Tentative identification of the second substrate binding site in Arabidopsis phytochelatin synthase

Phytochelatin synthase (PCS) uses the substrates glutathione (GSH, γGlu-Cys-Gly) and a cadmium (Cd)-bound GSH (Cd∙GS2) to produce the shortest phytochelatin product (PC2, (γGlu-Cys)2-Gly) through a ping-pong mechanism. The binding of the 2 substrates to the active site, particularly the second subst...

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Bibliographic Details
Published in:PloS one 2013-12, Vol.8 (12), p.e82675-e82675
Main Authors: Chia, Ju-Chen, Yang, Chien-Chih, Sui, Yu-Ting, Lin, Shin-Yu, Juang, Rong-Huay
Format: Article
Language:English
Subjects:
Amino acids
Aminoacyltransferases - chemistry
Aminoacyltransferases - genetics
Arabidopsis - enzymology
Arabidopsis - genetics
Arabidopsis Proteins - chemistry
Arabidopsis Proteins - genetics
Arabidopsis thaliana
Bacterial Proteins - chemistry
Bacterial Proteins - genetics
Binding Sites
Cadmium
Catalysis
Crystal structure
Crystals
Enzymatic activity
Enzyme activity
Enzymes
Glutathione
Glycine
Heavy metals
Life sciences
Mutation
Nostoc
Nostoc - enzymology
Nostoc - genetics
Phosphorylation
Phytochelatin synthase
Polypeptides
Protein Structure, Secondary
Proteins
Recognition
Structure
Studies
Substrates
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Summary:Phytochelatin synthase (PCS) uses the substrates glutathione (GSH, γGlu-Cys-Gly) and a cadmium (Cd)-bound GSH (Cd∙GS2) to produce the shortest phytochelatin product (PC2, (γGlu-Cys)2-Gly) through a ping-pong mechanism. The binding of the 2 substrates to the active site, particularly the second substrate binding site, is not well-understood. In this study, we generated a structural model of the catalytic domain of Arabidopsis AtPCS1 (residues 12-218) by using the crystal structure of the γGlu-Cys acyl-enzyme complex of the PCS of the cyanobacterium Nostoc (NsPCS) as a template. The modeled AtPCS1 revealed a cavity in proximity to the first substrate binding site, consisting of 3 loops containing several conserved amino acids including Arg152, Lys185, and Tyr55. Substitutions of these amino acids (R152K, K185R, or double mutation) resulted in the abrogation of enzyme activity, indicating that the arrangement of these 2 positive charges is crucial for the binding of the second substrate. Recombinant AtPCS1s with mutations at Tyr55 showed lower catalytic activities because of reduced affinity (3-fold for Y55W) for the Cd∙GS2, further suggesting the role of the cation-π interaction in recognition of the second substrate. Our study results indicate the mechanism for second substrate recognition in PCS. The integrated catalytic mechanism of PCS is further discussed.
ISSN:1932-6203
1932-6203
DOI:10.1371/journal.pone.0082675