Your search keyword '"Jinho Yeom"' showing total 8 results

1. Identification of a gene cluster for D-tagatose utilization in Escherichia coli B2 phylogroup

Author

Jinyoung Ha, Dohyeon Kim, Jinho Yeom, Youngshin Kim, Seung Min Yoo, and Sung Ho Yoon

Subjects

Genetics, Bacteriology, Science

Abstract

Summary: D-Tagatose is a promising low-calorie sugar-substituting sweetener in the food industry. Most ingested D-tagatose is fermented by intestinal microorganisms. Until now, Escherichia coli has been considered incapable of growing on D-tagatose. Here, we discovered a gene cluster involved in D-tagatose utilization in E. coli. The chromosome of the intestinal probiotic E. coli Nissle 1917 contains a six-gene cluster encoding the ABC transporter, D-tagatose kinase, D-tagatose-bisphosphate aldolase, and putative aldose 1-epimerase. The functionality of the gene cluster was experimentally validated. Based on single-gene deletions, D-tagatose dissimilation occurs via D-tagatose 6-phosphate to D-tagatose 1,6-bisphosphate to D-glyceraldehyde 3-phosphate plus dihydroxyacetone phosphate. Remarkably, this gene cluster was located in 93% of the completely sequenced genomes of the E. coli B2 phylogroup, which contains the majority of extraintestinal pathogenic and adherent-invasive E. coli strains prevalent in patients with inflammatory bowel disease. This highlights the importance of understanding the clinical significance of D-tagatose in microbiota alterations.

Published

2022

2. Biosensing Applications Using Nanostructure-Based Localized Surface Plasmon Resonance Sensors

Author

Dong Min Kim, Jong Seong Park, Seung-Woon Jung, Jinho Yeom, and Seung Min Yoo

Subjects

localized surface plasmon resonance, detection, nanoparticle, nanostructure, biomolecule, Chemical technology, TP1-1185

Abstract

Localized surface plasmon resonance (LSPR)-based biosensors have recently garnered increasing attention due to their potential to allow label-free, portable, low-cost, and real-time monitoring of diverse analytes. Recent developments in this technology have focused on biochemical markers in clinical and environmental settings coupled with advances in nanostructure technology. Therefore, this review focuses on the recent advances in LSPR-based biosensor technology for the detection of diverse chemicals and biomolecules. Moreover, we also provide recent examples of sensing strategies based on diverse nanostructure platforms, in addition to their advantages and limitations. Finally, this review discusses potential strategies for the development of biosensors with enhanced sensing performance.

Published

2021

3. High-throughput genetic engineering tools for regulating gene expression in a microbial cell factory

Author

Jinho Yeom, Jong Seong Park, Seung-Woon Jung, Sumin Lee, Hyukjin Kwon, and Seung Min Yoo

Subjects

General Medicine, Applied Microbiology and Biotechnology, Biotechnology

Abstract

With the rapid advances in biotechnological tools and strategies, microbial cell factory-constructing strategies have been established for the production of value-added compounds. However, optimizing the tradeoff between the biomass, yield, and titer remains a challenge in microbial production. Gene regulation is necessary to optimize and control metabolic fluxes in microorganisms for high-production performance. Various high-throughput genetic engineering tools have been developed for achieving rational gene regulation and genetic perturbation, diversifying the cellular phenotype and enhancing bioproduction performance. In this paper, we review the current high-throughput genetic engineering tools for gene regulation. In particular, technological approaches used in a diverse range of genetic tools for constructing microbial cell factories are introduced, and representative applications of these tools are presented. Finally, the prospects for high-throughput genetic engineering tools for gene regulation are discussed.

Published

2021

4. Tunable Gene Expression System Independent of Downstream Coding Sequence

Author

Seung-Woon Jung, Sang Yup Lee, Dokyun Na, Jinho Yeom, and Seung Min Yoo

Subjects

0106 biological sciences, Biochemical Phenomena, Biomedical Engineering, Gene Expression, Biology, 01 natural sciences, Biochemistry, Genetics and Molecular Biology (miscellaneous), Protein expression, Metabolic engineering, Open Reading Frames, 03 medical and health sciences, Synthetic biology, Eukaryotic translation, Downstream (manufacturing), 010608 biotechnology, Gene expression, Escherichia coli, Coding region, Gene Regulatory Networks, 030304 developmental biology, 0303 health sciences, Gene Expression Regulation, Bacterial, General Medicine, Cell biology, Metabolic Engineering, Synthetic Biology

Abstract

Fine control of the expression levels of proteins constitutes a major challenge in synthetic biology and metabolic engineering. However, the dependence of translation initiation on the downstream coding sequence (CDS) obscures accurate prediction of the protein expression levels from mRNA sequences. Here, we present a tunable gene-expression system comprising 24 expression cassettes that produce predefined relative expression levels of proteins ranging from 0.001 to 1 without being influenced by the downstream CDS. To validate the practical utility of the tunable expression system, it was applied to a synthetic circuit displaying three states of fluorescence depending on the difference in protein expression levels. To demonstrate the suitability of application to metabolic engineering, this system was used to diversify the levels of key metabolic enzymes. As a result, expression-optimized strains were capable of producing 2.25 g/L of cadaverine, 2.59 g/L of L-proline, and 95.7 mg/L of 1-propanol. Collectively, the tunable expression system could be utilized to optimize genetic circuits for desired operation and to optimize metabolic fluxes through biosynthetic pathways for enhancing production yields of bioproducts. This tunable system will be useful for studying basic and applied biological sciences in addition to applications in synthetic biology and metabolic engineering.

Published

2020

5. Synthetic fused sRNA for the simultaneous repression of multiple genes

Author

Jinho Yeom, Jong Seong Park, Yong Min Jeon, Beom Seop Song, and Seung Min Yoo

Subjects

RNA, Bacterial, Escherichia coli Proteins, Escherichia coli, RNA, Small Untranslated, General Medicine, Gene Expression Regulation, Bacterial, Host Factor 1 Protein, Applied Microbiology and Biotechnology, Biotechnology, Molecular Chaperones

Abstract

Efficient control over multiple gene expression still presents a major challenge. Synthetic sRNA enables targeted gene expression control in trans without directly modifying the chromosome, but its use to simultaneously target multiple genes can often cause cell growth defects because of the need for additional energy for transcription and lowering of their repression efficiency by limiting the amount of Hfq protein. To address these limitations, we present fusion sRNA (fsRNA) that simultaneously regulates the translation of multiple genes efficiently. It is constructed by linking the mRNA-binding modules for multiple targeted genes in one sRNA scaffold via one-pot generation using overlap extension PCR. The repression capacity of fsRNA was demonstrated by the construction of sRNAs to target four endogenous genes: caiF, hybG, ytfR and minD in Escherichia coli. Their cross-reactivity and the effect on cell growth were also investigated. As practical applications, we applied fsRNA to violacein- and protocatechuic acid-producing strains, resulting in increases of 13% violacein and 81% protocatechuic acid, respectively. The developed fsRNA-mediated multiple gene expression regulation system thus enables rapid and efficient development of optimised cell factories for valuable chemicals without cell growth defects and limiting cellular resources.Key points• Synthetic fusion sRNA (fsRNA)-based system was constructed for the repression of multiple target genes.• fsRNA repressed multiple genes by only expressing a single sRNA while minimising the cellular burden.• The application of fsRNA showed the increased production titers of violacein (13%) and protocatechuic acid (81%).

Published

2022

6. Biosensing Applications Using Nanostructure-Based Localized Surface Plasmon Resonance Sensors

Author

Jinho Yeom, Seung-Woon Jung, Jong Seong Park, Seung Min Yoo, and Dong Min Kim

Subjects

Nanostructure, Materials science, nanostructure, detection, Nanoparticle, Nanotechnology, 02 engineering and technology, Review, TP1-1185, 010402 general chemistry, 01 natural sciences, Biochemistry, Analytical Chemistry, localized surface plasmon resonance, Electrical and Electronic Engineering, Surface plasmon resonance, Instrumentation, Biochemical markers, chemistry.chemical_classification, Biomolecule, nanoparticle, Chemical technology, 021001 nanoscience & nanotechnology, Atomic and Molecular Physics, and Optics, biomolecule, 0104 chemical sciences, chemistry, 0210 nano-technology, Biosensor

Abstract

Localized surface plasmon resonance (LSPR)-based biosensors have recently garnered increasing attention due to their potential to allow label-free, portable, low-cost, and real-time monitoring of diverse analytes. Recent developments in this technology have focused on biochemical markers in clinical and environmental settings coupled with advances in nanostructure technology. Therefore, this review focuses on the recent advances in LSPR-based biosensor technology for the detection of diverse chemicals and biomolecules. Moreover, we also provide recent examples of sensing strategies based on diverse nanostructure platforms, in addition to their advantages and limitations. Finally, this review discusses potential strategies for the development of biosensors with enhanced sensing performance.

Published

2021

7. Recent advances in tuning the expression and regulation of genes for constructing microbial cell factories

Author

Jong Seong Park, Jinho Yeom, Seung Min Yoo, and Seung-Woon Jung

Subjects

0106 biological sciences, Regulation of gene expression, 0303 health sciences, Computer science, Bioengineering, 01 natural sciences, Applied Microbiology and Biotechnology, Expression (mathematics), Metabolic engineering, 03 medical and health sciences, Synthetic biology, Metabolic Engineering, 010608 biotechnology, Synthetic Biology, Biochemical engineering, Gene, 030304 developmental biology, Biotechnology

Abstract

To overcome environmental problems caused by the use of fossil resources, microbial cell factories have become a promising technique for the sustainable and eco-friendly development of valuable products from renewable resources. Constructing microbial cell factories with high titers, yields, and productivity requires a balance between growth and production; to this end, tuning gene expression and regulation is necessary to optimise and precisely control complicated metabolic fluxes. In this article, we review the current trends and advances in tuning gene expression and regulation and consider their engineering at each of the three stages of gene regulation: genomic, mRNA, and protein. In particular, the technological approaches utilised in a diverse range of genetic-engineering-based tools for the construction of microbial cell factories are reviewed and representative applications of these strategies are presented. Finally, the prospects for strategies and systems for tuning gene expression and regulation are discussed.

Published

2020

8. Nanoconfined 3D redox capacitor-based electrochemical sensor for ultrasensitive monitoring of metabolites in bacterial communication

Author

Ho Sang Jung, Dongho Kim, Jinho Yeom, Mijeong Kang, Jong Seong Park, Sung-Gyu Park, ChaeWon Mun, Seung Min Yoo, and Yeonggyu Jo

Subjects

Catechol, Metals and Alloys, High density, Condensed Matter Physics, Diagnostic monitoring, Redox, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, Electrochemical gas sensor, Chitosan, chemistry.chemical_compound, chemistry, Electrode, Materials Chemistry, Biophysics, Electrical and Electronic Engineering, Instrumentation, Redox cycling

Abstract

The ability to monitor metabolites related to cell communication is important for understanding bacterial physiology, identifying bacterial species in a cellular community, and providing insights into the stage of infection. Here, we developed a nanostructured electrochemical sensor comprising a 3D-redox-capacitor-coated electrode, which was prepared by grafting a redox capacitor molecule, catechol/o-quinone, at high density to a chitosan layer. It provided high sensitivity in detecting redox-active bacterial metabolites through a redox cycling reaction in the nanoconfined structures of the electrode. We used it to monitor the secretion of signalling-related metabolites at different growth phases of Pseudomonas aeruginosa. We also used the electrode to detect signalling-related metabolites in diverse simulated body fluids mixed with P. aeruginosa culture. It was able to provide information on bacterial communication and help in sensitive diagnostic monitoring of bacterial infection.

Published

2021