Search

Your search keyword '"Ginya H"' showing total 14 results
Start Over Author "Ginya H"
14 results on '"Ginya H"'

3. Silencing of p53 and CDKN1A establishes sustainable immortalized megakaryocyte progenitor cells from human iPSCs.

Author

Sone M, Nakamura S, Umeda S, Ginya H, Oshima M, Kanashiro MA, Paul SK, Hashimoto K, Nakamura E, Harada Y, Tsujimura K, Saraya A, Yamaguchi T, Sugimoto N, Sawaguchi A, Iwama A, Eto K, and Takayama N

Subjects
Blood Platelets metabolism, Cell Line, Cell Proliferation, Clone Cells, Gene Knockdown Techniques, HEK293 Cells, Humans, Polycomb Repressive Complex 1 metabolism, Proto-Oncogene Proteins c-myc metabolism, Up-Regulation, bcl-X Protein metabolism, Cyclin-Dependent Kinase Inhibitor p21 metabolism, Gene Silencing, Induced Pluripotent Stem Cells metabolism, Megakaryocyte Progenitor Cells metabolism, Tumor Suppressor Protein p53 metabolism
Abstract

Platelet transfusions are critical for severe thrombocytopenia but depend on blood donors. The shortage of donors and the potential of universal HLA-null platelet products have stimulated research on the ex vivo differentiation of human pluripotent stem cells (hPSCs) to platelets. We recently established expandable immortalized megakaryocyte cell lines (imMKCLs) from hPSCs by transducing MYC, BMI1, and BCL-XL (MBX). imMKCLs can act as cryopreservable master cells to supply platelet concentrates. However, the proliferation rates of the imMKCLs vary with the starting hPSC clone. In this study, we reveal from the gene expression profiles of several MKCL clones that the proliferation arrest is correlated with the expression levels of specific cyclin-dependent kinase inhibitors. Silencing CDKN1A and p53 with the overexpression of MBX was effective at stably inducing imMKCLs that generate functional platelets irrespective of the hPSC clone. Collectively, this improvement in generating imMKCLs should contribute to platelet industrialization and platelet biology., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2021
Full Text
View/download PDF

4. Genetic susceptibility to postherniotomy pain. The influence of polymorphisms in the Mu opioid receptor, TNF-α, GRIK3, GCH1, BDNF and CACNA2D2 genes.

Author

Kalliomäki ML, Sandblom G, Hallberg M, Grönbladh A, Gunnarsson U, Gordh T, Ginya H, and Nyberg F

Subjects
Brain-Derived Neurotrophic Factor, Calcium Channels genetics, Cohort Studies, Hernia, Herniorrhaphy, Humans, Receptors, Kainic Acid genetics, Receptors, Opioid, mu, GluK3 Kainate Receptor, Genetic Predisposition to Disease, Pain, Postoperative genetics, Tumor Necrosis Factor-alpha genetics
Abstract

Background and Aims: Despite improvements in surgical technique, 5%-8% of patients undergoing herniorrhaphy still suffer from clinically relevant persistent postherniotomy pain. This is a problem at both individual and society levels. The aim of this study was to determine whether or not a single nucleotide polymorphism in a specific gene contributes to the development of persistent pain after surgery., Methods: One hundred individuals with persistent postherniotomy pain, along with 100 without pain matched for age, gender and type of surgery were identified in a previous cohort study on patients operated for groin hernia. All patients underwent a thorough sensory examination and blood samples were collected. DNA was extracted and analysed for single nucleotide polymorphism in the Mu opioid receptor, TNF-α, GRIK3, GCH1, BDNF and CACNA2D2 genes., Results: Patients with neuropathic pain were found to have a homozygous single nucleotide polymorph in the TNF-α gene significantly more often than pain-free patients (P=0.036, one-tailed test)., Conclusions: SNP in the TNF-α gene has a significant impact on the risk for developing PPSP., Implications: The result suggests the involvement of genetic variance in the development of pain and this requires further investigation., (Copyright © 2015 Scandinavian Association for the Study of Pain. Published by Elsevier B.V. All rights reserved.)

Published
2016
Full Text
View/download PDF

5. Combined analysis of circulating β-endorphin with gene polymorphisms in OPRM1, CACNAD2 and ABCB1 reveals correlation with pain, opioid sensitivity and opioid-related side effects.

Author

Rhodin A, Grönbladh A, Ginya H, Nilsson KW, Rosenblad A, Zhou Q, Enlund M, Hallberg M, Gordh T, and Nyberg F

Subjects
ATP Binding Cassette Transporter, Subfamily B, Adult, Aged, Analgesics, Opioid therapeutic use, Female, Gene Frequency genetics, Genetic Predisposition to Disease, Humans, Male, Middle Aged, Pain drug therapy, Quality of Life, ATP Binding Cassette Transporter, Subfamily B, Member 1 genetics, Analgesics, Opioid adverse effects, Calcium Channels genetics, Pain genetics, Polymorphism, Single Nucleotide genetics, Receptors, Opioid, mu genetics, beta-Endorphin blood
Abstract

Background: Opioids are associated with wide inter-individual variability in the analgesic response and a narrow therapeutic index. This may be partly explained by the presence of single nucleotide polymorphisms (SNPs) in genes encoding molecular entities involved in opioid metabolism and receptor activation. This paper describes the investigation of SNPs in three genes that have a functional impact on the opioid response: OPRM1, which codes for the μ-opioid receptor; ABCB1 for the ATP-binding cassette B1 transporter enzyme; and the calcium channel complex subunit CACNA2D2. The genotyping was combined with an analysis of plasma levels of the opioid peptide β-endorphin in 80 well-defined patients with chronic low back pain scheduled for spinal fusion surgery, and with differential sensitivity to the opioid analgesic remifentanil. This patient group was compared with 56 healthy controls., Results: The plasma β-endorphin levels were significantly higher in controls than in pain patients.A higher incidence of opioid-related side effects and sex differences was found in patients with the minor allele of the ABCB1 gene. Further, a correlation between increased opioid sensitivity and the major CACNA2D2 allele was confirmed. A tendency of a relationship between opioid sensitivity and the minor allele of OPRM1 was also found., Conclusions: Although the sample cohort in this study was limited to 80 patients it appears that it was possible to observe significant correlations between polymorphism in relevant genes and various items related to pain sensitivity and opioid response. Of particular interest is the new finding of a correlation between increased opioid sensitivity and the major CACNA2D2 allele. These observations may open for improved strategies in the clinical treatment of chronic pain with opioids.

Published
2013
Full Text
View/download PDF

6. Quantification and improvement of error rate during ligase detection reaction.

Author

Ginya H, Matsushita R, and Yohda M

Subjects
Base Pair Mismatch genetics, Biotechnology methods, Enzyme Stability, Ligases genetics, Models, Theoretical, Polymerase Chain Reaction, Substrate Specificity, Ligases metabolism
Abstract

We estimated the actual error rate during ligase detection reaction (LDR), and confirmed that DNA sequences around 3' ends are greatly influenced on the specificity of LDR. Its specificity is increased about 1000 times by introducing a mismatch base near the 3' ends., (Copyright (c) 2009 The Society for Biotechnology, Japan. Published by Elsevier B.V. All rights reserved.)

Published
2010
Full Text
View/download PDF

7. Semi-quantitative discrimination of HBV mutants using allele-specific oligonucleotide hybridization with Handy Bio-Strand.

Author

Ginya H, Asahina J, Nakao R, Tamada Y, Takahashi M, Yohda M, and Yatsuhashi H

Subjects
DNA, Viral genetics, Humans, Polymerase Chain Reaction, Reproducibility of Results, Viral Load, Alleles, Hepatitis B virology, Hepatitis B virus genetics, Mutation genetics, Nucleic Acid Hybridization methods, Oligonucleotides genetics
Abstract

The analysis of hepatitis B virus (HBV) mutations is important for understanding HBV progression and for deciding on appropriate clinical treatments. However, it is difficult to determine the quantitative abundance of various mutants in heterogeneous mixtures by conventional methods such as direct sequencing or the TaqMan assay. In this study, we investigated the possibility of using both allele-specific oligonucleotide hybridization (ASOH) and allele-specific oligonucleotide competitive hybridization (ASOCH) with the Handy Bio-Strand system for the quantitative identification of three well-defined HBV variants: the basal core promoter (BCP) mutations (nt1762 and nt1764), the pre-core (PC) mutation (nt1896), and variance at nt1858. Using standardized mixtures of wild-type and mutant DNA, optimal hybridization conditions for ASOH and ASOCH were determined. Next, the performance of these methods was evaluated using actual serum DNAs from HBV patients. Excellent reproducibility was obtained both in the analysis of internal positive controls and in the semi-quantitative categorization of heterogeneous viral mixtures into five abundance groups (0%, 25%, 50%, 75%, and 100% mutant virus). Combined with real-time PCR to determine the HBV viral load, this hybridization method offers a new tool with applications both in HBV clinical research and treatment., (2009 The Society for Biotechnology, Japan. Published by Elsevier B.V. All rights reserved.)

Published
2010
Full Text
View/download PDF

8. Noncovalent immobilization of streptavidin on in vitro- and in vivo-biotinylated bacterial magnetic particles.

Author

Maeda Y, Yoshino T, Takahashi M, Ginya H, Asahina J, Tajima H, and Matsunaga T

Subjects
Acetyl-CoA Carboxylase chemistry, Carbon-Nitrogen Ligases chemistry, Carrier Proteins chemistry, Escherichia coli chemistry, Escherichia coli Proteins chemistry, Fatty Acid Synthase, Type II, Repressor Proteins chemistry, Biotinylation methods, Magnetics, Magnetospirillum chemistry, Nanoparticles chemistry, Streptavidin chemistry
Abstract

Biotinylated magnetic nanoparticles were constructed by displaying biotin acceptor peptide (BAP) or biotin carboxyl carrier protein (BCCP) on the surface of bacterial magnetic particles (BacMPs) synthesized by Magnetospirillum magneticum AMB-1. BAP-displaying BacMPs (BAP-BacMPs) were extracted from bacterial cells and incubated with biotin and Escherichia coli biotin ligase. Then the in vitro biotinylation of BAP-BacMPs was confirmed using alkaline phosphatase-labeled antibiotin antibody. In contrast, BacMPs displaying the intact 149 residues of AMB-1 BCCP (BCCP-BacMPs) and displaying the COOH-terminal 78 residues of BCCP (BCCP78-BacMPs) were biotinylated in AMB-1 cells. The in vivo biotinylation of BCCP-BacMPs and BCCP78-BacMPs was thought to be performed by endogenous AMB-1 biotin ligase. Streptavidin was introduced onto biotinylated BacMPs by simple mixing. In an analysis using tetramethyl rhodamine isocyanate-labeled streptavidin, approximately 15 streptavidin molecules were shown to be immobilized on a single BCCP-BacMP. Furthermore, gold nanoparticle-BacMP composites were constructed via the biotin-streptavidin interaction. The conjugation system developed in this work provides a simple, low-cost method for producing biotin- or streptavidin-labeled magnetic nanoparticles. Various functional materials can be site selectively immobilized on these specially designed BacMPs. By combining the site-selective biotinylation technology and the protein display technology, more innovative and attractive magnetic nanomaterials can be constructed.

Published
2008
Full Text
View/download PDF

9. Fully automated immunoassay for detection of prostate-specific antigen using nano-magnetic beads and micro-polystyrene bead composites, 'Beads on Beads'.

Author

Matsunaga T, Maeda Y, Yoshino T, Takeyama H, Takahashi M, Ginya H, Aasahina J, and Tajima H

Subjects
Antibodies immunology, Humans, Microscopy, Electron, Scanning, Immunoassay instrumentation, Immunoassay methods, Magnetics, Nanoparticles ultrastructure, Polystyrenes, Prostate-Specific Antigen analysis, Prostate-Specific Antigen immunology
Abstract

Magnetic beads have served as a conventional bioassay platform in biotechnology. In this study, a fully automated immunoassay was performed using novel nano- and microbead-composites constructed by assembling nano-magnetic beads onto polystyrene microbeads, designated 'Beads on Beads'. Nano-sized bacterial magnetic particles (BacMPs) displaying the immunoglobulin G (IgG)-binding domain of protein A (ZZ domain) were used for the construction of 'Beads on Beads' via the interaction of biotin-streptavidin. The efficient assembly of 'Beads on Beads' was performed by gradual addition of biotin-labeled BacMPs onto streptavidin-coated polystyrene microbeads. Approximately 2000 BacMPs were uniformly assembled on a single microbead without aggregation. The constructed 'Beads on Beads' were magnetized and separated from the suspension by using an automated magnetic separation system with a higher efficiency than BacMPs alone. Furthermore, fully automated detection of prostate-specific antigens was performed with the detection limit of 1.48 ng mL(-1). From this preliminary assay, it can be seen that 'Beads on Beads' could be a powerful tool in the development of high-throughput, fully automated multiplexed bioassays.

Published
2007
Full Text
View/download PDF

10. Development of the Handy Bio-Strand and its application to genotyping of OPRM1 (A118G).

Author

Ginya H, Asahina J, Yoshida M, Segawa O, Asano T, Ikeda H, Hatano YM, Shishido M, Johansson BM, Zhou Q, Hallberg M, Takahashi M, Nyberg F, Tajima H, and Yohda M

Subjects
Alleles, Base Sequence, DNA genetics, DNA isolation & purification, Equipment Design, Genotype, Humans, Oligonucleotide Array Sequence Analysis methods, Oligonucleotide Probes genetics, Oligonucleotide Array Sequence Analysis instrumentation, Polymorphism, Single Nucleotide, Receptors, Opioid, mu genetics
Abstract

We previously developed a three-dimensional microarray system, the Bio-Strand, which exhibits advantages in automated DNA analysis in combination with our Magtration Technology. In the current study, we have developed a compact system for the Bio-Strand, the Handy Bio-Strand, which consists of several tools for the preparation of Bio-Strand Tip, hybridization, and detection. Using the Handy Bio-Strand, we performed single nucleotide polymorphism (SNP) genotyping of OPRM1 (A118G) by allele-specific oligonucleotide competitive hybridization (ASOCH). DNA fragments containing SNP sites were amplified from genomic DNA by PCR and then were fixed on a microporous nylon thread. Thus, prepared Bio-Strand Tip was hybridized with allele-specific Cy5 probes (<15mer), on which the SNP site was designed to be located in the center. By optimizing the amount of competitors, the selectivity of Cy5 probes increased without a drastic signal decrease. OPRM1 (A118G) genotypes of 23 human genomes prepared from whole blood samples were determined by ASOCH using the Handy Bio-Strand. The results were perfectly consistent with those determined by PCR direct sequencing. ASOCH using the Handy Bio-Strand would be a very simple and reliable method for SNP genotyping for small laboratories and hospitals.

Published
2007
Full Text
View/download PDF

11. Pretreatment of polyamide monofilament with hydrochloric acid improves sensitivity of three-dimensional microarray, Bio-Strand.

Author

Tojo Y, Syou R, Yoshida M, Momose J, Ginya H, Takahashi M, Tajima H, and Yohda M

Subjects
Reproducibility of Results, Sensitivity and Specificity, Hydrochloric Acid pharmacology, Nylons pharmacology, Oligonucleotide Array Sequence Analysis methods
Abstract

A single-nucleotide-polymorphism-typing method using a novel three-dimensional DNA microarray, Bio-Strand, is promising because it is rapid, inexpensive and easily automated. It has been developed with the intent to overcome the drawbacks of conventional DNA microarrays, which use flat surfaces and impermeable materials such as glass slides; Bio-Strand as a novel DNA microarray, with its permeability, has a significantly improved stability compared with conventional DNA microarrays that use impermeable materials. In this study, we have developed a simple method of pretreating a polyamide monofilament to increase its surface area and to make it permeable, which makes Bio-Strand more sensitive and stable, allowing it to be adapted for clinical diagnostic applications. The fluorescence signal obtained with a nylon 6 monofilament pretreated under optimal conditions (hydrolysis by 5 M HCl/ethanol followed by washing with 50% ethanol and 100% ethanol) was significantly stronger than that obtained with an untreated monofilament.

Published
2006
Full Text
View/download PDF

12. Expression of alpha-(1,3)-fucosyltransferases which synthesize sialyl Le(x) and sialyl Le(a), the carbohydrate ligands for E- and P-selectins,in human malignant cell lines.

Author

Yago K, Zenita K, Ginya H, Sawada M, Ohmori K, Okuma M, Kannagi R, and Lowe JB

Subjects
Adenocarcinoma enzymology, Base Sequence, Blotting, Northern, Carcinoma, Squamous Cell enzymology, Cell Adhesion Molecules, E-Selectin, Flow Cytometry, Hepatoblastoma enzymology, Humans, Leukemia enzymology, Molecular Sequence Data, P-Selectin, Platelet Membrane Glycoproteins, Polymerase Chain Reaction, RNA, Messenger analysis, Tumor Cells, Cultured, Biomarkers, Tumor analysis, Fucosyltransferases analysis, Gangliosides analysis, Neoplasms enzymology
Abstract

Transcripts of alpha-(1,3)-fucosyltransferases in human epithelial cancer and leukemia cell lines were analyzed by Northern blotting and reverse transcriptase mediated-polymerase chain reaction using specific probes and primers which can discriminate between the transcripts derived from the four alpha-(1,3)-fucosyltransferase genes Fuc-TIII, IV, V, and VI. Flow cytometric analysis of the sialyl Le(x) and sialyl Le(a) antigens was also performed on the same cell lines. The sialyl Le(x) antigen was expressed on 14 of 15 epithelial cancer cell lines, and the sialyl Le(a) antigen was detected on 8 of them. The message of Fuc-TIII was detected in most of the epithelial cancer cell lines (14 of 15), which correlated with the surface expression of these carbohydrate determinants. In addition, the messages of Fuc-TIV and Fuc-TVI were detected in most epithelial cancer cell lines, while the message of Fuc-TV was undetectable in most of them. On the other hand, all leukemia cell lines were positively stained for sialyl Le(x), but none of them was stained for sialyl Le(a) in flow cytometry. The messages of Fuc-TIV++ were detected in all leukemia cell lines tested. Small quantities of Fuc-TIII, V, and/or VI messages were also detected in some leukemia cell lines in reverse transcriptase mediated-polymerase chain reaction analysis. These studies indicate that alpha-(1,3)-fucosyltransferase activities in epithelial cancer and leukemia cell lines are mixtures of multiple molecular species of alpha-(1,3)-fucosyltransferases. It is natural that epithelial cancer cells contain a significant amount of Fuc-TIII mRNA and leukemia cell lines contain Fuc-TIV mRNA, since their normal counterparts, normal epithelial cells and leukocytes, respectively, are known to contain these fucosyltransferases. The unexpectedly frequent occurrence of Fuc-TIV mRNA in epithelial cancer cell lines may be related to their retro-differentiation associated with tumorigenesis. Another unexpected finding was a weak but significant expression of the alpha-(1,3)-fucosyltransferases Fuc-TIII, V, and/or VI in leukemia cell lines detected by reverse transcriptase mediated-polymerase chain reaction analysis. Since these enzymes are known to be capable of synthesizing the sialyl Le(x) determinant, this finding implies a possibility that some of them may be involved in the synthesis of sialyl Le(x) in leukemia cells.

Published
1993

13. Positive effect of GAC gene product on the mRNA level of glyoxalase I gene in Saccharomyces cerevisiae.

Author

Inoue Y, Yano H, Ginya H, Tsuchiyama H, Murata K, and Kimura A

Subjects
Amino Acid Sequence, Base Sequence, Blotting, Northern, Blotting, Western, DNA, Fungal, Genes, Fungal, Lactoylglutathione Lyase metabolism, Molecular Sequence Data, Plasmids, RNA, Messenger metabolism, Restriction Mapping, Saccharomyces cerevisiae enzymology, Fungal Proteins genetics, Genes, Regulator, Lactoylglutathione Lyase genetics, Saccharomyces cerevisiae genetics
Abstract

A DNA fragment carrying a part of the structural gene for yeast (Saccharomyces cerevisiae) glyoxalase I was cloned from a lambda gt11 expression library using anti-glyoxalase IIgG as a probe. By Northern blotting analysis, the amount of glyoxalase I mRNA was found to increase in yeast cells containing plasmids carrying the GAC gene, which is a positive regulator for yeast glyoxalase I activity. This suggests that the GAC gene product may accelerate the transcription of glyoxalase I gene or may have some positive effects on the accumulation of glyoxalase I mRNA in yeast cells.

Published
1991

14. Nucleotide sequence of a gene which enhances the activity of glyoxalase I in Saccharomyces cerevisiae.

Author

Inoue Y, Feng L, Bong-Young C, Ginya H, Murata K, and Kimura A

Subjects
Amino Acid Sequence, Base Sequence, Chromosome Mapping, DNA, Fungal genetics, Lactoylglutathione Lyase metabolism, Molecular Sequence Data, Saccharomyces cerevisiae genetics, Lactoylglutathione Lyase genetics, Lyases genetics, Saccharomyces cerevisiae enzymology
Abstract

A gene whose product enhances glyoxalase I activity in yeast Saccharomyces cerevisiae cells was cloned as a 6-kbp DNA fragment in the vector YEp13. The DNA fragment was subcloned in approximately 2 kbp and its base sequence determined. An open reading frame with 318 nucleotide pairs (encoding 106 amino acids) was found. According to Northern blotting analysis, the yeast transformed with the hybrid plasmid harboring the 2-kbp fragment yielded two different transcripts. From the DNA sequence of the fragment, it is deduced that the gene product would contain seven cysteine residues, five of which would be located near the carboxy terminus of the peptide.

Published
1990

Catalog

Books, media, physical & digital resources
See catalog results