A phosphopantetheinylating polyketide synthase producing a linear polyene to initiate enediyne antitumor antibiotic biosynthesis

Zhang, Jian; Lanen, Steven G. Van; Ju, Jianhua; Li, Wen; Dorrestein, Pieter C.; Li, Wenli; Kelleher, Neil L.; Shen, Ben

doi:10.1073/pnas.0711625105

Cited by 94 publications

(147 citation statements)

References 54 publications

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“…Thus, the phylogenetic divergence between 9-and 10-membered PKSEs may reflect enediyne core-specific protein-protein interactions between the PKSE and corresponding accessory enzymes. This hypothesis is consistent with our earlier observation that only the 9-membered pksE genes, but not calE8, could restore C-1027 or NCS production in pksE null mutants (15). As an important first step toward elucidating pathway-directing interactions between PKSEs and accessory enzymes, we demonstrated the production of 1 by all possible PKSE-TE combinations.…”

Section: Resultssupporting

confidence: 78%

“…S2) and expected mass of 198.1 and confirmed to be identical to the previously characterized authentic standard (15). Productions of 1 by either the 9-or 10-membered PKSE-TE systems under the conditions examined are very similar as exemplified by the estimated yields of 1 at 1.3 AE 0.5 mg∕L for CalE8-CalE7 and 2.8 AE 1.0 mg∕L for MdpE-MdpE10, respectively.…”

Section: Resultssupporting

confidence: 53%

“…The difficulties with in vitro experimental systems for PKSE studies contrast sharply with our previously reported in vivo system, in which expression of pksE-TE from either the C-1027 or NCS biosynthetic machineries in either Escherichia coli or Streptomyces consistently provided 1 as the only major product (15). The apparent advantage of in vivo methods may reflect the difficulty of reconstituting the large multifunctional PKSE megaenzyme in vitro in the absence of the mild and regenerative conditions of the cell in vivo.…”

mentioning

confidence: 49%

“…2B). For instance, we previously reported that NcsE and SgcE-the PKSEs involved in the biosynthesis of the 9-membered enediynes NCS and C-1027, respectively-produced heptaene (1) when coexpressed with their associated TEs, NcsE10 and SgcE10 (15,16). In contrast, Liang and coworkers observed methyl hexaenone (2) as the major product of the in vitro combination of CalE8 and CalE7, the PKSE-TE pair from the 10-membered enediyne CAL (17).…”

mentioning

confidence: 96%

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Polyketide synthase chemistry does not direct biosynthetic divergence between 9- and 10-membered enediynes

Horsman

Chen²,

Thorson³

et al. 2010

Proc. Natl. Acad. Sci. U.S.A.

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109

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Enediynes are potent antitumor antibiotics that are classified as 9- or 10-membered according to the size of the enediyne core structure. However, almost nothing is known about enediyne core biosynthesis, and the determinants of 9- versus 10-membered enediyne core biosynthetic divergence remain elusive. Previous work identified enediyne-specific polyketide synthases (PKSEs) that can be phylogenetically distinguished as being involved in 9- versus 10-membered enediyne biosynthesis, suggesting that biosynthetic divergence might originate from differing PKSE chemistries. Recent in vitro studies have identified several compounds produced by the PKSE and associated thioesterase (TE), but condition-dependent product profiles make it difficult to ascertain a true catalytic difference between 9- and 10-membered PKSE-TE systems. Here we report that PKSE chemistry does not direct 9- versus 10-membered enediyne core biosynthetic divergence as revealed by comparing the products from three 9-membered and two 10-membered PKSE-TE systems under identical conditions using robust in vivo assays. Three independent experiments support a common catalytic function for 9- and 10-membered PKSEs by the production of a heptaene metabolite from: ( i ) all five cognate PKSE-TE pairs in Escherichia coli ; ( ii ) the C-1027 and calicheamicin cognate PKSE-TEs in Streptomyces lividans K4-114; and ( iii ) selected native producers of both 9- and 10-membered enediynes. Furthermore, PKSEs and TEs from different 9- and 10-membered enediyne biosynthetic machineries are freely interchangeable, revealing that 9- versus 10-membered enediyne core biosynthetic divergence occurs beyond the PKSE-TE level. These findings establish a starting point for determining the origins of this biosynthetic divergence.

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Section: Resultssupporting

confidence: 78%

Section: Resultssupporting

confidence: 53%

mentioning

confidence: 49%

mentioning

confidence: 96%

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Polyketide synthase chemistry does not direct biosynthetic divergence between 9- and 10-membered enediynes

Horsman

Chen²,

Thorson³

et al. 2010

Proc. Natl. Acad. Sci. U.S.A.

Self Cite

109

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“…Comparative analysis showed that ACPS-type PPTases usually contain about 120 amino acids carrying motif P2 [(V/I)G(V/I)D] and motif P3 [(F/W)(S/C/T/)xKE(A/S)xxK] (Lambalot et al 1996), whereas the Sfp-type PPTases contain about 220 amino acids with motifs P2 and P3 plus motif P1 [PxWPxGxxGS(M/L)THCxGY] (Sanchez et al 2001). The third type of PPTases is fused with fatty acid synthases or polyketide synthases as a functional domain (Murugan and Liang 2008;Zhang et al 2008).…”

Section: Introductionmentioning

confidence: 99%

A Sfp-type phosphopantetheinyl transferase ZmsO is essential for zeamines production and the virulence of Dickeya zeae

et al. 2016

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Zeamines are family of potent antibiotics and virulence determinants produced by the rice foot rot bacterial pathogen Dickeya zeae. So zeamines are important for the pathogenesis of D. zeae and development of new strategies against this devastating disease. In this study, we show that production of zeamines is positively modulated by ZmsO, which is a conserved Sfp-type phosphopantetheinyl thransferase (PPTase) associated with post-translational activation of fatty acid synthases and polyketide synthases. Deletion of zmsO significantly abolished zeamines production and attenuated the virulence of D. zeae without affect the growth rate. The zmsO gene is located at the upstream of zmsA and zmsK in the same gene cluster. Consistent with its role in post-translational modification, deletion of zmsO did not affect the transcriptional expression of zmsA and zmsK. In trans expression of the pcpS gene from Pseudomonas aeruginosa, which encodes a Sfp-type PPTase, in the zmsO deletion mutant could also fully restore the zeamines production and bacterial virulence, establishing the important role of Sfp-type PPTase in the zeamines biosynthesis and pathogenicity of D. zeae.

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Combinatorial Biosynthesis of Pharmaceutical Natural Products

Liu

2009

Biocatalysis for the Pharmaceutical Industry

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A phosphopantetheinylating polyketide synthase producing a linear polyene to initiate enediyne antitumor antibiotic biosynthesis

Cited by 94 publications

References 54 publications

Polyketide synthase chemistry does not direct biosynthetic divergence between 9- and 10-membered enediynes

Polyketide synthase chemistry does not direct biosynthetic divergence between 9- and 10-membered enediynes

A Sfp-type phosphopantetheinyl transferase ZmsO is essential for zeamines production and the virulence of Dickeya zeae

Combinatorial Biosynthesis of Pharmaceutical Natural Products

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