Your search keyword '"Juma KM"' showing total 10 results

1. Achieving unprecedented stability in lyophilized recombinase polymerase amplification with thermostable pyruvate kinase from Thermotoga maritima.

Author

Juma KM, Murakami Y, Morimoto K, Takita T, Kojima K, Suzuki K, Yanagihara I, Ikuta S, Fujiwara S, and Yasukawa K

Subjects

Humans, Recombinases metabolism, Recombinases chemistry, Recombinases genetics, Escherichia coli genetics, Escherichia coli metabolism, DNA-Directed DNA Polymerase metabolism, DNA-Directed DNA Polymerase chemistry, DNA-Directed DNA Polymerase genetics, Bacterial Proteins genetics, Bacterial Proteins metabolism, Bacterial Proteins chemistry, Thermotoga maritima enzymology, Thermotoga maritima genetics, Freeze Drying, Pyruvate Kinase metabolism, Pyruvate Kinase genetics, Pyruvate Kinase chemistry, Enzyme Stability, Nucleic Acid Amplification Techniques methods

Abstract

Recombinase polymerase amplification (RPA) is an isothermal DNA amplification reaction at around 41 °C using recombinase (Rec), single-stranded DNA-binding protein (SSB), strand-displacing DNA polymerase (Pol), and an ATP-regenerating enzyme. Considering the onsite use of RPA reagents, lyophilized RPA reagents with long storage stability are highly desired. In this study, as one of the approaches to solve this problem, we attempted to use a thermostable pyruvate kinase (PK). PK gene was isolated from a thermophilic bacterium Thermotoga maritima (Tma-PK). Tma-PK was expressed in Escherichia coli and purified from the cells. Tma-PK exhibited higher thermostability than human PK. The purified Tma-PK preparation was applied to RPA as an ATP-regenerating enzyme. Liquid RPA reagent with Tma-PK exhibited the same performance as that with human PK. Lyophilized RPA reagent with Tma-PK exhibited higher performance than that with human PK. Combined with our previous results of RPA reagents of thermostable Pol from a thermophilic bacterium, Aeribacillus pallidus, the results in this study suggest that thermostable enzymes are preferable to mesophilic ones as a component in lyophilized RPA reagents., (Copyright © 2024 The Society for Biotechnology, Japan. Published by Elsevier B.V. All rights reserved.)

Published

2024

2. Correction: Detection of SARS-CoV-2 spike protein D614G mutation using μTGGE.

Author

Juma KM, Morimoto K, Sharma V, Sharma K, Biyani R, Biyani M, Takita T, and Yasukawa K

Published

2024

3. Increase in the solubility of uvsY using a site saturation mutagenesis library for application in a lyophilized reagent for recombinase polymerase amplification.

Author

Morimoto K, Juma KM, Yamagata M, Takita T, Kojima K, Suzuki K, Yanagihara I, Fujiwara S, and Yasukawa K

Subjects

Solubility, Gene Library, Mutagenesis, Recombinases genetics, Amino Acids

Abstract

Background: Recombinase uvsY from bacteriophage T4, along with uvsX, is a key enzyme for recombinase polymerase amplification (RPA), which is used to amplify a target DNA sequence at a constant temperature. uvsY, though essential, poses solubility challenges, complicating the lyophilization of RPA reagents. This study aimed to enhance uvsY solubility., Methods: Our hypothesis centered on the C-terminal region of uvsY influencing solubility. To test this, we generated a site-saturation mutagenesis library for amino acid residues Lys91-Glu134 of the N-terminal (His) 6 -tagged uvsY., Results: Screening 480 clones identified A116H as the variant with superior solubility. Lyophilized RPA reagents featuring the uvsY variant A116H demonstrated enhanced performance compared to those with wild-type uvsY., Conclusions: The uvsY variant A116H emerges as an appealing choice for RPA applications, offering improved solubility and heightened lyophilization feasibility., (© 2024. The Author(s).)

Published

2024

4. Detection of SARS-CoV-2 spike protein D614G mutation using μTGGE.

Author

Juma KM, Morimoto K, Sharma V, Sharma K, Biyani R, Biyani M, Takita T, and Yasukawa K

Subjects

Denaturing Gradient Gel Electrophoresis, Mutation, SARS-CoV-2 genetics, Spike Glycoprotein, Coronavirus genetics

Abstract

Background: The accurate and expeditious detection of SARS-CoV-2 mutations is critical for monitoring viral evolution, assessing its impact on transmission, virulence, and vaccine efficacy, and formulating public health interventions. In this study, a detection system utilizing micro temperature gradient gel electrophoresis (μTGGE) was developed for the identification of the D614 and G614 variants of the SARS-CoV-2 spike protein., Methods: The in vitro synthesized D614 and G614 gene fragments of the SARS-CoV-2 spike protein were amplified via polymerase chain reaction and subjected to μTGGE analysis., Results: The migration patterns exhibited by the D614 and G614 variants on the polyacrylamide gel were distinctly dissimilar and readily discernible by μTGGE. In particular, the mid-melting pattern of D614 was shorter than that of G614., Conclusions: Our results demonstrate the capability of μTGGE for the rapid, precise, and cost-effective detection of SARS-CoV-2 spike protein D614 and G614 variants without the need for sequencing. Therefore, this approach holds considerable potential for use in point-of-care mutation assays for SARS-CoV-2 and other pathogens., (© 2024. The Author(s), under exclusive licence to Springer Nature B.V.)

Published

2024

5. Application of recombinant human pyruvate kinase in recombinase polymerase amplification.

Author

Kojima K, Morimoto K, Juma KM, Takita T, Saito K, Yanagihara I, Fujiwara S, and Yasukawa K

Abstract

Recombinase polymerase amplification (RPA) is an isothermal DNA amplification reaction at around 41°C using recombinase (Rec), single-stranded DNA-binding protein (SSB), strand-displacing DNA polymerase (Pol), and an ATP-regenerating enzyme. In this study, we attempted to use pyruvate kinase instead of creatine kinase (CK) that has been consistently used as an ATP-regenerating enzyme in RPA. Human pyruvate kinase M1 (PKM) was expressed in Escherichia coli and purified from the cells. RPA with PKM was performed at 41°C with the in vitro synthesized urease subunit β (ureB) DNA from Ureaplasma parvum serovar 3 as a standard DNA. The optimal concentrations of PKM and phosphoenolpyruvate were 20 ng/μL and 10 mM, respectively. The RPA reaction with PKM was more sensitive than that with CK. PKM exhibited higher thermostability than CK, suggesting that the RPA reagents with PKM are preferable to those with CK for onsite use., (Copyright © 2023 The Society for Biotechnology, Japan. Published by Elsevier B.V. All rights reserved.)

Published

2023

6. Recombinase polymerase amplification using novel thermostable strand-displacing DNA polymerases from Aeribacillus pallidus and Geobacillus zalihae.

Author

Juma KM, Inoue E, Asada K, Fukuda W, Morimoto K, Yamagata M, Takita T, Kojima K, Suzuki K, Nakura Y, Yanagihara I, Fujiwara S, and Yasukawa K

Subjects

DNA-Directed DNA Polymerase genetics, Nucleic Acid Amplification Techniques methods, Sensitivity and Specificity, Recombinases genetics, Recombinases metabolism, Geobacillus genetics

Abstract

Recombinase polymerase amplification (RPA) is an isothermal DNA amplification reaction at around 41 °C using recombinase (Rec), single-stranded DNA-binding protein (SSB), and strand-displacing DNA polymerase (Pol). Component instability and the need to store commercial kits in a deep freezer until use are some limitations of RPA. In a previous study, Bacillus stearothermophilus Pol (Bst-Pol) was used as a thermostable strand-displacing DNA polymerase in RPA. Here, we attempted to optimize the lyophilization conditions for RPA with newly isolated thermostable DNA polymerases for storage at room temperature. We isolated novel two thermostable strand-displacing DNA polymerases, one from a thermophilic bacterium Aeribacillus pallidus (H1) and the other from Geobacillus zalihae (C1), and evaluated their performances in RPA reaction. Urease subunit β (UreB) DNA from Ureaplasma parvum serovar 3 was used as a model target for evaluation. The RPA reaction with H1-Pol or C1-Pol was performed at 41 °C with the in vitro synthesized standard UreB DNA. The minimal initial copy numbers of standard DNA from which the amplified products were observed were 600, 600, and 6000 copies for RPA with H1-Pol, C1-Pol, and Bst-Pol, respectively. Optimization was carried out using RPA components, showing that the lyophilized RPA reagents containing H1-Pol exhibited the same performance as the corresponding liquid RPA reagents. In addition, lyophilized RPA reagents with H1-Pol showed almost the same activity after two weeks of storage at room temperature as the freshly prepared liquid RPA reagents. These results suggest that lyophilized RPA reagents with H1-Pol are preferable to liquid RPA reagents for onsite use., (Copyright © 2023 The Society for Biotechnology, Japan. Published by Elsevier B.V. All rights reserved.)

Published

2023

7. Modified uvsY by N-terminal hexahistidine tag addition enhances efficiency of recombinase polymerase amplification to detect SARS-CoV-2 DNA.

Author

Juma KM, Takita T, Yamagata M, Ishitani M, Hayashi K, Kojima K, Suzuki K, Ando Y, Fukuda W, Fujiwara S, Nakura Y, Yanagihara I, and Yasukawa K

Subjects

DNA, Viral genetics, SARS-CoV-2 genetics, Bacteriophage T4 enzymology, DNA, Viral chemistry, DNA-Binding Proteins chemistry, Membrane Proteins chemistry, Nucleic Acid Amplification Techniques, SARS-CoV-2 chemistry, Viral Proteins chemistry

Abstract

Background: Recombinase (uvsY and uvsX) from bacteriophage T4 is a key enzyme for recombinase polymerase amplification (RPA) that amplifies a target DNA sequence at a constant temperature with a single-stranded DNA-binding protein and a strand-displacing polymerase. The present study was conducted to examine the effects of the N- and C-terminal tags of uvsY on its function in RPA to detect SARS-CoV-2 DNA., Methods: Untagged uvsY (uvsY-Δhis), N-terminal tagged uvsY (uvsY-Nhis), C-terminal tagged uvsY (uvsY-Chis), and N- and C-terminal tagged uvsY (uvsY-NChis) were expressed in Escherichia coli and purified. RPA reaction was carried out with the in vitro synthesized standard DNA at 41 °C. The amplified products were separated on agarose gels., Results: The minimal initial copy numbers of standard DNA from which the amplified products were observed were 6 × 10 5 , 60, 600, and 600 copies for the RPA with uvsY-Δhis, uvsY-Nhis, uvsY-Chis, and uvsY-NChis, respectively. The minimal reaction time at which the amplified products were observed were 20, 20, 30, and 20 min for the RPA with uvsY-Δhis, uvsY-Nhis, uvsY-Chis, and uvsY-NChis, respectively. The RPA with uvsY-Nhis exhibited clearer bands than that with either of other three uvsYs., Conclusions: The reaction efficiency of RPA with uvsY-Nhis was the highest, suggesting that uvsY-Nhis is suitable for use in RPA., (© 2021. The Author(s), under exclusive licence to Springer Nature B.V.)

Published

2022

8. Optimization of reaction condition of recombinase polymerase amplification to detect SARS-CoV-2 DNA and RNA using a statistical method.

Author

Juma KM, Takita T, Ito K, Yamagata M, Akagi S, Arikawa E, Kojima K, Biyani M, Fujiwara S, Nakura Y, Yanagihara I, and Yasukawa K

Subjects

DNA Primers metabolism, DNA-Binding Proteins metabolism, Membrane Proteins metabolism, SARS-CoV-2 isolation & purification, Viral Proteins metabolism, DNA, Viral analysis, DNA-Directed DNA Polymerase metabolism, Nucleic Acid Amplification Techniques methods, Nucleic Acid Amplification Techniques standards, RNA, Viral analysis, Recombinases metabolism, SARS-CoV-2 genetics, Statistics as Topic

Abstract

Recombinase polymerase amplification (RPA) is an isothermal reaction that amplifies a target DNA sequence with a recombinase, a single-stranded DNA-binding protein (SSB), and a strand-displacing DNA polymerase. In this study, we optimized the reaction conditions of RPA to detect SARS-CoV-2 DNA and RNA using a statistical method to enhance the sensitivity. In vitro synthesized SARS-CoV-2 DNA and RNA were used as targets. After evaluating the concentration of each component, the uvsY, gp32, and ATP concentrations appeared to be rate-determining factors. In particular, the balance between the binding and dissociation of uvsX and DNA primer was precisely adjusted. Under the optimized condition, 60 copies of the target DNA were specifically detected. Detection of 60 copies of RNA was also achieved. Our results prove the fabrication flexibility of RPA reagents, leading to an expansion of the use of RPA in various fields., (Copyright © 2021 Elsevier Inc. All rights reserved.)

Published

2021

9. Development of robust isothermal RNA amplification assay for lab-free testing of RNA viruses.

Author

Biyani R, Sharma K, Kojima K, Biyani M, Sharma V, Kumawat T, Juma KM, Yanagihara I, Fujiwara S, Kodama E, Takamura Y, Takagi M, Yasukawa K, and Biyani M

Subjects

COVID-19 virology, COVID-19 Nucleic Acid Testing instrumentation, COVID-19 Nucleic Acid Testing methods, Equipment Design, Humans, Limit of Detection, Nucleic Acid Amplification Techniques instrumentation, RNA Viruses isolation & purification, RNA, Viral analysis, SARS-CoV-2 isolation & purification, Saliva virology, COVID-19 diagnosis, Nucleic Acid Amplification Techniques methods, Point-of-Care Systems, RNA Viruses genetics, RNA, Viral genetics, SARS-CoV-2 genetics

Abstract

Simple tests of infectiousness that return results in minutes and directly from samples even with low viral loads could be a potential game-changer in the fight against COVID-19. Here, we describe an improved isothermal nucleic acid amplification assay, termed the RICCA (RNA Isothermal Co-assisted and Coupled Amplification) reaction, that consists of a simple one-pot format of 'sample-in and result-out' with a primary focus on the detection of low copy numbers of RNA virus directly from saliva without the need for laboratory processing. We demonstrate our assay by detecting 16S rRNA directly from E. coli cells with a sensitivity as low as 8 CFU/μL and RNA fragments from a synthetic template of SARS-CoV-2 with a sensitivity as low as 1740 copies/μL. We further demonstrate the applicability of our assay for real-time testing at the point of care by designing a closed format for paper-based lateral flow assay and detecting heat-inactivated SARS-COV-2 virus in human saliva at concentrations ranging from 28,000 to 2.8 copies/μL with a total assay time of 15-30 min., (© 2021. The Author(s).)

Published

2021

10. Solvent engineering studies on recombinase polymerase amplification.

Author

Kojima K, Juma KM, Akagi S, Hayashi K, Takita T, O'Sullivan CK, Fujiwara S, Nakura Y, Yanagihara I, and Yasukawa K

Subjects

DNA Primers genetics, Temperature, Genetic Engineering, Nucleic Acid Amplification Techniques methods, Recombinases metabolism, Solvents

Abstract

Recombinase polymerase amplification (RPA) is a technique that is used to specifically amplify a target nucleic acid sequence. Unlike the polymerase chain reaction (PCR), RPA is performed at a constant temperature between 37 and 42°C. Therefore, it can be potentially used for the onsite detection of various pathogens when combined with DNA extraction and amplicon detection techniques. In this study, we prepared recombinant recombinase and single-stranded DNA-binding protein from T4 phage and used them to examine the effects of reaction conditions and additives on the efficiency of RPA. The results revealed that the optimal pH was 7.5-8.0, optimal potassium acetate concentration was 40-80 mM, and optimal reaction temperature was 37-45°C although dimethyl sulfoxide at 5% v/v and formamide at 5% v/v inhibited the reaction. Our results suggest that RPA could be conducted using a wider range of optimal reaction conditions than those required for PCR and that RPA is highly suitable for point-of-care use., (Copyright © 2020 The Society for Biotechnology, Japan. Published by Elsevier B.V. All rights reserved.)

Published

2021