EMD-5662
holo-ACP4-PikAIII/C209A/delta ACP5 (no pentaketide)
EMD-5662
Single-particle12.5 Å
Deposition: 02/05/2013Map released: 25/06/2014
Last modified: 22/10/2014
Sample Organism:
Streptomyces venezuelae
Sample: The 5th module from the pikromycin biosynthetic pathway (PikAIII) lacking the ACP domain with an N-terminal fusion to the ACP domain from module 4 of the pikromycin pathway (ACP4) - the ACP4 domain was phosphopantetheinylated
Deposition Authors: Dutta S, Whicher JR, Hansen DA
,
Hale WA,
Chemler JA,
Narayan AR,
Hakansson K ,
Sherman DH,
Smith JL,
Skiniotis G
Sample: The 5th module from the pikromycin biosynthetic pathway (PikAIII) lacking the ACP domain with an N-terminal fusion to the ACP domain from module 4 of the pikromycin pathway (ACP4) - the ACP4 domain was phosphopantetheinylated
Deposition Authors: Dutta S, Whicher JR, Hansen DA
,
Hale WA,
Chemler JA,
Narayan AR,
Hakansson K ,
Sherman DH,
Smith JL,
Skiniotis G
Structure of a modular polyketide synthase
Dutta S,
Whicher JR,
Hansen DA ,
Hale WA,
Chemler JA,
Congdon GR,
Narayan ARH,
Hakansson K ,
Sherman DH,
Smith JL,
Skiniotis G
(2014) Nature , 510 , 512 - 517
,
Hale WA,
Chemler JA,
Congdon GR,
Narayan ARH,
Hakansson K ,
Sherman DH,
Smith JL,
Skiniotis G
(2014) Nature , 510 , 512 - 517
Abstract:
Polyketide natural products constitute a broad class of compounds with diverse structural features and biological activities. Their biosynthetic machinery, represented by type I polyketide synthases (PKSs), has an architecture in which successive modules catalyse two-carbon linear extensions and keto-group processing reactions on intermediates covalently tethered to carrier domains. Here we used electron cryo-microscopy to determine sub-nanometre-resolution three-dimensional reconstructions of a full-length PKS module from the bacterium Streptomyces venezuelae that revealed an unexpectedly different architecture compared to the homologous dimeric mammalian fatty acid synthase. A single reaction chamber provides access to all catalytic sites for the intramodule carrier domain. In contrast, the carrier from the preceding module uses a separate entrance outside the reaction chamber to deliver the upstream polyketide intermediate for subsequent extension and modification. This study reveals for the first time, to our knowledge, the structural basis for both intramodule and intermodule substrate transfer in polyketide synthases, and establishes a new model for molecular dissection of these multifunctional enzyme systems.
Polyketide natural products constitute a broad class of compounds with diverse structural features and biological activities. Their biosynthetic machinery, represented by type I polyketide synthases (PKSs), has an architecture in which successive modules catalyse two-carbon linear extensions and keto-group processing reactions on intermediates covalently tethered to carrier domains. Here we used electron cryo-microscopy to determine sub-nanometre-resolution three-dimensional reconstructions of a full-length PKS module from the bacterium Streptomyces venezuelae that revealed an unexpectedly different architecture compared to the homologous dimeric mammalian fatty acid synthase. A single reaction chamber provides access to all catalytic sites for the intramodule carrier domain. In contrast, the carrier from the preceding module uses a separate entrance outside the reaction chamber to deliver the upstream polyketide intermediate for subsequent extension and modification. This study reveals for the first time, to our knowledge, the structural basis for both intramodule and intermodule substrate transfer in polyketide synthases, and establishes a new model for molecular dissection of these multifunctional enzyme systems.