Characterization of a Plant S-Adenosylmethionine Synthetase from Acacia Koa

22 Pages Posted: 2 Dec 2023

See all articles by Dulal Borthakur

Dulal Borthakur

affiliation not provided to SSRN

James T. Carrillo

affiliation not provided to SSRN

Abstract

The Acacia koa S-adenosylmethionine (SAM) synthetase was identified from transcriptome data and cloned into the T7-expression vector pEt14b. Assays indicate a thermoalkaliphic enzyme which tolerates conditions up to pH 10.5, 55 °C and 3 M KCl. In vitro examples of plant SAM-synthetase activity are scarce, however this study provides supporting evidence that these extremophilic properties may actually be typical for this plant enzyme. Enzyme kinetic constants (Km = 1.44 mM, Kcat = 1.29 s-1, Vmax 170 µM. min-1) are comparable to nonplant SAM-synthetases except that substrate inhibition was not apparent at 10 mM ATP/L-methionine. Methods were explored in this study to reduce feedback inhibition, which is known to limit SAM-synthetase activity in vitro. Four single-point mutation variants of the Acacia koa SAM-synthetase were produced, each with varying degrees of reduced reaction rate, greater sensitivity to product inhibition and loss of thermophilic properties. Although an enhanced mutant was not produced, this study describes the first mutagenesis of a plant SAM-synthetase. Overcoming feedback inhibition was accomplished by the addition of organic solvent to enzyme assays. Acetonitrile, methanol or dimethylformamide, when included as 25% of the assay volume, improved total SAM production by 30-65%.

Keywords: heterologous expression, recombinant enzyme, non-aqueous activity assay, feedback inhibition, hybrid enzyme

Suggested Citation

Borthakur, Dulal and Carrillo, James T., Characterization of a Plant S-Adenosylmethionine Synthetase from Acacia Koa. Available at SSRN: https://ssrn.com/abstract=4651464 or http://dx.doi.org/10.2139/ssrn.4651464

Dulal Borthakur (Contact Author)

affiliation not provided to SSRN ( email )

No Address Available

James T. Carrillo

affiliation not provided to SSRN ( email )

No Address Available

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