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      Structure of the Cannabis sativa olivetol‐producing enzyme reveals cyclization plasticity in type III polyketide synthases

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          Abstract

          In the native pathway to therapeutic cannabinoid biosynthesis in Cannabis sativa, the three‐step production of a key intermediate, olivetolic acid, is catalysed by the enzymes tetraketide synthase (TKS; linear tetraketide intermediate production in two stages) and olivetolic acid cyclase (OAC; final C2 → C7 aldol condensation). In the absence of OAC, a nonenzymatic C2 → C7 decarboxylative aldol condensation of the tetraketide intermediate occurs forming olivetol. TKS is a type III polyketide synthase, and the question arises why it is unable to form olivetolic acid directly, but instead forms this unwanted side product. We determined the TKS, CoA complex structure, and performed structurally guided mutagenesis studies to identify potential residues responsible for cyclization pathway discrimination in type III polyketide synthases. Prior studies suggested an ‘aldol switch’ is necessary to allow linear tetraketide intermediate release prior to cyclization, thereby enabling subsequent olivetolic acid production by OAC. However, our studies do not support the presence of a universal or predictable ‘aldol switch’ consensus sequence. Instead, we propose the mode of ordered active site water activation between type III polyketide synthases catalysing different cyclization mechanisms is subtle and homologue‐specific. Our work indicates that subtle structural variations between homologous enzymes can have a major mechanistic impact on the catalytic outcome. This highlights the importance of embedding high‐resolution structural analysis of multiple enzyme homologues with classical site‐directed mutagenesis studies when investigating highly similar enzymes with different mechanistic pathway outcomes.

          Enzymes

          TKS, http://www.chem.qmul.ac.uk/iubmb/enzyme/EC2/3/1/206.html; OAC, http://www.chem.qmul.ac.uk/iubmb/enzyme/EC4/4/1/26.html; chalcone synthase, http://www.chem.qmul.ac.uk/iubmb/enzyme/EC2/3/1/74.html; stilbene synthase, http://www.chem.qmul.ac.uk/iubmb/enzyme/EC2/3/1/95.html; 2‐PS, http://www.chem.qmul.ac.uk/iubmb/enzyme/EC2/3/1/-.html.

          Accession numbers

          The atomic coordinates and structure factors for the crystal structure of TKS have been deposited in the Protein Data Bank with accession number http://www.rcsb.org/pdb/search/structidSearch.do?structureId=6GW3.

          Abstract

          Tetraketide synthase from Cannabis sativa is a type III polyketide synthase involved in cannabinoid production. Unlike chalcone and stilbene synthases, it cannot catalyse classical cyclization reactions to generate chalcone or stilbene acid products. Instead, it releases a linear tetraketide product that undergoes a non‐enzymatic C2→C7 decarboxylative aldol condensation to form a stilbene. In this study by Nigel Scrutton and co‐authors, structure determination and mutagenesis studies are performed to investigate mechanistic details of this Cannabis sativa tetraketide synthase.

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          The draft genome and transcriptome of Cannabis sativa

          Harm van Bakel, Jake M Stout, Atina Cote (2011)
          Background Cannabis sativa has been cultivated throughout human history as a source of fiber, oil and food, and for its medicinal and intoxicating properties. Selective breeding has produced cannabis plants for specific uses, including high-potency marijuana strains and hemp cultivars for fiber and seed production. The molecular biology underlying cannabinoid biosynthesis and other traits of interest is largely unexplored. Results We sequenced genomic DNA and RNA from the marijuana strain Purple Kush using shortread approaches. We report a draft haploid genome sequence of 534 Mb and a transcriptome of 30,000 genes. Comparison of the transcriptome of Purple Kush with that of the hemp cultivar 'Finola' revealed that many genes encoding proteins involved in cannabinoid and precursor pathways are more highly expressed in Purple Kush than in 'Finola'. The exclusive occurrence of Δ9-tetrahydrocannabinolic acid synthase in the Purple Kush transcriptome, and its replacement by cannabidiolic acid synthase in 'Finola', may explain why the psychoactive cannabinoid Δ9-tetrahydrocannabinol (THC) is produced in marijuana but not in hemp. Resequencing the hemp cultivars 'Finola' and 'USO-31' showed little difference in gene copy numbers of cannabinoid pathway enzymes. However, single nucleotide variant analysis uncovered a relatively high level of variation among four cannabis types, and supported a separation of marijuana and hemp. Conclusions The availability of the Cannabis sativa genome enables the study of a multifunctional plant that occupies a unique role in human culture. Its availability will aid the development of therapeutic marijuana strains with tailored cannabinoid profiles and provide a basis for the breeding of hemp with improved agronomic characteristics.
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            The chalcone synthase superfamily of type III polyketide synthases.

            Michael B. Austin, Joseph P. Noel (2003)
            This review covers the functionally diverse type III polyketide synthase (PKS) superfamily of plant and bacterial biosynthetic enzymes. from the discovery of chalcone synthase (CHS) in the 1970s through the end of 2001. A broader perspective is achieved by a comparison of these CHS-like enzymes to mechanistically and evolutionarily related families of enzymes, including the type I and type II PKSs, as well as the thiolases and beta-ketoacyl synthases of fatty acid metabolism. As CHS is both the most frequently occurring and best studied type III PKS, this enzyme's structure and mechanism is examined in detail. The in vivo functions and biological activities of several classes of plant natural products derived from chalcones are also discussed. Evolutionary mechanisms of type III PKS divergence are considered, as are the biological functions and activities of each of the known and functionally divergent type III PKS enzymc families (currently twelve in plants and three in bacteria). A major focus of this review is the integration of information from genetic and biochemical studies with the unique insights gained from protein X-ray crystallography and homology modeling. This structural approach has generated a number of new predictions regarding both the importance and mechanistic role of various amino acid substitutions observed among functionally diverse type III PKS enzymes.
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              BglBrick vectors and datasheets: A synthetic biology platform for gene expression

              Taek Lee, Rachel Krupa, Fuzhong Zhang (2011)
              Background As engineered biological systems become more complex, it is increasingly common to express multiple operons from different plasmids and inducible expression systems within a single host cell. Optimizing such systems often requires screening combinations of origins of replication, expression systems, and antibiotic markers. This procedure is hampered by a lack of quantitative data on how these components behave when more than one origin of replication or expression system are used simultaneously. Additionally, this process can be time consuming as it often requires the creation of new vectors or cloning into existing but disparate vectors. Results Here, we report the development and characterization of a library of expression vectors compatible with the BglBrick standard (BBF RFC 21). We have designed and constructed 96 BglBrick-compatible plasmids with a combination of replication origins, antibiotic resistance genes, and inducible promoters. These plasmids were characterized over a range of inducer concentrations, in the presence of non-cognate inducer molecules, and with several growth media, and their characteristics were documented in a standard format datasheet. A three plasmid system was used to investigate the impact of multiple origins of replication on plasmid copy number. Conclusions The standardized collection of vectors presented here allows the user to rapidly construct and test the expression of genes with various combinations of promoter strength, inducible expression system, copy number, and antibiotic resistance. The quantitative datasheets created for these vectors will increase the predictability of gene expression, especially when multiple plasmids and inducers are utilized.
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                Author and article information

                Contributors
                Nigel S. Scrutton:
                ORCID: https://orcid.org/0000-0002-4182-3500
                nigel.scrutton@manchester.ac.uk
                Journal
                Journal ID (nlm-ta): FEBS J
                Journal ID (iso-abbrev): FEBS J
                Journal ID (doi): 10.1111/(ISSN)1742-4658
                Journal ID (publisher-id): FEBS
                Title: The Febs Journal
                Publisher: John Wiley and Sons Inc. (Hoboken )
                ISSN (Print): 1742-464X
                ISSN (Electronic): 1742-4658
                Publication date (Electronic): 28 October 2019
                Publication date (Print): April 2020
                Volume: 287
                Issue: 8 ( doiID: 10.1111/febs.v287.8 )
                Pages: 1511-1524
                Affiliations
                [ 1 ] Manchester Institute of Biotechnology and School of Chemistry The University of Manchester UK
                [ 2 ] BBSRC/EPSRC Synthetic Biology Research Centre SYNBIOCHEM The University of Manchester UK
                [ 3 ] EPSRC/BBSRC Future Biomanufacturing Research Hub The University of Manchester UK
                [ 4 ]Present address: Immunocore Limited Abingdon Oxfordshire OX14 4RY UK
                Author notes
                [*] [* ] Correspondence

                N. S. Scrutton, Manchester Institute of Biotechnology and School of Chemistry, The University of Manchester, Manchester M1 7DN, UK

                Tel: +44 (0) 161 306 5152

                E‐mail: nigel.scrutton@ 123456manchester.ac.uk

                Website: http://www.mib.ac.uk

                Author information
                https://orcid.org/0000-0002-4182-3500
                Article
                Publisher ID: FEBS15089
                DOI: 10.1111/febs.15089
                PMC ID: 7217186
                PubMed ID: 31605668
                SO-VID: 0a3f9a93-80fd-45e3-ad2d-15a613d36d14
                Copyright © © 2019 The Authors. The FEBS Journal published by John Wiley & Sons Ltd on behalf of Federation of European Biochemical Societies
                License:

                This is an open access article under the terms of the http://creativecommons.org/licenses/by/4.0/ License, which permits use, distribution and reproduction in any medium, provided the original work is properly cited.

                History
                Date received : 26 July 2019
                Date revision received : 10 September 2019
                Date accepted : 09 October 2019
                Page count
                Figures: 7, Tables: 1, Pages: 14, Words: 7752
                Funding
                Funded by: Biotechnology and Biological Sciences Research Council , open-funder-registry 10.13039/501100000268;
                Award ID: BB/M017702/1
                Award ID: BB/R505894/1
                Categories
                Subject: Editor's Choice
                Subject: Editor's Choice
                Custom metadata
                source-schema-version-number 2.0
                cover-date April 2020
                details-of-publishers-convertor Converter:WILEY_ML3GV2_TO_JATSPMC version:5.8.1 mode:remove_FC converted:12.05.2020

                ScienceOpen disciplines: Molecular biology
                Keywords: cannabinoid pathway,olivetol synthase,olivetolic acid,structure‐guided mutagenesis,type iii polyketide synthase
                Data availability:
                ScienceOpen disciplines: Molecular biology
                Keywords: cannabinoid pathway, olivetol synthase, olivetolic acid, structure‐guided mutagenesis, type iii polyketide synthase

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