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Featured researches published by Cheng-Hsilin Hsieh.


Protein Science | 2007

Expression of proteins with dimethylarginines in Escherichia coli for protein-protein interaction studies

Cheng-Hsilin Hsieh; San-Yuan Huang; Yu-Ching Wu; Li-Fan Liu; Chau-Chung Han; Yi-Chen Liu; Ming F. Tam

Protein arginine methylation often modulates protein–protein interactions. To isolate a sufficient quantity of proteins enriched in methyl arginine(s) from natural sources for biochemical studies is laborious and difficult. We describe here an expression system that produces recombinant proteins that are enriched in ω‐NG,NG‐asymmetry dimethylarginines. A yeast type I arginine methyltransferase gene (HMT1) is put on a plasmid under the control of the Escherichia coli methionine aminopeptidase promoter for constitutive expression. The protein targeted for post‐translational modification is put on the same plasmid behind a T7 promoter for inducible expression of His6‐tagged proteins. Sbp1p and Stm1p were used as model proteins to examine this expression system. The 13 arginines within the arginine‐glycine‐rich motif of Sbp1p and the RGG sequence near the C terminus of Stm1p were methylated. Unexpectedly, the arginine residue on the thrombin cleavage site (LVPRGS) of the fusion proteins can also be methylated by Hmt1p. Sbp1p and Sbp1p/hmt1 were covalently attached to solid supports for the isolation of interacting proteins. The results indicate that arginine methylation on Sbp1p exerts both positive and negative effects on protein–protein interaction.


Biochemical Journal | 1997

Mass spectrometric analysis of rat ovary and testis cytosolic glutathione S-transferases (GSTs): identification of a novel class-Alpha GST, rGSTA6*, in rat testis

Cheng-Hsilin Hsieh; Shu-Ping Tsai; Horng-I Yeh; Tsuey-Chyi Sheu; Ming F. Tam


Rapid Communications in Mass Spectrometry | 2006

Matrix‐assisted laser desorption/ionization of peptides on AnchorChip™ targets with α‐cyano‐4‐hydroxycinnamic acid and nitrocellulose as matrix

Yu-Ching Wu; Cheng-Hsilin Hsieh; Ming F. Tam


Biochemical Journal | 1995

Mass spectrometric analysis of rat liver cytosolic glutathione S-transferases: modifications are limited to N-terminal processing.

Horng-I Yeh; Cheng-Hsilin Hsieh; Lian-Yung Wang; Shu-Ping Tsai; Hsiu-Ya Hsu; Ming F. Tam


Journal of Molecular Biology | 2000

Tyr115, gln165 and trp209 contribute to the 1, 2-epoxy-3-(p-nitrophenoxy)propane-conjugating activity of glutathione S-transferase cGSTM1-1.

Ming-Kai Chern; Tien-Chung Wu; Cheng-Hsilin Hsieh; Chia-Cheng Chou; Li-Fan Liu; I-Ching Kuan; Yi-Hong Yeh; Chwan-Deng Hsiao; Ming F. Tam


Biochemical Journal | 1999

Characterization and cloning of avian-hepatic glutathione S-transferases.

Cheng-Hsilin Hsieh; Li-Fan Liu; Shu-Ping Tsai; Ming F. Tam


Analytical Biochemistry | 2004

Escherichia coli methionine aminopeptidase with Tyr168 to alanine substitution can improve the N-terminal processing of recombinant proteins with valine at the penultimate position

Li-Fan Liu; Cheng-Hsilin Hsieh; Pei-Fen Liu; Shu-Ping Tsai; Ming F. Tam


Biochemical Journal | 1998

Amino acid sequence of glutathione S-transferase rGSTM5* from rat testis.

Ming F. Tam; Cheng-Hsilin Hsieh; Shu-Ping Tsai; Tsuey-Chyi S. Tam


Biochemical Journal | 1996

Rat kidney glutathione S-transferase 1 subunits have C-terminal truncations

Horng-I Yeh; Jing-Yu Lee; Shu-Ping Tsai; Cheng-Hsilin Hsieh; Ming F. Tam


Biochemical Journal | 1994

Modification of glutathione S-transferase 3-3 mutants with 2-(S-glutathionyl)-3,5,6-trichloro-1,4-benzoquinone. Identification of the C-terminal tryptic fragment as part of the H-site and evidence that 2-(S-glutathionyl)-3,5,6-trichloro-1,4-benzoquinone is not specific for cysteine labelling

Jeng-Liang Hong; Li-Fan Liu; Lian-Yung Wang; Shu-Ping Tsai; Cheng-Hsilin Hsieh; Chwan-Deng Hsiao; Ming F. Tam

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