Polyketide synthase

From Wikipedia the free encyclopedia

Polyketide synthases (PKSs) are a family of multi-domain enzymes or enzyme complexes that produce polyketides, a large class of secondary metabolites, in bacteria, fungi, plants, and a few animal lineages. The biosyntheses of polyketides share striking similarities with fatty acid biosynthesis.[1][2]

The PKS genes for a certain polyketide are usually organized in one operon or in gene clusters. Type I and type II PKSs form either large modular protein complexes or dissociable molecular assemblies; type III PKSs exist as smaller homodimeric proteins.[3][4]

Classification[edit]

Reaction mechanisms of type I, II and III PKSs. Decarboxylation of malonyl unit followed by thio-Claisen condensation. a) (cis-AT) type I PKS with acyl carrier protein (ACP), keto synthase (KS) and acyl transferase (AT) domains covalently bound to another . b) Type II PKS with KSα-KSβ heterodimer and ACP as separate proteins. c) ACP-independent Type III PKS.

PKSs can be classified into three types:

  • Type I PKSs are large, complex protein structures with multiple modules which in turn consist of several domains that are usually covalently connected to each other and fulfill different catalytic steps. The minimal composition of a type I PKS module consists of an acyltransferase (AT) domain, which is responsible for choosing the building block to be used, a keto synthase (KS) domain, which catalyzes the C-C bond formation and an acyl carrier protein (ACP) domain, also known as thiolation domain. The latter contains a conserved Ser residue, post-translationally modified with a phosphopantetheine at the end of which the polyketide chain is covalently bound during biosynthesis as a thioester. Moreover, multiple other optional domains can also exist within a module like ketoreductase or dehydratase domains which alter the default 1,3-dicarbonyl functionality of the installed ketide by sequential reduction to an alcohol and double bond, respectively.[5][6] These domains work together like an assembly line. This type of type I PKSs is also referred to as cis-acyltransferase polyketide synthases (cis-AT PKSs). In contrast to that, so called trans-AT PKSs evolved independently and lack AT domains in their modules. This activity is provided by free-standing AT domains instead. Moreover, they often contain uncommon domains with unique catalytic activities.[7]
  • Type II PKSs behave very similarly to type I PKS but with one key difference: Instead of one large megaenzyme, type II PKSs are separate, monofunctional enzymes. The smallest possible type II PKS consists of an ACP, as well as two heterodimeric KS units (KSα, which catalyzes the C-C bond formation and KSβ, also known as 'chain length factor' — CLF, since it can determine the carbon chain length[8]), which fulfill a similar function as the AT, KS and ACP domains in type I PKSs, even though type II PKSs are lacking a separate AT domain. Additionally, type II PKSs often work iteratively where multiple chain elongation steps are carried out by the same enzyme, similar to type III PKSs.[9][10]
  • Type III PKSs are small homodimers of 40 kDa proteins that combine all the activities from the essential type I and II PKS domains. However, in contrast to type I and II PKSs they do not require an ACP-bound substrate. Instead, they can use a free acyl-CoA substrate for chain elongation.[11][12][13] Moreover, type III PKSs contain a Cys-His-Asn catalytic triad in their active center, with the cysteine residue acting as the attacking nucleophile, whereas type I and II PKSs are characterized by a Cys-His-His catalytic triad.[14] Typical products of type III PKSs include phenolic lipids like alkylresorcinols
  • In addition to these three types of PKSs, they can be further classified as iterative or noniterative. Iterative Type I PKSs reuse domains in a cyclic fashion. Other classifications include the degree of reduction performed during the synthesis of the growing polyketide chain.
    • NR-PKSs — non-reducing PKSs, the products of which are true polyketides
    • PR-PKSs — partially reducing PKSs
    • FR-PKSs — fully reducing PKSs, the products of which are fatty acid derivatives

Modules and domains[edit]

Biosynthesis of the doxorubicin precursor, є-rhodomycinone. The polyketide synthase reactions are shown on top.

Each type I polyketide-synthase module consists of several domains with defined functions, separated by short spacer regions. The order of modules and domains of a complete polyketide-synthase is as follows (in the order N-terminus to C-terminus):

  • Starting or loading module: AT-ACP-
  • Elongation or extending modules: -KS-AT-[DH-ER-KR]-ACP-
  • Termination or releasing domain: -TE

Domains:

The polyketide chain and the starter groups are bound with their carboxy functional group to the SH groups of the ACP and the KS domain through a thioester linkage: R-C(=O)OH + HS-protein <=> R-C(=O)S-protein + H2O.

The ACP carrier domains are similar to the PCP carrier domains of nonribosomal peptide synthetases, and some proteins combine both types of modules.

Stages[edit]

The growing chain is handed over from one thiol group to the next by trans-acylations and is released at the end by hydrolysis or by cyclization (alcoholysis or aminolysis).

Starting stage:

  • The starter group, usually acetyl-CoA or its analogues, is loaded onto the ACP domain of the starter module catalyzed by the starter module's AT domain.

Elongation stages:

  • The polyketide chain is handed over from the ACP domain of the previous module to the KS domain of the current module, catalyzed by the KS domain.
  • The elongation group, usually malonyl-CoA or methylmalonyl-CoA, is loaded onto the current ACP domain catalyzed by the current AT domain.
  • The ACP-bound elongation group reacts in a Claisen condensation with the KS-bound polyketide chain under CO2 evolution, leaving a free KS domain and an ACP-bound elongated polyketide chain. The reaction takes place at the KSn-bound end of the chain, so that the chain moves out one position and the elongation group becomes the new bound group.
  • Optionally, the fragment of the polyketide chain can be altered stepwise by additional domains. The KR (keto-reductase) domain reduces the β-keto group to a β-hydroxy group, the DH (dehydratase) domain splits off H2O, resulting in the α-β-unsaturated alkene, and the ER (enoyl-reductase) domain reduces the α-β-double-bond to a single-bond. It is important to note that these modification domains actually affect the previous addition to the chain (i.e. the group added in the previous module), not the component recruited to the ACP domain of the module containing the modification domain.
  • This cycle is repeated for each elongation module.

Termination stage:

  • The TE domain hydrolyzes the completed polyketide chain from the ACP-domain of the previous module.

Pharmacological relevance[edit]

Polyketide synthases are an important source of naturally occurring small molecules used for chemotherapy.[15] For example, many of the commonly used antibiotics, such as tetracycline and macrolides, are produced by polyketide synthases. Other industrially important polyketides are sirolimus (immunosuppressant), erythromycin (antibiotic), lovastatin (anticholesterol drug), and epothilone B (anticancer drug).[16]

Polyketides are a large family of natural products widely used as drugs, pesticides, herbicides, and biological probes.[17]

There are antifungal and antibacterial polyketide compounds, namely ophiocordin and ophiosetin.[citation needed]

And are researched for the synthesis of biofuels and industrial chemicals.[18]

Ecological significance[edit]

Only about 1% of all known molecules are natural products, yet it has been recognized that almost two thirds of all drugs currently in use are at least in part derived from a natural source.[19] This bias is commonly explained with the argument that natural products have co-evolved in the environment for long time periods and have therefore been pre-selected for active structures. Polyketide synthase products include lipids with antibiotic, antifungal, antitumor, and predator-defense properties; however, many of the polyketide synthase pathways that bacteria, fungi and plants commonly use have not yet been characterized.[20][21] Methods for the detection of novel polyketide synthase pathways in the environment have therefore been developed. Molecular evidence supports the notion that many novel polyketides remain to be discovered from bacterial sources.[22][23]

See also[edit]

References[edit]

  1. ^ Khosla, C.; Gokhale, R. S.; Jacobsen, J. R.; Cane, D. E. (1999). "Tolerance and Specificity of Polyketide Synthases". Annual Review of Biochemistry. 68: 219–253. doi:10.1146/annurev.biochem.68.1.219. PMID 10872449.
  2. ^ Jenke-Kodama, H.; Sandmann, A.; Müller, R.; Dittmann, E. (2005). "Evolutionary Implications of Bacterial Polyketide Synthases". Molecular Biology and Evolution. 22 (10): 2027–2039. doi:10.1093/molbev/msi193. PMID 15958783.
  3. ^ Weng, Jing-Ke; Noel, Joseph P. (2012). "Structure–Function Analyses of Plant Type III Polyketide Synthases". Natural Product Biosynthesis by Microorganisms and Plants, Part A. Methods in Enzymology. Vol. 515. pp. 317–335. doi:10.1016/B978-0-12-394290-6.00014-8. ISBN 978-0-12-394290-6. PMID 22999180.
  4. ^ Pfeifer, Blaine A.; Khosla, Chaitan (March 2001). "Biosynthesis of Polyketides in Heterologous Hosts". Microbiology and Molecular Biology Reviews. 65 (1): 106–118. doi:10.1128/MMBR.65.1.106-118.2001. PMC 99020. PMID 11238987.
  5. ^ Sattely, Elizabeth S.; Fischbach, Michael A.; Walsh, Christopher T. (2008). "Total biosynthesis: in vitro reconstitution of polyketide and nonribosomal peptide pathways". Natural Product Reports. 25 (4): 757–793. doi:10.1039/b801747f. PMID 18663394.
  6. ^ Weissman, Kira J. (2020). "Bacterial Type I Polyketide Synthases". Comprehensive Natural Products III: 4–46. doi:10.1016/b978-0-12-409547-2.14644-x. ISBN 9780081026915. S2CID 201202295.
  7. ^ Helfrich, Eric J. N.; Piel, Jörn (2016). "Biosynthesis of polyketides by trans-AT polyketide synthases". Natural Product Reports. 33 (2): 231–316. doi:10.1039/c5np00125k. PMID 26689670.
  8. ^ "The polyketide metabolites". General Pharmacology: The Vascular System. 23 (6): 1228. November 1992. doi:10.1016/0306-3623(92)90327-g.
  9. ^ Hertweck, Christian; Luzhetskyy, Andriy; Rebets, Yuri; Bechthold, Andreas (2007). "Type II polyketide synthases: gaining a deeper insight into enzymatic teamwork". Nat. Prod. Rep. 24 (1): 162–190. doi:10.1039/B507395M. PMID 17268612.
  10. ^ Sattely, Elizabeth S.; Fischbach, Michael A.; Walsh, Christopher T. (2008). "Total biosynthesis: in vitro reconstitution of polyketide and nonribosomal peptide pathways". Natural Product Reports. 25 (4): 757–793. doi:10.1039/b801747f. PMID 18663394.
  11. ^ Abe, Ikuro; Morita, Hiroyuki (2010). "Structure and function of the chalcone synthase superfamily of plant type III polyketide synthases". Natural Product Reports. 27 (6): 809–838. doi:10.1039/b909988n. PMID 20358127.
  12. ^ Shen, B (April 2003). "Polyketide biosynthesis beyond the type I, II and III polyketide synthase paradigms". Current Opinion in Chemical Biology. 7 (2): 285–295. doi:10.1016/S1367-5931(03)00020-6. PMID 12714063.
  13. ^ Wong, Chin Piow; Morita, Hiroyuki (2020). "Bacterial Type III Polyketide Synthases". Comprehensive Natural Products III: 250–265. doi:10.1016/b978-0-12-409547-2.14640-2. ISBN 9780081026915. S2CID 195410516.
  14. ^ Shimizu, Yugo; Ogata, Hiroyuki; Goto, Susumu (3 January 2017). "Type III Polyketide Synthases: Functional Classification and Phylogenomics". ChemBioChem. 18 (1): 50–65. doi:10.1002/cbic.201600522. PMID 27862822. S2CID 45980356.
  15. ^ Koehn, F. E.; Carter, G. T. (2005). "The evolving role of natural products in drug discovery". Nature Reviews Drug Discovery. 4 (3): 206–220. doi:10.1038/nrd1657. PMID 15729362. S2CID 32749678.
  16. ^ Wawrik, B.; Kerkhof, L.; Zylstra, G. J.; Kukor, J. J. (2005). "Identification of Unique Type II Polyketide Synthase Genes in Soil". Applied and Environmental Microbiology. 71 (5): 2232–2238. Bibcode:2005ApEnM..71.2232W. doi:10.1128/AEM.71.5.2232-2238.2005. PMC 1087561. PMID 15870305.
  17. ^ Pankewitz, Florian; Hilker, Monika (May 2008). "Polyketides in insects: ecological role of these widespread chemicals and evolutionary aspects of their biogenesis". Biological Reviews. 83 (2): 209–226. doi:10.1111/j.1469-185X.2008.00040.x. PMID 18410406. S2CID 27702684.
  18. ^ Cai, Wenlong; Zhang, Wenjun (1 April 2018). "Engineering modular polyketide synthases for production of biofuels and industrial chemicals". Current Opinion in Biotechnology. 50: 32–38. doi:10.1016/j.copbio.2017.08.017. PMC 5862724. PMID 28946011.
  19. ^ Von Nussbaum, F.; Brands, M.; Hinzen, B.; Weigand, S.; Häbich, D. (2006). "Antibacterial Natural Products in Medicinal Chemistry—Exodus or Revival?". Angewandte Chemie International Edition. 45 (31): 5072–5129. doi:10.1002/anie.200600350. PMID 16881035.
  20. ^ Castoe, T. A.; Stephens, T.; Noonan, B. P.; Calestani, C. (2007). "A novel group of type I polyketide synthases (PKS) in animals and the complex phylogenomics of PKSs". Gene. 392 (1–2): 47–58. doi:10.1016/j.gene.2006.11.005. PMID 17207587.
  21. ^ Ridley, C. P.; Lee, H. Y.; Khosla, C. (2008). "Chemical Ecology Special Feature: Evolution of polyketide synthases in bacteria". Proceedings of the National Academy of Sciences. 105 (12): 4595–4600. Bibcode:2008PNAS..105.4595R. doi:10.1073/pnas.0710107105. PMC 2290765. PMID 18250311.
  22. ^ Metsä-Ketelä, M.; Salo, V.; Halo, L.; Hautala, A.; Hakala, J.; Mäntsälä, P.; Ylihonko, K. (1999). "An efficient approach for screening minimal PKS genes from Streptomyces". FEMS Microbiology Letters. 180 (1): 1–6. doi:10.1016/S0378-1097(99)00453-X (inactive 2024-03-07). PMID 10547437.{{cite journal}}: CS1 maint: DOI inactive as of March 2024 (link)
  23. ^ Wawrik, B.; Kutliev, D.; Abdivasievna, U. A.; Kukor, J. J.; Zylstra, G. J.; Kerkhof, L. (2007). "Biogeography of Actinomycete Communities and Type II Polyketide Synthase Genes in Soils Collected in New Jersey and Central Asia". Applied and Environmental Microbiology. 73 (9): 2982–2989. Bibcode:2007ApEnM..73.2982W. doi:10.1128/AEM.02611-06. PMC 1892886. PMID 17337547.

External links[edit]

Retrieved from "https://en.wikipedia.org/w/index.php?title=Polyketide_synthase&oldid=1212338957"