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Featured researches published by Jong-Shin Yoo.


Proteomics | 2008

Comparison of the extracellular proteomes of Escherichia coli B and K-12 strains during high cell density cultivation.

Xiao-Xia Xia; Mee-Jung Han; Sang Yup Lee; Jong-Shin Yoo

Escherichia coli BL21 (DE3) and W3110 strains, belonging to the family B and K‐12, respectively, have been most widely employed for recombinant protein production. During the excretory production of recombinant proteins by high cell density cultivation (HCDC) of these strains, other native E. coli proteins were also released. Thus, we analyzed the extracellular proteomes of E. coli BL21 (DE3) and W3110 during HCDC. E. coli BL21 (DE3) released more than twice the amount of protein compared with W3110 during HCDC. A total of 204 protein spots including 83 nonredundant proteins were unambiguously identified by 2‐DE and MS. Of these, 32 proteins were conserved in the two strains, while 20 and 33 strain‐specific proteins were identified for E. coli BL21 (DE3) and W3110, respectively. More than 70% of identified proteins were found to be of periplasmic origin. The outer membrane proteins, OmpA and OmpF, were most abundant. Two strains showed much different patterns in their released proteins. Also, cell density‐dependent variations in the released proteins were observed in both strains. These findings summarized as reference proteome maps will be useful for studying protein release in further detail, and provide new strategies for enhanced excretory production of recombinant proteins.


Applied and Environmental Microbiology | 2003

Engineering Escherichia coli for Increased Productivity of Serine-Rich Proteins Based on Proteome Profiling

Mee-Jung Han; Ki Jun Jeong; Jong-Shin Yoo; Sang Yup Lee

ABSTRACT Variations in proteome profiles of Escherichia coli in response to the overproduction of human leptin, a serine-rich (11.6% of total amino acids) protein, were examined by two-dimensional gel electrophoresis. The levels of heat shock proteins increased, while those of protein elongation factors, 30S ribosomal protein, and some enzymes involved in amino acid biosynthesis decreased, after leptin overproduction. Most notably, the levels of enzymes involved in the biosynthesis of serine family amino acids significantly decreased. Based on this information, we designed a strategy to enhance the leptin productivity by manipulating the cysK gene, encoding cysteine synthase A. By coexpression of the cysK gene, we were able to increase the cell growth rate by approximately twofold. Also, the specific leptin productivity could be increased by fourfold. In addition, we found that cysK coexpression can improve the production of another serine-rich protein, interleukin-12 β chain, suggesting that this strategy may be useful for the production of other serine-rich proteins as well. The approach taken in this study should be useful in designing a strategy for improving recombinant protein production.


BMC Microbiology | 2009

Transcriptome and proteome analyses of adaptive responses to methyl methanesulfonate in Escherichia coli K-12 and ada mutant strains

Jong Hwan Baek; Mee-Jung Han; Sang Yup Lee; Jong-Shin Yoo

BackgroundThe Ada-dependent adaptive response system in Escherichia coli is important for increasing resistance to alkylation damage. However, the global transcriptional and translational changes during this response have not been reported. Here we present time-dependent global gene and protein expression profiles following treatment with methyl methanesulfonate (MMS) in E. coli W3110 and its ada mutant strains.ResultsTranscriptome profiling showed that 1138 and 2177 genes were differentially expressed in response to MMS treatment in the wild-type and mutant strains, respectively. A total of 81 protein spots representing 76 nonredundant proteins differentially expressed were identified using 2-DE and LC-MS/MS. In the wild-type strain, many genes were differentially expressed upon long-exposure to MMS, due to both adaptive responses and stationary phase responses. In the ada mutant strain, the genes involved in DNA replication, recombination, modification and repair were up-regulated 0.5 h after MMS treatment, indicating its connection to the SOS and other DNA repair systems. Interestingly, expression of the genes involved in flagellar biosynthesis, chemotaxis, and two-component regulatory systems related to drug or antibiotic resistance, was found to be controlled by Ada.ConclusionThese results show in detail the regulatory components and pathways controlling adaptive response and how the related genes including the Ada regulon are expressed with this response.


Biotechnology and Bioengineering | 2003

Combined transcriptome and proteome analysis of Escherichia coli during high cell density culture

Mee-Jung Han; Sang Yup Lee; Ki Jun Jeong; Jong-Shin Yoo


Proteomics | 2006

The proteome of Mannheimia succiniciproducens, a capnophilic rumen bacterium

Jeong Wook Lee; Sang Yup Lee; Hyohak Song; Jong-Shin Yoo


2011 International Meeting of the Microbiological Society of Korea | 2011

Metabolic Evolution of Mannheimia succinicproducens for the Succinate Production and its Proteomic Characteristics.

J.W. Lee; Jong-Shin Yoo; SangYup Lee


European BioPerspectives celebrating the 25th DECHEMA annual convention of biotechnologists | 2007

The proteome of succinic acid overproducing bacterium, Mannheimia succiniciproducens

J.W. Lee; Hyohak Song; Sy Choi; Jong-Shin Yoo; SangYup Lee


Annual Meeting of Korean Society for Biotechnology and Bioengineering Symposium | 2006

A proteomic view of Mannheimia succiniciproducens, succinic acid-producing capnophilic rumen bacterium

J.W. Lee; SangYup Lee; Hyohak Song; Jong-Shin Yoo


The 62th Korean Society for Biochemistry and Molecular Biology(KSBMB) annual meeting | 2005

Proteomic Signature of a Response to Long Chain Fatty Acid in Escherichia coli and Its Application

J.W. Lee; M.J. Han; Jong-Shin Yoo; SangYup Lee


KHUPO 5th International Proteomics Conference AOHUPO Workshop/Symposium | 2005

Analysis of poly(3-Hydroxybutyrate) granule-associated proteome in recombinant Escherichia coli

M.J. Han; S.J Park; J.W. Lee; Jong-Shin Yoo; Sang Yup Lee

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Kwangjoon Jeong

Chonnam National University

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