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Cloning of a Novel Feruloyl Esterase from Rumen Microbial Metagenome for Substantial Yield of Mono- and Diferulic Acids from Natural Substrates. | LitMetric

AI Article Synopsis

  • A feruloyl esterase gene named RuFae4 was isolated from rumen microbes, cloned into E. coli, and shown to effectively release ferulic acid (FA) and diferulic acid (diFA) from wheat insoluble arabinoxylan (WIA).
  • The enzyme demonstrated a significant ability to release FA (205 µg) and diFA (0.84 µg) under optimal conditions (37°C, pH 6.5) and achieved about 48.3% of the total FA in the substrate.
  • When combined with GH10 endoxylanase, RuFae4 enhanced FA and diFA yields by 17 and 10 times respectively, indicating that the GH10 enzyme played

Article Abstract

A feruloyl esterase (FAE) gene was isolated from a rumen microbial metagenome, cloned into E. coli, and expressed in active form. The enzyme (RuFae4) was classified as a Type D feruloyl esterase based on its action on synthetic substrates and ability to release diferulates. The RuFae4 alone released ferulic acid (FA) and diferulic acid (diFA) from wheat insoluble arabinoxylan (WIA) and other natural substrates. The diFA released was confirmed by mass spectrometry. A maximum of 205±5.7 µg FA and 0.84±0.1 µg diFA were released (37°C, pH 6.5, 2 hr) when a saturating amount of RuFae4 (23 nmole for 100 mg WIA) was used. These yields represent 48.3% of FA, and 6.6% of diFAs present in the WIA substrate. Addition of GH10 endoxylanase (EX) to RuFae4 both at 1 nmole concentrations increased the release of FA and diFAs by 17 and 10 fold, respectively. Addition of GH11 EX resulted in smaller increase in the amount of both FA and diFAs. Applying additive amount of the two enzymes did not lead to additive increase in the product yields, suggesting that it was primarily the GH10 enzyme contributing synergism to FA/diFA release in mixed reactions.

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Source
http://dx.doi.org/10.2174/0929866522666150428114053DOI Listing

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