Your search keyword '"Horiguchi-Yamada J"' showing total 3 results

1. Segregation of megakaryocytic or erythroid cells from a megakaryocytic leukemia cell line (JAS-R) by adhesion during culture.

Author

Yamada H, Sekikawa T, Iwase S, Arakawa Y, Suzuki H, Agawa M, Akiyama M, Takeda N, and Horiguchi-Yamada J

Subjects

Cell Line, Tumor, Humans, Oligonucleotide Array Sequence Analysis, Reverse Transcriptase Polymerase Chain Reaction, Cell Adhesion, Erythrocytes pathology, Leukemia, Megakaryoblastic, Acute pathology, Megakaryocytes pathology

Abstract

Adhesion is one of the important biologic characteristics of leukemic cells. We previously reported a new megakaryocytic-erythroid cell line, JAS-R. In this study, JAS-R cells were segregated into two types by the differences of attachment to culture dishes. One type (designated as JAS-RAD cells) adhered to the substratum of the culture dishes, while the other (JAS-REN cells) grew as a single-cell suspension. Adhesion of JAS-RAD was inhibited by treatment with RGDS oligopeptide. Flow cytometric analysis revealed that JAS-RAD cells had high expression of CD41a and CD61 versus low CD235a expression, and JAS-REN showed low expression of CD41a, and CD61, and high CD235a. The two phenotypes were reciprocally exchangeable by selecting adherent or suspended cells from each type of culture. Microarray analysis and RT-PCR revealed that JAS-RAD cells expressed four major alpha-granule genes and JAS-REN cells expressed beta-globin. Interestingly, erythropoietin was only secreted by JAS-RAD cells. With regard to transcription factors, it was shown that GFI1, FLI1 and RUNX1 were strongly expressed in JAS-RAD cells while GATA1, FOG1 and NFE2 were equally expressed by both types. These findings indicate that adhesion via integrins is related to the phenotypic shift of JAS-R cells between megakaryocytic and erythroid lineages.

Published

2007

2. Depsipeptide-resistant KU812 cells show reversible P-glycoprotein expression, hyper-acetylated histones, and modulated gene expression profile.

Author

Yamada H, Arakawa Y, Saito S, Agawa M, Kano Y, and Horiguchi-Yamada J

Subjects

Acetylation drug effects, Alcohol Dehydrogenase biosynthesis, Alcohol Oxidoreductases, Animals, Carbonyl Reductase (NADPH), Cell Line, Tumor, Down-Regulation drug effects, Gene Expression Regulation, Neoplastic drug effects, Humans, Nuclear Proteins biosynthesis, ATP Binding Cassette Transporter, Subfamily B, Member 1 biosynthesis, Antibiotics, Antineoplastic pharmacology, Depsipeptides pharmacology, Drug Resistance, Neoplasm drug effects, Histones metabolism, Protein Processing, Post-Translational drug effects

Abstract

Depsipeptide (FK228), a histone deacetylase inhibitor, is a promising new anticancer agent. The mechanism of resistance to this agent was studied using KU812 cells. Depsipeptide-resistant KU812 cells expressed P-glycoprotein (P-gp) and their resistance was abolished by co-treatment with verapamil. P-gp expression returned to the parental cell level when resistant cells were cultured in depsipeptide-free medium, while resistant cells cultured in the medium containing 16 nM depsipeptide still showed hyper-acetylation of histones. Moreover, resistant cells showed erythroid differentiation. Microarray analysis revealed that 28 genes showed increased expression and three genes showed decreased expression in resistant cells compared with parental cells. These 31 genes had various functions relating to signal transduction, cell cycle, apoptosis, and control of cell morphology and differentiation. Among the 28 genes that were upregulated, 15 genes also showed an increased expression in parental cells treated with 4 nM depsipeptide for 48 h, while the other 13 genes including P-gp were different. Among the three genes with decreased expression, HEP27 was most dramatically downregulated. These findings suggest that continuous exposure to depsipeptide reversibly induces P-gp, which contributes to the onset of resistance, but the altered gene expression profile of resistant cells may also play a role.

Published

2006

3. Ectopic cyclin D1 expression blocks STI571-induced erythroid differentiation of K562 cells.

Author

Kawano T, Horiguchi-Yamada J, Saito S, Iwase S, Furukawa Y, Kano Y, and Yamada H

Subjects

Benzamides, Benzoquinones, Down-Regulation, Drug Resistance, Neoplasm, Erythroid Precursor Cells pathology, Glycophorins metabolism, Humans, Imatinib Mesylate, K562 Cells, Lactams, Macrocyclic, Mitogen-Activated Protein Kinase 1 metabolism, Mitogen-Activated Protein Kinase 3, Mitogen-Activated Protein Kinase Kinases metabolism, Mitogen-Activated Protein Kinases metabolism, Phosphorylation, Protein-Tyrosine Kinases antagonists & inhibitors, Quinones pharmacology, Rifabutin analogs & derivatives, Signal Transduction, Transfection, Cell Differentiation drug effects, Cyclin D1 metabolism, Enzyme Inhibitors pharmacology, Erythroid Precursor Cells drug effects, Piperazines pharmacology, Pyrimidines pharmacology

Abstract

Bcr-Abl tyrosine kinase inhibitor induces apoptosis and erythroid differentiation of K562 cells. During this erythroid differentiation, c-Myc and cyclin D1 transcripts are transiently downregulated. Accordingly, we studied the effect of cyclin D1 overexpression on erythroid differentiation. After treatment with 250 nM STI571, 90% of K562 and 25% of K562/D1 cells underwent erythroid differentiation. The basal expression of glycophorin A in K562/D1 cells was markedly diminished compared with that by parental cells. STI571 treatment failed to induce glycophorin A expression in K562/D1 cells. During STI571 treatment, ERK activity was downregulated in parental cells, while it was constantly activated in K562/D1 cells. These results suggest that ectopic expression of cyclin D1 causes the resistance of K562 cells to erythroid differentiation by modulating ERK regulation.

Published

2004