4.7 Article

Characterization of redox state and reductase activity of protein disulfide isomerase under different redox environments using a sensitive fluorescent assay

Journal

FREE RADICAL BIOLOGY AND MEDICINE
Volume 43, Issue 1, Pages 62-70

Publisher

ELSEVIER SCIENCE INC
DOI: 10.1016/j.freeradbiomed.2007.03.025

Keywords

protein disulfide isomerase; disulfide exchange; cell surface protein disulfide isomerease; fluorescence self-quenching; redox buffer

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In this study, dicosin glutathione disulfide (Di-E-GSSG) was synthesized by the reaction of eosin isothiocyanate with GSSG. Di-E-GSSG had low fluorescence which increased similar to 70-fold on reduction of its disulfide bond. The substrate was used to monitor the disulfide reductase activity of PDI. Di-E-GSSG is the most sensitive pseudo substrate for PDI reductase activity reported to date. This probe was further used as an analytical reagent to develop an end point assay for measuring the redox state of PDI. The reduction of Di-E-GSSG by reduced enzyme was studied in the absence of reducing agents and the redox state of PDI was monitored as a function of the stoichiometric changes in the amount of eosinglutathione (EGSH) generated by the active-site dithiols of PDI. The redox state of PDI was also studied under variable [GSH]/[GSSG] ratios. The results indicate that PDI is in similar to 1/2-reduced state where the [GSHI/[GSSG] ratio is between 1: 1 and 3: 1, conditions similar to the lumen of endoplasmic reticulum or in the extracellular environment. On the other hand, [GSH]/[GSSGI ratios of >= 8: 1, such as in cytosol, all active-site thiols would be reduced. The study was extended to utilize Di-E-GSSG to investigate the effect of variable redox ratios on the platelet surface PDI reductase activity. (c) 2007 Elsevier Inc. All rights reserved.

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