4.6 Article

Methionine and S-Adenosylmethionine Regulate Monascus Pigments Biosynthesis in Monascus purpureus

Journal

FRONTIERS IN MICROBIOLOGY
Volume 13, Issue -, Pages -

Publisher

FRONTIERS MEDIA SA
DOI: 10.3389/fmicb.2022.921540

Keywords

methionine; S-adenosylmethionine; SAM synthetase; Monascus pigments; Monascus purpureus

Categories

Funding

  1. National Natural Science Foundation of China [31401669]
  2. Joint Program of Beijing Natural Science Foundation
  3. Beijing Municipal Education Commission [KZ201910011014]
  4. Support Project of High-level Teachers in Beijing Municipal Universities [IDHT20180506]
  5. Talent Training Quality Construction-First Class Professional Construction [PXM2019-014213-000010]

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The study reveals that amino acid metabolism can regulate the biosynthesis of Monascus pigments (MPs), and methionine and S-adenosylmethionine (SAM) play different roles in the regulation of MPs biosynthesis in Monascus purpureus RP2. The expression of SAM synthetase leads to an increased expression of transcriptional regulatory proteins of the MPs biosynthesis gene cluster, while the addition of SAM results in increased expression of MPs biosynthesis activators and the global regulator LaeA. These findings provide a new perspective for understanding the regulation of MPs biosynthesis in M. purpureus.
Amino acid metabolism could exert regulatory effects on Monascus pigments (MPs) biosynthesis. In this work, MPs biosynthesis regulated by methionine and S-adenosylmethionine (SAM) was investigated in Monascus purpureus RP2. The results indicated that the addition of methionine in fermentation significantly reduced MPs production by 60-70%, and it induced a higher expression of SAM synthetase Mon2A2272 and consequently led to SAM accumulation. However, the addition of SAM in fermentation promoted MPs production by a maximum of 35%, while over-expression of the gene Mon2A2272 led to a decrease in MPs yield, suggesting that SAM synthetase and SAM were likely to play different regulatory roles in MPs biosynthesis. Furthermore, the gene transcription profile indicated that SAM synthetase expression led to a higher expression of the transcriptional regulatory protein of the MPs biosynthesis gene cluster, while the addition of SAM gave rise to a higher expression of MPs biosynthesis activator and the global regulator LaeA, which probably accounted for changes in MPs production and the mycelium colony morphology of M. purpureus RP2 triggered by methionine and SAM. This work proposed a possible regulation mechanism of MPs biosynthesis by SAM metabolism from methionine. The findings provided a new perspective for a deep understanding of MPs biosynthesis regulation in M. purpureus.

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