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103. Validation of the immunochromatographic strip for [alpha]-thalassemia screening: a multicenter study.

Author

Winichagoon, Pranee, Kumpan, Pornnapa, Holmes, Paula, Finlayson, Jill, Newbound, Christopher, Kabral, Arnold, Li, Benjamin, Nuinoon, Manit, Fawcett, Terry, Tayapiwatana, Chatchai, Kasinrerk, Watchara, and Fucharoen, Suthat

Abstract

[alpha](0)-Thalassemia occurs from a deletion of 2 linked [alpha]-globin genes and interaction of these defective genes leads to hemoglobin (Hb) Bart's hydrops fetalis, the most severe and lethal thalassemia syndrome. Identification of [alpha](0)-thalassemia carriers is thus essential for the prevention and control program. An immunochromatographic (IC) strip test was developed for rapid screening of [alpha](0)-thalassemia by testing for Hb Bart's in the blood samples using a specific monoclonal antibody against Hb Bart's. To evaluate its sensitivity and specificity, the IC strip test was assessed in a cohort with various thalassemia genotypes from 4 different laboratories in Thailand and Australia. The result showed 97% sensitivity in [alpha]-thalassemia carriers with 2 [alpha]-globin genes deletion and Hb H disease. This is, in particular, the useful rapid screening test for regions where [beta]-thalassemia and homozygous Hb E are also common. Similar hematologic and Hb data make it impossible to address the concomitant inheritance of [alpha](0)-thalassemia in these samples without polymerase chain reaction (PCR)-based techniques, leading to misdiagnosis of the risk of having Hb Bart's hydrops fetalis. However, [alpha]-globin genotyping should be carried out in samples with positive IC strip as positive reactivity was also observed in homozygous [alpha](+)-thalassemia carriers who have 2 trans [alpha]-globin gene deletions. These results indicate that in combination with red blood cell indices, the IC strip test could rule out mass populations for further [alpha](0)-thalassemia detection by PCR-based analysis. The Alpha Thal IC strip also has the potential to replace testing for Hb H inclusion bodies, as it appears to be more sensitive, specific, and less labor intensive. [ABSTRACT FROM AUTHOR]

Published
2015
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104. Enhanced Production of Functional Extracellular Single Chain Variable Fragment Against HIV-1 Matrix Protein from Escherichia coli by Sequential Simplex Optimization.

Author

Intachai, Kannaporn, Singboottra, Panthong, Leksawasdi, Noppol, Kasinrerk, Watchara, Tayapiwatana, Chatchai, and Butr-Indr, Bordin

Subjects
EXTRACELLULAR matrix proteins, RECOMBINANT proteins, HIV-1 glycoprotein 120, ESCHERICHIA coli proteins, SIMPLEX algorithm
Abstract

The optimal culture condition for extracellular recombinant single chain variable fragment anti HIV-1 p17 protein (scFv anti-p17) production inEscherichia coliHB2151 was investigated by the sequential simplex optimization (SS) method. Five variable parameters were submitted in the fermentation process. The most favorable condition obtained from 19 independent experiments was as followed: 58 µM of IPTG induction to 1.7 OD600 nm at 25.5°C for 16 h with 202 rpm agitation rate. The amount of secreted scFv anti-p17 at the optimal condition was 38% higher than under the control condition. The binding activity of soluble extracellular scFv anti-p17 protein increased 95.5% and 73.2% in comparison with the control condition and non-optimized condition respectively. The soluble scFv anti-p17 from crude HB2151 lysated was subsequently purified by immobilized metal ion affinity chromatography (IMAC) with His-tag. The purified scFv anti-p17 was intact and retained its antigen-binding affinity against HIV-1 p17. We demonstrated that the sequential simplex optimization method was a key for exertion of high yield with fewer experimental requirements for acquiring of large scale secretory protein production. [ABSTRACT FROM PUBLISHER]

Published
2015
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109. Simple method for screening of alpha-thalassaemia 1 carriers.

Author

Tayapiwatana, Chatchai, Kuntaruk, Surakit, Tatu, Thanusak, Chiampanichayakul, Sawitree, Munkongdee, Thongperm, Winichagoon, Pranee, Fuchareon, Suthat, and Kasinrerk, Watchara

Subjects
ALPHA-Thalassemia, CHROMATOGRAPHIC analysis, COMPARATIVE studies, DIAGNOSTIC reagents & test kits, HEMOGLOBINS, IMMUNOASSAY, RESEARCH methodology, MEDICAL cooperation, MEDICAL screening, META-analysis, MONOCLONAL antibodies, RESEARCH, EVALUATION research, GENETIC carriers, DIAGNOSIS
Abstract

Alpha-thalassaemia 1 genetic disorder occurs when there is a deletion of two linked alpha-globin genes. The interaction between these abnormal genes leads to the most severe type of thalassaemia disease, haemoglobin (Hb) Bart's hydrops fetalis. The identification of alpha-thalassaemia 1 carriers and genetic counselling are essential for the prevention and control of severe thalassaemia diseases. In this study, we have developed a rapid screening method for identifying alpha-thalassaemia 1. A sandwich-type immunochromatographic (IC) strip test was developed, using the generated monoclonal anti-Hb Bart's antibody, to trace the Hb Bart's in haemolysates. When assayed by our IC strip test, all alpha-thalassaemia 1, HbH disease, HbH-Constant Spring (H-CS) disease, HbH-CS and heterozygous HbE (CSEA) Bart's disease, and homozygous alpha-thalassaemia 2 showed positive results. No false negative results were observed in these blood samples. In alpha-thalassaemia 2 heterozygotes, 83% of them showed positive reactivity. Among HbE (both homozygotes and heterozygotes), beta-thalassaemia (heterozygotes, homozygotes and beta-thalassaemia/HbE) and normal subjects, the IC strip test revealed negative reactivity of 100, 85 and 97%, respectively. These results indicate that this novel immunodiagnostic kit, in combination with red blood cell indices, is suitable for screening and ruling out mass populations for the presence of alpha-thalassaemia 1. [ABSTRACT FROM AUTHOR]

Published
2009
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110. Lekteplase--a Secreted Tissue Plasminogen Activator Derivative from Escherichia coli.

Author

Manosroi, Jiradey, Tayapiwatana, Chatchai, Manosroi, Aranya, Beer, Jurgen, Bergemann, Klaus, and Werner, Rolf Gunter

Subjects
ESCHERICHIA coli, SERINE proteinases, PLASMINOGEN activators
Abstract

Fermentation studies of batch-mode cultivation in 4-L fermenters were carried out to obtain an active recombinant DNA-derived tissue plasminogen activator (t-PA) deletion mutant, lekteplase, secreted and correctly folded from Escherichia coli. The OmpA signal sequence was used to deliver the heterologous product composed of kringle 2 plus serine protease domain (K[sub2]S) to the medium. Supplementing the complex medium with 10 % glycerol and 20 mmol/l magnesium chloride led to an increase in cell numbers with final cell density reaching an OD[sub600] of 24. The expression level of lekteplase in the medium detected by sandwich ELISA was 100 mg/L. Enzymatic activity of lysine-sepharose purified product was demonstrated by amidolytic assay, in vitro fibrin clot lysis, and copolymerization PAGE. [ABSTRACT FROM AUTHOR]

Published
2002

111. Combined Antiviral Therapy Using Designed Molecular Scaffolds Targeting Two Distinct Viral Functions, HIV-1 Genome Integration and Capsid Assembly

Author

Sudarat Hadpech, Pierre Boulanger, Koollawat Chupradit, Chatchai Tayapiwatana, Bruce E. Torbett, Wannisa Khamaikawin, Sawitree Nangola, Supachai Sakkhachornphop, Aftab A. Ansari, Siddappa N. Byrareddy, Nattawat Onlamoon, Somphot Saoin, Saw See Hong, Rétrovirus et Pathologie Comparée (RPC), Institut National de la Recherche Agronomique (INRA)-École pratique des hautes études (EPHE), Université Paris sciences et lettres (PSL)-Université Paris sciences et lettres (PSL)-Université Claude Bernard Lyon 1 (UCBL), Université de Lyon-Université de Lyon-Ecole Nationale Vétérinaire de Lyon (ENVL), Thailand Research Fund through the Royal Golden Jubilee Ph.D. program= [PHD/0024/2552], Cluster and Program Management Office (CPMO), National Science and Technology Development Agency (NSTDA), National Research Council of Thailand (NRCT), Health Systems Research Institute (HSRI), National Research University project under the Thailand's Office of the Commission on Higher Education, National Institutes of Health (NIH) [CFAR-P30 AI036214, GM083658, HL091219], Tayapiwatana, Chatchai, Infections Virales et Pathologie Comparée - UMR 754 (IVPC), Institut National de la Recherche Agronomique (INRA)-École pratique des hautes études (EPHE)-Université Claude Bernard Lyon 1 (UCBL), and Université de Lyon-Université de Lyon

Subjects
capside, Genetic enhancement, viruses, [SDV]Life Sciences [q-bio], anti-HIV-1 molecular scaffolds, designed ankyrin repeat proteins, designed zinc-finger proteins, HIV-1-resistant cells, Biology, Viral vector, 03 medical and health sciences, analyse de génome, 0302 clinical medicine, Complementary DNA, Drug Discovery, Vector (molecular biology), sida, Gene, 030304 developmental biology, Zinc finger, 0303 health sciences, lcsh:RM1-950, myr, virus diseases, Virology, antiviral, 3. Good health, lcsh:Therapeutics. Pharmacology, Capsid, SIV, SHIV, 030220 oncology & carcinogenesis, Molecular Medicine, Original Article
Abstract

International audience; Designed molecular scaffolds have been proposed as alternative therapeutic agents against HIV-1. The ankyrin repeat protein (Ank(GAG)1D4) and the zinc finger protein (2LTRZFP) have recently been characterized as intracellular antivirals, but these molecules, used individually, do not completely block HIV-1 replication and propagation. The capsid-binder Ank(GAG)1D4, which inhibits HIV-1 assembly, does not prevent the genome integration of newly incoming viruses. 2LTRZFP, designed to target the 2-LTR-circle junction of HIV-1 cDNA and block HIV-1 integration, would have no antiviral effect on HIV-1-infected cells. However, simultaneous expression of these two molecules should combine the advantage of preventive and curative treatments. To test this hypothesis, the genes encoding the N-myristoylated Myr(+)Ank(GAG)1D4 protein and the 2LTRZFP were introduced into human T-cells, using a third-generation lentiviral vector. SupT1 cells stably expressing 2LTRZFP alone or with Myr(+)Ank(GAG)1D4 showed a complete resistance to HIV-1 in viral challenge. Administration of the Myr(+)Ank(GAG)1D4 vector to HIV-1-preinfected SupT1 cells resulted in a significant antiviral effect. Resistance to viral infection was also observed in primary human CD4+ T-cells stably expressing Myr(+)Ank(GAG)1D4, and challenged with HIV-1, SIVmac, or SHIV. Our data suggest that our two anti-HIV-1 molecular scaffold prototypes are promising antiviral agents for anti-HIV-1 gene therapy.

Published
2015

112. Rapid lateral flow test for Mycobacterium tuberculosis complex and non-tuberculous mycobacteria differentiation.

Author

Phunpae P, Thongkum W, Panyasit W, Laopajon W, Takheaw N, Pata S, Yasamut U, Kasinrerk W, and Tayapiwatana C

Subjects
Humans, Chromatography, Affinity methods, Sensitivity and Specificity, Mycobacterium Infections, Nontuberculous diagnosis, Mycobacterium Infections, Nontuberculous microbiology, Acyltransferases, Antibodies, Bacterial immunology, Mycobacterium tuberculosis growth & development, Mycobacterium tuberculosis isolation & purification, Mycobacterium tuberculosis genetics, Antibodies, Monoclonal immunology, Nontuberculous Mycobacteria isolation & purification, Nontuberculous Mycobacteria classification, Nontuberculous Mycobacteria growth & development, Antigens, Bacterial analysis, Antigens, Bacterial immunology, Tuberculosis diagnosis, Tuberculosis microbiology, Bacterial Proteins genetics
Abstract

The diagnosis of mycobacterial infections, including both the Mycobacterium tuberculosis complex (MTBC) and non-tuberculous mycobacteria (NTM), poses a significant global medical challenge. This study proposes a novel approach using immunochromatographic (IC) strip tests for the simultaneous detection of MTBC and NTM. Traditional methods for identifying mycobacteria, such as culture techniques, are hindered by delays in distinguishing between MTBC and NTM, which can affect patient care and disease control. Molecular methods, while sensitive, are resource-intensive and unable to differentiate between live and dead bacteria. In this research, we developed unique monoclonal antibodies (mAbs) against Ag85B, a mycobacterial secretory protein, and successfully implemented IC strip tests named 8B and 9B. These strips demonstrated high concordance rates with conventional methods for detecting MTBC, with positivity rates of 93.9% and 85.9%, respectively. For NTM detection, the IC strip tests achieved a 63.2% detection rate compared to culture methods, considering variations in growth rates among different NTM species. Furthermore, this study highlights a significant finding regarding the potential of MPT64 and Ag85B proteins as markers for MTBC detection. In conclusion, our breakthrough method enables rapid and accurate detection of both MTBC and NTM bacteria within the BACTEC MGIT system. This approach represents a valuable tool in clinical settings for distinguishing between MTBC and NTM infections, thereby enhancing the management and control of mycobacterial diseases. KEY POINTS: • Panel of mAbs for differentiating MTB versus NTM • IC strips for diagnosing MTBC and NTM after the BACTEC MGIT • Combined detection of MTP64 and Ag85B enhances diagnostic accuracy., (© 2024. The Author(s).)

Published
2024
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113. Evaluating the ability of different chaperones in improving soluble expression of a triple-mutated human interferon gamma in Escherichia coli.

Author

Yasamut U, Thongheang K, Weechan A, Sornsuwan K, Juntit OA, and Tayapiwatana C

Subjects
Humans, Mutation, Recombinant Proteins genetics, Recombinant Proteins metabolism, Plasmids genetics, Escherichia coli genetics, Escherichia coli metabolism, Interferon-gamma metabolism, Interferon-gamma genetics, Molecular Chaperones genetics, Molecular Chaperones metabolism, Solubility
Abstract

Human interferon gamma (hIFN-γ) plays a pivotal role as a soluble cytokine with diverse functions in both innate and adaptive immunity. In a previous investigation, we pinpointed three critical amino acid residues, i.e., threonine (T) 27, phenylalanine (F) 29, and leucine (L) 30, on the IFN-γ structure, which are integral to the epitope recognized by anti-IFN-γ autoantibodies. It is crucial to impede the interaction between this epitope and autoantibodies for effective therapy in adult-onset immunodeficiency (AOID). However, the challenge arises from the diminished solubility of the T27AF29L30A mutant in Escherichia coli BL21(DE3). This study delves into a targeted strategy aimed at improving the soluble expression of IFN-γ T27AF29AL30A. This is achieved through the utilization of five chaperone plasmids: pG-KJE8, pKJE7, pGro7, pG-Tf2, and pTf16. These plasmids, encoding cytoplasmic chaperones, are co-expressed with the IFN-γ mutant in E. coli BL21(DE3), and we meticulously analyze the proteins in cell lysate and inclusion bodies using SDS-PAGE and Western blotting. Our findings reveal the remarkable efficacy of pG-KJE8, which houses cytoplasmic chaperones DnaK-DnaJ-GrpE and GroEL-GroES, in significantly enhancing the solubility of IFN-γ T27AF29AL30A. Importantly, this co-expression not only addresses solubility concerns but also preserves the functional dimerized structure, as confirmed by sandwich ELISA. This promising outcome signifies a significant step forward in developing biologic strategies for AOID., (Copyright © 2024 The Society for Biotechnology, Japan. Published by Elsevier B.V. All rights reserved.)

Published
2024
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114. Engineered CD147-Deficient THP-1 Impairs Monocytic Myeloid-Derived Suppressor Cell Differentiation but Maintains Antibody-Dependent Cellular Phagocytosis Function for Jurkat T-ALL Cells with Humanized Anti-CD147 Antibody.

Author

Pamonsupornwichit T, Sornsuwan K, Juntit OA, Yasamut U, Takheaw N, Kasinrerk W, Wanachantararak P, Kodchakorn K, Nimmanpipug P, Intasai N, and Tayapiwatana C

Subjects
Humans, Jurkat Cells, THP-1 Cells, Myeloid-Derived Suppressor Cells metabolism, Myeloid-Derived Suppressor Cells immunology, Antibodies, Monoclonal, Humanized pharmacology, Animals, CHO Cells, Cricetulus, Monocytes metabolism, Monocytes immunology, Macrophages metabolism, Macrophages immunology, CRISPR-Cas Systems, Phagocytosis, Basigin metabolism, Basigin genetics, Cell Differentiation
Abstract

CD147 is upregulated in cancers, including aggressive T-ALL. Traditional treatments for T-ALL often entail severe side effects and the risk of relapse, highlighting the need for more efficacious therapies. ADCP contributes to the antitumor response by enhancing the ability of phagocytic cells to engulf cancer cells upon antibody binding. We aimed to engineer CD147 KO THP-1 cells and evaluated their differentiation properties compared to the wild type. A humanized anti-CD147 antibody, HuM6-1B9, was also constructed for investing the phagocytic function of CD147 KO THP-1 cells mediated by HuM6-1B9 in the phagocytosis of Jurkat T cells. The CD147 KO THP-1 was generated by CRISPR/Cas9 and maintained polarization profiles. HuM6-1B9 was produced in CHO-K1 cells and effectively bound to CD147 with high binding affinity (K D : 2.05 ± 0.30 × 10 -9 M). Additionally, HuM6-1B9 enhanced the phagocytosis of Jurkat T cells by CD147 KO THP-1-derived LPS-activated macrophages (M-LPS), without self-ADCP. The formation of THP-1-derived mMDSC was limited in CD147 KO THP-1 cells, highlighting the significant impact of CD147 deletion. Maintaining expression markers and phagocytic function in CD147 KO THP-1 macrophages supports future engineering and the application of induced pluripotent stem cell-derived macrophages. The combination of HuM6-1B9 and CD147 KO monocyte-derived macrophages holds promise as an alternative strategy for T-ALL.

Published
2024
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115. Development and evaluation of a high-sensitivity RT-PCR lateral flow assay for early detection of HIV-1 infection.

Author

Sakkhachornphop S, Thongkum W, Sornsuwan K, Juntit OA, Jirakunachayapisan K, Kongyai N, and Tayapiwatana C

Abstract

Early diagnosis of HIV-1 is crucial to minimize transmission, morbidity, and mortality, particularly for neonates with developing immune systems. This study aimed to develop and evaluate a simplified, high-sensitivity assay for early HIV-1 detection before seroconversion. The assay utilizes reverse-transcription-polymerase chain reaction (RT-PCR) to amplify the HIV-1 RNA protease gene. Digoxigenin (dig)-labeled forward, and biotin-labeled universal reverse primers are used, generating digoxigenin-amplicon-biotin (DAB) products. These products are detected using a lateral flow assay (LFA) containing a conjugated pad with colloidal gold-labeled 6-histidine tag-fused maltose-binding protein-monomeric streptavidin ( 6HIS MBP-mSA-CGC). Anti-dig monoclonal antibody (mAb) and biotinylated-BSA are immobilized in the test and control line zones, respectively. Five plasma samples with known viral load (VL) were used to simulate the efficacy of early HIV-1 detection. RNA extracted from these samples was amplified by RT-PCR using the labeled primers, and DAB products were examined on agarose gel electrophoresis and LFA. RT-PCR from diluted clinical samples yielded visible DNA bands in agarose gel electrophoresis, consistent with positive LFA results. Conversely, negative samples only displayed the control line on LFA. This assay exhibited a limit of detection (LOD) of 82.29 RNA copies/mL, comparable to other nucleic acid amplification tests (NAATs). This novel technique provides a highly sensitive assay for early HIV-1 diagnosis, even with low VL, making it suitable for resource-limited settings., Competing Interests: The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (© 2024 The Authors.)

Published
2024
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116. Transcriptomic analysis of glucosidase II beta subunit (GluIIß) knockout A549 cells reveals its roles in regulation of cell adhesion molecules (CAMs) and anti-tumor immunity.

Author

Khaodee W, Xiyuan G, Han MTT, Tayapiwatana C, Chiampanichayakul S, Anuchapreeda S, and Cressey R

Subjects
Humans, A549 Cells, Gene Expression Profiling, Cytokines, Cell Adhesion, Cell Adhesion Molecule-1, Leukocytes, Mononuclear, Cell Adhesion Molecules genetics, alpha-Glucosidases
Abstract

Glucosidase II beta subunit (GluIIß), encoded from PRKCSH, is a subunit of the glucosidase II enzyme responsible for quality control of N-linked glycoprotein folding and suppression of GluIIß led to inhibitory effect of the receptor tyrosine kinase (RTKs) activities known to be critical for survival and development of cancer. In this study, we investigated the effect of GluIIß knockout on the global gene expression of cancer cells and its impact on functions of immune cells. GluIIß knockout lung adenocarcinoma A549 cell line was generated using CRISPR/Cas9-based genome editing system and subjected to transcriptomic analysis. Among 23,502 expressed transcripts, 1068 genes were significantly up-regulated and 807 genes greatly down-regulated. The KEGG enrichment analysis showed significant down-regulation of genes related extracellular matrix (ECM), ECM-receptor interaction, cytokine-cytokine receptor interaction and cell adhesion molecules (CAMs) in GluIIß knockout cells. Of 9 CAMs encoded DEG identified by KEGG enrichment analysis, real time RT-PCR confirmed 8 genes to be significantly down-regulated in all 3 different GluIIß knockout clones, which includes cadherin 4 (CDH4), cadherin 2 (CDH2), versican (VCAN), integrin subunit alpha 4 (ITGA4), endothelial cell-selective adhesion molecule (ESAM), CD274 (program death ligand-1 (PD-L1)), Cell Adhesion Molecule 1 (CADM1), and Nectin Cell Adhesion Molecule 3 (NECTIN3). Whereas PTPRF (Protein Tyrosine Phosphatase Receptor Type F) was significantly decreased only in 1 out of 3 knockout clones. Microscopic analysis revealed distinctively different cell morphology of GluIIβ knockout cells with lesser cytoplasmic and cell surface area compared to parental A549 cells and non-targeted transfected cells.Further investigations revealed that Jurkat E6.1 T cells or human peripheral blood mononuclear cells (PBMCs) co-cultured with GluIIß knockout A549 exhibited significantly increased viability and tumor cell killing activity compared to those co-cultured with non-target transfected cells. Analysis of cytokine released from Jurkat E6.1 T cells co-cultured with GluIIß knockout A549 cells showed significant increased level of angiogenin and significant decreased level of ENA-78. In conclusion, knockout of GluIIß from cancer cells induced altered gene expression profile that improved anti-tumor activities of co-cultured T lymphocytes and PBMCs thus suppression of GluIIß may represent a novel approach of boosting anti-tumor immunity., (© 2024. The Author(s).)

Published
2024
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117. Development of an immunochromatographic strip test for rapid detection of a potent neutralizing anti-interferon gamma antibody in adult-onset immunodeficiency.

Author

Yasamut U, Thongkum W, Wongsawat E, and Tayapiwatana C

Abstract

Background: Adult-onset immunodeficiency (AOID) is associated with the presence of anti-interferon gamma autoantibodies (anti-IFN-γ autoAbs), which neutralizes IFN-γ signaling and leads to susceptibility to intracellular opportunistic infections. However, measuring neutralizing autoAbs is not practical for general clinical laboratories., Objective: This study aims to develop a competitive immunochromatographic (IC) strip test for detecting autoAbs that recognize the same epitope as a potent neutralizing antibody., Methods: The competitive IC strip test detecting autoAbs that recognize the same epitope as mouse anti-IFN-γ monoclonal antibody, clone B27 (B27 mAb) was fabricated and used to determine B27 epitope recognizing autoAb (B27 AAb) in AOID plasma. The competitive ELISA was used as a comparative method. AR patients., Results: The efficacy of the IC strip test was compared with competitive ELISA and found a percent positive agreement of 91.30%, a percent negative agreement of 79.31%, and a percent overall agreement of 84.62%., Conclusions: The results from the competitive IC strip test were consistent with those from competitive ELISA, indicating that the generated IC strip could detect B27 AAb in AOID plasma.

Published
2023
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118. Biological properties of reverse ankyrin engineered for dimer construction to enhance HIV-1 capsid interaction.

Author

Juntit OA, Yasamut U, Sakkhachornphop S, Chupradit K, Thongkum W, Srisawat C, Chokepaichitkool T, Kongtawelert P, and Tayapiwatana C

Abstract

Background: Assembly and budding in the late-stage of human immunodeficiency virus type 1 (HIV-1) production rely on Gag protein polymerization at the inner leaflet of the plasma membrane. We previously generated a monomeric ankyrin repeat protein (Ank1D4) that specifically interacts with capsid protein (CAp24) of HIV-1, however this protein had modest binding affinity., Objective: This study aimed to improve the avidity of Ank1D4 by generating two Ank1D4 dimers: (Ank1D4NC-NC) and its inverted form (Ank1D4NC-CN), with each domain connected by a flexible (G4S)4 linker peptide., Methods: Binding properties of monomeric and dimeric Ank1D4 was performed by capture enzyme-linked immunosorbent assay (ELISA). Sandwich ELISA was used to examine bifunctional module of dimeric Ank1D4. Ank1D4NC-NC and Ank1D4NC-CN were evaluated using bio-layer interferometry (BLI), compared to monomeric Ank1D4., Results: Similar binding surfaces were observed in both dimers which was comparable with monomeric Ank1D4. The interaction of Ank1D4NC-CN with CAp24 was significantly greater than that of Ank1D4NC-NC and Ank1D4 by capture ELISA. Ank1D4NC-CN also exhibited bifunctionality using a sandwich ELISA. The KD of Ank1D4NC-CN, Ank1D4NC-NC and monomeric Ank1D4 was 3.5 nM, 53.7 nM, and 126.2 nM, respectively using bio-layer interferometry analysis., Conclusions: This study provides a strategy for increasing Ank1D4 avidity through the construction of novel inverted dimers with a flexible linker. Ank1D4NC-CN may provide an alternative treatment strategy for inhibiting HIV-1 replication.

Published
2022
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119. Determination of a distinguished interferon gamma epitope recognized by monoclonal antibody relating to autoantibody associated immunodeficiency.

Author

Yasamut U, Wisitponchai T, Lee VS, Yamabhai M, Rangnoi K, Thongkum W, Chupradit K, and Tayapiwatana C

Subjects
Adult, Amino Acids, Antibodies, Monoclonal, Autoantibodies, Epitopes, Humans, Immunologic Deficiency Syndromes, Interferon-gamma metabolism
Abstract

Anti-interferon gamma autoantibodies (anti-IFN-γ autoAbs) neutralize the IFN-γ-mediated functions, contributing to immunodeficiency. A particular autoAb in patient serum had been previously demonstrated to recognize the same determinant on IFN-γ as the neutralizing anti-IFN-γ monoclonal antibody clone B27 (B27 mAb). This study explored the epitope recognized by B27 mAb. The specific peptide sequence recognized by B27 mAb, TDFLRMMLQEER, was retrieved from a phage display random peptide library. Sequence alignment and homology modeling demonstrated that the queried phage peptide sequence and structure were similar to amino acids at position 27-40 (TLFLGILKNWKEES) of the human IFN-γ. This determinant resides in the contact surface of IFN-γ and interferon gamma receptor 1. To elucidate the crucial amino acids, mutations were introduced by substituting T27 and T27F29L30 with alanine or deleting the amino acid residues T27-L33. The binding of B27 mAb to IFN-γ T27A using western blotting was lesser than that to wild-type. The interaction with triple mutant and T27-L33 deletion mutant using western blotting and sandwich ELISA was abolished. The finding demonstrated that T27, F29, and L30 are critical residues in the B27 antigenic determinant. Identification of the functional domain of IFN-γ decrypted the relevance of neutralizing autoAb in adult-onset immunodeficiency., (© 2022. The Author(s).)

Published
2022
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120. Immunoreactivity of humanized single-chain variable fragment against its functional epitope on domain 1 of CD147.

Author

Intasai N, Rangnoi K, Yamabhai M, Pamonsupornwichit T, Thongkum W, Yasamut U, Chupradit K, Takheaw N, Nimmanpipug P, and Tayapiwatana C

Subjects
Animals, Epitopes, Humans, Jurkat Cells, Lymphocyte Activation, Mice, Single-Chain Antibodies metabolism
Abstract

Domain 1 of CD147 participates in matrix metalloproteinase (MMP) production and is a candidate for targeted therapy to prevent cancer invasion and metastasis. A functional mouse anti-CD147 monoclonal antibody, M6-1B9, was found to recognize domain 1 of CD147, and its respective mouse single-chain variable fragment (ScFvM61B9) was subsequently generated. The EDLGS epitope candidate for M6-1B9 was identified using the phage display peptide technique in this study. For future clinical applications, humanized ScFv specific to domain 1 of CD147 (HuScFvM61B9) was partially adopted from the hypervariable sequences of parental mouse ScFvM61B9 and grafted onto suitable human immunoglobulin frameworks. Molecular modelling and simulation were performed in silico to generate the conformational structure of HuScFvM61B9. These results elucidated the amino acid residues that contributed to the interactions between CDRs and the epitope motif. The expressed HuScFvM61B9 specifically interacted with CD147 at the same epitope as the original mAb, M6-1B9, and retained immunoreactivity against CD147 in SupT1 cells. The reactivity of HuScFvM61B9 was confirmed using CD147 knockout Jurkat cells. In addition, the inhibitory effect of HuScFvM61B9 on OKT3-induced T-cell proliferation as M6-1B9 mAb was preserved. As domain 1 is responsible for cancer invasion and metastasis, HuScFvM61B9 would be a candidate for cancer targeted therapy in the future., (© 2022. The Author(s).)

Published
2022
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121. Deciphering critical amino acid residues to modify and enhance the binding affinity of ankyrin scaffold specific to capsid protein of human immunodeficiency virus type 1.

Author

Saoin S, Wisitponchai T, Intachai K, Chupradit K, Moonmuang S, Nangola S, Kitidee K, Fanhchaksai K, Lee VS, Hong SS, Boulanger P, Chuankhayan P, Chen CJ, and Tayapiwatana C

Subjects
Amino Acid Sequence, Amino Acids, Ankyrins chemistry, Ankyrins metabolism, Ankyrins pharmacology, Antiviral Agents metabolism, Capsid Proteins metabolism, Humans, Protein Binding, Recombinant Fusion Proteins metabolism, Structure-Activity Relationship, Antiviral Agents chemistry, Antiviral Agents pharmacology, HIV-1 drug effects, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins pharmacology
Abstract

Background: AnkGAG1D4 is an artificial ankyrin repeat protein which recognizes the capsid protein (CA) of the human immunodeficiency virus type 1 (HIV-1) and exhibits the intracellular antiviral activity on the viral assembly process. Improving the binding affinity of AnkGAG1D4 would potentially enhance the AnkGAG1D4-mediated antiviral activity., Objective: To augment the affinity of AnkGAG1D4 scaffold towards its CA target, through computational predictions and experimental designs., Method: Three dimensional structure of the binary complex formed by AnkGAG1D4 docked to the CA was used as a model for van der Waals (vdW) binding energy calculation. The results generated a simple guideline to select the amino acids for modifications. Following the predictions, modified AnkGAG1D4 proteins were produced and further evaluated for their CA-binding activity, using ELISA-modified method and bio-layer interferometry (BLI)., Results: Tyrosine at position 56 (Y56) in AnkGAG1D4 was experimentally identified as the most critical residue for CA binding. Rational substitutions of this residue diminished the binding affinity. However, vdW calculation preconized to substitute serine for tyrosine at position 45. Remarkably, the affinity for the viral CA was significantly enhanced in AnkGAG1D4-S45Y mutant, with no alteration of the target specificity., Conclusions: The S-to-Y mutation at position 45, based on the prediction of interacting amino acids and on vdW binding energy calculation, resulted in a significant enhancement of the affinity of AnkGAG1D4 ankyrin for its CA target. AnkGAG1D4-S45Y mutant represented the starting point for further construction of variants with even higher affinity towards the viral CA, and higher therapeutic potential in the future.

Published
2018
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122. Combined Antiviral Therapy Using Designed Molecular Scaffolds Targeting Two Distinct Viral Functions, HIV-1 Genome Integration and Capsid Assembly.

Author

Khamaikawin W, Saoin S, Nangola S, Chupradit K, Sakkhachornphop S, Hadpech S, Onlamoon N, Ansari AA, Byrareddy SN, Boulanger P, Hong SS, Torbett BE, and Tayapiwatana C

Abstract

Designed molecular scaffolds have been proposed as alternative therapeutic agents against HIV-1. The ankyrin repeat protein (Ank(GAG)1D4) and the zinc finger protein (2LTRZFP) have recently been characterized as intracellular antivirals, but these molecules, used individually, do not completely block HIV-1 replication and propagation. The capsid-binder Ank(GAG)1D4, which inhibits HIV-1 assembly, does not prevent the genome integration of newly incoming viruses. 2LTRZFP, designed to target the 2-LTR-circle junction of HIV-1 cDNA and block HIV-1 integration, would have no antiviral effect on HIV-1-infected cells. However, simultaneous expression of these two molecules should combine the advantage of preventive and curative treatments. To test this hypothesis, the genes encoding the N-myristoylated Myr(+)Ank(GAG)1D4 protein and the 2LTRZFP were introduced into human T-cells, using a third-generation lentiviral vector. SupT1 cells stably expressing 2LTRZFP alone or with Myr(+)Ank(GAG)1D4 showed a complete resistance to HIV-1 in viral challenge. Administration of the Myr(+)Ank(GAG)1D4 vector to HIV-1-preinfected SupT1 cells resulted in a significant antiviral effect. Resistance to viral infection was also observed in primary human CD4+ T-cells stably expressing Myr(+)Ank(GAG)1D4, and challenged with HIV-1, SIVmac, or SHIV. Our data suggest that our two anti-HIV-1 molecular scaffold prototypes are promising antiviral agents for anti-HIV-1 gene therapy.

Published
2015
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123. A dot-ELISA test using a Gnathostoma spinigerum recombinant matrix metalloproteinase protein for the serodiagnosis of human gnathostomiasis.

Author

Saenseeha S, Penchom J, Yamasaki H, Laummaunwai P, Tayapiwatana C, Kitkhuandee A, Maleewong W, and Intapan PM

Subjects
Animals, Enzyme-Linked Immunosorbent Assay, Humans, Recombinant Proteins, Sensitivity and Specificity, Serologic Tests, Gnathostomiasis diagnosis, Matrix Metalloproteinases
Abstract

Gnathostomiasis caused by Gnathostoma spinigerum, is a hazardous food- borne helminthic zoonosis, and is endemic especially in developing countries in Asia. Definitive diagnosis, relying upon identification of worms from human tissues or body, is rarely accomplished. Consequently, sensitive supporting tools such as serological tests have been used widely. But these methods are time con- suming, need sophisticated equipment and are impractical in some settings. In the present study a dot enzyme-linked immunosorbent assay (dot-ELISA), using C. spin igerum recombinant matrix metalloproteinase protein as the antigen, was developed and assessed using sera of gnathostomiasis and other parasitosis pa- tients as well as healthy controls. The accuracy, sensitivity, specificity, positive and negative predictive values were 97.4%, 100%, 96.1%, 92.9%, and 100%, respectively. The dot-ELISA appears to be a suitable rapid test for diagnostic purpose as well as epidemiological studies.

Published
2014

124. Accuracy of immunochromatographic strip test in diagnosis of alpha-thalassemia-1 carrier.

Author

Wanapirak C, Piyamongkol W, Sirichotiyakul S, Tayapiwatana C, Kasinrerk W, and Tongsong T

Subjects
Adult, Biomarkers blood, Carrier State diagnosis, Female, Gestational Age, Humans, Polymerase Chain Reaction, Predictive Value of Tests, Pregnancy, Reagent Strips, Sensitivity and Specificity, Young Adult, alpha-Thalassemia blood, Chromatography methods, Immunoassay methods, Prenatal Diagnosis methods, alpha-Thalassemia diagnosis
Abstract

Objective: To determine the accuracy of alpha-thal immunochromatographic (IC) strip in diagnosis of alpha-thalassemia 1 carrier among pregnant women, using PCR for alpha-thalassemia 1 (SEA type) as a gold standard., Material and Method: Asymptomatic pregnant women attending the antenatal care clinic were recruited Their blood samples were taken for IC Strip Test (alpha Thal IC strip, i+Med Laboratories Company Limited) in predicting alpha-thalassemia 1 carrier and separately sent for PCR for diagnosis of alpha-thalassemia 1 carrier as a gold standard, Results: Four hundred ninety nine pregnant women were recruited into the present study at various gestational weeks. The accuracy of alpha-Thal IC strip test was relatively high as shown in Table 1. Of them, 62 cases were proven to be alpha-thalassemia 1 trait and all ofthem had the results of positive IC strip, giving a sensitivity of 100%. However 45 pregnant women of non-alpha-thalassemia 1 trait had positive test, giving a specificity of 89%., Conclusion: The present study was solid evidence for clinical application of alpha-thal IC strip in screening program of thalassemia to reduce the need for PCR in diagnosis of a-thalassemia 1 carrier because of its very high sensitivity. The negative test reassures the non alpha-thalassemia 1 carrier status. Moreover, due to its simplicity, convenience to use, low cost, less-time consuming, clear interpretation and no need for either equipment or expensive laboratories, it may probably be very helpful in a massive screening program.

Published
2011

125. Hydrophobic allergens from the bottom fraction membrane of Hevea brasiliensis.

Author

Mengumpun K, Tayapiwatana C, Hamilton RG, Sangsupawanich P, and Wititsuwannakul R

Subjects
Allergens isolation & purification, Cell Fractionation, Gloves, Protective adverse effects, Health Care Sector, Health Personnel, Humans, Hydrophobic and Hydrophilic Interactions, Immunoglobulin E blood, Latex Hypersensitivity blood, Membranes, Occupational Exposure, Plant Proteins isolation & purification, Rubber adverse effects, Allergens immunology, Hevea, Latex Hypersensitivity immunology, Plant Proteins immunology
Abstract

Several proteins of rubber latex have been recognized as allergens causing immediate hypersensitivity in humans. In this study, a bottom fraction membrane (BFM) protein preparation from Hevea brasiliensis trees grown in southern Thailand was used to detect specific IgE in four groups of serum samples. The first group included 170 samples of latex glove factory workers (LGWs); group 2 consisted of the sera of 35 health care workers (HCWs) who were repeatedly exposed to powdered latex gloves; groups 3 and 4 were 31 positive and 22 negative sera, respectively, obtained from Johns Hopkins University School of Medicine, Baltimore, USA, tested for IgE to latex allergen. It was found that 56/170 (33%), 5/35 (14%), 11/31 (35.5%) and 1/22 (4.5%) samples of the LGWs, HCWs, CAP+ and CAP- groups had significant IgE to the BFM proteins, respectively. However, of all subjects only one subject of group 1 had experienced allergic morbidity consisting of eczema, conjunctivitis and asthma. The IgE of this subject bound to a 55 kDa component in the rubber latex BFM preparation. Thus, this protein may be regarded as a novel, although minor, latex allergen. Further investigation is needed to characterize the component and to pinpoint its allergenic role.

Published
2008

126. Potent inhibition of OKT3-induced T cell proliferation and suppression of CD147 cell surface expression in HeLa cells by scFv-M6-1B9.

Author

Intasai N, Tragoolpua K, Pingmuang P, Khunkaewla P, Moonsom S, Kasinrerk W, Lieber A, and Tayapiwatana C

Subjects
Cell Membrane immunology, Cell Proliferation, Gelatinases metabolism, HEK293 Cells, HeLa Cells, Humans, Recombinant Proteins genetics, Recombinant Proteins metabolism, Single-Chain Antibodies genetics, T-Lymphocytes metabolism, Basigin metabolism, Muromonab-CD3 immunology, Single-Chain Antibodies metabolism, T-Lymphocytes cytology, T-Lymphocytes immunology
Abstract

CD147, a multifunctional type I transmembrane glycoprotein, has been implicated in various physiological and pathological processes. It is involved in signal transduction pathways and also plays a crucial role in the invasive and metastatic activity of malignant tumor cells. Diminished expression of this molecule has been shown to be beneficial in suppression of tumor progression. In a previous study, we generated and characterized a recombinant antibody fragment, scFv, which reacted specifically to CD147. In the present study, we further investigated the biological properties, function and the effect of generated scFv on CD147 expression. The in vitro study showed that soluble scFv-M6-1B9 produced from E. coli HB2151 bound to CD147 surface molecule and inhibited OKT3-induced T cell proliferation. Furthermore, soluble lysate of scFv-M6-1B9 from 293A cells, transduced with a scFv-M6-1B9 expressing adenovirus vector, recognized both recombinant and native CD147. These results indicate that scFv-M6-1B9 binds with high efficiency and specificity. Importantly, scFv-M6-1B9 intrabody reduced the expression of CD147 on the cell surface of HeLa cells suggesting that scFv-M6-1B9 is biologically active. In conclusion, our present study demonstrated that scFv-M6-1B9 has a great potential to target both the intracellular and the extracellular CD147. The generated scFv-M6-1B9 may be an effective agent to clarify the cellular function of CD147 and may aid in efforts to develop a novel treatment in various human carcinomas.

Published
2008
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127. Lekteplase--a secreted tissue plasminogen activator derivative from Escherichia coli.

Author

Manosroi J, Tayapiwatana C, Manosroi A, Beer J, Bergemann K, and Werner RG

Subjects
Base Sequence, Bioreactors, Blotting, Western, Clot Retraction, Electrophoresis, Polyacrylamide Gel, Escherichia coli drug effects, Escherichia coli genetics, Fermentation, Glycerol pharmacology, Immunoassay, Magnesium Chloride pharmacology, Molecular Sequence Data, Plasmids genetics, Serine Endopeptidases metabolism, Tissue Plasminogen Activator metabolism, Escherichia coli metabolism, Tissue Plasminogen Activator pharmacology
Abstract

Fermentation studies of batch-mode cultivation in 4-L fermenters were carried out to obtain an active recombinant DNA-derived tissue plasminogen activator (t-PA) deletion mutant, lekteplase, secreted and correctly folded from Escherichia coli. The OmpA signal sequence was used to deliver the heterologous product composed of kringle 2 plus serine protease domain (K2S) to the medium. Supplementing the complex medium with 10% glycerol and 20 mmol/l magnesium chloride led to an increase in cell numbers with final cell density reaching an OD600 of 24. The expression level of lekteplase in the medium detected by sandwich ELISA was 100 mg/L. Enzymatic activity of lysine-sepharose purified product was demonstrated by amidolytic assay, in vitro fibrin clot lysis, and copolymerization PAGE.

Published
2002
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