4.7 Article

Electron cryomicroscopy observation of acyl carrier protein translocation in type I fungal fatty acid synthase

Journal

SCIENTIFIC REPORTS
Volume 9, Issue -, Pages -

Publisher

NATURE PUBLISHING GROUP
DOI: 10.1038/s41598-019-49261-3

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Funding

  1. Canada Foundation for Innovation and Ontario Research Fund
  2. Princess Margaret Cancer Research Institute
  3. Princess Margaret Cancer Foundation (PMCF)
  4. Natural Sciences and Engineering Research Council of Canada (NSERC)
  5. PMCF
  6. Canada Research Chair in Microbial Genomics and Infectious Disease
  7. Canadian Institutes of Health Research Foundation [FDN-154288]

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During fatty acid biosynthesis, acyl carrier proteins (ACPs) from type I fungal fatty acid synthase (FAS) shuttle substrates and intermediates within a reaction chamber that hosts multiple spatially-fixed catalytic centers. A major challenge in understanding the mechanism of ACP-mediated substrate shuttling is experimental observation of its transient interaction landscape within the reaction chamber. Here, we have shown that ACP spatial distribution is sensitive to the presence of substrates in a catalytically inhibited state, which enables high-resolution investigation of the ACP-dependent conformational transitions within the enoyl reductase (ER) reaction site. In two fungal FASs with distinct ACP localization, the shuttling domain is targeted to the ketoacyl-synthase (KS) domain and away from other catalytic centers, such as acetyl-transferase (AT) and ER domains by steric blockage of the KS active site followed by addition of substrates. These studies strongly suggest that acylation of phosphopantetheine arm of ACP may be an integral part of the substrate shuttling mechanism in type I fungal FAS.

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