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A novel assay for phosphoserine phosphatase exploiting serine acetyltransferase as the coupling enzyme

Academic Article
Publication Date:
2021
abstract:
Phosphoserine phosphatase (PSP) catalyzes the final step of de novo L-serine biosynthesis-- the hydrolysis of phosphoserine to serine and inorganic phosphate--in humans, bacteria, and plants. In published works, the reaction is typically monitored through the discontinuous malachite green phosphate assay or, more rarely, through a continuous assay that couples phosphate release to the phosphorolysis of a chromogenic nucleoside by the enzyme purine nucleoside phosphorylase (PNP). These assays suffer from numerous drawbacks, and both rely on the detection of phosphate. We describe a new continuous assay that monitors the release of serine by exploiting bacterial serine acetyltransferase (SAT) as a reporter enzyme. SAT acetylates serine, consuming acetyl-CoA and releasing CoA-SH. CoA-SH spontaneously reacts with Ellman's reagent to produce a chromophore that absorbs light at 412 nm. The catalytic parameters estimated through the SAT-coupled assay are fully consistent with those obtained with the published methods, but the new assay exhibits several advantages. Particularly, it depletes L-serine, thus allowing more prolonged linearity in the kinetics. Moreover, as the SAT-coupled assay does not rely on phosphate detection, it can be used to investigate the inhibitory effect of phosphate on PSP.
Iris type:
01.01 Articolo in rivista
Keywords:
5; 5'-dithionitrobenzoate (DTNB); Ellman's reagent; Enzymatic assay; Malachite green assay; Phosphoserine phosphatase; Serine acetyltransferase; Serine detection; Serine phosphorylated pathway
List of contributors:
Bettati, Stefano
Handle:
https://iris.cnr.it/handle/20.500.14243/401861
Published in:
LIFE
Journal
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