Your search keyword '"Seong Hee Bhoo"' showing total 5 results

1. Fine Mutational Analysis of 2B8 and 3H7 Tag Epitopes with Corresponding Specific Monoclonal Antibodies

Author

Kanidta Sangsawang, Man-Ho Cho, Seong Hee Bhoo, and Tae-Lim Kim

Subjects

0301 basic medicine, 030103 biophysics, medicine.drug_class, DNA Mutational Analysis, Peptide, Biology, 3H7 monoclonal antibody, Monoclonal antibody, Epitope, Article, 03 medical and health sciences, Epitopes, Mice, Bacterial Proteins, Antibody Specificity, tag, medicine, Animals, Amino Acid Sequence, 2B8 monoclonal antibody, Molecular Biology, Peptide sequence, chemistry.chemical_classification, Linear epitope, DrB-phP protein, Antibodies, Monoclonal, Cell Biology, General Medicine, Molecular biology, Amino acid, epitope mapping, 030104 developmental biology, Epitope mapping, chemistry, biology.protein, Deinococcus, Antibody

Abstract

Bacteriophytochromes are phytochrome-like light-sensing photoreceptors that use biliverdin as a chromophore. To study the biochemical properties of the Deinococcus radiodurans bacteriophytochrome (DrBphP) protein, two anti-DrBphP mouse monoclonal antibodies (2B8 and 3H7) were generated. Their specific epitopes were identified in our previous report. We present here fine epitope mapping of these two antibodies by using truncation and substitution of original epitope sequences in order to identify minimized epitope peptides. The previously reported original epitope sequences for 2B8 and 3H7 were truncated from both sides. Our analysis showed that the minimal peptide sequence lengths for 2B8 and 3H7 antibodies were nine amino acids (RDPLPFFPP) and six amino acids (PGEIEE), respectively. We further characterized these peptides in order to investigate their reactivity after single deletion and single substitution of the original peptides. We found that single-substituted 2B8 epitope (RDPLPAFPP) and dual-substituted 3H7 epitope (PGEIAD) showed significantly increased reactivity. These two antibodies with high reactivity for the short modified peptide sequences are valueble for developing new peptide tags for protein research.

Published

2015

2. Improvement of plant protein solubilization and 2-DE gel resolution through optimization of the concentration of Tris in the solubilization buffer

Author

Heeyoun Hwang, Seong Hee Bhoo, Tae-Ryong Hahn, Man-Ho Cho, and Jin-Hwan Cho

Subjects

Tris, Proteomics, Resolution (mass spectrometry), Buffer (optical fiber), Acetone, chemistry.chemical_compound, Chemical Precipitation, Electrophoresis, Gel, Two-Dimensional, Tromethamine, Molecular Biology, Plant Proteins, Chromatography, Isoelectric focusing, Osmolar Concentration, food and beverages, Oryza, Cell Biology, General Medicine, Molecular biology, chemistry, Solubility, Solubilization, Plant protein, Seedlings, Proteome

Abstract

It is important to solubilize acetone-precipitated proteins before isoelectric focusing (IEF) to achieve high resolution 2-DE gels. To resolve the maximum possible number of plant protein spots, we developed an improved solubilization buffer for plant proteins. We demonstrated that the resolution of 2-DE gels increased dramatically as the concentration of Tris-base increased, with maximum solubilization obtained at 200 mM Tris-base (Ly200T). The Ly200T buffer was more effective than the commonly used solubilization buffer containing 40 mM Tris at solubilizing acetone-precipitated plant proteins. Use of the Ly200T buffer to solubilize proteins resulted in an increase in intensity of approximately 30% of plant protein spots in the larger-than-40 kDa region of the gel. The Ly200T buffer also improved the resolution of abundant and basic proteins. Thus, the Ly200T buffer can be used to achieve greater resolution of protein spots in plant proteomics research.

Published

2009

3. Altered expression of pyrophosphate: fructose-6-phosphate 1-phosphotransferase affects the growth of transgenic Arabidopsis plants

Author

Yong-Kook Kwon, Man-Ho Cho, Jong-Seong Jeon, Seong Hee Bhoo, Tae-Ryong Hahn, and Hyemin Lim

Subjects

Transgene, Genetic Vectors, Arabidopsis, Down-Regulation, Carbohydrate metabolism, Genes, Plant, Pyrophosphate, chemistry.chemical_compound, RNA interference, Gene Expression Regulation, Plant, Gene expression, Glycolysis, Photosynthesis, Molecular Biology, biology, Reverse Transcriptase Polymerase Chain Reaction, Gene Expression Profiling, Phosphotransferases, Wild type, Cell Biology, General Medicine, biology.organism_classification, Plants, Genetically Modified, Plant Leaves, Phenotype, chemistry, Biochemistry, Carbohydrate Metabolism

Abstract

Pyrophosphate: fructose-6-phosphate 1-phosphotransferase (PFP) catalyzes the reversible interconversion of fructose-6-phosphate and fructose-1,6-bisphosphate, a key step in the regulation of the metabolic flux toward glycolysis or gluconeogenesis. To examine the role of PFP in plant growth, we have generated transgenic Arabidopsis plants that either overexpress or repress Arabidopsis PFP sub-unit genes. The overexpressing lines displayed increased PFP activity and slightly faster growth relative to wild type plants, although their photosynthetic activities and the levels of metabolites appeared not to have significantly changed. In contrast, the RNAi lines showed significantly retarded growth in parallel with the reduced PFP activity. Analysis of photosynthetic activity revealed that the growth retardation phenotype of the RNAi lines was accompanied by the reduced rates of CO(2) assimilation. Microarray analysis of our transgenic plants further revealed that the altered expression of AtPFPbeta affects the expression of several genes involved in diverse physiological processes. Our current data thus suggest that PFP is important in carbohydrate metabolism and other cellular processes.

Published

2008

4. Comparative proteomic analysis of blue light signaling components in the Arabidopsis cryptochrome 1 mutant

Author

Bong-Kwan, Phee, Sebyul, Park, Jin-Hwan, Cho, Jong-Seong, Jeon, Seong Hee, Bhoo, and Tae-Ryong, Hahn

Subjects

Cryptochromes, Proteomics, Flavoproteins, Light, Arabidopsis Proteins, Gene Expression Regulation, Plant, Mutation, Arabidopsis, Photosynthesis, Signal Transduction

Abstract

An Arabidopsis hy4 mutant that is specifically impaired in its ability to undergo blue light dependent photomorphogenesis was used to identify cryptochrome 1 signaling-related components. Proteomic analysis revealed about 205 differentially expressed protein spots in the blue light-irradiated hy4 mutant compared to the wild-type. The proteins corresponding to 28 up-regulated and 33 down-regulated spots were identified. Obvious morphological changes in the hy4 mutant were closely related to the expression of various transcription factors. Our findings suggest that blue light signals may be involved in many cellular processes including disease resistance and stress responses.

Published

2007

5. Characterization of rice mutants with enhanced susceptibility to rice blast

Author

Hye-Kyung, Kim, Sang-Kyu, Lee, Jung-Il, Cho, Sichul, Lee, Gynheung, An, Nam-Soo, Jwa, Byung-Ryun, Kim, Young-Chan, Cho, Seong-Sook, Han, Seong-Hee, Bhoo, Youn-Hyung, Lee, Yeon-Kyu, Hong, Gihwan, Yi, Dae-Sup, Park, Tae-Ryong, Hahn, and Jong-Seong, Jeon

Subjects

Genetic Markers, DNA, Plant, Mutation, Oryza, Disease Susceptibility, Phosphate-Binding Proteins, Carrier Proteins, Plants, Genetically Modified, Chromosomes, Plant, Immunity, Innate, Plant Diseases, Plant Proteins

Abstract

As a first step towards identifying genes involving in the signal transduction pathways mediating rice blast resistance, we isolated 3 mutants lines that showed enhanced susceptibility to rice blast KJ105 (91-033) from a T-DNA insertion library of the japonica rice cultivar, Hwayeong. Since none of the susceptible phenotypes co-segregated with the T-DNA insertion we adapted a map-based cloning strategy to isolate the gene(s) responsible for the enhanced susceptibility of the Hwayeong mutants. A genetic mapping population was produced by crossing the resistant wild type Hwayeong with the susceptible cultivar, Nagdong. Chi-square analysis of the F2 segregating population indicated that resistance in Hwayeong was controlled by a single major gene that we tentatively named Pi-hy. Randomly selected susceptible plants in the F2 population were used to build an initial map of Pi-hy. The SSLP marker RM2265 on chromosome 2 was closely linked to resistance. High resolution mapping using 105 F2 plants revealed that the resistance gene was tightly linked, or identical, to Pib, a resistance gene with a nucleotide binding sequence and leucine-rich repeats (NB-LRR) previously isolated. Sequence analysis of the Pib locus amplified from three susceptible mutants revealed lesions within this gene, demonstrating that the Pi-hy gene is Pib. The Pib mutations in 1D-22-10-13, 1D-54-16-8, and 1C-143-16-1 were, respectively, a missense mutation in the conserved NB domain 3, a nonsense mutation in the 5th LRR, and a nonsense mutation in the C terminus following the LRRs that causes a small deletion of the C terminus. These findings provide evidence that NB domain 3 and the C terminus are required for full activity of the plant R gene. They also suggest that alterations of the resistance gene can cause major differences in pathogen specificity by affecting interactions with an avirulence factor.

Published

2006