In vitro kinetic study of the squalestatin tetraketide synthase dehydratase reveals the stereochemical course of a fungal highly reducing polyketide synthase

Emma Liddle; Alan Scott; Li Chen Han; David Ivison; Thomas J. Simpson; Christine L. Willis; Russell J. Cox

doi:10.1039/c6cc10172k

In vitro kinetic study of the squalestatin tetraketide synthase dehydratase reveals the stereochemical course of a fungal highly reducing polyketide synthase

Emma Liddle
, Alan Scott
, Li Chen Han
, David Ivison
, Thomas J. Simpson
, Christine L. Willis
, Russell J. Cox^*

^*Korrespondierende*r Autor*in für diese Arbeit

Institut für Organische Chemie

University of Bristol

Publikation: Beitrag in Fachzeitschrift › Artikel › Forschung › Peer-Review

Abstract

Six potential diketide substrates for the squalestatin tetraketide synthase (SQTKS) dehydratase (DH) domain were synthesised as N-acetyl cysteamine thiolesters (SNAC) and tested in kinetic assays as substrates with an isolated DH domain. 3R-3-hydroxybutyryl SNAC 3R-16 was turned over by the enzyme, but its enantiomer was not. Of the four 2-methyl substrates only 2R,3R-2-methyl-3-hydroxybutyryl SNAC 2R,3R-8 was a substrate. Combined with stereochemical information from the isolated SQTKS enoyl reductase (ER) domain, our results provide a near complete stereochemical description of the first cycle of beta-modification reactions of a fungal highly reducing polyketide synthase (HR-PKS). The results emphasise the close relationship between fungal HR-PKS and vertebrate fatty acid synthases (vFAS).

Originalsprache	Englisch
Seiten (von - bis)	1727-1730
Seitenumfang	4
Fachzeitschrift	Chemical communications
Jahrgang	53
Ausgabenummer	10
DOIs	https://doi.org/10.1039/c6cc10172k
Publikationsstatus	Veröffentlicht - 1 Jan. 2017

ASJC Scopus Sachgebiete

Katalyse
Elektronische, optische und magnetische Materialien
Keramische und Verbundwerkstoffe
Allgemeine Chemie
Oberflächen, Beschichtungen und Folien
Metalle und Legierungen
Werkstoffchemie

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10.1039/c6cc10172k

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title = "In vitro kinetic study of the squalestatin tetraketide synthase dehydratase reveals the stereochemical course of a fungal highly reducing polyketide synthase",

abstract = "Six potential diketide substrates for the squalestatin tetraketide synthase (SQTKS) dehydratase (DH) domain were synthesised as N-acetyl cysteamine thiolesters (SNAC) and tested in kinetic assays as substrates with an isolated DH domain. 3R-3-hydroxybutyryl SNAC 3R-16 was turned over by the enzyme, but its enantiomer was not. Of the four 2-methyl substrates only 2R,3R-2-methyl-3-hydroxybutyryl SNAC 2R,3R-8 was a substrate. Combined with stereochemical information from the isolated SQTKS enoyl reductase (ER) domain, our results provide a near complete stereochemical description of the first cycle of beta-modification reactions of a fungal highly reducing polyketide synthase (HR-PKS). The results emphasise the close relationship between fungal HR-PKS and vertebrate fatty acid synthases (vFAS).",

author = "Emma Liddle and Alan Scott and Han, \{Li Chen\} and David Ivison and Simpson, \{Thomas J.\} and Willis, \{Christine L.\} and Cox, \{Russell J.\}",

note = "Funding information: We thank EPSRC (EP/F066104/1) for LCMS equipment, BBSRC (BB/I003355/1) for funding AS and BrisSynBio Synthetic Biology Research Centre, (BB/L01386X/1) for funding L-CH. E. L. and D. I. were funded by the School of Chemistry, University of Bristol. We thank Dr J. E. Nettleship at the Oxford Protein Production Facility (OPPF) for assistance with protein production. Hao Yao and Oliver Piech (LUH) are thanked for technical assistance.",

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AU - Liddle, Emma

AU - Scott, Alan

AU - Han, Li Chen

AU - Ivison, David

AU - Simpson, Thomas J.

AU - Willis, Christine L.

AU - Cox, Russell J.

N1 - Funding information: We thank EPSRC (EP/F066104/1) for LCMS equipment, BBSRC (BB/I003355/1) for funding AS and BrisSynBio Synthetic Biology Research Centre, (BB/L01386X/1) for funding L-CH. E. L. and D. I. were funded by the School of Chemistry, University of Bristol. We thank Dr J. E. Nettleship at the Oxford Protein Production Facility (OPPF) for assistance with protein production. Hao Yao and Oliver Piech (LUH) are thanked for technical assistance.

PY - 2017/1/1

Y1 - 2017/1/1

N2 - Six potential diketide substrates for the squalestatin tetraketide synthase (SQTKS) dehydratase (DH) domain were synthesised as N-acetyl cysteamine thiolesters (SNAC) and tested in kinetic assays as substrates with an isolated DH domain. 3R-3-hydroxybutyryl SNAC 3R-16 was turned over by the enzyme, but its enantiomer was not. Of the four 2-methyl substrates only 2R,3R-2-methyl-3-hydroxybutyryl SNAC 2R,3R-8 was a substrate. Combined with stereochemical information from the isolated SQTKS enoyl reductase (ER) domain, our results provide a near complete stereochemical description of the first cycle of beta-modification reactions of a fungal highly reducing polyketide synthase (HR-PKS). The results emphasise the close relationship between fungal HR-PKS and vertebrate fatty acid synthases (vFAS).

AB - Six potential diketide substrates for the squalestatin tetraketide synthase (SQTKS) dehydratase (DH) domain were synthesised as N-acetyl cysteamine thiolesters (SNAC) and tested in kinetic assays as substrates with an isolated DH domain. 3R-3-hydroxybutyryl SNAC 3R-16 was turned over by the enzyme, but its enantiomer was not. Of the four 2-methyl substrates only 2R,3R-2-methyl-3-hydroxybutyryl SNAC 2R,3R-8 was a substrate. Combined with stereochemical information from the isolated SQTKS enoyl reductase (ER) domain, our results provide a near complete stereochemical description of the first cycle of beta-modification reactions of a fungal highly reducing polyketide synthase (HR-PKS). The results emphasise the close relationship between fungal HR-PKS and vertebrate fatty acid synthases (vFAS).

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