containing variable region, and a phage clone containing γ constant region, 14q32.33 translocation was detected as split signals of the IgH gene in 31 patients with plasma cell malignancies and 3 with MGUS. In contrast, of 40 patients who were assessed by G-banding, 3 (7.5%) showed the 14q+ chromosome. DCFISH detected a split of the IgH gene on interphase nuclei in 34 (73.9%) of 46 patients analyzed, whereas on metaphase spreads, it was in 22 (51.2%) of 43 patients analyzed. Interphase DCFISH was particularly useful to detect 14q32.33 translocation in 17 (65.4%) of 26 patients with normal karyotypes. Donor sites were identified in 11 of 22 patients demonstrated as carrying 14q32.33 translocation by metaphase FISH. Chromosome t(11; 14)(q13.3; q32.33) was detected in 5 patients, t(8; 14)(q24.1; q32.33) in 2, t(14; 18)(q32.33; q21.3) in 2, and t(7; 14)(q32.1; q32.33) in 1. A complex 14q32.33 translocation involving 3q and 16q24 was detected in 1 patient. Myeloma cells with t(7; 14) showed myelomonocytoid surface antigen. Because rearrangements of 14q32.33 were closely associated with translocation of proto-oncogenes into the IgH gene, our findings indicate that 14q32.33 translocation with various partner chromosomes is a critical event in the pathogenesis of MM and MGUS.

Published
1997
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10. Report of the Sixth International Workshop on Human Chromosome 21 Mapping 1996

Author

J. Derré, M. Taniwaki, C. Cassano, F. Hecht, S. Jitrapakdee, H.-U.G. Weier, R. Rinke, E. Takahashi, T. Watari, Y. Nakamura, A. Tanigami, J. Adélaïde, T. Foulon, P. Chardon, H. Ichise, A. Jones, C.D.K. Bottema, T. Shiratsuchi, P. Coullin, N. Namba, M. Rocchi, R. Mori, P. Gaudray, C. Theillet, R. Berger, J.J. Chen, S.J. O’Brien, F. Canavez, D.H. Ledbetter, T. Kawabe, F. Pröls, D. Chérif, J.E. Swallow, J. de Gunzburg, H. Tanaka, P.H. Vogt, G.C. Webb, H. Hayes, M.A.M. Moreira, N. Mueller-Lantzsch, C. Gouzy, L.B. Nielsen, S. Bekri, J.Y. Wang, Y. Endo, A. Lori, C.-B. Kang, M. Negrini, S.G. Young, J.F. Cochran, J. Aurich-Costa, A. Tamura, D.W. Bianchi, S. Kojima, V. lacobazzi, G. Ershova, D.K. Zhen, P. Parham, A. Courseaux, Y. Nozawa, C. Morelli, R. Dalgleish, F. Caroli-Bosc, Y. Akao, G.P. Robertson, R. Hliscs, K. Narahara, E. Meese, A. Hasegawa, Y. Kuga, P.K. Gill, S. Chételin, T. Tokino, S. Sonta, X. Luan, T. Ono, M. MacDougall, K.-W. Cho, J. Grosgeorge, R. Scarpato, S. Nakashima, F. Palmieri, M. Suzuki, E.J. Androphy, J. Kaplan, G. Panasiuk, B. Rautenstrauss, B.K. Hecht, D. Perucca-Lostanlen, S.D. Pack, D. Birnbaum, K. Kita, Y. Matsuda, Jc. Wallace, T. Okamoto, H.N. Seuánez, S. Yoshimura, G. Barbanti-Brodano, K. Hayakawa, S. Cadel, M. Andoh, W.-L. Kuo, H.-Y. Youn, M. Vaiman, D. Simmons, R. Barale, T. Sato, L. Viggiano, D. Polikoff, A. Munnich, S. Merscher, H. Satoh, U. Claussen, C. Rogel-Gaillard, J. Mayer, V. Nancy, R. Marzella, H. Sakai, H. Kyushioki, T.G. Lugo, P.M. Kelley, I. Kondo, T. Duell, M.-J. Pébusque, P. Mühlig, T.T. Gu, W.K. Merrison, D. Kowbel, Y. Seino, M.N. Fukuda, B.R. DuPont, H. Tsujimoto, M. Wernick, J.M. Boyle, M.. Horie, K. Myambo, M. Okuda, C.C. Collins, H. Hirawake, H. Nishimori, S. Harris, A. Hufford, P. Cohen, F. Cardona, and T. Liehr

Subjects
geography, geography.geographical_feature_category, Evolutionary biology, Centromere, Spring (hydrology), Genetics, Biology, Chromosome 21, Molecular Biology, Genetics (clinical)
Published
1997
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11. 151Eu Mössbauer effect study of T′- and T*-phase superconductors

Author

M. Kusuhashi, M. Taniwaki, and H. Itho

Subjects
Superconductivity, Lanthanide, Nuclear and High Energy Physics, Materials science, Condensed matter physics, Mössbauer effect, Doping, Electron, Condensed Matter Physics, Atomic and Molecular Physics, and Optics, symbols.namesake, Phase (matter), Mössbauer spectroscopy, symbols, Physical and Theoretical Chemistry, Debye model
Abstract

The (La,Eu(2CuO4 system shows superconductivity by dopingCe orSr. Carriers inT′-phase doped withCe are electrons and those inT*-phase doped withSr are holes. In this work,151Eu Mossbauer analysis is applied for theT′-phase(La1−xEux)2−yCeyCuO4 and theT*-phase(La1−xEux)2−ySryCuO4 in order to compare the electronic state and the lattice vibration ofEu in these superconductors. In addition, correlations betweenTc and Mossbauer parameters are examined. The isomer shift of151Eu is 0.784–0.840 mm/s in theT*-phase and 0.689–0.733 mm/s in theT′-phase, which shows that the lanthanide in these superconductors is tri-valent. The Debye temperature of151Eu is 180–208 K in theT*-phase and 160–192 K in theT′-phase. The difference of isomer shift between these two phases is explained by theEu−O distance. For(La1−xEux)2−yCeyCuO4, a light correlation betweenTc and the Debye temperature is observed, which means the importance of the lattice vibration in high-Tc superconductivity.

Published
1992
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12. High Power Co Laser And Its Power Delivery Through Optical Fibers

Author

M. Taniwaki, Y. Kikuchi, K. Igarashi, and S. Sato

Subjects
Optical amplifier, Optical fiber, Materials science, business.industry, Laser pumping, Optical modulation amplitude, Laser, law.invention, Optics, law, Fiber laser, Diode-pumped solid-state laser, Optoelectronics, Laser power scaling, business
Published
2005
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13. Laser ionization time‐of‐flight mass spectrometric study on laser ablation of a graphite‐like material of (BC2N)ncomposition

Author

Fumio Kokai, M. Taniwaki, Y. Koga, Yozo Kakudate, Shuzo Fujiwara, K. Fukuda, and M. Kawaguchi

Subjects
chemistry.chemical_classification, Laser ablation, Chemistry, medicine.medical_treatment, Analytical chemistry, General Physics and Astronomy, Mass spectrometry, Laser, Ablation, Atmospheric-pressure laser ionization, law.invention, law, Ionization, medicine, Compounds of carbon, Graphite, Atomic physics
Abstract

Laser ionization time‐of‐flight mass spectrometry has been used to probe Nd:YAG laser ablation products from a new graphite‐like material of (BC2N)n composition. Neutral species mainly composed of one, two, and three atoms were detected. A center‐of‐mass velocity of 1.2×105 cm/s was obtained for the expansion of the products. An influence of collision‐induced reactions is suggested for the product generation.

Published
1995
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14. [Small lymphocytic lymphoma/chronic lymphocytic leukemia with t(11;14)]

Author

K, Ueda, M, Nakao, Y, Akano, K, Nomura, Y, Fujita, T, Okamoto, S, Yokota, S, Horiike, S, Nakamura, and M, Taniwaki

Subjects
Aged, 80 and over, Chromosome Aberrations, Chromosomes, Human, Pair 14, B-Lymphocytes, Chromosomes, Human, Pair 11, Humans, Female, CD5 Antigens, Leukemia, Lymphocytic, Chronic, B-Cell, Aged
Abstract

A 83-year-old woman was referred to our hospital because of swollen lymph nodes, marked splenomegaly, and bone marrow abnormality. Histological examination of the lymph nodes revealed characteristic findings for small lymphocytic lymphoma/chronic lymphocytic leukemia (SLL/CLL). The immunophenotype of the tumor cells was CD5+, 10-, 19+, 20+, 23-, IgM+D+. Interphase fluorescent in situ hybridization (FISH) detected t(11;14), and immunohistochemical studies demonstrated cyclin D1 expression. In both SLL/CLL and mantle cell lymphoma (MCL), the normal counterpart of the tumor cells is thought to be CD5-positive B1 cells. The present case may therefore have been borderline between SLL/CLL and MCL.

Published
2001

17. Langerhans cell histiocytosis of an adult with tumors in liver and spleen

Author

K, Yagita, M, Iwai, M, Yagita-Toguri, H, Kimura, M, Taniwaki, S, Misawa, T, Okanoue, K, Kashima, and Y, Tsuchihashi

Subjects
Antigens, CD1, Male, Histiocytosis, Langerhans-Cell, Splenic Neoplasms, Liver Neoplasms, S100 Proteins, Humans, Histiocytes, Middle Aged, Tomography, X-Ray Computed, Immunohistochemistry
Abstract

We describe a 58-year-old male with multiple histiocytic tumors in the liver and spleen. Multiple tumors in the liver and spleen were seen by image analysis, and splenectomy showed a large splenic tumor with a small nodule and a swelling lymph node in the hilus. Histological features of the tumors in the liver and spleen revealed proliferation of histiocytic cells with large and clear cytoplasm and a horseshoe-shaped nucleus. Immunohistochemical studies revealed the presence of S-100 protein and CD1a antigen in the tumor cells, and neither lymphocytic marker nor lysozyme was detected. No definite Birbeck granules were seen ultrastructurally, thus the tumor cells could be classified into Langerhans cell type without Birbeck granules. Administration of adriamycin, vincristine, cyclophosphamide and prednisolone reduced size and number of the liver tumors, and the histiocytic cells could not be detected in repeatedly biopsied tissue from liver tumor. We present the clinical, immunohistological and cytological features in a visceral type of adult Langerhans cell histiocytosis, which responded well to chemotherapy.

Published
2001

18. The CDCREL1 gene fused to MLL in de novo acute myeloid leukemia with t(11;22)(q23;q11.2) and its frequent expression in myeloid leukemia cell lines

Author

K, Tatsumi, T, Taki, M, Taniwaki, H, Nakamura, J, Taguchi, Y Z, Chen, F, Bessho, M, Yanagisawa, and Y, Hayashi

Subjects
Adult, Male, Base Sequence, Oncogene Proteins, Fusion, Gene Expression Regulation, Leukemic, Chromosomes, Human, Pair 11, Chromosomes, Human, Pair 22, Molecular Sequence Data, Cell Cycle Proteins, Histone-Lysine N-Methyltransferase, Translocation, Genetic, DNA-Binding Proteins, Leukemia, Myeloid, Acute, Platelet Glycoprotein GPIb-IX Complex, Proto-Oncogenes, Tumor Cells, Cultured, Humans, Amino Acid Sequence, RNA, Messenger, Myeloid-Lymphoid Leukemia Protein, Septins, Transcription Factors
Abstract

We report on an adult patient with de novo acute myeloid leukemia (AML) with a t(11;22)(q23;q11.2) involving CDCREL1 and MLL genes. Reverse transcriptase (RT)-polymerase chain reaction (PCR) followed by direct sequencing analysis revealed the MLL-CDCREL1 fusion transcript in his leukemic cells. Analysis of the fusion transcript showed that exon 6 of MLL was fused to exon 4 of CDCREL1, which contains an AT-hook domain of MLL and a GTP binding domain of CDCREL1. To investigate the roles of CDCREL1 further, we examined the expression of the CDCREL1 gene in various cell lines. Expression of CDCREL1 was detected in 11 (85%) of 13 AML cell lines and 3 (21%) of 14 acute lymphoblastic leukemia (ALL) cell lines, but none of 11 EB virus transformed B-cell lines by RT-PCR. The expression rate of CDCREL1 was significantly higher in AML cell lines than in ALL cell lines (P = 0.0035). Platelet glycoprotein 1B beta (GP1B beta), which is located downstream of CDCREL1 and is cotranscribed with CDCREL1 due to a nonconsensus polyadenylation sequence, was expressed in all these cell lines. The higher expression rate of CDCREL1 in AML cell lines than in ALL cell lines suggests that this gene may play some role in myeloid leukemogenesis.

Published
2001

19. A novel human multiple myeloma-derived cell line, NCU-MM-1, carrying t(2;11)(q11;q23) and t(8;22)(q24;q11) chromosomal translocations with overexpression of c-Myc protein

Author

S, Iida, I, Hanamura, T, Suzuki, T, Kamiya, M, Kato, Y, Hayami, K, Miura, S, Harada, K, Tsuboi, A, Wakita, Y, Akano, M, Taniwaki, M, Nitta, and R, Ueda

Subjects
Chromosomes, Human, Pair 11, Cell Culture Techniques, Gene Expression, Proto-Oncogene Mas, Translocation, Genetic, Cell Line, Proto-Oncogene Proteins c-myc, Chromosomes, Human, Pair 2, Cytogenetic Analysis, Humans, Female, Immunoglobulin Light Chains, Multiple Myeloma, Aged, Chromosomes, Human, Pair 8
Abstract

A novel cell line, designated as NCU-MM-1, was established from a 66-year-old female patient with multiple myeloma (MM) that had shown rapid progression from solitary plasmacytoma to plasma cell leukemia. Interestingly, cytogenetic analysis including fluorescence in situ hybridization analysis disclosed that this cell line carried 2 kinds of chromosomal translocations involving immunoglobulin light chain (IgL) gene loci without the presence of 14q32 translocations (14q+). The Ig lambda locus juxtaposed to the c-MYC locus at 8q24 on the derivative (8) chromosome and a concomitant overexpression of the c-Myc protein was observed. On the derivative (11) chromosome, the Ig kappa locus was also fused to the chromosome 11q23 locus, which is known to be a nonrandom translocation breakpoint in mature B-cell malignancies. The NCU-MM-1 cell line may thus be useful not only for the identification of the responsible proto-oncogene(s) mapped to 11q23, deregulated by the Ig kappa enhancer sequences, but also for clarification of the molecular origin of MM lacking 14q+ chromosomes because IgL rearrangements can physiologically begin to occur in the pre-B-cell stage.

Published
2000

20. Randomized comparison of mobilization kinetics of circulating CD34+ cells between biweekly CHOP and dose-escalated CHOP with the prophylactic use of lenograstim (glycosylated rHuG-CSF) in aggressive non-Hodgkin's lymphoma. The lenograstim/Lymphoma Study Group

Author

K, Itoh, T, Ohtsu, Y, Sasaki, M, Ogura, Y, Morishima, M, Kasai, T, Chou, K, Yoshida, T, Ohno, F, Mizorogi, N, Uike, T, Sai, M, Taniwaki, S, Ikeda, and K, Tobinai

Subjects
Adult, Male, Lymphoma, Non-Hodgkin, Hematopoietic Stem Cell Transplantation, Middle Aged, Combined Modality Therapy, Transplantation, Autologous, Hematopoietic Stem Cell Mobilization, Lenograstim, Recombinant Proteins, Adjuvants, Immunologic, Doxorubicin, Vincristine, Antineoplastic Combined Chemotherapy Protocols, Granulocyte Colony-Stimulating Factor, Humans, Prednisone, Female, Cyclophosphamide, Aged
Abstract

High-dose chemotherapy with autologous hematopoietic stem cell transplantation has been expected to result in a promising outcome in high risk aggressive non-Hodgkin's lymphoma (NHL). However, it remains unknown what type of initial chemotherapy is optimal, especially regarding progenitor cell mobilization. Sixty-three untreated patients with aggressive NHL in a high risk group were randomized to either a biweekly arm with 8 cycles of standard CHOP or 6 cycles of the dose-escalated CHOP arm with cyclophosphamide 1.5 g/m2 and doxorubicin 70 mg/m2. Lenograstim (glycosylated rHuG-CSF 2.0 microg/kg/day) was administered daily from day 3 to patients in both arms. The mobilization effect of the two regimens on circulating CD34+ cells was evaluated. Twenty-seven of 29 patients in the biweekly CHOP arm and 33 of 34 patients in the dose-escalated CHOP were assessable. Dose-escalated CHOP yielded a significantly higher number of circulating CD34+ cells in the first cycle compared with biweekly CHOP (p=0.05). The peak number of circulating CD34+ cells with biweekly CHOP did not significantly change from cycle to cycle; however, in dose-escalated CHOP, the peak number of circulating CD34+ cells mobilized after the fifth and sixth cycle was lower than after the first cycle (p=0.07 and 0.009, respectively). Routine conventional-dose chemotherapy and low-dose G-CSF can mobilize sufficient CD34+ cells in patients with aggressive NHL. The mobilization kinetics of circulating progenitor cells in patients with aggressive NHL is dependent on the dosage and schedule of CHOP.

Published
2000

21. MLL-CBP fusion transcript in a therapy-related acute myeloid leukemia with the t(11;16)(q23;p13) which developed in an acute lymphoblastic leukemia patient with Fanconi anemia

Author

K, Sugita, T, Taki, Y, Hayashi, H, Shimaoka, H, Kumazaki, H, Inoue, Y, Konno, M, Taniwaki, H, Kurosawa, and M, Eguchi

Subjects
Male, Base Sequence, Chromosomes, Human, Pair 11, Molecular Sequence Data, Nuclear Proteins, Neoplasms, Second Primary, Histone-Lysine N-Methyltransferase, Precursor Cell Lymphoblastic Leukemia-Lymphoma, CREB-Binding Protein, Translocation, Genetic, DNA-Binding Proteins, Fanconi Anemia, Phenotype, Karyotyping, Leukemia, Monocytic, Acute, Proto-Oncogenes, Trans-Activators, Humans, Amino Acid Sequence, Child, Chromosomes, Human, Pair 16, Myeloid-Lymphoid Leukemia Protein, Transcription Factors
Abstract

We describe a boy with Fanconi anemia (FA) who developed acute lymphoblastic leukemia (ALL) (FAB-LI) followed by acute myeloid leukemia (AML) (FAB-M5) at relapse. The patient was diagnosed with early pre-B-cell ALL without preceding aplastic anemia and was treated with ALL-oriented chemotherapy which included doxorubicin (a total dose of 140 mg/m(2) administered), which is a topoisomerase II inhibitor. Complete remission was obtained, but after 38 weeks AML developed. The karyotype of ALL cells at diagnosis showed 46,XY, and that of AML cells at relapse was 46,XY, t(11;16)(q23;p13). An MLL gene rearrangement and MLL-CBP chimeric mRNA were found in AML, but not in ALL. A diagnosis of FA was confirmed by an increased number of chromosomal breaks and rearrangements in peripheral blood lymphocytes cultured with mitogen in the presence of mitomycin C. We conclude that this FA patient developed ALL followed by a therapy-related t(11;16)-AML resulting in an MLL-CBP fusion. Further examination of such patients would shed light on leukemogenesis in FA patients. Genes Chromosomes Cancer 27:264-269, 2000.

Published
2000

22. Bowel perforation during chemotherapy for non-hodgkin's lymphoma

Author

C, Sakakura, A, Hagiwara, M, Nakanishi, R, Yasuoka, M, Shirasu, T, Togawa, M, Taniwaki, and H, Yamagishi

Subjects
Male, Intestinal Perforation, Antineoplastic Combined Chemotherapy Protocols, Intestinal Neoplasms, Humans, Jejunal Diseases, Lymphoma, Large B-Cell, Diffuse, Radionuclide Imaging, Digestive System Surgical Procedures, Aged
Abstract

Bowel perforation in patients with primary malignant lymphoma usually occurs at the site of tumor. A 78 year-old man underwent chemotherapy for malignant lymphoma. He presented with abdominal pain. An emergency operation was performed under a diagnosis of panperitonitis. At laparotomy, an anal-side perforation approximately 20 cm from the Treiz ligament was observed. Drainage and partial resection of the jejunum was performed. Histopathologic examination demonstrated that there was no characteristic finding of malignant lymphoma around the perforation site in the case. Perforation of the small intestine is one of the most critical complications during the chemotherapy for malignant lymphoma. In cases of chemotherapy for malignant lymphoma, especially systemic administration, we should keep in mind the possibility of perforation of the small intestine. Fortunately, emergency surgery saved the patient presented in this report. Early diagnosis and treatment are important to improve prognosis of bowel perforation in patients with primary malignant lymphoma.

Published
2000

23. Expression of fibroblast growth factor and FGF-receptor family genes in human myeloma cells, including lines possessing t(4;14)(q16.3;q32. 3) and FGFR3 translocation

Author

Haruko Sakaguchi, Osamu Yamada, Ayako Ueki, Junichi Kurebayashi, M Taniwaki, Yoshihito Yawata, Takemi Otsuki, Kenichiro Yata, and N Nakazawa

Subjects
Male, Cancer Research, DNA, Complementary, Fibroblast Growth Factor 4, HL-60 Cells, Biology, Translocation, Genetic, Growth factor receptor, immune system diseases, Proto-Oncogene Proteins, hemic and lymphatic diseases, Tumor Cells, Cultured, medicine, Humans, Protein Isoforms, Receptor, Fibroblast Growth Factor, Type 3, RNA, Neoplasm, Autocrine signalling, Multiple myeloma, Aged, Cell Line, Transformed, Chromosomes, Human, Pair 14, Reverse Transcriptase Polymerase Chain Reaction, Fibroblast growth factor receptor 2, Fibroblast growth factor receptor 1, Antibodies, Monoclonal, Fibroblast growth factor receptor 4, Middle Aged, Protein-Tyrosine Kinases, Fibroblast growth factor receptor 3, medicine.disease, Receptors, Fibroblast Growth Factor, Fibroblast Growth Factors, Gene Expression Regulation, Neoplastic, stomatognathic diseases, Oncology, Fibroblast growth factor receptor, Immunology, Cancer research, Fibroblast Growth Factor 1, Female, Fibroblast Growth Factor 2, Chromosomes, Human, Pair 4, Multiple Myeloma, Cell Division
Abstract

Recently several chromosomal translocations involved in myeloma cases and myeloma cell lines; i.e., t(11;14)(q13;q32), t('8;14)(q24;q32), t(4;14)(q16.3;q32.3), t(6;14)(p25;q32), and t(14;16)(q32.3;q23), have been identified. These translocations are considered to dysregulate genes which may be concerned with myelomagenesis; i.e., PRAD1/cyclin D1, the c-myc oncogene, FGFR3 (fibroblast growth factor receptor 3), MMSET (multiple myeloma SET domain), MUM1 (multiple myeloma oncogene 1)/IRF4 (interferon regulatory factor 4), and the c-maf oncogene, respectively. However, the cellular biological roles of these genes have not yet been elucidated in myeloma cells. Because two of the seven human myeloma cell lines which were established at Kawasaki Medical School, Okayama, Japan, KMS-11 and KMS-18, have been proven to possess t(4;14)(q16.3;q32.3), we studied the expression levels of the FGFR3 gene in these seven cell lines and 13 primary myeloma specimens. The expression levels of 12 known FGF family genes (FGF-1 to 12) and 4 FGFR genes (FGFR1 to 4) were also examined in seven cell lines. In addition, the growth status of the KMS-11 and KMS-18 lines with FGF-1 or anti-FGF-4 neutralizing monoclonal antibody (MoAb) supplementation was investigated because FGF-1 and 4 are known as the principal ligands for FGFR3. FGFR3 overexpression was observed in both of the cell lines possessing t(4;14)(q16.3;q32.3) and in 3 of 13 case specimens. Anti-FGF-4 neutralizing MoAb caused significant growth inhibition in these two cell lines possessing t(4;14)(q16.3;q32.3). These findings indicate that t(4;14) (q16. 3;q32.3) may provide myeloma cells with a growth advantage via an autocrine mechanism between FGFR3 and FGF-4.

Published
1999
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24. Consistent detection of CALM-AF10 chimaeric transcripts in haematological malignancies with t(10;11)(p13;q14) and identification of novel transcripts

Author

M, Narita, K, Shimizu, Y, Hayashi, T, Taki, M, Taniwaki, F, Hosoda, H, Kobayashi, H, Nakamura, N, Sadamori, H, Ohnishi, F, Bessho, M, Yanagisawa, and M, Ohki

Subjects
Adult, Male, Oncogene Proteins, Fusion, Chromosomes, Human, Pair 10, Reverse Transcriptase Polymerase Chain Reaction, Chromosomes, Human, Pair 11, Molecular Sequence Data, Chromosome Breakage, Translocation, Genetic, Immunophenotyping, Leukemia, Lymphoid, Leukemia, Myeloid, Tumor Cells, Cultured, Humans, Female, Amino Acid Sequence, Child, In Situ Hybridization, Fluorescence, Transcription Factors
Abstract

The t(10;11)(p13-14;q14-21) is a rare but recurring translocation associated with acute lymphoblastic leukaemia (ALL) and acute myeloid leukaemia (AML). Recently the CALM gene was cloned from the t(10;11) breakpoint of U937 and fused to AF10, a putative transcription factor, which had been identified as one of the fusion partners of the MLL gene. In order to define the involvement of these genes in primary leukaemias and cell lines with t(10;11), we analysed the expression of fusion transcripts by reverse transcriptase-polymerase chain reaction (RT-PCR) in five patient samples including ALL, AML and lymphoblastic lymphoma, and three monocytic cell lines (P31/Fujioka, KP-Mo-TS and U937). The CALM-AF10 fusion transcript was detected in all samples; however, the AF10-CALM fusion was not detected in two patient samples and one cell line. In RT-PCR analysis there were six isoforms of the CALM-AF10 fusion transcripts and five of AF10-CALM fusion transcripts. We also detected novel transcripts in U937. Sequence analysis revealed that all these isoforms had in-frame junctions and that some of them resulted from alternative splicing at different exons of CALM and others from different breakpoints at CALM and/or AF10. There were at least two different breakpoints of CALM and three of AF10 gene. Our results suggest that the CALM-AF10 fusion gene is a constant feature and is involved in the pathogenesis of haematological malignancies with t(10;11)(p13-14;q14-21), showing various and often multilineage phenotypes. Thus, t(10;11) needs to be investigated by RT-PCR for identification of the genes involved.

Published
1999

25. A new translocation, t(2;4;12)(p21;q12;p13), in CD7-positive acute myeloid leukemia: a variant form of t(4;12)

Author

H, Hamaguchi, K, Nagata, K, Yamamoto, M, Kobayashi, T, Takashima, and M, Taniwaki

Subjects
Adult, Male, Chromosomes, Human, Pair 12, Proto-Oncogene Proteins c-ets, Genetic Variation, Antigens, CD7, Translocation, Genetic, DNA-Binding Proteins, Repressor Proteins, Leukemia, Myeloid, Chromosomes, Human, Pair 2, Karyotyping, Acute Disease, Humans, Chromosomes, Human, Pair 4, In Situ Hybridization, Fluorescence, Transcription Factors
Abstract

We describe a 41-year-old man with CD7-positive acute myeloid leukemia (AML-M0) with trilineage-myelodysplasia. Chromosome analysis of the bone marrow cells showed 46.XY.t(2;4;12) (p21;q12;p13). Cytological and clinical features of our case were quite similar to those of AML with t(4;12)(q11-12;p13). The karyotypic interpretation was confirmed by fluorescence in situ hybridization (FISH) by using the whole-chromosome painting probes specific for chromosomes 2, 4, and 12. FISH analysis with the use of the YAC 936e2 probe, which covers the TEL gene, did not show the split signal, suggesting that a gene other than TEL was involved in the leukemogenesis of the present case. Our case with AML with t(2;4;12)(p21;q12;p13) appears to be the first case of a variant type of AML with t(4;12) (q11-12;p13).

Published
1999

26. [B cell acute lymphocytic leukemia with marked leukocytosis and t(3;15)(q27;q2?2)]

Author

K, Yata, H, Wada, T, Sugihara, O, Yamada, T, Otsuki, N, Nakazawa, M, Taniwaki, T, Akasaka, H, Ohno, and Y, Yawata

Subjects
DNA-Binding Proteins, Male, Chromosomes, Human, Pair 15, Adolescent, Leukocytosis, Proto-Oncogene Proteins, Leukemia, B-Cell, Proto-Oncogene Proteins c-bcl-6, Humans, Chromosomes, Human, Pair 3, Translocation, Genetic, Transcription Factors
Abstract

We report on a 16-year-old boy with B cell acute lymphocytic leukemia presenting marked leukocytosis (388,000/microliter) and resistance to multidrug chemotherapy. Karyotypical analysis revealed a novel t(3;15)(q27;q2?2) chromosomal abnormality. Because 3q27 is known to be a locus of the bcl-6 gene, which is frequently involved in B cell malignancies, molecular biological analyses were performed. Although no rearrangement was detected in 5 genes including bcl-6 on 3q27 and 2 genes on 15q2, reverse transcriptase-polymerase chain reaction procedures detected relatively strong mRNA expression of the bcl-6, smrp, dvl3, and tpml genes. These results indicate that immature leukemic cells with CD10 and CD34 positivity and rearrangement of the T cell receptor beta gene may coexist with relatively mature subpopulations that are positive for CD19 and CD20 surface markers, bcl-6 expression, and rearrangement of the gene for immunoglobulin kappa.

Published
1999

27. [Syngeneic peripheral blood stem cell transplantation for chronic myelogenous leukemia associated with Klinefelter's syndrome]

Author

H, Fujii, Y, Ueda, H, Nakagawa, Y, Sasai, S, Horiike, and M, Taniwaki

Subjects
Male, Transplantation, Isogeneic, Klinefelter Syndrome, Leukemia, Myelogenous, Chronic, BCR-ABL Positive, Remission Induction, Diseases in Twins, Hematopoietic Stem Cell Transplantation, Humans, Twins, Monozygotic, Middle Aged, Tissue Donors
Abstract

We report on a patient with Klinefelter's syndrome who underwent successful syngeneic peripheral blood stem cell transplantation (PBSCT) for chronic myelogenous leukemia (CML). A-46-year-old man was given a diagnosis of chronic phase CML in May 1994 on the basis of findings of leukocytosis (54,000/microliter) and bone marrow chromosomal abnormalities [47, XXY, t(9; 22; 14) (q34; q11; q24)]. Hydroxyurea and interferon alpha were administered. In August 1996, a syngeneic transplant was performed following myeloablative therapy, using peripheral blood stem cells collected from the patient's identical twin brother, who had been pretreated with rhG-CSF. Following transplantation (4.0 x 10(6) CD34+ cells/kg) and the subsequent administration of rhG-CSF, the patient rapidly achieved normal tri-lineage hematopoiesis. A post-transplant chromosomal analysis of the patient's bone marrow cells detected the 47, XXY karyotype. Although the major BCR-ABL gene had been detected in bone marrow by RT-PCR methods prior to the syngeneic PBSCT (August 1996), it was not detected after PBSCT (January 1997). In March 1998, interphase fluorescence in situ hibridization (FISH) procedures disclosed XXY signal patterns in peripheral blood lymphocyte samples from the patient and donor, at frequencies of 96% and 97%, respectively. Both the patient and donor had high levels of serum FSH and LH and low levels of serum testosterone.

Published
1999

28. Internal tandem duplication of the FLT3 gene and clinical evaluation in childhood acute myeloid leukemia. The Children's Cancer and Leukemia Study Group, Japan

Author

T, Iwai, S, Yokota, M, Nakao, T, Okamoto, M, Taniwaki, N, Onodera, A, Watanabe, A, Kikuta, A, Tanaka, K, Asami, I, Sekine, H, Mugishima, Y, Nishimura, S, Koizumi, Y, Horikoshi, J, Mimaya, S, Ohta, K, Nishikawa, A, Iwai, T, Shimokawa, M, Nakayama, K, Kawakami, T, Gushiken, N, Hyakuna, and T, Fujimoto

Subjects
Adult, Male, Repetitive Sequences, Amino Acid, Molecular Sequence Data, Receptor Protein-Tyrosine Kinases, Receptors, Cell Surface, Exons, Prognosis, Polymerase Chain Reaction, Survival Analysis, Introns, fms-Like Tyrosine Kinase 3, Bone Marrow, Leukemia, Myeloid, Gene Duplication, Proto-Oncogene Proteins, Acute Disease, Proto-Oncogenes, Humans, Female, Amino Acid Sequence, Phosphorylation, Child
Abstract

We analyzed tandem duplication in the juxtamembrane (JM) domain of the FLT3 (FMS-like tyrosine kinase 3/FLK2, CD135) gene in 94 children with acute myeloid leukemia (AML) and evaluated its correlation with clinical features. Longer polymerase chain reaction (PCR) products were observed in five patients; 1/3 of M0, 119 of M1, 1/39 of M2, 1/9 of M3 and 1/12 of M5. The sequence analyses of abnormal PCR products showed that all the abnormal products were derived from tandem duplications involving the JM domain and that all the lengthened sequences were in-frame as we previously reported. Statistical analyses revealed a significantly lower incidence of the tandem duplication in childhood AML patients than in adult patients (P0.05), and significantly shorter disease-free survival in patients with mutant FLT3 than in patients with wild-type FLT3 (P0.05). Our results suggest that the tandem duplication in the JM domain of the FLT3 gene is not a frequent phenomenon but might be a factor of poor prognosis in childhood patients with AML.

Published
1999

30. [Clinical evaluation of panipenem/betamipron as a second line chemotherapy in severe infections associated with hematological disorders]

Author

N, Nakazawa, T, Okamoto, M, Kobayashi, T, Iwai, Y, Sasai, A, Tamura, S, Horiike, S, Yokota, M, Taniwaki, K, Kashima, S, Misawa, S, Tuda, and Y, Ohkawara

Subjects
Adult, Aged, 80 and over, Male, Leukemia, Lymphoma, Pyelonephritis, Anemia, Aplastic, Drug Resistance, Microbial, Bacterial Infections, Pneumonia, Middle Aged, Treatment Outcome, Sepsis, beta-Alanine, Humans, Drug Therapy, Combination, Female, Thienamycins, Multiple Myeloma, Aged
Abstract

Thirty three patients with severe infections associated with hematological disorders were treated with panipenem/betamipron as a second line chemotherapy. Of these, 30 patients were evaluated for effectiveness. An excellent response was obtained in 14 patients (46.7%) and a good response in 5 (16.7%), and the overall efficacy rate was 63.3%. Efficacy rates were 3/6 in patients with sepsis, 68.4% (13/19) in patients with fever of undetermined origin, 2/4 in patients with pneumonia. In patients whose peripheral granulocyte count was below 100/microliter at the start of chemotherapy, the efficacy rate was 3/7. Side effects were observed in 5 of 33 patients (15.2%). These results show that PAPM/BP is useful as a second line chemotherapy for the treatment of severe infections in patients with hematological disorders.

Published
1998

31. [Clinical evaluation of cefozopran for infections associated with hematological malignancies]

Author

Y, Sasai, T, Iwai, A, Tamura, N, Nakazawa, Y, Ueda, H, Kaneko, S, Horiike, S, Yokota, M, Taniwaki, K, Kashima, S, Misawa, S, Tsuda, and Y, Ohgawara

Subjects
Adult, Aged, 80 and over, Male, Leukemia, Leukemia, T-Cell, Lymphoma, Anemia, Aplastic, Bacterial Infections, Pneumonia, Middle Aged, Peritonitis, Precursor Cell Lymphoblastic Leukemia-Lymphoma, Hodgkin Disease, Severity of Illness Index, Cephalosporins, Leukemia, Myeloid, Acute, Leukocyte Count, Sepsis, Acute Disease, Humans, Female, Bronchitis, Multiple Myeloma, Aged, Granulocytes
Abstract

Cefozopran (CZOP) was used as an initial antibacterial therapy for infections in patients with hematological malignancies. CZOP was given at a daily dose of 4 g by drip intravenously to patients who were febrile over 38 degrees C and were suspected as having bacterial infections. As underlying diseases, 8 patients had acute lymphoblastic leukemia (ALL), 9 acute myeloblastic leukemia (AML), 2 aplastic anemia (AA), 2 adult T cell leukemia/lymphoma (ATLL), 28 non Hodgkin lymphoma (NHL), and 2 multiple myeloma (MM). Bacterial infections diagnosed were sepsis in 7 patients, suspected sepsis in 32, bronchitis in 6, pneumonia in 5 and acute peritonitis in 1. Clinical responses among 51 evaluable cases were excellent in 14, good in 15, fair in 3, poor in 19 and the overall response rate was 57%. The overall response rates for AML, ALL, AA, ATLL, NHL and MM were 56%, 63%, 100%, 50%, 50%, and 100%, respectively. Those for sepsis, suspected sepsis, bronchitis, pneumonia and acute peritonitis were 14%, 63%, 100%, 40%, and 0%, respectively. This therapy was effective in 53% (9/17) of patients whose granulocyte count remained below 500/microliter throughout the course of CZOP therapy. Six bacterial and one fungal strains were isolated from blood and sputum of six patients including five sepsis cases; two bacteria were eradicated and bacterial change was observed in one case. As side adverse effects, 10 patients had liver dysfunction, 1 anemia, 2 proteinemia, 1 indirect bilirubinemia, 2 thrombocytopenia, and 1 eosinophilia. We tried to establish a scoring system for the severities of patients with their infections, underlying diseases, treatments for the underlying disease, and granulocyte counts in order to evaluate the efficacy of CZOP more precisely. This scoring system was consisted of three grades; severe, moderate, and mild. CZOP was effective on mild and moderate grades. These results indicate that the initial antibacterial therapy by CZOP is useful for the treatment of mild and moderate grade infections complicated with hematological malignancies.

Published
1998

32. Frequent aberration of FHIT gene expression in acute leukemias

Author

T, Iwai, S, Yokota, M, Nakao, N, Nakazawa, M, Taniwaki, T, Kimura, Y, Sonoda, H, Kaneko, T, Okuda, H, Azuma, T, Oka, T, Takeda, A, Watanabe, A, Kikuta, K, Asami, I, Sekine, T, Matsushita, T, Tsuchiya, J, Mimaya, S, Koizumi, S, Ohta, M, Miyake, Y, Takaue, A, Iwai, and T, Fujimoto

Subjects
Adult, Leukemia, Gene Expression, Proteins, Precursor Cell Lymphoblastic Leukemia-Lymphoma, Leukemia, Myelomonocytic, Acute, Acid Anhydride Hydrolases, Neoplasm Proteins, Leukemia, Myeloid, Acute, Leukemia, Promyelocytic, Acute, Bone Marrow, Acute Disease, Leukemia, Monocytic, Acute, Humans, Leukemia, Erythroblastic, Acute, RNA, Messenger, Child, Gene Deletion
Abstract

We analyzed the mRNA expression of the FHIT gene by reverse transcription-PCR (RT-PCR) in 54 cases of acute lymphoblastic leukemia (ALL; 11 cases of T-cell ALL [T-ALL] and 43 cases of non-T-ALL) and 40 cases of acute myeloid leukemia (AML). In 46% of the ALL cases and 55% of the AML cases, FHIT expression was absent or markedly decreased. Only abnormal short bands were detected in 30% of the ALL cases and 5% of the AML cases. Eighteen of 19 abnormal transcripts had the same fusion of exons 2-7, and all lacked the starting codon in exon 5. No obvious normal-sized PCR products were detected in cases exhibiting abnormal transcripts. These findings suggest that the expression of functional FHIT protein was lost in the majority of ALL (76%) and AML (60%) cases. Differential quantitative PCR of exons 3-9 of the FHIT gene and RT-PCR of the PTPRG gene, which is centromeric to the FHIT gene, showed the presence of the target sequences. Fluorescence in situ hybridization analysis using probes covering exons 5 and 8 revealed no difference in the signal patterns between leukemia and normal cells, showing one or two signal doublets in more than 90% of nuclei, and indicated that gross segments of the FHIT gene were not homozygously deleted in these cases. A small number of transcripts with an aberrant fusion between exons 2 and 7 were detected by RT-PCR in the bone marrow cells from four healthy individuals. Granulocytes, lymphocytes, and monocytes in the bone marrow cells of a healthy individual contained transcripts with the same fusion. This unique fusion of exons 2 and 7 might be preferentially seen in either neoplastic or normal hematopoietic cells, regardless of their lineage. The finding that FHIT expression was abolished in the majority of leukemia cases might support the hypothesis that the FHIT gene acts as a tumor suppressor, at least in leukemia.

Published
1998

33. ABI-1, a human homolog to mouse Abl-interactor 1, fuses the MLL gene in acute myeloid leukemia with t(10;11)(p11.2;q23)

Author

T, Taki, N, Shibuya, M, Taniwaki, R, Hanada, K, Morishita, F, Bessho, M, Yanagisawa, and Y, Hayashi

Subjects
Male, DNA, Complementary, Oncogene Proteins, Fusion, RNA Splicing, Molecular Sequence Data, Leukemia, Myelomonocytic, Acute, Translocation, Genetic, Mice, Species Specificity, Proto-Oncogenes, Animals, Humans, Amino Acid Sequence, RNA, Messenger, RNA, Neoplasm, Adaptor Proteins, Signal Transducing, Homeodomain Proteins, Base Sequence, Sequence Homology, Amino Acid, Chromosomes, Human, Pair 10, Gene Expression Regulation, Leukemic, Chromosomes, Human, Pair 11, Infant, DNA, Neoplasm, Histone-Lysine N-Methyltransferase, Neoplasm Proteins, DNA-Binding Proteins, Cytoskeletal Proteins, Sequence Alignment, Myeloid-Lymphoid Leukemia Protein, Transcription Factors
Abstract

Recurrent translocation t(10;11) has been reported to be associated with acute myeloid leukemia (AML). Recently, two types of chimeric transcripts, MLL-AF10 in t(10;11)(p12;q23) and CALM-AF10 in t(10;11)(p13;q14), were isolated. t(10;11) is strongly associated with complex translocations, including invins(10;11) and inv(11)t(10;11), because the direction of transcription of AF10 is telomere to centromere. We analyzed a patient of AML with t(10;11)(p11.2;q23) and identified ABI-1 on chromosome 10p11.2, a human homolog to mouse Abl-interactor 1 (Abi-1), fused with MLL. Whereas the ABI-1 gene bears no homology with the partner genes of MLL previously described, the ABI-1 protein exhibits sequence similarity to protein of homeotic genes, contains several polyproline stretches, and includes a src homology 3 (SH3) domain at the C-terminus that is required for binding to Abl proteins in mouse Abi-1 protein. Recently, e3B1, an eps8 SH3 binding protein 1, was also isolated as a human homolog to mouse Abi-1. Three types of transcripts of ABI-1 gene were expressed in normal peripheral blood. Although e3B1 was considered to be a full-length ABI-1, the MLL-ABI-1 fusion transcript in this patient was formed by an alternatively spliced ABI-1. Others have shown that mouse Abi-1 suppresses v-ABL transforming activity and that e3B1, full-length ABI-1, regulates cell growth. In-frame MLL-ABI-1 fusion transcripts combine the MLL AT-hook motifs and DNA methyltransferase homology region with the homeodomain homologous region, polyproline stretches, and SH3 domain of alternatively spliced transcript of ABI-1. Our results suggest that the ABI-1 gene plays a role in leukemogenesis by translocating to MLL.

Published
1998

34. A variant Burkitt-type translocation (8;22)(q24;q11) in multiple myeloma. Report of a new case and review of the literature

Author

K, Yamamoto, H, Hamaguchi, K, Nagata, and M, Taniwaki

Subjects
Adult, Male, Oncogene Proteins, Chromosomes, Human, Pair 22, Genes, myc, Middle Aged, Protein-Tyrosine Kinases, Burkitt Lymphoma, Translocation, Genetic, Karyotyping, Proto-Oncogene Proteins, Proto-Oncogene Proteins c-bcr, Humans, Female, Multiple Myeloma, Chromosomes, Artificial, Yeast, In Situ Hybridization, Fluorescence, Aged, Chromosomes, Human, Pair 8
Abstract

We report here a new case of multiple myeloma (IgG, kappa, stage IIIA) with a variant Burkitt-type translocation (8;22)(q24;q11). Bone marrow plasma cells were morphologically immature with fine nuclear chromatin and nucleoli. Chromosome analysis showed complex aberrations; that is, 53,XX, der(1)add(1)(p11)dup(1)(q12q32),+3,+5,t(8;22)(q24;q11),+9,add(10)( p13), +11,+15,add(19)(q13),+21. Fluorescence in situ hybridization analysis with the yeast artificial chromosome (YAC) clone I2 containing the C-MYC gene at 8q24 and the chromosome-22-specific DNA library pBS22 revealed that 12 was located on the der(8)t(8;22). A fusion signal derived from I2 and the YAC clone B99E1 containing the BCR gene at 22q11 was also observed on the der(8)t(8;22). Our results indicate that the breakpoint at 8q24 in this patient was located far downstream of the C-MYC gene. This breakpoint site is similar to Burkitt lymphoma with t(8;22)(q24;q11). A review of eight cases in the literature and the present case of multiple myeloma with t(8;22)(q24;q11) showed that most of them were of advanced stage and had an immature phenotype. It is suggested that the C-MYC gene may be activated by t(8;22)(q24;q11) and implicated in disease progression in multiple myeloma.

Published
1998

35. Trisomy 12 and t(14;18) in B-cell chronic lymphocytic leukemia

Author

K, Kojima, M, Taniwaki, T, Yoshino, Y, Katayama, K, Sunami, S, Fukuda, E, Omoto, M, Harada, and T, Sezaki

Subjects
Chromosomes, Human, Pair 14, Male, Blotting, Southern, Chromosomes, Human, Pair 12, Humans, Trisomy, Middle Aged, Chromosomes, Human, Pair 18, Leukemia, Lymphocytic, Chronic, B-Cell, In Situ Hybridization, Fluorescence, Translocation, Genetic
Abstract

We report a case of B-cell chronic lymphocytic leukemia (B-CLL) in which trisomy 12 and t(14;18)(q32;q21) were simultaneously detected in the same leukemic clone. Southern blot analysis showed that the BCL2/IgJH rearrangement occurred at the major breakpoint region in the hot spot of the BCL2 gene. Double color fluorescence in situ hybridization analysis using multiple probes indicated that clonal B-cell with t(14;18) represented a subpopulation of the total leukemic cells and that trisomy 12 followed t(14;18) as the cytogenetic aberration in the development of B-CLL. Our findings suggests that both the t(14;18) and the trisomy are secondary chromosomal changes in the leukemogenesis of B-CLL.

Published
1998

36. [Clinical study on the inhibitory effect of a 5-HT3 antagonist, granisetron, for nausea and vomiting induced by chemotherapy (CHOP, VEPA, high-dose ETP) for non-Hodgkin's lymphoma]

Author

Y, Sasai, S, Misawa, T, Iwai, A, Tamura, N, Nakazawa, Y, Ueda, H, Kaneko, S, Horiike, S, Yokota, M, Taniwaki, K, Kashima, S, Tsuda, Y, Ookawara, M, Nakao, H, Nakagawa, and H, Fujii

Subjects
Adult, Aged, 80 and over, Male, Vomiting, Lymphoma, Non-Hodgkin, Nausea, Middle Aged, Granisetron, Bleomycin, Doxorubicin, Vincristine, Antineoplastic Combined Chemotherapy Protocols, Antiemetics, Humans, Prednisone, Female, Serotonin Antagonists, Cyclophosphamide, Aged, Etoposide
Abstract

The antiemetic effect of granisetron on nausea and vomiting induced by cancer chemotherapy (CHOP, VEPA, VEPA-B, massive dose of ETP) was studied in fifty patients with non-Hodgkin's lymphoma. There was almost no difference in the inhibitory effect by regimen, with the rates of perfect inhibition of nausea and vomiting standing at 55.6% to 60%. Nausea and vomiting was perfectly controlled in 60% of 35 patients receiving CHOP therapy. As a part of this study, a comparison was made of perfect inhibitory effect on nausea and vomiting by potency of chemotherapy under the potency scale of 750 mg/m2 of CPA as 1, revealing no significant difference in the rates of complete inhibition as 71.4% for a drug potency of less than 0.8 vs 52.4% for 0.8 or above (p = 0.26). However, it was clear that the higher the dose of chemotherapy, the lower the rate of complete inhibition. The results confirmed the high efficacy and safety of granisetron in the treatment of nausea and vomiting induced by cancer chemotherapy.

Published
1998

38. Establishment of a new human myeloma cell line, KMS-18, having t(4;14)(p16.3;q32.3) derived from a case phenotypically transformed from Ig A-lambda to BJP-lambda, and associated with hyperammonemia

Author

Hideho Wada, N Nakazawa, Ayako Ueki, M Taniwaki, Haruko Sakaguchi, Takemi Otsuki, Osamu Yamada, and Yoshihito Yawata

Subjects
Male, Cancer Research, Herpesvirus 4, Human, Carcinoma, Hepatocellular, Cell, Cell Culture Techniques, Chromosomal translocation, Polymerase Chain Reaction, Translocation, Genetic, Mycoplasma, immune system diseases, Ammonia, Antigens, CD, hemic and lymphatic diseases, medicine, Tumor Cells, Cultured, Humans, Multiple myeloma, In Situ Hybridization, Fluorescence, Chromosomes, Human, Pair 14, biology, Cell growth, Liver Neoplasms, Chromosome Mapping, Hyperammonemia, Cell cycle, Middle Aged, medicine.disease, Molecular biology, medicine.anatomical_structure, Phenotype, Oncology, Cell culture, Hematologic Neoplasms, Karyotyping, Immunology, biology.protein, Antibody, Chromosomes, Human, Pair 4, Multiple Myeloma
Abstract

A new human myeloma cell line, KMS-18, was established from a 58-year-old male with multiple myeloma associated with hyperammonemia. The original leukemic cells and established KMS-18 cells possessed several of the same chromosomal abnormalities, including add(1)(q32), add(10) (q24) and add(17)(p11). In addition, the KMS-18 cells showed novel t(4;14)(p16.3;q32.3) masked translocation which was determined by the FISH method. Moreover, we compared the ammonia production in culture medium of the KMS-18 cell line with that of non-myeloma hematological malignant cell lines and a hepatocellular carcinoma cell line. KMS-18 produced higher levels of ammonia in medium than the other cell lines examined. This new cell line may prove helpful in analyzing the role and biological mechanisms of the t(4;14)(p16.3;q32.3) translocation in myeloma and also in investigating hyperammonemia in cases with myeloma.

Published
1998

39. Establishment of a novel human B-cell line (OZ) with t(14;18)(q32;q21) and aberrant p53 expression was associated with the homozygous deletions of p15INK4B and p16INK4A genes

Author

M, Nagai, M, Fujita, M, Ohmori, S, Matsubara, M, Taniwaki, S, Horiike, T, Tasaka, H P, Koeffler, and J, Takahara

Subjects
Adult, Male, Cell Cycle Proteins, Translocation, Genetic, Fatal Outcome, Bone Marrow, Biomarkers, Tumor, Tumor Cells, Cultured, Humans, Neoplasm Invasiveness, Cyclin-Dependent Kinase Inhibitor p16, Cyclin-Dependent Kinase Inhibitor p15, Chromosome Aberrations, Chromosomes, Human, Pair 14, B-Lymphocytes, Genes, p16, Tumor Suppressor Proteins, Homozygote, DNA, Neoplasm, Aneuploidy, Antigens, CD20, Genes, p53, Genes, bcl-2, Neoplasm Proteins, Gene Expression Regulation, Neoplastic, Karyotyping, Lymph Nodes, Lymphoma, Large B-Cell, Diffuse, Tumor Suppressor Protein p53, Carrier Proteins, Chromosomes, Human, Pair 18, Gene Deletion
Abstract

The novel human pre-B cell line OZ was established from a patient with an aggressive form of non-Hodgkin's lymphoma. Karyotypic analysis of both the primary tumour and OZ cells revealed several marker chromosomes, including the t(14;18)(q32;q21) translocation, which involves the Bcl-2 gene, and alterations on chromosome 17p. Southern blot analysis found identical rearrangements in the 5' region of Bcl-2 gene in the primary tumour and OZ cells. Homozygous deletions of the p15INK4B and p16INK4A genes, however, were present only in OZ cells. Western blot analysis detected aberrant small molecular-weight p53 proteins in both cell types. In addition, OZ cells no longer expressed the CD20 antigen. These findings suggest that Bcl-2 gene rearrangement and aberrant p53 expression resulted in the original B-cell tumour. A subsequent transforming event involving the p15INK4B and p16INK4A genes may have generated more immature cells with a growth advantage during in vitro culture. The genetic alterations involving p53, p15INK4B, and p16INK4A may be implicated in the aggressive form of t(14;18)(q32;q21)-bearing tumours and their poor prognosis.

Published
1997

40. Detection of 14q32.33 translocation and t(11;14) in interphase nuclei of chronic B-cell leukemia/lymphomas by in situ hybridization

Author

T, Takashima, M, Itoh, Y, Ueda, K, Nishida, T, Tamaki, S, Misawa, T, Abe, M, Seto, T, Machii, and M, Taniwaki

Subjects
Adult, Aged, 80 and over, Cell Nucleus, Chromosomes, Human, Pair 14, Male, Adolescent, Lymphoma, Chromosomes, Human, Pair 11, Middle Aged, Translocation, Genetic, Chronic Disease, Leukemia, B-Cell, Humans, Female, Interphase, In Situ Hybridization, Fluorescence, Aged
Abstract

Abnormalities of chromosome 14 involving band q32.33 are among the most commonly observed cytogenetic alterations in B-cell malignancies. To assess the incidence and pathogenetic implications of 14q32.33 translocation in chronic B-cell leukemia/lymphomas, we performed fluorescence in situ hybridization (FISH) analysis with variable region (V(H)) and gamma constant region (Cgamma) gene probes in 37 patients with these disorders. Chromosome 14q32.33 translocation was detected in 2 of 18 patients with chronic lymphocytic leukemia (CLL), 1 of 2 with CLL of mixed cell types (CLL/PL), 1 of 2 with pro-lymphocytic leukemia (PLL), 5 of 6 with leukemic mantle-cell lymphoma (MCL), 2 of 7 with splenic B-cell leukemia/lymphoma of possible marginal zone origin (SBLL) and 2 with leukemic follicular lymphoma (FL). To further characterize 14q32.33 translocations in these patients, we developed a new procedure using double-color FISH with PRAD1, BCL2, V(H) and Cgamma gene probes. Chromosome t(11;14) was detected in 1 patient with CLL/PL, 1 with PLL and 5 with MCL. Chromosome t(14;18) was detected in 2 patients with FL. In a PLL patient with t(11;14), the cosmid CPP29 containing the PRAD1 gene and its 5'-flanking region split and co-localized with both Cgamma and V(H) gene probes, thus spanning the breakpoint. In CLL and SBLL patients, donor chromosomes were other than chromosomes 2, 11, 18 and 19, suggesting the involvement of a novel oncogene(s) in the pathogenesis of these diseases. Interphase FISH rapidly detected 14q32.33 translocation, t(11;14) and t(14;18) in B-cell malignancies with low mitotic activity at the single-cell level, facilitating the correlation of the molecular features of these translocations with clinical characteristics.

Published
1997

41. A nodal gamma/delta T-cell lymphoma with an association of Epstein-Barr virus

Author

Y, Kagami, S, Nakamura, R, Suzuki, Y, Yatabe, Y, Okada, T, Kobayasi, M, Taniwaki, M, Seto, M, Ogura, and T, Suchi

Subjects
Immunoenzyme Techniques, Herpesvirus 4, Human, Cell Transformation, Neoplastic, Humans, Female, Lymph Nodes, Cell Transformation, Viral, Flow Cytometry, Lymphoma, T-Cell, In Situ Hybridization, Aged
Abstract

The postthymic gamma/delta T-cell lymphoma is rare, and most occur as extranodal tumors, e.g., in hepatosplenic or cutaneous forms. We here report an unusual nodal case that initially presented as a T-zone lymphoma. The neoplasm recurred as systemic lymphadenopathy 25 months after complete remission with terminal high-grade transformation. Phenotypic analysis showed CD1-, CD2+, CD3+, CD4-, CD5-, CD7+, CD8+, CD10-, CD16-, CD19-, CD20-, CD21-, CD25-, CD56-, CD57-, T-cell receptor (TCR) alpha/beta antigens negative, TCR gamma/delta antigens positive, and an HLA-DR+ phenotype. Cytogenetic studies showed clonal chromosomal translocations involving chromosomes 1, 5, 6, 8, 15, and X in eight of 15 cells; t(X;5;1)(q13;q13;p22) and t(6;15;8)(p22;q26;q13). Genotypic analysis showed the same clone, characterized by the TCR gamma-chain gene rearrangement pattern, to be present in both initial and recurrent tumors. The lymphoma cells were also demonstrated to express the latent membrane protein-1 by immunohistochemistry and EBV-encoded small RNAs by in situ hybridization. Southern blot analysis using the probe of the terminal repeat demonstrated incorporation of multiple copies of EBV in the recurrent tumor. However, the initial lesion, which contained a smaller number of EBV-positive cells, showed no such evidence of clonal proliferation. These data suggest that EBV may be associated with high-grade transformation, although its exact role in lymphomagenesis remains uncertain. The present study also adds to our understanding of the clinicopathologic spectrum of gamma/delta T-cell neoplasia.

Published
1997

42. Tandem duplication of the MLL gene in myelodysplastic syndrome-derived overt leukemia with trisomy 11

Author

K, Yamamoto, H, Hamaguchi, K, Nagata, M, Kobayashi, and M, Taniwaki

Subjects
Chromosome Aberrations, Leukemia, Chromosomes, Human, Pair 11, Chromosome Disorders, Trisomy, Histone-Lysine N-Methyltransferase, Chromosome Banding, DNA-Binding Proteins, Gene Expression Regulation, Neoplastic, Multigene Family, Myelodysplastic Syndromes, Proto-Oncogenes, Humans, Female, RNA, Messenger, RNA, Neoplasm, In Situ Hybridization, Fluorescence, Myeloid-Lymphoid Leukemia Protein, Aged, Transcription Factors
Abstract

Trisomy 11 as a sole chromosomal abnormality is a rare aberration observed in myelodysplastic syndrome (MDS) or acute myeloblastic leukemia (AML). Recently a partial tandem duplication of the MLL gene, located on chromosome band 11q23, has been identified in de novo AML with trisomy 11. We describe a 72-year-old woman suffering from MDS-derived overt leukemia with trisomy 11 and a tandem duplication of the MLL gene. At first the patient was found to have myeloblasts with Auer rods in the peripheral blood and diagnosed as MDS, refractory anemia with excess of blasts in transformation (RAEB-T). After 2 months a picture of overt leukemia (AML; M2) developed as shown by an increased number of myeloblasts. Various chemotherapy regimens had little effect, and she died of disease progression 15 months after admission. During her clinical course, the chromosome analyses consistently showed 47,XX, +11. Southern blot analysis of leukemic blasts on admission and in accelerated phase revealed identical rearranged bands of the MLL gene. Fluorescence in situ hybridization analysis excluded the possibility of masked translocation of the MLL gene to other chromosomes. Reverse transcriptase-polymerase chain reaction (RT-PCR) analysis using a forward exon 6 primer and a backward exon 3 primer demonstrated an in-frame fusion of exon 8 with exon 2. Our results indicated that a partial tandem duplication of exons 2-8 of the MLL gene could be observed in MDS-derived overt leukemia as well as de novo AML with trisomy 11.

Published
1997

43. Rapid detection of lymphoma-specific translocations in interphase nuclei of non-Hodgkin's lymphoma by fluorescence in situ hybridization

Author

M, Taniwaki, Y, Ueda, K, Nishida, T, Takashima, K, Kashima, F, Matsuda, and G A, Silverman

Subjects
Cell Nucleus, Chromosomes, Human, Pair 14, Gene Rearrangement, Lymphoma, B-Cell, Genes, Immunoglobulin, Chromosomes, Human, Pair 11, Chromosome Mapping, Translocation, Genetic, DNA-Binding Proteins, Proto-Oncogene Proteins, Proto-Oncogene Proteins c-bcl-6, Humans, Chromosomes, Human, Pair 3, Chromosomes, Human, Pair 18, DNA Probes, Interphase, In Situ Hybridization, Fluorescence, Transcription Factors
Abstract

We have recently developed a method to detect tumor-specific rearrangement of the IgH gene in interphase nuclei by fluorescence in situ hybridization. Tumor-specific IgH gene rearrangement is equivalent to 14q32.33 translocation. Using this approach, we detected 14q32.33 translocation in 29 of 70 patients with B-cell non-Hodgkin's lymphoma (NHL). Chromosome t(3;14) was found in 10 of these 29 patients, and were demonstrated as a fusion signal of BCL6 and VH gene probes in interphase nuclei. Furthermore, in another series of 11 patients and a NHL cell line, we demonstrated t(14;18) and t(11;14) in interphase and metaphase cells with a combination of BCL2 (or PRAD1) with IgH gene probes. Interphase FISH with lymphoma-associated gene probes is a rapid procedure for cytogenetic diagnosis of B-cell NHL.

Published
1997

44. Microsatellite instability is an early genetic event in myelodysplastic syndrome but is infrequent and not associated with TGF-beta receptor type II gene mutation

Author

H, Kaneko, S, Horiike, M, Taniwaki, and S, Misawa

Subjects
Chromosome Aberrations, Bone Marrow, Transforming Growth Factor beta, Karyotyping, Myelodysplastic Syndromes, Mutation, Humans, Chromosome Disorders, DNA, Satellite, Receptors, Transforming Growth Factor beta, Microsatellite Repeats
Abstract

We examined microsatellite instability (MSI) at 10 loci of dinucleotide repeats using the polymerase chain reaction (PCR) in patients with myelodysplastic syndrome (MDS). Bone marrow DNA was obtained from 45 patients repeatedly during the disease course and fibroblast DNA was also collected from 19 of them as a normal control. Three of the 19 patients showed an alteration at more than three loci, when the allele length was compared between their fibroblast DNA and the initial marrow DNA. On the other hand, none of the 45 patients showed an alteration when the initial sample was compared with the latest one. One of the three patients with MSI had refractory anemia and two refractory anemia with ring sideroblasts and none of them showed disease progression, complex chromosome abnormality, karyotypic evolution, or mutation of N-RAS or TP53. Moreover, a frameshift mutation within 10 repeating adenines of transforming growth factor beta type II receptor gene, which was recently recognized as a critical target of MSI, was not found in any of the patients including the three with MSI. These findings suggest that MSI is an early but infrequent genetic event and is independent of other critical genetic aberrations in the development of MDS.

Published
1996

45. Detection and quantification of TEL/AML1 fusion transcripts by polymerase chain reaction in childhood acute lymphoblastic leukemia

Author

M, Nakao, S, Yokota, S, Horiike, M, Taniwaki, K, Kashima, Y, Sonoda, S, Koizumi, Y, Takaue, T, Matsushita, T, Fujimoto, and S, Misawa

Subjects
Male, Neoplasm, Residual, Adolescent, Base Sequence, Oncogene Proteins, Fusion, Proto-Oncogene Proteins c-ets, Molecular Sequence Data, Precursor Cell Lymphoblastic Leukemia-Lymphoma, Burkitt Lymphoma, Polymerase Chain Reaction, Neoplasm Proteins, DNA-Binding Proteins, Repressor Proteins, Phenotype, Child, Preschool, Proto-Oncogene Proteins, Core Binding Factor Alpha 2 Subunit, Humans, Leukemia-Lymphoma, Adult T-Cell, Female, RNA, Messenger, Child, Transcription Factors
Abstract

We investigated TEL/AML1 fusion mRNA in 108 children with acute lymphoblastic leukemia (ALL) (86 B-lineage ALL, 15 T-ALL, two mixed lineage ALL, and five other phenotypes) using reverse transcriptase-polymerase chain reaction (RT-PCR). TEL/AML1 transcripts were found in 14 patients (13%) including three relapsed patients, and were unexceptionally limited to B-lineage ALL patients. The incidence of TEL/AML1 transcripts among B-lineage ALL was 16% (14/86). The reciprocal AML1/TEL transcripts were detected in 12 (86%) of the 14 cases expressing a TEL/AML1 transcript. In three cases, the TEL gene was fused to exon 3 of the AML1 gene, and to exon 2 in the remaining cases. To evaluate the amount of TEL/AML1 molecules for the quantification of a minimal residual disease (MRD), a plasmid vector which contained either a long TEL/AML1 PCR product (464 bp) or a short one (425 bp) was used as a competitor. We amplified RNAs obtained from bone marrow (BM) at complete remission or from peripheral blood stem cell (PBSC) harvests in two representative cases. For one PBSC harvest showing a positive result, a competitive PCR was carried out to quantify the amount of MRD. A 1:4 dilution series of competitor vectors was constructed, and each vector was added to a PCR reaction which contain a constant amount of cDNA obtained from the PBSC harvest. An equivalent point was compared to that of corresponding samples at diagnosis. Using this method, MRD in the PBSC harvest was 3.9:10(3). Our results elucidated the incidence, lineage-specificity, and variant forms of TEL/AML1 fusion transcripts in childhood ALL. Since the percentage of other chromosomal translocations in childhood ALL is not more than 5%, TEL/AML1 transcript would be the most feasible clone-specific marker for these patients. In addition, our method could be a powerful tool for quantification of the TEL/AML1 transcript and for the detection of MRD.

Published
1996

46. Establishment of the novel B acute lymphoblastic leukemia (FAB L3) cell line KHM-10B with a 13q34 abnormality and constitutive expression of c-myc and max during cell cycle

Author

T, Sonoki, H, Matsuzaki, K, Miyamoto, M, Taniwaki, T, Yoshino, H, Hata, M, Yoshida, F, Matsuno, A, Nagasaki, and N, Kuribayashi

Subjects
Adult, Chromosome Aberrations, Male, Base Sequence, Chromosomes, Human, Pair 13, Basic Helix-Loop-Helix Leucine Zipper Transcription Factors, Cell Cycle, Molecular Sequence Data, Burkitt Lymphoma, Translocation, Genetic, DNA-Binding Proteins, Proto-Oncogene Proteins c-myc, Basic-Leucine Zipper Transcription Factors, Karyotyping, Tumor Cells, Cultured, Humans, Transcription Factors
Abstract

We established and characterized a new acute lymphoblastic leukemia (ALL-L3 according to FAB classification, or Burkitt's type) cell line, KHM-10B. The morphology of the patient's lymphoblasts and KHM-10B cells corresponded to that of ALL-L3 cells. The cells were positive for HLA-DR, CD19 and surface immunoglobulin (mu, lambda). Southern blot analysis revealed that the fresh lymphoblasts and KHM-10B shared the same immunoglobulin gene rearrangement. Conventional cytogenetic analysis of fresh lymphoblasts from the patient and KHM-10B cells revealed the 13q34 abnormality, the second most common additional abnormality in Burkitt's lymphoma, but no detectable 8q24 involvement. Rearrangement of the c-myc oncogene was not detected by Southern blot analysis. However, a fluorescence in situ hybridization (FISH) assay identified a t(8;22)(q24;q11). The KHM-10B cells were arrested at S phase with hydroxyurea and thymidine, and the synchronized cells progressed through the cell cycle in drug-free medium. The expression of c-myc and max was observed throughout the cell cycle, as was found in the Burkitt's lymphoma cell in Raji. Our findings indicate that FISH analysis is of diagnostic value in detecting obscure chromosomal translocations and that max, as well as c-myc, is expressed constitutively in ALL-L3 and Burkitt's lymphoma cell lines.

Published
1995

47. Double mutations of the N-ras gene in a patient with acute myelomonocytic leukemia

Author

S, Horiike, S, Misawa, H, Kaneko, H, Nakai, Y, Ueda, M, Nakao, K, Hirakawa, M, Taniwaki, and K, Kashima

Subjects
Male, Prednisolone, Genetic Vectors, Vinblastine, Leukemia, Myelomonocytic, Acute, Fatal Outcome, Antineoplastic Combined Chemotherapy Protocols, Humans, Point Mutation, Aclarubicin, Codon, Alleles, Etoposide, Chromosomes, Human, Pair 12, Mercaptopurine, Daunorubicin, Cytarabine, Middle Aged, Genes, ras, Doxorubicin, Vincristine, Karyotyping, Disease Progression, Chromosome Deletion, Mitoxantrone, Chromosomes, Human, Pair 9
Abstract

We report a patient with acute myelomonocytic leukemia (AMMoL) who showed two independent point mutations of the N-ras gene at codons 12 and 13. Longitudinal analysis revealed that one mutation at codon 13 was detectable throughout his disease course and the other at codon 12 emerged as a second mutation 14 months after the diagnosis was made, at the refractory stage. Cloning to vector and subsequent sequencing confirmed that these mutations occurred in different alleles. Chromosome findings showed a simple abnormal karyotype at presentation and further karyotypic aberrations during his disease course, concomitantly with the second mutation of the N-ras gene. These findings revealed a close relationship among the disease progression, karyotypic evolution and a newly-appearing N-ras mutation.

Published
1995

48. Interphase and metaphase detection of the breakpoint of 14q32 translocations in B-cell malignancies by double-color fluorescence in situ hybridization

Author

M, Taniwaki, K, Nishida, Y, Ueda, S, Misawa, M, Nagai, S, Tagawa, T, Yamagami, H, Sugiyama, M, Abe, and S, Fukuhara

Subjects
Chromosomes, Human, Pair 14, Lymphoma, B-Cell, Genes, Immunoglobulin, Rhodamines, Immunoglobulin gamma-Chains, Immunoglobulin Variable Region, Cosmids, Burkitt Lymphoma, Translocation, Genetic, Leukemia, Plasma Cell, Tumor Cells, Cultured, Humans, Chromosomes, Human, Pair 3, Chromosomes, Human, Pair 18, Immunoglobulin Heavy Chains, Chromosomes, Artificial, Yeast, Interphase, Fluorescein-5-isothiocyanate, In Situ Hybridization, Fluorescence, Metaphase, Chromosomes, Human, Pair 8, Fluorescent Dyes
Abstract

The breakpoint of 14q32 translocations found in B-cell malignancies was delineated specifically in both metaphase spreads and interphase nuclei by double-color fluorescence in situ hybridization (FISH) using bacteriophage clones containing the human immunoglobulin gamma chain gene locus (Ig gamma) and a cosmid clone, CY24-68, containing VH segments. CY24-68 is more telomeric than Ig gamma, separated by approximately 1 megabase (Mb). FISH studies were performed on four patients with non-Hodgkin's lymphoma (NHL), one with acute lymphoblastic leukemia (ALL), one with plasma cell leukemia (PCL), and three cell lines. In each patient with t(8;14), t(14;18), and t(3;14), the signal of Ig gamma gene was observed on der(14) and that of CY24-68 at respective partner sites of these translocations, 8q24.1, 18q21.3, and 3q27. Interphase nuclei with a signal of Ig gamma clearly separated from that of CY24-68 were more frequently encountered in all of the patients (45% to 74%) than those in normal controls (4% to 5%). Even in cases where only interphase nuclei were available for FISH studies, 14q32 translocations are detected as shown in two patients each with NHL and t(11;14)-carrying PCL. In two cell lines, HS-1 derived from ALL carrying t(8;14) and FR4 derived from a plasmacytoma carrying a complex form of t(8;14), the signal of Ig gamma was observed at the breakpoint region 8q24.1 of the der(8) in addition to the der(14), indicating that translocation event occurred within the Ig gamma locus. Intense Ig gamma signal was found at the breakpoint region on the der(14)t(11;14) in HBL-2 derived from NHL, indicating amplification of the Ig gamma gene, and presumably the resultant chimeric DNA between Ig gamma and DNA sequences at 11q13. The present approach allowed us to unequivocally detect tumor-specific breakpoints of 14q32 translocations. Furthermore, interphase FISH provides a rapid diagnostic procedure to detect 14q32 translocations in B-cell malignancies.

Published
1995

49. [A combined consecutive therapy with fosfomycin and sulbactam/cefoperazone for bacterial infections associated with hematological diseases]

Author

S, Misawa, S, Tsuda, M, Taniwaki, S, Horiike, Y, Ariyama, K, Hirakawa, Y, Ueda, H, Kaneko, M, Nakao, and K, Kashima

Subjects
Adult, Aged, 80 and over, Male, Cefoperazone, Bacterial Infections, Middle Aged, Hematologic Diseases, Drug Administration Schedule, Drug Combinations, Fosfomycin, Sulbactam, Granulocyte Colony-Stimulating Factor, Injections, Intravenous, Humans, Drug Therapy, Combination, Female, Aged
Abstract

A combination antibacterial therapy with fosfomycin (FOM) and sulbactam/cefoperazone (SBT/CPZ) was applied to 78 patients with severe infections associated with hematological diseases. In this protocol, FOM was followed by SBT/CPZ and each drug was administered for 1 hour intravenously and consecutively. Among 72 evaluable patients, 43 patients had acute leukemia, myeloblastic or lymphoblastic, 22 had malignant lymphoma, 3 had multiple myeloma, and 4 had other hematological diseases as underlying diseases. Bacterial infections diagnosed were sepsis in 21 patients, suspected sepsis in 47, and other infections in 4. The overall efficacy rate of this treatment was 72.2%, and those for individual infections were 66.7% for sepsis, 74.5% for suspected sepsis, and 75.0% for other infectious diseases. Among 22 bacteria separated from patients with sepsis, 78.6% (11/14 strains) were eradicated by this treatment. This protocol was also effective in 57.1% (8/14) of patients whose granulocyte count was less than 100/mm3 during the course of treatment as well as in 83.3% (15/18) of patients with granulocyte count over 500/mm3. There was no difference in effectiveness between those patients to whom G-CSF was administered and those to whom it was not (17/24, 70.8% vs 35/48, 72.9%). As an adverse reaction, a transient increase of GOT and/or GPT was observed in 2 patients (2.8%). The consecutive administration treatment of FOM and SBT/CPZ is thus an effective and safe regimen for the treatment of patients with hematological diseases complicated by severe infections.

Published
1995

50. Neurofibromatosis 1 gene (NF1) mutation is a rare genetic event in myelodysplastic syndrome regardless of the disease progression

Author

H, Kaneko, S, Horiike, H, Nakai, Y, Ueda, M, Nakao, K, Hirakawa, S, Yokota, M, Taniwaki, S, Misawa, and K, Kashima

Subjects
Base Sequence, Myelodysplastic Syndromes, Genes, Neurofibromatosis 1, Molecular Sequence Data, Mutation, Disease Progression, Exons, Polymerase Chain Reaction
Abstract

Neurofibromatosis 1 gene (NF1) is a tumor suppressor gene and the product of which down-regulates Nras protein by its GTPase activating protein-related domain (NF1-GRD). Although the incidence of NF1 mutation was reported to be rare in the chronic phase of myelodysplastic syndrome (MDS), there have been no previous reports on its configuration in patients showing the disease progression. We examined NF1 in 50 patients with MDS including 9 who had progressed to more advanced stages and 16 to acute leukemia. Six patients had an Nras mutation. We carried out allele specific restriction analysis (ASRA) to detect a mutation at the first nucleotide A of codon 1423 (AAG), a mutational hot spot. We also employed a polymerase chain reaction mediated single strand conformation polymorphism (PCR-SSCP) method to confirm the result of ASRA and to detect a point mutation in other sequences of FLR exon. In consequence, ASRA disclosed wild type configuration and PCR-SSCP showed no aberrant band in any sample examined whether the samples harboured an Nras mutation or not. We conclude that NF1 mutation does not play a crucial role in the development and the progression of MDS.

Published
1995

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