Your search keyword '"Lutz Heide"' showing total 126 results

1. Specific induction of secondary product formation in transgenic plant cell cultures using an inducible promoter

Author

Susanne Sommer, Andreas Bechthold, Lutz Heide, and M. Siebert

Subjects

Genetics, Nicotiana tabacum, Transgene, Plant Science, General Medicine, Biology, Secondary metabolite, biology.organism_classification, medicine.disease_cause, Molecular biology, Transformation (genetics), Cell culture, medicine, Subculture (biology), Secondary metabolism, Agronomy and Crop Science, Escherichia coli, medicine.drug

Abstract

This paper describes the artificial induction of secondary metabolite production in transgenic plant cell cultures using a recombinant, inducible plant promoter. The bacterial gene ubiC from Escherichia coli encodes the enzyme chorismate pyruvate lyase (CPL) which catalyses the conversion of chorismate to 4-hydroxybenzoate (4HB). This gene was fused to the tetracycline-inducible plant promoter Triple-Op. After transformation into Nicotiana tabacum W38 TET, transgenic cell cultures were established. Addition of chlorotetracycline to the medium led to specific induction of CPL activity. The optimal chlorotetracycline concentration was approximately 2 mg/l medium. Three to 5 h after induction, the ubiC mRNA concentration reached a maximum, while highest specific CPL activity was detected after 8 days. The artificial secondary metabolite 4HB was converted to glucosides, and their accumulation reached maximum levels after 5 weeks of subculture. The induction was reversible.

Published

2019

2. A Membrane-Bound Prenyltransferase Catalyzes the O-Prenylation of 1,6-Dihydroxyphenazine in the Marine BacteriumStreptomycessp. CNQ-509

Author

Franziska Leipoldt, Marco Steimle, Jörn Kalinowski, Philipp Zeyhle, Harald Gross, Lutz Heide, Manuela Rösch, and Judith S. Bauer

Subjects

Prenyltransferase, Phenazine, Locus (genetics), Biology, enzyme catalysis, Biochemistry, Streptomyces, Substrate Specificity, chemistry.chemical_compound, Bacterial Proteins, Prenylation, Biosynthesis, Molecular Biology, Gene, phenazine, Organic Chemistry, Dimethylallyltranstransferase, biology.organism_classification, Kinetics, Membrane protein, chemistry, Multigene Family, Biocatalysis, prenyltransferase, Phenazines, Molecular Medicine, biosynthesis

Abstract

Streptomyces sp. CNQ-509 produces the rare O-prenylated phenazines marinophenazines A and B. To identify the enzyme catalyzing the O-prenyl transfer in marinophenazine biosynthesis, we sequenced the genome of S. sp. CNQ-509. This led to the identification of two genomic loci harboring putative phenazine biosynthesis genes. The first locus contains orthologues for all seven genes involved in phenazine-1-carboxylic acid biosynthesis in pseudomonads. The second locus contains two known phenazine biosynthesis genes and a putative prenyltransferase gene termed cnqPT1. cnqPT1 codes for a membrane protein with sequence similarity to the prenyltransferase UbiA of ubiquinone biosynthesis. The enzyme CnqPT1 was identified as a 1,6-dihydroxyphenazine geranyltransferase, which catalyzes the C-O bond formation between C-1 of the geranyl moiety and O-6 of the phenazine scaffold. CnqPT1 is the first example of a prenyltransferase catalyzing O-prenyl transfer to a phenazine.

Published

2014

3. Five gene products are required for assembly of the central pyrrole moiety of coumermycin A1

Author

Jaroslav Spizek, Bertolt Gust, Lutz Heide, Jitka Novotna, and Andreas Kulik

Subjects

Adenosine Triphosphatases, Aminocoumarins, biology, Streptomyces rishiriensis, Streptomyces coelicolor, Bioengineering, Protein Serine-Threonine Kinases, biology.organism_classification, Applied Microbiology and Biotechnology, Streptomyces, Coumermycin A1, Anti-Bacterial Agents, Biochemistry, Gene cluster, Dicarboxylic Acids, Pyrroles, Heterologous expression, Threonine, Kinase activity, Gene Deletion, Plasmids, Biotechnology

Abstract

Coumermycin A1 is an aminocoumarin antibiotic produced by Streptomyces rishiriensis. It exhibits potent antibacterial and anticancer activity. The coumermycin A1 molecule contains two terminal 5-methyl-pyrrole-2-carboxylic acid moieties and one central 3-methylpyrrole-2,4-dicarboxylic acid moiety (CPM). While the biosynthesis of the terminal moieties has been elucidated in detail, the pathway leading to the CPM remains poorly understood. In this work, the minimal set of genes required for the generation of the CPM scaffold was identified. It comprises the five genes couR1, couR2a, couR2b, couR3, and couR4 which are grouped together in a contiguous 4.7 kb region within the coumermycin A1 biosynthetic gene cluster. The DNA fragment containing these genes was cloned into an expression plasmid and heterologously expressed in Streptomyces coelicolor M1146. Thereupon, the formation of CPM could be shown by HPLC and by HPLC-MS/MS, in comparison to an authentic CPM standard. This proves that the genes couR1–couR4 are sufficient to direct the biosynthesis of CPM, and that the adjacent genes couR5 and couR6 are not required for this pathway. The enzyme CouR3 was expressed in Escherichia coli and purified to near homogeneity. The protein exhibited an ATPase activity similar to that reported for its close ortholog, the threonine kinase PduX. However, we could not show a threonine kinase activity of CouR3, and; therefore, the substrate of CouR3 in CPM biosynthesis is still unknown and may be different from threonine.

Published

2013

4. Structural Basis of the Interaction of MbtH-like Proteins, Putative Regulators of Nonribosomal Peptide Biosynthesis, with Adenylating Enzymes

Author

Thilo Stehle, Björn Boll, Dominik A. Herbst, Georg Zocher, and Lutz Heide

Subjects

Models, Molecular, Molecular Sequence Data, Biology, Crystallography, X-Ray, Biochemistry, Protein Structure, Secondary, Protein structure, Bacterial Proteins, Nonribosomal peptide, Escherichia coli, medicine, heterocyclic compounds, Amino Acid Sequence, Peptide Biosynthesis, Peptide Synthases, Molecular Biology, Peptide sequence, Adenylylation, chemistry.chemical_classification, Alanine, Aspartic Acid, Tryptophan, Cell Biology, Adenosine Monophosphate, Recombinant Proteins, Enzyme structure, Anti-Bacterial Agents, Protein Structure, Tertiary, Aminoglycosides, chemistry, Multigene Family, Protein Structure and Folding, Mutation, Peptide Biosynthesis, Nucleic Acid-Independent, Streptolydigin, medicine.drug

Abstract

The biosynthesis of nonribosomally formed peptides (NRPs), which include important antibiotics such as vancomycin, requires the activation of amino acids through adenylate formation. The biosynthetic gene clusters of NRPs frequently contain genes for small, so-called MbtH-like proteins. Recently, it was discovered that these MbtH-like proteins are required for some of the adenylation reactions in NRP biosynthesis, but the mechanism of their interaction with the adenylating enzymes has remained unknown. In this study, we determined the structure of SlgN1, a 3-methylaspartate-adenylating enzyme involved in the biosynthesis of the hybrid polyketide/NRP antibiotic streptolydigin. SlgN1 contains an MbtH-like domain at its N terminus, and our analysis defines the parameters required for an interaction between MbtH-like domains and an adenylating enzyme. Highly conserved tryptophan residues of the MbtH-like domain critically contribute to this interaction. Trp-25 and Trp-35 form a cleft on the surface of the MbtH-like domain, which accommodates the alanine side chain of Ala-433 of the adenylating domain. Mutation of Ala-433 to glutamate abolished the activity of SlgN1. Mutation of Ser-23 of the MbtH-like domain to tyrosine resulted in strongly reduced activity. However, the activity of this S23Y mutant could be completely restored by addition of the intact MbtH-like protein CloY from another organism. This suggests that the interface found in the structure of SlgN1 is the genuine interface between MbtH-like proteins and adenylating enzymes.

Published

2013

5. An Artificial Pathway to 3,4-Dihydroxybenzoic Acid Allows Generation of New Aminocoumarin Antibiotic Recognized by Catechol Transporters of E. coli

Author

Silke Alt, Lutz Heide, Andreas Kulik, Nadja Burkard, and Stephanie Grond

Subjects

Operon, Mutant, Clinical Biochemistry, Receptors, Cell Surface, Streptomyces coelicolor, Corynebacterium, medicine.disease_cause, Biochemistry, chemistry.chemical_compound, Biosynthesis, Disk Diffusion Antimicrobial Tests, Gene cluster, Drug Discovery, medicine, Escherichia coli, Hydroxybenzoates, Topoisomerase II Inhibitors, Molecular Biology, Pharmacology, Clorobiocin, biology, Oxo-Acid-Lyases, General Medicine, biology.organism_classification, 4-Hydroxybenzoate-3-Monooxygenase, Anti-Bacterial Agents, chemistry, DNA Gyrase, Multigene Family, bacteria, Molecular Medicine, Heterologous expression, Novobiocin, Bacterial Outer Membrane Proteins

Abstract

SummaryAn artificial operon was synthesized, consisting of the genes for chorismate pyruvate-lyase of E. coli and for 4-hydroxybenzoate 3-hydroxylase of Corynebacterium cyclohexanicum. This operon, directing the biosynthesis of 3,4-dihdroxybenzoate, was expressed in the heterologous expression host Streptomyces coelicolor M512, together with a modified biosynthetic gene cluster for the aminocoumarin antibiotic clorobiocin. The resulting strain produced a clorobiocin derivative containing a 3,4-dihdroxybenzoyl moiety. Its structure was confirmed by MS and NMR analysis, and it was found to be a potent inhibitor of the gyrases from Escherichia coli and Staphylococcus aureus. Bioassays against different E. coli mutants suggested that this compound is actively imported by catechol siderophore transporters in the cell envelope. This study provides an example of the structure of a natural product that can be rationally modified by synthetic biology.

Published

2011

6. Identification and structural elucidation of new caprazamycins from Streptomyces sp. MK730-62F2 by liquid chromatography/electrospray ionization tandem mass spectrometry

Author

Bernd Kammerer, Lutz Heide, Bertolt Gust, Leonard Kaysser, Emmanuel Wemakor, and Stefanie Siebenberg

Subjects

Chromatography, biology, Electrospray ionization, Organic Chemistry, biology.organism_classification, Tandem mass spectrometry, Streptomyces, Analytical Chemistry, Triple quadrupole mass spectrometer, chemistry.chemical_compound, chemistry, Fragmentation (mass spectrometry), Streptomyces sp. MK730-62F2, Ionization, Spectroscopy, Boronic acid

Abstract

The development of reliable analytic methods, capable of separating mixtures of secondary metabolites as well as providing structural information, is essential for the investigation of secondary metabolites, e.g. from Streptomyces. Here we report a liquid chromatography/electrospray ionization tandem mass spectrometry (LC/ESI-MS/MS) method using a triple quadrupole mass analyzer for the structural elucidation of caprazamycins and liposidomycins from culture extracts of the wild-type producer strains. Comparison of the fragmentation patterns in positive as well as in negative ionization mode revealed several characteristic product ions used for identification of six new caprazamycins. Furthermore, a chromatographic method for the purification of nucleosides from cell cultures using a boronic acid gel was adapted for the partial purification of the culture extracts. Copyright © 2011 John Wiley & Sons, Ltd.

Published

2011

7. The biosynthetic genes for prenylated phenazines are located at two different chromosomal loci of Streptomyces cinnamonensis DSM 1042

Author

Lutz Heide, Elisa Haug-Schifferdecker, Hans-Peter Fiedler, Bertolt Gust, Katrin Flinspach, Kerstin Seeger, and Andreas Kulik

Subjects

Genetics, biology, Operon, Bioengineering, Locus (genetics), biology.organism_classification, Applied Microbiology and Biotechnology, Biochemistry, Streptomyces, Complementation, Gene cluster, Cosmid, Mevalonate pathway, Gene, Biotechnology

Abstract

Streptomyces cinnamonensis DSM 1042 produces two types of isoprenoid secondary metabolites: the prenylated naphthalene derivative furanonaphthoquinone I (FNQ I), and isoprenylated phenazines which are termed endophenazines. Previously, a 55 kb gene cluster was identified which contained genes for both FNQ I and endophenazine biosynthesis. However, several genes required for the biosynthesis of these metabolites were not present in this cluster. We now re-screened the cosmid library for genes of the mevalonate pathway and identified a separate genomic locus which contains the previously missing genes. This locus (15 kb) comprised orthologues of four phenazine biosynthesis genes known from Pseudomonas strains. Furthermore, the locus contained a putative operon of six genes of the mevalonate pathway, as well as the gene epzP which showed sequence similarity to a recently discovered class of prenyltransferases. Inactivation and complementation experiments proved the involvement of epzP in the prenylation reaction in endophenazine biosynthesis. This newly identified genomic locus is more than 40 kb distant from the previously identified cluster. The protein EpzP was expressed in Escherichia coli in form of a his-tag fusion protein and purified. The enzyme catalysed the prenylation of 5,10-dihydrophenazine-1-carboxylic acid (dihydro-PCA) using dimethylallyl diphosphate (DMAPP) as isoprenoid substrate. K(m) values were determined as 108 µM for dihydro-PCA and 25 µM for DMAPP.

Published

2010

8. Reducing the variability of antibiotic production in Streptomyces by cultivation in 24-square deepwell plates

Author

Prashant Madhusudhan Bapat, Anna Eliasson Lantz, Lutz Heide, Bertolt Gust, and Stefanie Siebenberg

Subjects

Microorganism, Cell Culture Techniques, Bioengineering, Applied Microbiology and Biotechnology, Streptomyces, law.invention, Microbiology, Laboratory flask, Bioreactors, Erlenmeyer flask, law, medicine, Food science, Mycelium, Novobiocin, biology, Streptomycetaceae, Equipment Design, biology.organism_classification, Anti-Bacterial Agents, Equipment Failure Analysis, Bacteria, Biotechnology, medicine.drug

Abstract

Highly reproducible production values of the aminocoumarin antibiotic novobiocin were achieved by cultivation of a heterologous Streptomyces producer strain in commercially available square deepwell plates consisting of 24 wells of 3 ml culture volume each. Between parallel cultivation batches in the deepwell plates, novobiocin accumulation showed standard deviations of 4–9%, compared to 39% in baffled Erlenmeyer flasks. Mycelia used as inoculum could be frozen in the presence of 20% peptone and stored at − 70 °C, allowing repeated cultivations from the same batch of inoculum over extended periods of time. Originally, novobiocin titers in the deepwell plate (5–12 mg l− 1) were lower than in Erlenmeyer flasks (24 mg l− 1). Optimization of the inoculation procedure as well as addition of a siloxylated ethylene oxide/propylene oxide copolymer, acting as oxygen carrier, to the production medium increased novobiocin production to 54 mg l− 1. The additional overexpression of the pathway-specific positive regulator gene novG increased novobiocin production to 163 mg l− 1. Harvesting the precultures in a defined section of growth phase greatly reduced variability between different batches of inoculum. The use of deepwell plates may considerably reduce the workload and cost of investigations of antibiotic biosynthesis in streptomycetes and other microorganisms due to the high reproducibility and the low requirement for shaker space and culture medium.

Published

2010

9. Transcriptional regulation of the novobiocin biosynthetic gene cluster

Author

Johannes Härle, Bertolt Gust, Lutz Heide, Christiane Wolz, Jean-Luc Pernodet, Christiane Goerke, Volker Dangel, Institut de génétique et microbiologie [Orsay] (IGM), and Université Paris-Sud - Paris 11 (UP11)-Centre National de la Recherche Scientifique (CNRS)

Subjects

Transcription, Genetic, Operon, MESH: Streptomyces, MESH: Base Sequence, DNA gyrase, MESH: Genetic Vectors, MESH: Reverse Transcriptase Polymerase Chain Reaction, Gene cluster, Promoter Regions, Genetic, MESH: Bacterial Proteins, Regulator gene, Genetics, MESH: Gene Expression Regulation, Bacterial, 0303 health sciences, Reverse Transcriptase Polymerase Chain Reaction, MESH: Novobiocin, Streptomyces, RNA, Bacterial, [SDV.MP]Life Sciences [q-bio]/Microbiology and Parasitology, Terminator (genetics), DNA Gyrase, Multigene Family, MESH: Genes, Bacterial, MESH: RNA, Bacterial, Novobiocin, MESH: DNA Gyrase, Plasmids, medicine.drug, DNA, Bacterial, Genetic Vectors, Molecular Sequence Data, Biology, Models, Biological, Microbiology, 03 medical and health sciences, Bacterial Proteins, MESH: Plasmids, MESH: Promoter Regions, Genetic, medicine, [SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology, RNA, Messenger, Gene, MESH: RNA, Messenger, 030304 developmental biology, MESH: Molecular Sequence Data, Binding Sites, Base Sequence, 030306 microbiology, MESH: Transcription, Genetic, MESH: Models, Biological, Promoter, Gene Expression Regulation, Bacterial, MESH: DNA, Bacterial, Molecular biology, MESH: Binding Sites, Genes, Bacterial, MESH: Multigene Family

Abstract

The aminocoumarin antibiotic novobiocin is a gyrase inhibitor formed by a Streptomyces strain. The biosynthetic gene cluster of novobiocin spans 23.4 kb and contains 20 coding sequences, among them the two regulatory genes novE and novG. We investigated the location of transcriptional promoters within this cluster by insertion of transcriptional terminator cassettes and RT-PCR analysis of the resulting mutants. The cluster was found to contain eight DNA regions with promoter activity. The regulatory protein NovG binds to a previously identified binding site within the promoter region located upstream of novH, but apparently not to any of the other seven promoters. Quantitative real-time PCR was used to compare the number of transcripts in a strain carrying an intact novobiocin cluster with strains carrying mutated clusters. Both in-frame deletion of the regulatory gene novG and insertion of a terminator cassette into the biosynthetic gene novH led to a strong reduction of the number of transcripts of the genes located between novH and novW. This suggested that these 16 biosynthetic genes form a single operon. Three internal promoters are located within this operon but appear to be of minor importance, if any, under our experimental conditions. Transcription of novG was found to depend on the presence of NovE, suggesting that the two regulatory genes, novE and novG, act in a cascade-like mechanism. The resistance gene gyrBR , encoding an aminocoumarin-resistant gyrase B subunit, may initially be co-transcribed with the genes from novH to novW. However, when the gyrase inhibitor novobiocin accumulates in the cultures, gyrBR is transcribed from its own promoter. Previous work has suggested that this promoter is controlled by the superhelical density of chromosomal DNA.

Published

2009

10. Genetic engineering of antibiotic biosynthesis for the generation of new aminocoumarins

Author

Lutz Heide

Subjects

Aminocoumarins, Clorobiocin, Bioengineering, General Medicine, Biology, biology.organism_classification, Applied Microbiology and Biotechnology, Streptomyces, DNA gyrase, Coumermycin A1, Anti-Bacterial Agents, Metabolic engineering, Biochemistry, Coumarins, Gene cluster, medicine, Cloning, Molecular, Genetic Engineering, Novobiocin, Biotechnology, medicine.drug

Abstract

The aminocoumarin antibiotics novobiocin, clorobiocin and coumermycin A1 are inhibitors of gyrase and highly effective antibacterial agents. Their biosynthetic gene clusters have been cloned from the respective Streptomyces producer strains, and the function of nearly all genes contained therein has been elucidated by genetic and biochemical methods. Efficient methods have been developed for the genetic manipulation and the heterologous expression of the clusters, and more than 100 new derivatives of these antibiotics have been generated by metabolic engineering, mutasynthesis and chemoenzymatic synthesis, providing a model for the power of genetic and genomic methods for the generation of new bioactive compounds.

Published

2009

11. The structure of dimethylallyl tryptophan synthase reveals a common architecture of aromatic prenyltransferases in fungi and bacteria

Author

Christoph Schall, Thilo Stehle, Ute Metzger, Shu-Ming Li, Inge A. Unsöld, Lutz Heide, Georg Zocher, and Edyta Stec

Subjects

Models, Molecular, Stereochemistry, Molecular Sequence Data, Prenyltransferase, Tryptophan synthase, Crystallography, X-Ray, Catalysis, Substrate Specificity, Fungal Proteins, chemistry.chemical_compound, Hemiterpenes, Organophosphorus Compounds, Biosynthesis, Dimethylallyltranstransferase, Catalytic Domain, Transferase, Magnesium, Amino Acid Sequence, Indole test, Fungal protein, Alkyl and Aryl Transferases, Multidisciplinary, Bacteria, Molecular Structure, Sequence Homology, Amino Acid, biology, Terpenes, Aspergillus fumigatus, Fungi, Tryptophan, Biological Sciences, Protein Structure, Tertiary, Models, Chemical, chemistry, Biochemistry, biology.protein

Abstract

Ergot alkaloids are toxins and important pharmaceuticals that are produced biotechnologically on an industrial scale. The first committed step of ergot alkaloid biosynthesis is catalyzed by dimethylallyl tryptophan synthase (DMATS; EC 2.5.1.34). Orthologs of DMATS are found in many fungal genomes. We report here the x-ray structure of DMATS, determined at a resolution of 1.76 Å. A complex of DMATS from Aspergillus fumigatus with its aromatic substrate L-tryptophan and with an analogue of its isoprenoid substrate dimethylallyl diphosphate reveals the structural basis of this enzyme-catalyzed Friedel-Crafts reaction, which shows strict regiospecificity for position 4 of the indole nucleus of tryptophan as well as unusual independence of the presence of Mg 2+ ions. The 3D structure of DMATS belongs to a rare β/α barrel fold, called prenyltransferase barrel, that was recently discovered in a small group of bacterial enzymes with no sequence similarity to DMATS. These bacterial enzymes catalyze the prenylation of aromatic substrates in the biosynthesis of secondary metabolites (i.e., a reaction similar to that of DMATS).

Published

2009

12. Aromatic Prenylation in Phenazine Biosynthesis

Author

Orwah Saleh, Hans-Peter Fiedler, Björn Boll, Bertolt Gust, and Lutz Heide

Subjects

biology, Stereochemistry, Phenazine, Pseudomonas, Prenyltransferase, Streptomyces coelicolor, Cell Biology, biology.organism_classification, Biochemistry, Streptomyces, chemistry.chemical_compound, chemistry, Gene cluster, Heterologous expression, Molecular Biology, Streptomyces anulatus

Abstract

The bacterium Streptomyces anulatus 9663, isolated from the intestine of different arthropods, produces prenylated derivatives of phenazine 1-carboxylic acid. From this organism, we have identified the prenyltransferase gene ppzP. ppzP resides in a gene cluster containing orthologs of all genes known to be involved in phenazine 1-carboxylic acid biosynthesis in Pseudomonas strains as well as genes for the six enzymes required to generate dimethylallyl diphosphate via the mevalonate pathway. This is the first complete gene cluster of a phenazine natural compound from streptomycetes. Heterologous expression of this cluster in Streptomyces coelicolor M512 resulted in the formation of prenylated derivatives of phenazine 1-carboxylic acid. After inactivation of ppzP, only nonprenylated phenazine 1-carboxylic acid was formed. Cloning, overexpression, and purification of PpzP resulted in a 37-kDa soluble protein, which was identified as a 5,10-dihydrophenazine 1-carboxylate dimethylallyltransferase, forming a C–C bond between C-1 of the isoprenoid substrate and C-9 of the aromatic substrate. In contrast to many other prenyltransferases, the reaction of PpzP is independent of the presence of magnesium or other divalent cations. The Km value for dimethylallyl diphosphate was determined as 116 μm. For dihydro-PCA, half-maximal velocity was observed at 35 μm. Kcat was calculated as 0.435 s-1. PpzP shows obvious sequence similarity to a recently discovered family of prenyltransferases with aromatic substrates, the ABBA prenyltransferases. The present finding extends the substrate range of this family, previously limited to phenolic compounds, to include also phenazine derivatives.

Published

2009

13. Prenyl transfer to aromatic substrates: genetics and enzymology

Author

Lutz Heide

Subjects

Indole test, chemistry.chemical_classification, Genetics, Indoles, Stereochemistry, Prenyltransferase, Fungi, Quinones, Plants, Biology, Dimethylallyltranstransferase, Hydrocarbons, Aromatic, Biochemistry, Prenylflavonoid, Analytical Chemistry, chemistry.chemical_compound, Enzyme, Biosynthesis, chemistry, Prenylation, Pt-barrel, Humans

Abstract

Aromatic prenyltransferases catalyze the transfer of prenyl moieties to aromatic acceptor molecules and give rise to an astounding diversity of primary and secondary metabolites in plants, fungi and bacteria. Significant progress has been made in the biochemistry and genetics of this heterogeneous group of enzymes in the past years. After 30 years of extensive research on plant prenylflavonoid biosynthesis, finally the first aromatic prenyltransferases involved in the formation of these compounds have been cloned. In bacteria, investigations of the newly discovered family of ABBA prenyltransferases revealed a novel type of protein fold, the PT barrel. In fungi, a group of closely related indole prenyltransferase was found to carry out aromatic prenylations with different substrate specificity and regiospecificity, and to catalyze both regular and reverse prenylations.

Published

2009

14. Use of a Halogenase of Hormaomycin Biosynthesis for Formation of New Clorobiocin Analogues with 5-Chloropyrrole Moieties

Author

Bertolt Gust, Lutz Heide, Jörn Piel, Bernd Kammerer, Lucia Westrich, and Christine Anderle

Subjects

Stereochemistry, Molecular Sequence Data, Mutant, Biology, Thioester, Biochemistry, Streptomyces, chemistry.chemical_compound, Biosynthesis, Depsipeptides, Moiety, Pyrroles, Cloning, Molecular, Molecular Biology, chemistry.chemical_classification, Depsipeptide, Clorobiocin, Organic Chemistry, Gene Expression Regulation, Bacterial, Sequence Analysis, DNA, biology.organism_classification, Anti-Bacterial Agents, Acyl carrier protein, chemistry, biology.protein, Molecular Medicine, Oxidoreductases, Novobiocin, Bacillus subtilis

Abstract

The depsipeptide antibiotic hormaomycin, which is produced by Streptomyces griseoflavus W-384, contains a 5-chloropyrrole moiety. In the producer strain we identified the gene hrmQ that shows sequence similarity to FADH(2)-dependent halogenases. This gene was cloned and heterologously expressed in Streptomyces roseochromogenes var. oscitans DS12.976, which is the producer of the aminocoumarin antibiotic clorobiocin, which contains a 5-methylpyrrole moiety. For the present experiment, we used a mutant of this strain in which the respective pyrrole-5-methyltransferase had been inactivated. Expression of the halogenase hrmQ in this mutant strain led to the formation of two new clorobiocin derivatives that carried a 5-chloropyrrole moiety. These compounds were isolated on a preparative scale, their structures were elucidated by (1)H NMR spectroscopy and mass spectrometry, and their antibacterial activity was determined. The substrate of HrmQ is likely to be a pyrrole-2-carboxyl-S-[acyl carrier protein] thioester. If this assumption is true, this study presents the first experiment in combinatorial biosynthesis that uses a halogenase that acts on an acyl carrier protein-bound substrate.

Published

2008

15. novE and novG act as positive regulators of novobiocin biosynthesis

Author

Bertolt Gust, Lutz Heide, Alessandra S. Eustáquio, and Volker Dangel

Subjects

DNA, Bacterial, Gene Dosage, Gene Expression, Biochemistry, Microbiology, Streptomyces, chemistry.chemical_compound, Bacterial Proteins, Biosynthesis, Gene cluster, Escherichia coli, Genetics, medicine, heterocyclic compounds, Cloning, Molecular, Molecular Biology, Novobiocin, Antibacterial agent, Regulator gene, biology, Streptomycetaceae, Gene Expression Profiling, Genetic Complementation Test, Gene Expression Regulation, Bacterial, General Medicine, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, Recombinant Proteins, Anti-Bacterial Agents, DNA-Binding Proteins, carbohydrates (lipids), Mutagenesis, Insertional, chemistry, Multigene Family, Heterologous expression, Gene Deletion, Protein Binding, medicine.drug

Abstract

The biosynthetic gene cluster of the aminocoumarin antibiotic novobiocin contains two putative regulatory genes, i.e., novE and novG. Functional proof for the role of NovG as a positive regulator of novobiocin biosynthesis had been provided previously, and we now investigated the role of novE. Heterologous expression experiments with the novobiocin biosynthetic gene cluster showed that the entire putative promoter region of novE is required to achieve optimal novobiocin production. Overexpression of novE, using a replicative vector, resulted in an increase of novobiocin formation. In contrast, inactivation of novE by in frame deletion resulted in a strong reduction of novobiocin biosynthesis. Novobiocin production could be restored by an intact copy of novE, but also by the regulatory gene novG. These observations suggest that novE is a positive regulator of novobiocin biosynthesis. NovE was expressed in E. coli and purified. However, in contrast to parallel experiments with NovG, no DNA-binding properties could be shown for NovE. RT-PCR experiments showed that expression of novG was detectable in the absence of NovE, and also that expression of novE occurred in absence of NovG.

Published

2008

16. Assembly and Heterologous Expression of the Coumermycin A1 Gene Cluster and Production of New Derivatives by Genetic Engineering

Author

Bernd Kammerer, Bertolt Gust, Lutz Heide, and Manuel Wolpert

Subjects

Aminocoumarins, Gene Expression, Heterologous, Biochemistry, Mass Spectrometry, Databases, Genetic, Gene cluster, Molecular Biology, Chromatography, High Pressure Liquid, Genetics, Clorobiocin, Molecular Structure, biology, Organic Chemistry, Streptomyces coelicolor, Methyltransferases, biology.organism_classification, Streptomyces, Coumermycin A1, Anti-Bacterial Agents, Gene Expression Regulation, Multigene Family, Methyltransferase Gene, Mutation, Cosmid, Molecular Medicine, Heterologous expression, Genetic Engineering, Bacillus subtilis

Abstract

Many secondary metabolites of clinical importance have been isolated from different Streptomyces species. As most of the natural producers remain difficult to handle genetically, heterologous expression of an entire biosynthetic gene cluster in a well characterised host allows improved possibilities for modifications of the desired compound by manipulation of the biosynthetic genes. However, the large size of a functional gene cluster often prevents its direct cloning into a single cosmid clone. Here we describe a successful strategy to assemble the entire coumermycin A1 biosynthetic gene cluster (38.6 kb) into a single cosmid clone by lambda RED recombination technology. Heterologous expression of the reconstituted gene cluster in Streptomyces coelicolor M512 resulted in the heterologous production of coumermycin A1. Inactivation of the methyltransferase gene couO--responsible for the C-methylation at the 8-positions of the aminocoumarin moieties in coumermycin A1--and heterologous expression of the modified cluster resulted in an accumulation of a C-8-unsubstituted coumermycin A1 derivative. Subsequent expression of the halogenase gene clo-hal from the clorobiocin gene cluster in the heterologous producer strain led to the formation of two new hybrid antibiotics, containing either one or two chlorine atoms. The identities of the new compounds were verified by LC-MS, and their antibacterial activities were tested against Bacillus subtilis in an agar diffusion assay.

Published

2008

17. The ABBA family of aromatic prenyltransferases: broadening natural product diversity

Author

Tomohisa Kuzuyama, Stéphane Richard, Joseph P. Noel, Lutz Heide, and M. Tello

Subjects

Models, Molecular, Protein Conformation, Stereochemistry, Prenyltransferase, Biology, Protein Engineering, Models, Biological, Article, Amino Acids, Aromatic, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Bacterial Proteins, Prenylation, Dimethylallyltranstransferase, Pt-barrel, Molecular Biology, Phylogeny, Pharmacology, chemistry.chemical_classification, Biological Products, Natural product, Biodiversity, Cell Biology, Terpenoid, Amino acid, chemistry, Biochemistry, Multigene Family, Apigenin, Molecular Medicine

Abstract

Aromatic prenyltransferases (PTases) catalyze the transfer of a C5 (dimethylallyl), C10 (geranyl) or C15 (farnesyl) prenyl group derived from the corresponding isoprenyl diphosphate metabolites onto a variety of electron-rich aromatic acceptors. Prenyl groups appear in a wide variety of bioactive natural products of microbial and plant origin, including amino acids, stilbenes, alkaloids, polyketides and phenylpropanoids such as flavonoids, creating natural product hybrids with altered or enhanced bioactivities. Prenylation of flavonoids enhances some of the desirable pharmacological properties of these plant compounds [1], as demonstrated for apigenin and liquiritigenin [2]. Prenylation appears in many cases to provide a higher level of bioactivity compared to the non-prenylated precursor, often by increasing affinity for biological membranes and interactions with cellular targets [3]. With the recent identification of these enzymes there is increased interest in the role of these regiospecific catalysts in expanding the diversity and bioactivities of several important classes of natural products in vivo and in vitro.

Published

2008

18. Biosynthesis of the Isoprenoid Moieties of Furanonaphthoquinone I and Endophenazine A in Streptomyces cinnamonensis DSM 1042

Author

T. A. M. Gulder, Yvonne Haagen, Gerhard Bringmann, Lutz Heide, and Tanja Gulder

Subjects

Magnetic Resonance Spectroscopy, Molecular Structure, biology, Terpenes, Operon, Stereochemistry, Streptomycetaceae, Organic Chemistry, Mevalonic Acid, Mevalonate kinase, biology.organism_classification, Streptomyces, chemistry.chemical_compound, Polyketide, Biosynthesis, chemistry, Biochemistry, Gene cluster, biology.protein, Phenazines, Mevalonate pathway, Chromatography, High Pressure Liquid, Naphthoquinones

Abstract

Streptomyces cinnamonensis DSM 1042 produces the polyketide-isoprenoid compound furanonaphthoquinone I (FNQ I) and isoprenylated phenazines, predominantly endophenazine A. However, the recently identified biosynthetic gene cluster for these compounds only contains a single gene for a mevalonate pathway enzyme, that is, a putative mevalonate kinase gene. This is in strong contrast to all Streptomyces strains examined so far, where all six genes encoding the mevalonate pathway enzymes are clustered in a single operon of 6.8 kb and, thus, raised the question about the biosynthetic origin of the isoprenoid moieties of FNQ I and endophenazine A. In this study, we investigated the incorporation of [13C2]acetate and [2-13C]glycerol into FNQ I and endophenazine A. The results unequivocally prove that the isoprenoid building blocks of both compounds are predominantly formed via the mevalonate pathway (approximately 80%) but that the MEP pathway (approximately 20%) contributes to the biosynthesis of these molecules, too. In actinomycetes, this is the first experimentally proven example of the utilization of both biosynthetic routes for the formation of one single secondary metabolite. The incorporation pattern of [2-13C]glycerol was consistent with a "reverse" prenyl transfer, that is, with the formation of a C-C bond from C-3 of GPP to the polyketide nucleus of FNQ I.

Published

2007

19. Effects of deletions of mbtH-like genes on clorobiocin biosynthesis in Streptomyces coelicolor

Author

Manuel Wolpert, Lutz Heide, Bernd Kammerer, and Bertolt Gust

Subjects

Molecular Sequence Data, Streptomyces coelicolor, Mycobactin, medicine.disease_cause, Microbiology, Open Reading Frames, Bacterial Proteins, Coumarins, Gene cluster, medicine, Amino Acid Sequence, Gene, Chromatography, High Pressure Liquid, Genetics, Mutation, Clorobiocin, Molecular Structure, biology, Streptomycetaceae, Genetic Complementation Test, Mycobacterium tuberculosis, biology.organism_classification, Complementation, Biochemistry, Multigene Family, Sequence Alignment, Gene Deletion, Novobiocin

Abstract

In the biosynthetic gene cluster of the aminocoumarin antibiotic clorobiocin, the small ORF cloY encodes a 71 aa protein which shows significant sequence similarity to mbtH from the mycobactin biosynthetic gene cluster of Mycobacterium tuberculosis. mbtH-like genes are frequently found in the biosynthetic gene clusters of peptide antibiotics and siderophores, but their function has remained enigmatic. In a recent publication it has been suggested that these genes may have no function for secondary metabolite biosynthesis. An in-frame deletion of cloY in the clorobiocin cluster has now been carried out. When the modified cluster was expressed in the heterologous host Streptomyces coelicolor M512, clorobiocin was still formed. However, when the two further mbtH-like genes from elsewhere in the host genome were inactivated as well, clorobiocin formation was reduced dramatically. Complementation with cloY or with any of three other mbtH-like genes restored clorobiocin formation. This is the first report proving the requirement of an mbtH-like gene for secondary metabolite formation, and the first proof that different mbtH-like genes can functionally replace each other. Feeding of an mbtH-defective triple mutant strain with an intact 3-amino-4,7-dihydroxy-coumarin moiety restored antibiotic production, showing that cloY is specifically required for the formation of this moiety of the clorobiocin molecule.

Published

2007

20. Diversity of ABBA Prenyltransferases in Marine Streptomyces sp. CNQ-509: Promiscuous Enzymes for the Biosynthesis of Mixed Terpenoid Compounds

Author

Leonard Kaysser, Lutz Heide, Jörn Kalinowski, Philipp Zeyhle, Andreas Kulik, and Franziska Leipoldt

Subjects

Prenyltransferase, lcsh:Medicine, Naphthols, Streptomyces, Mass Spectrometry, Protein Structure, Secondary, Substrate Specificity, Terpene, chemistry.chemical_compound, Biosynthesis, Dimethylallyltranstransferase, Amino Acid Sequence, Secondary metabolism, lcsh:Science, chemistry.chemical_classification, Prenylation, Multidisciplinary, biology, Molecular Structure, Terpenes, lcsh:R, biology.organism_classification, Terpenoid, Enzyme, chemistry, Biochemistry, lcsh:Q, Research Article

Abstract

Terpenoids are arguably the largest and most diverse family of natural products, featuring prominently in e.g. signalling, self-defence, UV-protection and electron transfer. Prenyltransferases are essential players in terpenoid and hybrid isoprenoid biosynthesis that install isoprene units on target molecules and thereby often modulate their bioactivity. In our search for new prenyltransferase biocatalysts we focused on the marine-derived Streptomyces sp. CNQ-509, a particularly rich source of meroterpenoid chemistry. Sequencing and analysis of the genome of Streptomyces sp. CNQ-509 revealed seven putative phenol/phenazine-specific ABBA prenyltransferases, and one putative indole-specific ABBA prenyltransferase. To elucidate the substrate specificity of the ABBA prenyltransferases and to learn about their role in secondary metabolism, CnqP1 –CnqP8 were produced in Escherichia coli and incubated with various aromatic and isoprenoid substrates. Five of the eight prenyltransferases displayed enzymatic activity. The efficient conversion of dihydroxynaphthalene derivatives by CnqP3 (encoded by AA958_24325) and the co-location of AA958_24325 with genes characteristic for the biosynthesis of THN (tetrahydroxynaphthalene)-derived natural products indicates that the enzyme is involved in the formation of debromomarinone or other naphthoquinone-derived meroterpenoids. Moreover, CnqP3 showed high flexibility towards a range of aromatic and isoprenoid substrates and thus represents an interesting new tool for biocatalytic applications.

Published

2015

21. Biosynthesis of the unusual 5,5-gem-dimethyl-deoxysugar noviose: investigation of the C-methyltransferase gene cloU

Author

Shu-Ming Li, Anja Freitag, and Lutz Heide

Subjects

Clorobiocin, biology, Stereochemistry, Streptomycetaceae, Molecular Sequence Data, Monosaccharides, Methyltransferases, biology.organism_classification, Microbiology, Streptomyces, Anti-Bacterial Agents, chemistry.chemical_compound, Biochemistry, Biosynthesis, chemistry, Methyltransferase Gene, Gene cluster, medicine, Moiety, Amino Acid Sequence, Novobiocin, medicine.drug

Abstract

The aminocoumarin antibiotic clorobiocin contains an unusual branched deoxysugar with a 5,5-gem-dimethyl structure. Inactivation of the putative C-methyltransferase gene cloU was carried out, which led to the loss of the axial methyl group at C-5 of this deoxysugar moiety. This result establishes the function of cloU, and at the same time it proves that the biosynthesis of the deoxysugar moiety of clorobiocin proceeds via a 3,5-epimerization of the dTDP-4-keto-6-deoxyglucose intermediate. The inactivation was carried out on a cosmid which contained the entire clorobiocin biosynthetic gene cluster. Expression of the modified cluster in a heterologous host led to the formation of desmethyl-clorobiocin and a structural isomer thereof. Both compounds were isolated on a preparative scale, their structures were elucidated by 1H-NMR and mass spectroscopy and their antibacterial activity was assayed.

Published

2006

22. Structure-Activity Relationships of Aminocoumarin-Type Gyrase and Topoisomerase IV Inhibitors Obtained by Combinatorial Biosynthesis

Author

Shu-Ming Li, Ruth H. Flatman, Alessandra S. Eustáquio, Lutz Heide, and Anthony Maxwell

Subjects

Aminocoumarins, DNA Topoisomerase IV, Topoisomerase IV, Stereochemistry, DNA gyrase, Acylation, Structure-Activity Relationship, chemistry.chemical_compound, Biosynthesis, medicine, Combinatorial Chemistry Techniques, Topoisomerase II Inhibitors, Pharmacology (medical), Enzyme Inhibitors, Novobiocin, Pharmacology, Clorobiocin, biology, Topoisomerase, Chemistry, Anti-Bacterial Agents, Infectious Diseases, chemistry, biology.protein, medicine.drug

Abstract

Novobiocin and clorobiocin are gyrase inhibitors produced by Streptomyces strains. Structurally, the two compounds differ only by substitution at two positions: CH 3 versus Cl at position 8′ of the aminocoumarin ring and carbamoyl versus 5-methyl-pyrrol-2-carbonyl (MePC) at the 3"-OH of noviose. Using genetic engineering, we generated a series of analogs carrying H, CH 3 , or Cl at 8′ and H, carbamoyl, or MePC at 3"-OH. Comparison of the gyrase inhibitory activities of all nine structural permutations confirmed that acylation of 3"-OH is essential for activity, with MePC being more effective than carbamoyl. Substitution at 8′ further enhanced activity, but the effect of CH 3 or Cl depended on the nature of the acyl group at 3": in the presence of carbamoyl at 3", CH 3 resulted in higher activity; in the presence of MePC at 3", Cl resulted in higher activity. This suggests that the structures of both natural compounds are highly evolved for optimal interaction with gyrase. In a second series of experiments, clorobiocin derivatives with and without the methyl group at 4"-OH of noviose, and with different positions of the MePC group of noviose, were tested. Again clorobiocin was superior to all of its analogs. The activities of all compounds were also tested against topoisomerase IV (topo IV). Clorobiocin stood out as a remarkably effective topo IV inhibitor. The relative activities of the different compounds toward topo IV showed a pattern similar to that of the relative gyrase-inhibitory activities. This is the first report of a systematic evaluation of a series of aminocoumarins against both gyrase and topo IV. The results give further insight into the structure-activity relationships of aminocoumarin antibiotics.

Published

2006

23. Acyl Transfer in Clorobiocin Biosynthesis: Involvement of Several Proteins in the Transfer of the Pyrrole-2-carboxyl Moiety to the Deoxysugar

Author

Emmanuel Wemakor, Shu-Ming Li, Anja Freitag, and Lutz Heide

Subjects

Clorobiocin, Proline, biology, Acylation, Organic Chemistry, Streptomyces coelicolor, Carbohydrates, Cosmids, biology.organism_classification, Biochemistry, Streptomyces, Multienzyme Complexes, Gene cluster, medicine, Cosmid, Molecular Medicine, Moiety, Heterologous expression, Molecular Biology, Novobiocin, medicine.drug

Abstract

Clorobiocin is an aminocoumarin antibiotic containing a pyrrole-2-carboxyl moiety, attached through an ester bond to a deoxysugar. The pyrrole moiety is important for the binding of the antibiotic to its biological target, gyrase. The complete biosynthetic gene cluster for clorobiocin has been cloned and sequenced from the natural producer, Streptomyces roseochromogenes DS 12.976. In this study, the genes cloN1 and cloN7 were deleted separately from a cosmid containing the complete clorobiocin cluster. The modified cosmids were introduced into the genome of the heterologous host Streptomyces coelicolor M512 by using the integration functions of the PhiC31 phage. While a heterologous producer strain harbouring the intact clorobiocin biosynthetic gene cluster accumulated clorobiocin, the cloN1- and cloN7-defective integration mutants accumulated a clorobiocin derivative that lacked the pyrrole-2-carboxyl moiety, while also producing free pyrrole-2-carboxylic acid. The structures of these metabolites were confirmed by NMR and MS analysis. These results showed that CloN1 and CloN7, together with the previously investigated CloN2, are involved in the transfer of the pyrrole-2-carboxyl moiety to the deoxysugar of clorobiocin. A possible mechanism for the role of these three proteins in the acyl-transfer process is suggested.

Published

2005

24. Heterologous Expression of Novobiocin and Clorobiocin Biosynthetic Gene Clusters

Author

Keith F. Chater, Lutz Heide, Ute Galm, Bertolt Gust, Shu-Ming Li, and Alessandra S. Eustáquio

Subjects

Recombination, Genetic, Genetics, Clorobiocin, Ecology, biology, Molecular Sequence Data, Streptomyces coelicolor, Genetics and Molecular Biology, biology.organism_classification, Applied Microbiology and Biotechnology, Streptomyces, Multigene Family, Gene cluster, Escherichia coli, medicine, Amino Acid Sequence, Heterologous expression, Homologous recombination, Gene, Novobiocin, Food Science, Biotechnology, medicine.drug

Abstract

A method was developed for the heterologous expression of biosynthetic gene clusters in different Streptomyces strains and for the modification of these clusters by single or multiple gene replacements or gene deletions with unprecedented speed and versatility. -Red-mediated homologous recombination was used for genetic modification of the gene clusters, and the attachment site and integrase of phage C31 were employed for the integration of these clusters into the heterologous hosts. This method was used to express the gene clusters of the aminocoumarin antibiotics novobiocin and clorobiocin in the well-studied strains Streptomyces coelicolor and Streptomyces lividans, which, in contrast to the natural producers, can be easily genetically manipulated. S. coelicolor M512 derivatives produced the respective antibiotic in yields comparable to those of natural producer strains, whereas S. lividans TK24 derivatives were at least five times less productive. This method could also be used to carry out functional investigations. Shortening of the cosmids’ inserts showed which genes are essential for antibiotic production. The development of new antimicrobial agents is crucial to reduce the future clinical impact of resistant pathogens (35). Natural products play a dominant role in antimicrobial drug discovery (19), and streptomycetes produce two-thirds of the clinically useful antibiotics of natural origin (12). Structural modification of these natural products is often necessary in drug development, e.g., for improvements in efficacy and pharmacokinetics (32). The manipulation of genes which encode enzymes of the biosynthetic pathways represents a promising approach for introducing structural changes (33). The functional analysis of biosynthetic genes is, however, a prerequisite for such approaches. Moreover, a principal limitation is often presented by the lack of suitable protocols for the genetic manipulation of natural producers (11).

Published

2005

25. Functional characterizations of novWUS involved in novobiocin biosynthesis from Streptomyces spheroides

Author

Jae Kyung Sohng, Ta Thi Thu Thuy, Chun-Gyu Kim, Hei Chan Lee, and Lutz Heide

Subjects

Biophysics, Biology, medicine.disease_cause, Biochemistry, Streptomyces, Catalysis, chemistry.chemical_compound, Biosynthesis, Deoxy Sugars, Escherichia coli, medicine, Thymine Nucleotides, Base sequence, Molecular Biology, Polyacrylamide gel electrophoresis, Gene, Chromatography, High Pressure Liquid, Novobiocin, Streptomyces spheroides, Base Sequence, Nucleoside Diphosphate Sugars, NAD, biology.organism_classification, Models, Chemical, chemistry, Multigene Family, Electrophoresis, Polyacrylamide Gel, Carbohydrate Epimerases, medicine.drug

Abstract

NovW, novU, and novS gene products represent dTDP-4-keto-6-deoxy-D-glucose 3,5 epimarase, C-methyltransferase and dTDP-glucose-4-ketoreductase involved in noviose biosynthetic pathway, respectively. We have expressed three genes to elucidate the functions of NovW, NovU, and NovS in Escherichia coli. NovW and NovU catalyze the formation of dTDP-4-keto-6-deoxy-5-C-methyl-L-lyxo-hexose from dTDP-4-keto-6-deoxy-D-glucose. NovS reduces the product formed from the reaction of NovW with dTDP-4-keto-6-deoxy-D-glucose in the presence of NADH to result in dTDP-l-rhamnose. Furthermore, a pathway for the biosynthesis of noviose is proposed.

Published

2005

26. Production of 8′-Halogenated and 8′-Unsubstituted Novobiocin Derivatives in Genetically Engineered Streptomyces coelicolor Strains

Author

Lutz Heide, Alessandra S. Eustáquio, Stefan Pelzer, Shu-Ming Li, Keith F. Chater, Wolfgang Wohlleben, and Bertolt Gust

Subjects

medicine.drug_class, Clinical Biochemistry, Streptomyces coelicolor, Glycopeptide antibiotic, medicine.disease_cause, Biochemistry, chemistry.chemical_compound, Halogens, Biosynthesis, Gene cluster, Drug Discovery, medicine, Gene Silencing, Escherichia coli, Molecular Biology, Novobiocin, Pharmacology, Clorobiocin, biology, General Medicine, biology.organism_classification, Anti-Bacterial Agents, chemistry, Multigene Family, Cosmid, bacteria, Molecular Medicine, Genetic Engineering, medicine.drug

Abstract

In the present study, we produced a hybrid antibiotic, carrying a chlorine atom instead of a methyl group at position 8 of the aminocoumarin moiety of novobiocin. This compound was not accessible by conventional gene inactivation/gene expression experiments due to difficulties in the genetic manipulation of the novobiocin producer Streptomyces spheroides. However, the desired compound was obtained after modification of the novobiocin biosynthetic gene cluster by using λ-Red-mediated recombination in Escherichia coli, followed by integration of the resulting modified cosmid into the φC31 attachment site of Streptomyces coelicolor and coexpression of the halogenase Clo-hal of clorobiocin biosynthesis. The halogenase BhaA, responsible for chlorination of tyrosyl moieties of the glycopeptide antibiotic balhimycin, was unable to functionally replace the halogenase Clo-hal, suggesting that the two enzymes have different substrate specificities.

Published

2004

27. Assembly of Dimeric Variants of Coumermycins by Tandem Action of the Four Biosynthetic Enzymes CouL, CouM, CouP, and NovN

Author

Caren L. Freel Meyers, Markus Oberthür, Lutz Heide, Daniel Kahne, and Christopher T. Walsh

Subjects

Aminocoumarins, Operon, Biochemistry, DNA gyrase, Mass Spectrometry, Substrate Specificity, Ligases, Coumarins, Glycosyltransferase, Escherichia coli, medicine, Novobiocin, chemistry.chemical_classification, Clorobiocin, DNA ligase, Molecular Structure, biology, Genetic Variation, Glycosyltransferases, Streptomyces, Anti-Bacterial Agents, Enzyme, chemistry, biology.protein, Dimerization, Chromatography, Liquid, medicine.drug

Abstract

Coumermycin A(1) is a member of the aminocoumarin family of antibiotics. Unlike its structural relatives, novobiocin and clorobiocin, coumermycin A(1) is a dimer built on a 3-methyl-2,4-dicarboxypyrrole scaffold and bears two decorated noviose sugar components which are the putative target binding motifs for DNA gyrase. Starting with this scaffold, we have utilized the ligase CouL for mono- and bisamide formation with aminocoumarins to provide substrates for the glycosyltransferase CouM. CouM was subsequently shown to catalyze mono- and bisnoviosylation of the resulting CouL products. CouP was shown to possess 4'-O-methyltransferase activity on products from tandem CouL, CouM assays. A fourth enzyme, NovN, the 3'-O-carbamoyltransferase from the novobiocin operon, was then able to carbamoylate either or both arms of the CouP product. The tandem action of CouL, CouM, CouP, and NovN thus generates a biscarbamoyl analogue of the pseudodimer coumermycin A(1). Starting from alternative dicarboxy scaffolds, these four enzymes can be utilized in tandem to create additional variants of dimeric aminocoumarin antibiotics.

Published

2004

28. Randomized controlled trial of a traditional preparation of Artemisia annua L. (Annual Wormwood) in the treatment of malaria

Author

Markus S Mueller, Klaus Dietz, Lutz Heide, Steffen Borrmann, Nyabuhanga Runyambo, and Irmela Wagner

Subjects

food.ingredient, Artemisia annua, law.invention, food, Randomized controlled trial, law, parasitic diseases, medicine, Artemisinin, Quinine, Traditional medicine, biology, business.industry, Public Health, Environmental and Occupational Health, food and beverages, Plasmodium falciparum, General Medicine, biology.organism_classification, medicine.disease, Infectious Diseases, Herb, Artemisia, Parasitology, business, Malaria, medicine.drug

Abstract

The Chinese medicinal plant Artemisia annua L. (Annual Wormwood) contains the antimalarial compound artemisinin. The locally grown herb may offer an additional tool for the control of malaria, especially in poor countries where modern antimalarial drugs are often unavailable. In an open, randomized, controlled pilot trial, we investigated the efficacy and safety of traditional tea preparations of Artemisia annua in the treatment of uncomplicated malaria. Treatment resulted in a quick resolution of parasitaemia and of clinical symptoms. After 7 d of medication, cure rates were on average 74% for the Artemisia preparations compared with 91% for quinine. However, recrudescence rates were high in the Artemisia groups. Therefore, monotherapy with Artemisia annua L. cannot be recommended as alternative to modern antimalarials, but may deserve further investigation.

Published

2004

29. New Aminocoumarin Antibiotics from a cloQ-Defective Mutant of the Chorobiocin Producer Streptomyces reseochromogenes DS12.976

Author

Lutz Heide, Shu-Ming Li, Ute Galm, and Anja Freitag

Subjects

Stereochemistry, Mutant, Microbial Sensitivity Tests, Bacillus subtilis, Streptomyces, Structure-Activity Relationship, chemistry.chemical_compound, Biosynthesis, Drug Discovery, medicine, Vanillic acid, Moiety, Novobiocin, Pyrrole, Pharmacology, Clorobiocin, biology, General Medicine, biology.organism_classification, Anti-Bacterial Agents, Biochemistry, chemistry, Fermentation, medicine.drug

Abstract

Three new antibiotics, vanillobiocin, isovanillobiocin and declovanillobiocin, were isolated from the culture broth of a cloQ-defective mutant of the clorobiocin producer Streptomyces roseochromogenes, which is blocked in the biosynthesis of the prenylated 4-hydroxybenzoic acid moiety of clorobiocin. Spectroscopic analysis showed that the isolated compounds were similar to clorobiocin, but contained vanillic acid as the acyl component instead of the prenylated 4-hydroxybenzoic acid present in clorobiocin. Isovanillobiocin differs from vanillobiocin by the position of the pyrrole unit attached to the sugar moiety of the antibiotic. Declovanillobiocin lacks the chlorine atom at the aminocoumarin ring. All three compounds had lower antibiotic activity against Bacillus subtilis than clorobiocin.

Published

2004

30. An unusual amide synthetase (CouL) from the coumermycin A1 biosynthetic gene cluster from Streptomyces rishiriensis DSM 40489

Author

Andrea Porzel, Shu-Ming Li, Jürgen Schmidt, Marion Steffensky, Elisabeth Schmutz, and Lutz Heide

Subjects

Aminocoumarins, Stereochemistry, Streptomyces rishiriensis, Molecular Sequence Data, Biology, Biochemistry, Mixed Function Oxygenases, Substrate Specificity, chemistry.chemical_compound, Biosynthesis, Coumarins, Multienzyme Complexes, Amide, medicine, Amino Acid Sequence, Cloning, Molecular, Novobiocin, chemistry.chemical_classification, Clorobiocin, Sequence Homology, Amino Acid, Streptomyces, Coumermycin A1, Amino acid, Kinetics, Dicarboxylic acid, chemistry, medicine.drug

Abstract

The aminocoumarin antibiotic coumermycin A1 produced by Streptomyces rishiriensis DSM 40489 contains two amide bonds. The biosynthetic gene cluster of coumermycin contains a putative amide synthetase gene, couL, encoding a protein of 529 amino acids. CouL was overexpressed as hexahistidine fusion protein in Escherichia coli and purified by metal affinity chromatography, resulting in a nearly homogenous protein. CouL catalysed the formation of both amide bonds of coumermycin A1, i.e. between the central 3-methylpyrrole-2,4-dicarboxylic acid and two aminocoumarin moieties. Gel exclusion chromatography showed that the enzyme is active as a monomer. The activity was strictly dependent on the presence of ATP and Mn2+ or Mg2+. The apparent Km values were determined as 26 micro m for the 3-methylpyrrole-2,4-dicarboxylic acid and 44 micro m for the aminocoumarin moiety, respectively. Several analogues of the pyrrole dicarboxylic acid were accepted as substrates. In contrast, pyridine carboxylic acids were not accepted. 3-Dimethylallyl-4-hydroxybenzoic acid, the acyl component in novobiocin biosynthesis, was well accepted, despite its structural difference from the genuine acyl substrate of CouL.

Published

2003

31. CloN2, a novel acyltransferase involved in the attachment of the pyrrole-2-carboxyl moiety to the deoxysugar of clorobiocin

Author

Shu-Ming Li, Lutz Heide, Bernd Kammerer, Hui Xu, and Rainer Kahlich

Subjects

Magnetic Resonance Spectroscopy, Proline, Stereochemistry, Mutant, Microbiology, Streptomyces, Mass Spectrometry, chemistry.chemical_compound, Plasmid, Biosynthesis, Moiety, Pyrrole, Clorobiocin, Binding Sites, Molecular Structure, biology, Chemistry, Genetic Complementation Test, biology.organism_classification, Anti-Bacterial Agents, Models, Chemical, Genes, Bacterial, Acyltransferase, Mutation, Acyltransferases, Gene Deletion, Novobiocin, Chromatography, Liquid

Abstract

The aminocoumarin antibiotic clorobiocin contains a 5-methylpyrrole-2-carboxylic acid unit, attached via an ester bond to the 3-OH group of the deoxysugar moiety. To investigate candidate genes responsible for the formation of this ester bond, a gene inactivation experiment was carried out in the clorobiocin producer Streptomyces roseochromogenes var. oscitans DS 12.976. An in-frame deletion was created in the coding sequence of the gene cloN2. The production of secondary metabolites in the wild-type and in the cloN2 mutant was analysed. The wild-type showed clorobiocin as the main product, whereas the cloN2 mutant accumulated a new aminocoumarin derivative, novclobiocin 104, lacking the pyrrole moiety at the 3-OH of the deoxysugar. In addition, free pyrrole-2-carboxylic acid accumulated in the culture extract of the cloN2 mutant. The structures of the metabolites were confirmed by NMR and LC-MS analysis. Clorobiocin production was successfully restored in the cloN2 mutant by introducing a replicative plasmid containing the cloN2 sequence. These results prove an involvement of cloN2 in the formation of the ester bond between the pyrrole moiety and the deoxysugar in clorobiocin biosynthesis. Furthermore, they indicate that the C-methylation at position 5 of the pyrrole moiety occurs after the attachment of pyrrole-2-carboxylic acid unit to the deoxysugar moiety.

Published

2003

32. Clorobiocin Biosynthesis in Streptomyces

Author

Bertolt Gust, Lutz Heide, Shu-Ming Li, Keith F. Chater, Alessandra S. Eustáquio, and Thomas Luft

Subjects

Pharmacology, Clorobiocin, biology, Stereochemistry, Clinical Biochemistry, Mutant, General Medicine, biology.organism_classification, Biochemistry, DNA gyrase, Streptomyces, chemistry.chemical_compound, Biosynthesis, chemistry, Methyltransferase Gene, Drug Discovery, polycyclic compounds, medicine, Molecular Medicine, Molecular Biology, Novobiocin, medicine.drug, Methyl group

Abstract

Clorobiocin ( clo ) and novobiocin ( nov ) are potent inhibitors of bacterial DNA gyrase. The two substances differ in the substitution pattern at C-8′ of the aminocoumarin ring, carrying a chlorine atom or a methyl group, respectively. By gene inactivation, clo-hal was identified as the gene of the halogenase responsible for the introduction of the chlorine atom of clorobiocin. Inactivation of cloZ did not affect clorobiocin formation, showing that this ORF is not essential for clorobiocin biosynthesis. Expression of the methyltransferase gene novO in the clo-hal − mutant led to the very efficient formation of a hybrid antibiotic containing a methyl group instead of a chlorine atom at C-8′. Comparison of the antibacterial activity of clorobiocin analogs with -Cl, -H, or -CH 3 at C-8′ showed that chlorine leads to 8-fold higher activity than hydrogen and to 2-fold higher activity than a methyl group.

Published

2003

33. Resistance Genes of Aminocoumarin Producers: Two Type II Topoisomerase Genes Confer Resistance against Coumermycin A 1 and Clorobiocin

Author

Shu-Ming Li, Agnes Mühlenweg, Elisabeth Schmutz, and Lutz Heide

Subjects

Aminocoumarins, DNA, Bacterial, Microbial Sensitivity Tests, Biology, DNA gyrase, Plasmid, Coumarins, Mechanisms of Resistance, medicine, Pharmacology (medical), In Situ Hybridization, Phylogeny, Novobiocin, Pharmacology, Genetics, Clorobiocin, Streptomyces coelicolor, biology.organism_classification, Streptomyces, Coumermycin A1, Anti-Bacterial Agents, Blotting, Southern, DNA Topoisomerases, Type II, Infectious Diseases, DNA Gyrase, Multigene Family, Antibiotic transport, Type II topoisomerase, Plasmids, medicine.drug

Abstract

The aminocoumarin resistance genes of the biosynthetic gene clusters of novobiocin, coumermycin A 1 , and clorobiocin were investigated. All three clusters contained a gyrB R resistance gene, coding for a gyrase B subunit. Unexpectedly, the clorobiocin and the coumermycin A 1 clusters were found to contain an additional, similar gene, named parY R . Its predicted gene product showed sequence similarity with the B subunit of type II topoisomerases. Expression of gyrB R and likewise of parY R in Streptomyces lividans TK24 resulted in resistance against novobiocin and coumermycin A 1 , suggesting that both gene products are able to function as aminocoumarin-resistant B subunits of gyrase. Southern hybridization experiments showed that the genome of all three antibiotic producers and of Streptomyces coelicolor contained two additional genes which hybridized with either gyrB R or parY R and which may code for aminocoumarin-sensitive GyrB and ParY proteins. Two putative transporter genes, novA and couR5 , were found in the novobiocin and the coumermycin A 1 cluster, respectively. Expression of these genes in S. lividans TK24 resulted in moderate levels of resistance against novobiocin and coumermycin A 1 , suggesting that these genes may be involved in antibiotic transport.

Published

2003

34. [Untitled]

Author

Lutz Heide, Susanne Sommer, Annegret Köhle, Shu-Ming Li, Helga Ninnemann, and Lieselotte Schilde-Rentschler

Subjects

biology, Nicotiana tabacum, fungi, food and beverages, Plant physiology, Plant Science, Genetically modified crops, Secondary metabolite, biology.organism_classification, Solanum tuberosum, chemistry.chemical_compound, 4-Hydroxybenzoic acid, Biochemistry, Glucoside, chemistry, Genetics, medicine, Agronomy and Crop Science, Molecular Biology, Solanaceae, Biotechnology, medicine.drug

Abstract

The bacterial gene ubiC encodes chorismate pyruvate-lyase (CPL), which converts chorismate to 4-hydroxybenzoate (4HB). The ubiC gene was expressed in tobacco (Nicotiana tabacum L., Solanaceae) and potato (Solanum tuberosum L., Solanaceae) under the control of the very strong constitutive plant promotor (ocs3) mas. High accumulation of 4HB glucosides as new, artificial secondary metabolites was observed in the transgenic plants. 4HB glucoside content reached 5.1% of dry weight in tobacco cell cultures and 4.0% of dry weight in the leaves of potato shoots. This is the highest content of an artificial secondary metabolite produced by genetic engineering of plants reported so far. Surprisingly, no growth retardation and no phenotypical changes were observed in the transgenic cell cultures and plants. Glucosylation of 4HB was achieved by endogeneous, constitutively expressed glucosyltransferases. The total amount of 4HB glucoside acccumulated showed a strict linear dependence on the expression level of ubiC.

Published

2003

35. Molecular cloning and sequence analysis of the clorobiocin biosynthetic gene cluster: new insights into the biosynthesis of aminocoumarin antibiotics The GenBank accession number for the sequence of cosmid K1F2 is AF329398

Author

Shu-Ming Li, Florence Pojer, and Lutz Heide

Subjects

Genetics, Clorobiocin, Sequence analysis, Mutant, Biology, biology.organism_classification, Microbiology, Streptomyces, Coumermycin A1, Biochemistry, Gene cluster, medicine, Gene, Novobiocin, medicine.drug

Abstract

The biosynthetic gene cluster of the aminocoumarin antibiotic clorobiocin was cloned by screening of a cosmid library of Streptomyces roseochromogenes DS 12.976 with two heterologous probes from the novobiocin biosynthetic gene cluster. Sequence analysis revealed 27 ORFs with striking similarity to the biosynthetic gene clusters of novobiocin and coumermycin A(1). Inactivation of a putative aldolase gene, cloR, by in-frame deletion led to the abolishment of the production of clorobiocin. Feeding of the mutant with 3-dimethylallyl-4-hydroxybenzoic acid (Ring A of clorobiocin) restored clorobiocin production. Here, it is suggested that the formation of Ring A of clorobiocin may proceed via a retro-aldol reaction catalysed by CloR, i.e. by a mechanism different from the previously elucidated benzoic acid biosynthetic pathway in Streptomyces maritimus. A comparison of the gene clusters for clorobiocin, novobiocin and coumermycin A(1) showed that the structural differences between the three antibiotics were reflected remarkably well by differences in the organization of their respective biosynthetic gene clusters.

Published

2002

36. ChemInform Abstract: New Aminocoumarins from the Rare Actinomycete Catenulispora acidiphila DSM 44928: Identification, Structure Elucidation, and Heterologous Production

Author

Haiyang Xia, Judith Zettler, Andreas Kulik, Nadja Burkard, Stephanie Grond, Lutz Heide, and Alexander Kristian Apel

Subjects

Aminocoumarins, biology, Stereochemistry, Chemistry, Sequence analysis, Putative gene, Streptomyces coelicolor, Gene cluster, Heterologous, General Medicine, Heterologous expression, biology.organism_classification, Structural motif

Abstract

Genome mining led to the discovery of a novel aminocoumarin gene cluster in the rare actinomycete Catenulispora acidiphila DSM 44928. Sequence analysis revealed the presence of genes putatively involved in export/resistance, regulation, and biosynthesis of the aminocoumarin moiety and its halogenation, as well as several genes with so far unknown function. Two new aminocoumarins, cacibiocin A and B, were identified in the culture broth of C. acidiphila. Heterologous expression of the putative gene cluster in Streptomyces coelicolor M1152 confirmed that this cluster is responsible for cacibiocin biosynthesis. Furthermore, total production levels of cacibiocins could be increased by heterologous expression and screening of different culture media from an initial yield of 4.9 mg L(-1) in C. acidiphila to 60 mg L(-1) in S. coelicolor M1152. By HR-MS and NMR analysis, cacibiocin A was found to contain a 3-amino-4,7-dihydroxycoumarin moiety linked by an amide bond to a pyrrole-2,5-dicarboxylic acid. The latter structural motif has not been identified previously in any natural compound. Additionally, cacibiocin B contains two chlorine atoms at positions 6' and 8' of the aminocoumarin moiety.

Published

2014

37. Draft Genome Sequence of Streptomyces niveus NCIMB 11891, Producer of the Aminocoumarin Antibiotic Novobiocin

Author

Lutz Heide, Alexander Kristian Apel, Katrin Flinspach, Jörn Kalinowski, and Christian Rückert

Subjects

Whole genome sequencing, Genetics, Streptomyces niveus, Secondary metabolite, Biology, DNA gyrase, Microbiology, Putative gene, Gene cluster, medicine, Prokaryotes, Molecular Biology, Gene, Novobiocin, medicine.drug

Abstract

Streptomyces niveus NCIMB 11891 is the producer of the gyrase inhibitor novobiocin, which belongs to the aminocoumarin class of antibiotics. The genome sequence of this strain was found to contain, besides the gene cluster for novobiocin, a putative gene cluster for the macrolactam antibiotic BE-14106 and further secondary metabolite gene clusters.

Published

2014

38. Draft Genome Sequence of Streptomyces roseochromogenes subsp. oscitans DS 12.976, Producer of the Aminocoumarin Antibiotic Clorobiocin

Author

Jörn Kalinowski, Christian Rückert, Alexander Kristian Apel, and Lutz Heide

Subjects

Genetics, Whole genome sequencing, Clorobiocin, medicine.drug_class, Antibiotics, Biology, Secondary metabolite, biology.organism_classification, Streptomyces, Microbiology, Gene cluster, medicine, Prokaryotes, Molecular Biology, medicine.drug

Abstract

Streptomyces roseochromogenes subsp. oscitans DS 12.976 is the producer of the gyrase-inhibiting aminocoumarin antibiotic clorobiocin. Here, we present a draft genome sequence of this strain, in which we identified the clorobiocin gene cluster as well as an unusually high number (43) of further putative secondary metabolite clusters.

Published

2014

39. Cloning, Overexpression, and Purification of Novobiocic Acid Synthetase from Streptomyces spheroides NCIMB 11891

Author

Shu-Ming Li, Lutz Heide, and Marion Steffensky

Subjects

Molecular Sequence Data, Adenylate kinase, Biology, Biochemistry, Chromatography, Affinity, Substrate Specificity, chemistry.chemical_compound, Biosynthesis, Affinity chromatography, Amide Synthases, Escherichia coli, medicine, Peptide bond, heterocyclic compounds, Amino Acid Sequence, Cloning, Molecular, Molecular Biology, Novobiocin, chemistry.chemical_classification, Base Sequence, Sequence Homology, Amino Acid, Cell Biology, Recombinant Proteins, Streptomyces, Amino acid, Molecular Weight, Kinetics, Enzyme, chemistry, Chromatography, Gel, Sequence Alignment, Acyl group, medicine.drug

Abstract

Novobiocic acid synthetase, a key enzyme in the biosynthesis of the antibiotic novobiocin, was cloned from the novobiocin producer Streptomyces spheroides NCIMB 11891. The enzyme is encoded by the gene novL, which codes for a protein of 527 amino acids with a calculated mass of 56,885 Da. The protein was overexpressed as a His(6) fusion protein in Escherichia coli and purified to apparent homogeneity by affinity chromatography and gel chromatography. The purified enzyme catalyzed the formation of an amide bond between 3-dimethylallyl-4-hydroxybenzoic acid (ring A of novobiocin) and 3-amino-4,7-dihydroxy-8-methyl coumarin (ring B of novobiocin) in an ATP-dependent reaction. NovL shows homology to the superfamily of adenylate-forming enzymes, and indeed the formation of an acyl adenylate from ring A and ATP was demonstrated by an ATP-PP(i) exchange assay. The purified enzyme exhibited both activation and transferase activity, i.e. it catalyzed both the activation of ring A as acyl adenylate and the subsequent transfer of the acyl group to the amino group of ring B. It is active as a monomer as determined by gel filtration chromatography. The reaction was specific for ATP as nucleotide triphosphate and dependent on the presence of Mg(2+) or Mn(2+). Apparent K(m) values for ring A and ring B were determined as 19 and 131 micrometer respectively. Of several analogues of ring A, only 3-geranyl-4-hydroxybenzoate and to a lesser extent 3-methyl-4-aminobenzoate were accepted as substrates.

Published

2000

40. Identification of the Novobiocin Biosynthetic Gene Cluster of Streptomyces spheroides NCIB 11891

Author

Agnes Mühlenweg, Shu-Ming Li, Zhao-Xin Wang, Marion Steffensky, and Lutz Heide

Subjects

DNA, Bacterial, Molecular Sequence Data, Biology, Streptomyces, Amide Synthases, Gene cluster, medicine, Pharmacology (medical), Amino Acid Sequence, Cloning, Molecular, ORFS, Novobiocin, Gene Library, Antibacterial agent, Pharmacology, Sequence Homology, Amino Acid, Streptomycetaceae, Chemistry, Biosynthesis, biochemical phenomena, metabolism, and nutrition, Cosmids, biology.organism_classification, Molecular biology, carbohydrates (lipids), Mutagenesis, Insertional, Open reading frame, Infectious Diseases, Genes, Bacterial, Multigene Family, Heterologous expression, medicine.drug

Abstract

The novobiocin biosynthetic gene cluster from Streptomyces spheroides NCIB 11891 was cloned by using homologous deoxynucleoside diphosphate (dNDP)-glucose 4,6-dehydratase gene fragments as probes. Double-stranded sequencing of 25.6 kb revealed the presence of 23 putative open reading frames (ORFs), including the gene for novobiocin resistance, gyrB r , and at least 11 further ORFs to which a possible role in novobiocin biosynthesis could be assigned. An insertional inactivation experiment with a dNDP-glucose 4,6-dehydratase fragment resulted in abolishment of novobiocin production, since biosynthesis of the deoxysugar moiety of novobiocin was blocked. Heterologous expression of a key enzyme of novobiocin biosynthesis, i.e., novobiocic acid synthetase, in Streptomyces lividans TK24 further confirmed the involvement of the analyzed genes in the biosynthesis of the antibiotic.

Published

2000

41. [Untitled]

Author

Susanne Sommer, Lutz Heide, Robert Boehm, Klaus Severin, and Shu-Ming Li

Subjects

Signal peptide, Regulation of gene expression, Agrobacterium, Endoplasmic reticulum, Structural gene, Biology, biology.organism_classification, Molecular biology, Membrane protein, Biochemistry, Gene expression, Genetics, Animal Science and Zoology, Agronomy and Crop Science, Integral membrane protein, Biotechnology

Abstract

The ubiA gene from E. coli codes for 4-hydroxybenzoate: polyprenyldiphosphate 3-polyprenyltransferase, an integral membrane protein involved in ubiquinone biosynthesis. This prokaryotic membrane protein was stably expressed in tobacco using Agrobacterium tumefaciens-mediated transformation. Transgenic lines containing a direct fusion of the ubiA structural gene to a 35S-derived promoter gave very low enzyme activity levels (average 0.16 pkat/mg). Inclusion of an N-terminal ER-specific signal peptide from a lectin gene from Phaseolus vulgaris resulted in an average activity of 1.08 pkat/mg in the transgenic tobacco lines. The additional inclusion of a C-terminal HDEL tetrapeptide, responsible for the retention of proteins in the endoplasmic reticulum of eukaryotic cells, increased the activity to 18.6 pkat/mg. When the promotor of this construct was changed from the 35S derivative to the recently described very strong plant promoter (ocs)3mas, the activity increased further to 128.6 pkat/mg. The most active tobacco line showed activities of the introduced enzyme which exceeded those of wild-type E. coli (the source of ubiA) by a factor of 1100. These results demonstrate the efficacy of plant ER-specific signal peptides for the active expression of a prokaryotic membrane protein in plants.

Published

2000

42. [Untitled]

Author

Annegret Köhle, Susanne Sommer, Koichiro Shimomura, Kazufumi Yazaki, Lutz Heide, and Andreas Bechthold

Subjects

biology, Agrobacterium, Plant Science, General Medicine, biology.organism_classification, medicine.disease_cause, Lithospermum erythrorhizon, Naphthoquinone, chemistry.chemical_compound, Transformation (genetics), Biochemistry, Glucoside, chemistry, Biosynthesis, Genetics, Aromatic amino acids, medicine, Agronomy and Crop Science, Escherichia coli

Abstract

The biosynthetic pathway to 4-hydroxybenzoate (4HB), a precursor of the naphthoquinone pigment shikonin, was modified in Lithospermum erythrorhizon hairy root cultures by introduction of the bacterial gene ubiC. This gene of Escherichia coli encodes chorismate pyruvate-lyase (CPL), an enzyme that converts chorismate into 4HB and is not normally present in plants. The ubiC gene was fused to the sequence for a chloroplast transit peptide and placed under control of a constitutive plant promoter. This construct was introduced into L. erythrorhizon by Agrobacterium rhizogenes-mediated transformation. The resulting hairy root cultures showed high CPL activity. 4HB produced by the CPL reaction was utilized for shikonin biosynthesis, as shown by in vivo inhibition of the native pathway to 4HB with 2-aminoindan-2-phosphonic acid (AIP), an inhibitor of phenylalanine ammonia-lyase. A feeding experiment with [1,7-13C2]shikimate showed that in the absence of AIP the artificially introduced CPL reaction contributed ca. 20% of the overall 4HB biosynthesis in the transgenic cultures. ubiC transformation did not lead to a statistically significant increase of shikonin formation, but to a 5-fold increase of the accumulation of menisdaurin, a nitrile glucoside which is presumably related to aromatic amino acid metabolism.

Published

1999

43. Complete genome sequence of Streptomyces sp. CNQ-509, a prolific producer of meroterpenoid chemistry

Author

Jörn Kalinowski, Leonard Kaysser, Paul R. Jensen, Lutz Heide, William Fenical, Franziska Leipoldt, Christian Rückert, and Philipp Zeyhle

Subjects

Whole genome sequencing, Genetics, Lineage (genetic), Base Sequence, Bioengineering, General Medicine, Biology, biology.organism_classification, Applied Microbiology and Biotechnology, Genome, Streptomyces, chemistry.chemical_compound, Biosynthesis, chemistry, Putative gene, Monoterpenes, Base sequence, Genome, Bacterial, Biotechnology

Abstract

Streptomyces sp. CNQ-509 is a marine actinomycete belonging to the MAR4 streptomycete lineage. MAR4 strains have been linked to the production of diverse and otherwise rare meroterpenoid compounds. The genome sequence of Streptomyces sp. CNQ-509 was found to contain 29 putative gene clusters for the biosynthesis of secondary metabolites, some of them potentially involved in the formation of meroterpenoid molecules.

Published

2015

44. Expression of Bacterial Chorismate Pyruvate-Lyase in Tobacco: Evidence for the Presence of Chorismate in the Plant Cytosol

Author

Lutz Heide and Susanne Sommer

Subjects

Physiology, Nicotiana tabacum, Plant Science, Biology, Gene product, chemistry.chemical_compound, 4-Hydroxybenzoic acid, Consensus Sequence, Tobacco, Escherichia coli, Shikimate pathway, Plastid, chemistry.chemical_classification, Base Sequence, fungi, Oxo-Acid-Lyases, food and beverages, Cell Biology, General Medicine, Shikimic acid, Plants, Genetically Modified, biology.organism_classification, Recombinant Proteins, Plants, Toxic, Cytosol, Enzyme, Biochemistry, chemistry, Agrobacterium tumefaciens, Sequence Alignment

Abstract

The bacterial gene ubiC encodes chorismate pyruvate-lyase, an enzyme which converts chorismate to 4-hydroxybenzoate and which is not normally present in plants. The UbiC protein was expressed in tobacco, with targeting of the gene product either to the plastids or to the cytosol. In both cases, chorismate pyruvate-lyase activity and a resulting formation of 4-hydroxybenzoate was detected. This suggests that chorismate, a metabolite of the shikimate pathway, is present not only in the plastids but also in the cytosol of plant cells.

Published

1998

45. 4-Hydroxybenzoate 3-geranyltransferase from Lithospermum erythrorhizon : purification of a plant membrane-bound prenyltransferase

Author

Shu-Ming Li, M. Melzer, Agnes Mühlenweg, and Lutz Heide

Subjects

Prenyltransferase, Lithospermum, Digitonin, Cyclopentanes, Plant Science, Acetates, Cofactor, Substrate Specificity, chemistry.chemical_compound, Genetics, Magnesium, Oxylipins, Magnesium ion, Cells, Cultured, chemistry.chemical_classification, Alkyl and Aryl Transferases, biology, Chemistry, Temperature, Membrane Proteins, Geranyltranstransferase, Hydrogen-Ion Concentration, Plants, Dimethylallyltranstransferase, Lithospermum erythrorhizon, biology.organism_classification, Enzyme, Solubility, Biochemistry, Hydroxybenzoate, biology.protein

Abstract

Geranyldiphosphate:4-hydroxybenzoate 3-geranyltransferase is a regulatory enzyme in the biosynthesis of shikonin, a phytoalexin and pharmaceutical produced by cell cultures of Lithospermum erythrorhizon Sieb. et Zucc. In Linsmaier-Skoog medium, the activity of this enzyme could be enhanced more than 200-fold by addition of methyl jasmonate, and this culture material was used for the solubilization and purification of the enzyme. Of various detergents examined, digitonin was the most suitable for the solubilization of the enzyme. The solubilized enzyme was purified 800-fold by chromatography over diethylaminoethyl (DEAE)-Sephacel, Heparin-Sepharose, Reactive Green 19-Agarose, and Cholic Acid-Agarose. The purified enzyme required magnesium ions as cofactor and was highly specific for geranyldiphosphate (GPP) and 4-hydroxybenzoate (4HB) as substrates. The K(m) values for 4HB and GPP were calculated by the method of Lineweaver and Burk as 18.4 microM and 13.8 microM, respectively.

Published

1998

46. Novobiocin biosynthesis inStreptomyces spheroides: identification of a dimethylallyl diphosphate:4-hydroxyphenylpyruvate dimethylallyl transferase

Author

Bernhard Vogler, Marion Steffensky, Lutz Heide, and Shu-Ming Li

Subjects

chemistry.chemical_classification, biology, Streptomycetaceae, Prenyltransferase, biology.organism_classification, Microbiology, Streptomyces, chemistry.chemical_compound, Enzyme, Biosynthesis, chemistry, Biochemistry, Dimethylallyltranstransferase, Genetics, medicine, Transferase, Molecular Biology, Novobiocin, medicine.drug

Abstract

A dimethylallyl diphosphate:4-hydroxyphenylpyruvate dimethylallyl transferase from the novobiocin producer Streptomyces spheroides DSM 40292 was identified, partially purified and characterized. The enzyme was soluble, and specific for 4-hydroxyphenylpyruvate and dimethylallyl diphosphate as substrates. It is most likely involved in the biosynthesis of the prenylated 4-hydroxybenzoate moiety of the aminocoumarin antibiotic novobiocin.

Published

1998

47. Shikonin: A geranyl diphosphate-derived plant hemiterpenoid formed via the mevalonate pathway

Author

Lutz Heide, Susanne Hennig, and Shu-Ming Li

Subjects

biology, Chemistry, Stereochemistry, organic chemicals, Organic Chemistry, Lithospermum erythrorhizon, biology.organism_classification, Biochemistry, Terpenoid, chemistry.chemical_compound, Biosynthesis, Cell culture, Labelling, Drug Discovery, Mevalonate pathway

Abstract

Feeding of [1- 13 C]glucose to cell cultures of Lithospermum erythrorhizon revealed a labelling pattern in the isoprenoid part of shikonin consistent with a biosynthesis via the mevalonate pathway. This is in contrast to other plant monoterpenoids.

Published

1998

48. Crystallization and preliminary X-ray analysis of the aromatic prenyltransferase CloQ from the clorobiocin biosynthetic cluster ofStreptomyces roseochromogenes

Author

Florence Pojer, Sascha Keller, David M. Lawson, and Lutz Heide

Subjects

Prenyltransferase, Biophysics, Crystallography, X-Ray, Biochemistry, Streptomyces, DNA gyrase, chemistry.chemical_compound, Bacterial Proteins, Biosynthesis, Structural Biology, Genetics, medicine, Novobiocin, chemistry.chemical_classification, Clorobiocin, biology, clorobiocin, CloQ, Dimethylallyltranstransferase, Condensed Matter Physics, biology.organism_classification, Anti-Bacterial Agents, Amino acid, Crystallography, Monomer, chemistry, Crystallization Communications, prenyltransferases, antibiotic biosynthesis, medicine.drug

Abstract

An aromatic prenyltransferase (CloQ) from S. roseochromogenes that is implicated in clorobiocin biosynthesis has been crystallized in space group I4122. X-ray data to 2.2 Å resolution were collected in-house., Crystals of recombinant CloQ (subunit MW = 35 626 Da; 324 amino acids), an aromatic prenyltransferase from Streptomyces roseochromogenes, were grown by vapour diffusion. The protein crystallizes in space group I4122, with unit-cell parameters a = b = 135.19, c = 98.13 Å. Native data from a single crystal were recorded to a resolution of 2.2 Å in-house. Preliminary analysis of these data indicated that the asymmetric unit corresponds to a monomer, giving an estimated solvent content of 60.6%. CloQ is involved in the biosynthesis of the aminocoumarin antibiotic clorobiocin, which targets the essential bacterial enzyme DNA gyrase.

Published

2006

49. Purification of UDP-glucose: 4-hydroxybenzoate glucosyltransferase from cell cultures of Lithospermum erythrorhizon

Author

Shu-Ming Li, Lutz Heide, and Zhao-Xin Wang

Subjects

chemistry.chemical_classification, Chromatography, biology, Chemistry, Elution, Plant Science, General Medicine, Horticulture, Lithospermum erythrorhizon, biology.organism_classification, Biochemistry, Enzyme, Column chromatography, Affinity chromatography, Hydroxybenzoate, biology.protein, Glucosyltransferase, NAD+ kinase, Molecular Biology

Abstract

UDP-glucose: 4-hydroxybenzoate glucosyltransferase (4HB glucosyltransferase, EC 2.4.1.194) was purified to near homogeneity from cell suspension cultures of Lithospermum erythrorhizon , using ammonium sulphate precipitation, and column chromatography on DEAE Sephacel, Superdex 200, hydroxyapatite, HiTrap blue, Mono P and Mono Q. Affinity chromatography on HiTrap blue was the crucial step for the success of this scheme. After removal of NAD-dependent enzymes from the HiTrap blue column with NAD (5 mM), the 4HB glucosyltransferase was eluted specifically with UDP-glucose (0–20 mM). The above purification procedure resulted in an enzyme fraction with 27 300-fold higher specific 4HB glucosyltransferase activity than the crude enzyme extract. The enzyme is a monomer of about M r , 51 k, determined by SDS-PAGE. © 1997 Published by Elsevier Science Ltd. All rights reserved

Published

1997

50. 4-hydroxybenzoate prenyltransferases in cell-free extracts of Lithospermum erythrorhizon cell cultures

Author

Shu-Ming Li, Robert Boehm, Lutz Heide, and M. Melzer

Subjects

chemistry.chemical_classification, Methyl jasmonate, biology, Stereochemistry, Plant Science, General Medicine, Horticulture, Lithospermum erythrorhizon, biology.organism_classification, Biochemistry, Naphthoquinone, Cell-free system, chemistry.chemical_compound, Enzyme, chemistry, Biosynthesis, Prenylation, Hydroxybenzoate, Molecular Biology

Abstract

Aromatic prenylation reactions of 4-hydroxybenzoate (4HB) are involved in the biosynthesis of ubiquinones and of shikonin, a naphthoquinone pigment derived from 4HB and geranyldiphosphate (GPP) in Lithospermum erythrorhizon. The enzymic prenylation of 4HB with GPP and with solanesyldiphosphate (SPP) was measured in cell-free extracts from L. erythrorhizon cell cultures. The conversion of GPP was induced by methyl jasmonate, an inducer of shikonin biosynthesis, whilst the conversion of SPP was not, suggesting that the two reactions are carried out by different enzymes. Either reaction was found both in the microsomal fraction and in the organellar membrane fraction. The activity of the 4HB geranyltransferase in the microsomal fraction could be separated from the 4HB solanesyltransferase by partial purification using DEAE Sephacel and Heparin Sepharose affinity columns. The results indicate the presence of two distinct enzymes, GPP:4-HB geranyltransferase and SPP:4-HB solanesyltransferase. The enzymes are apparently quite specific for the chain length of the isoprenoid precursors, which is in contrast to the broad substrate specificity of the polyprenyldiphosphate: 4-HB polyprenyltransferase from Escherichia coli.

Published

1997