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Human peroxiredoxin 1 and 2 are not duplicate proteins - The unique presence of Cys(83) in Prx1 underscores the structural and functional differences between Prx1 and Prx2

Authors
Lee, WeonSupChoi, Kyoung-SooRiddell, JonahIp, ClementGhosh, DebashisPark, Jong-HoonPark, Young-Mee
Issue Date
Jul-2007
Publisher
AMER SOC BIOCHEMISTRY MOLECULAR BIOLOGY INC
Citation
JOURNAL OF BIOLOGICAL CHEMISTRY, v.282, no.30, pp 22011 - 22022
Pages
12
Journal Title
JOURNAL OF BIOLOGICAL CHEMISTRY
Volume
282
Number
30
Start Page
22011
End Page
22022
URI
https://scholarworks.sookmyung.ac.kr/handle/2020.sw.sookmyung/14662
DOI
10.1074/jbc.M610330200
ISSN
0021-9258
1083-351X
Abstract
Human peroxiredoxins 1 and 2, also known as Prx1 and Prx2, are more than 90% homologous in their amino acid sequences. Prx1 and Prx2 are elevated in various cancers and are shown to influence diverse cellular processes. Although their growth regulatory role has traditionally been attributed to the peroxidase activity, the physiological significance of this function is unclear because the proteins are highly susceptible to inactivation by H2O2. A chaperone activity appears to emerge when their peroxidase activity is lost. Structural studies suggest that they may form a homodimer or doughnut-shaped homodecamer. However, little information is available whether human Prx1 and Prx2 are duplicative in structure and function. We noted that Prx1 contains a cysteine (Cys(83)) at the putative dimer-dimer interface, which is absent in Prx2. We studied the role of Cys(83) in regulating the peroxidase and chaperone activities of Prx1, because the redox status of Cys(83) might influence the oligomeric structure and consequently the functions of Prx1. We show that Prx1 is more efficient as a molecular chaperone, whereas Prx2 is better suited as a peroxidase enzyme. Substituting Cys(83) with Ser(83) (Prx1C83S) results in dramatic changes in the structural and functional characteristics of Prx1 in a direction similar to those of Prx2. Here we also report the first crystal structure of human Prx1 and the presence of the Cys(83)-Cys(83) bond at the dimer-dimer interface of decameric Prx1. These findings are consistent with the hypothesis that human Prx1 and Prx2 possess unique functions and regulatory mechanisms and that Cys(83) bestows a distinctive identity to Prx1.
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