Your search keyword '"Akihiro Abe"' showing total 5 results

1. Truncated RUNX1 Generated by the Fusion of RUNX1 to Antisense GRIK2 via a Cryptic Chromosome Translocation Enhances Sensitivity to Granulocyte Colony-Stimulating Factor

Author

Akihiro Abe, Yoko Inaguma, Akihiro Tomita, Hideyuki Yamamoto, Akira Katsumi, Nobuhiko Emi, Yukiya Yamamoto, Chisako Iriyama, Masutaka Tokuda, Akinao Okamoto, and Masataka Okamoto

Subjects

0303 health sciences, Daunorubicin, 030305 genetics & heredity, Myeloid leukemia, Combination chemotherapy, Chromosomal translocation, Biology, medicine.disease, Fusion protein, 03 medical and health sciences, chemistry.chemical_compound, Leukemia, RUNX1, chemistry, hemic and lymphatic diseases, embryonic structures, Genetics, medicine, Cytarabine, Cancer research, Molecular Biology, Genetics (clinical), 030304 developmental biology, medicine.drug

Abstract

Fusions of the Runt-related transcription factor 1 (RUNX1) with different partner genes have been associated with various hematological disorders. Interestingly, the C-terminally truncated form of RUNX1 and RUNX1 fusion proteins are similarly considered important contributors to leukemogenesis. Here, we describe a 59-year-old male patient who was initially diagnosed with acute myeloid leukemia, inv(16)(p13;q22)/CBFB-MYH11 (FAB classification M4Eo). He achieved complete remission and negative CBFB-MYH11 status with daunorubicin/cytarabine combination chemotherapy but relapsed 3 years later. Cytogenetic analysis of relapsed leukemia cells revealed CBFB-MYH11 negativity and complex chromosomal abnormalities without inv(16)(p13;q22). RNA-seq identified the glutamate receptor, ionotropic, kinase 2 (GRIK2) gene on 6q16 as a novel fusion partner for RUNX1 in this case. Specifically, the fusion of RUNX1 to the GRIK2 antisense strand (RUNX1-GRIK2as) generated multiple missplicing transcripts. Because extremely low levels of wild-type GRIK2 were detected in leukemia cells, RUNX1-GRIK2as was thought to drive the pathogenesis associated with the RUNX1-GRIK2 fusion. The truncated RUNX1 generated from RUNX1-GRIK2as induced the expression of the granulocyte colony-stimulating factor (G-CSF) receptor on 32D myeloid leukemia cells and enhanced proliferation in response to G-CSF. In summary, the RUNX1-GRIK2as fusion emphasizes the importance of aberrantly truncated RUNX1 in leukemogenesis.

Published

2020

2. Truncated RUNX1 Generated by the Fusion of RUNX1 to Antisense GRIK2 via a Cryptic Chromosome Translocation Enhances Sensitivity to Granulocyte Colony-Stimulating Factor

Author

Akihiro, Abe, Yukiya, Yamamoto, Akira, Katsumi, Hideyuki, Yamamoto, Akinao, Okamoto, Yoko, Inaguma, Chisako, Iriyama, Masutaka, Tokuda, Masataka, Okamoto, Nobuhiko, Emi, and Akihiro, Tomita

Subjects

Male, Middle Aged, Polymerase Chain Reaction, DNA, Antisense, Translocation, Genetic, Leukemia, Myeloid, Acute, Receptors, Kainic Acid, Core Binding Factor Alpha 2 Subunit, Granulocyte Colony-Stimulating Factor, Receptors, Granulocyte Colony-Stimulating Factor, Humans, RNA, Messenger, Gene Fusion, Cell Proliferation, Sequence Deletion

Abstract

Fusions of the Runt-related transcription factor 1 (RUNX1) with different partner genes have been associated with various hematological disorders. Interestingly, the C-terminally truncated form of RUNX1 and RUNX1 fusion proteins are similarly considered important contributors to leukemogenesis. Here, we describe a 59-year-old male patient who was initially diagnosed with acute myeloid leukemia, inv(16)(p13;q22)/CBFB-MYH11 (FAB classification M4Eo). He achieved complete remission and negative CBFB-MYH11 status with daunorubicin/cytarabine combination chemotherapy but relapsed 3 years later. Cytogenetic analysis of relapsed leukemia cells revealed CBFB-MYH11 negativity and complex chromosomal abnormalities without inv(16)(p13;q22). RNA-seq identified the glutamate receptor, ionotropic, kinase 2 (GRIK2) gene on 6q16 as a novel fusion partner for RUNX1 in this case. Specifically, the fusion of RUNX1 to the GRIK2 antisense strand (RUNX1-GRIK2as) generated multiple missplicing transcripts. Because extremely low levels of wild-type GRIK2 were detected in leukemia cells, RUNX1-GRIK2as was thought to drive the pathogenesis associated with the RUNX1-GRIK2 fusion. The truncated RUNX1 generated from RUNX1-GRIK2as induced the expression of the granulocyte colony-stimulating factor (G-CSF) receptor on 32D myeloid leukemia cells and enhanced proliferation in response to G-CSF. In summary, the RUNX1-GRIK2as fusion emphasizes the importance of aberrantly truncated RUNX1 in leukemogenesis.

Published

2020

3. NUP214-RAC1 and RAC1-COL12A1 Fusion in Complex Variant Translocations Involving Chromosomes 6, 7 and 9 in an Acute Myeloid Leukemia Case with DEK-NUP214

Author

Akinao Okamoto, Akihiro Abe, Yukiya Yamamoto, Masutaka Tokuda, Nobuhiko Emi, Motohiro Tsuzuki, Tadaharu Kanie, Masataka Okamoto, Akila Mayeda, Yoshiki Akatsuka, Yoko Inaguma, Shuichi Mizuta, Masamitsu Yanada, Sachiko Iba, Toshiki Kameyama, and Satoko Morishima

Subjects

Genetics, Breakpoint, Intron, Myeloid leukemia, Locus (genetics), Chromosomal translocation, Biology, Molecular biology, Fusion gene, Exon, Complex Karyotype, Molecular Biology, Genetics (clinical)

Abstract

DEK-NUP214 gene fusion in acute myeloid leukemia (AML) is associated with poor prognosis. It is most often a sole translocation and more rarely observed as complex chromosomal forms. We describe an AML case with complex karyotype abnormalities involving chromosome bands 6p23, 6q13, 7p22, and 9q34. RNA sequencing analysis revealed that exon 17 of NUP214 (9q34) was fused to exon 2 of RAC1 (7p22). We also detected that the 5′-end of intron 1 of RAC1 was fused with the antisense strand of intron 5 of COL12A1 (6q13). RT-PCR analysis confirmed the expression of DEK-NUP214, NUP214-RAC1, RAC1-COL12A1, NUP214, and RAC1. These results suggest that the 5′- and 3′-ends of NUP214 from the breakpoint in the same locus were fused to RAC1 and DEK, respectively, and the 5′-end of RAC1 was fused to COL12A1. The reading frame of NUP214 was not matched with RAC1; however, high expression of the RAC1 protein was detected by Western blotting. This study identifies the variant complex fusion genesNUP214-RAC1 and RAC1- COL12A1 in a case of AML.

Published

2015

4. Contents Vol. 146, 2015

Author

Duílio Mazzoni Zerbinato de Andrade Silva, Satz Mengensatzproduktion, John P. Murnane, Horacio Schneider, Yukiya Yamamoto, Akihiro Abe, Willam Oliveira da Silva, Yoko Inaguma, Kristine Nyhan, Jocicléia Thums Konerat, Zong-Ming Liu, Toshiki Kameyama, Motohiro Tsuzuki, Cleuton Lima Miranda, Shuichi Mizuta, Tadaharu Kanie, Manolo Penitente, Peter Zauber, Julio Cesar Pieczarka, Shao-Qian Cui, Filomena Adega, Masamitsu Yanada, Yoshiki Akatsuka, Akinao Okamoto, Christine Janson, Vladimir Pavan Margarido, Masutaka Tokuda, Ana Luiza de Brito Portela-Castro, Tae-Soo Jang, Druckerei Stückle, Hanna Weiss-Schneeweiss, Ricardo Utsunomia, Masataka Okamoto, Marlene Sabbath-Solitare, Huan Wang, Sandro Natal Daniel, Satoko Morishima, Daniela Ferreira, Iracilda Sampaio, Sachiko Iba, Cleusa Yoshiko Nagamachi, Lei Yang, Diogo Teruo Hashimoto, Claudia Regina Silva, Akila Mayeda, Viviani F. de Sene, Raquel Chaves, Isabel Cristina Martins-Santos, Vanessa Bueno, Stephen Marotta, Elizandra M. Cardoso, Rogério Vieira Rossi, Fausto Foresti, Yan-Wei Rao, Susana Meles, Fábio Porto-Foresti, José Carlos Pansonato-Alves, João Castro, Claudio Oliveira, Nobuhiko Emi, and Xiao-Jing Jia

Subjects

Botany, Genetics, Zoology, Biology, Molecular Biology, Genetics (clinical)

Published

2015

5. NUP214-RAC1 and RAC1-COL12A1 Fusion in Complex Variant Translocations Involving Chromosomes 6, 7 and 9 in an Acute Myeloid Leukemia Case with DEK-NUP214

Author

Akihiro, Abe, Yukiya, Yamamoto, Sachiko, Iba, Akinao, Okamoto, Masutaka, Tokuda, Yoko, Inaguma, Masamitsu, Yanada, Satoko, Morishima, Tadaharu, Kanie, Motohiro, Tsuzuki, Yoshiki, Akatsuka, Shuichi, Mizuta, Masataka, Okamoto, Toshiki, Kameyama, Akila, Mayeda, and Nobuhiko, Emi

Subjects

Adult, Collagen Type XII, Male, Nuclear Pore Complex Proteins, rac1 GTP-Binding Protein, Leukemia, Myeloid, Acute, Reverse Transcriptase Polymerase Chain Reaction, Sequence Analysis, RNA, Spectral Karyotyping, Chromosomes, Human, Humans, Translocation, Genetic

Abstract

DEK-NUP214 gene fusion in acute myeloid leukemia (AML) is associated with poor prognosis. It is most often a sole translocation and more rarely observed as complex chromosomal forms. We describe an AML case with complex karyotype abnormalities involving chromosome bands 6p23, 6q13, 7p22, and 9q34. RNA sequencing analysis revealed that exon 17 of NUP214 (9q34) was fused to exon 2 of RAC1 (7p22). We also detected that the 5'-end of intron 1 of RAC1 was fused with the antisense strand of intron 5 of COL12A1 (6q13). RT-PCR analysis confirmed the expression of DEK-NUP214, NUP214-RAC1, RAC1-COL12A1, NUP214, and RAC1. These results suggest that the 5'- and 3'-ends of NUP214 from the breakpoint in the same locus were fused to RAC1 and DEK, respectively, and the 5'-end of RAC1 was fused to COL12A1. The reading frame of NUP214 was not matched with RAC1; however, high expression of the RAC1 protein was detected by Western blotting. This study identifies the variant complex fusion genesNUP214-RAC1 and RAC1- COL12A1 in a case of AML.

Published

2015