Penicillin production in industrial strain Penicillium chrysogenum P2niaD18 is not dependent on the copy number of biosynthesis genes

Ziemons, Sandra; Koutsantas, Katerina; Becker, Kordula; Dahlmann, Tim A.; Kück, Ulrich

doi:10.1186/s12896-017-0335-8

Cited by 36 publications

(21 citation statements)

References 48 publications

(71 reference statements)

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“…This fits with the type of mutagenesis and artificial selection used for this process. Experimental work showed that tandem duplication of the pcbAB – pcbC – penDE cluster does not directly increase penicillin production over short time periods—a strain of P2niaD18 that was modified to lose one copy did not produce significantly less penicillin over a 96-h assay period 57 . Substantial copy number multiplication of the region among industrial strains still seems to implicate gene duplication in penicillin production, but perhaps only under specific growth conditions or over longer periods 18 , 51 .…”

Section: Discussionmentioning

confidence: 99%

Comparative genomics of Alexander Fleming’s original Penicillium isolate (IMI 15378) reveals sequence divergence of penicillin synthesis genes

Pathak

Nowell

Wilson

et al. 2020

Sci Rep

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Antibiotics were derived originally from wild organisms and therefore understanding how these compounds evolve among different lineages might help with the design of new antimicrobial drugs. We report the draft genome sequence of Alexander Fleming’s original fungal isolate behind the discovery of penicillin, now classified as Penicillium rubens Biourge (1923) (IMI 15378). We compare the structure of the genome and genes involved in penicillin synthesis with those in two ‘high producing’ industrial strains of P. rubens and the closely related species P. nalgiovense. The main effector genes for producing penicillin G (pcbAB, pcbC and penDE) show amino acid divergence between the Fleming strain and both industrial strains, whereas a suite of regulatory genes are conserved. Homologs of penicillin N effector genes cefD1 and cefD2 were also found and the latter displayed amino acid divergence between the Fleming strain and industrial strains. The draft assemblies contain several partial duplications of penicillin-pathway genes in all three P. rubens strains, to differing degrees, which we hypothesise might be involved in regulation of the pathway. The two industrial strains are identical in sequence across all effector and regulatory genes but differ in duplication of the pcbAB–pcbC–penDE complex and partial duplication of fragments of regulatory genes. We conclude that evolution in the wild encompassed both sequence changes of the effector genes and gene duplication, whereas human-mediated changes through mutagenesis and artificial selection led to duplication of the penicillin pathway genes.

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Section: Discussionmentioning

confidence: 99%

Comparative genomics of Alexander Fleming’s original Penicillium isolate (IMI 15378) reveals sequence divergence of penicillin synthesis genes

Pathak

Nowell

Wilson

et al. 2020

Sci Rep

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“…For example, the industrial strain RutC 30 of Trichoderma reesei (used for enzyme production) is derived from a natural strain QM6A through repeated mutagenesis resulting in 15- to 20-fold improvement in cellulase biosynthesis (Peterson and Nevalainen, 2012). Another example is the enhancement of penicillin biosynthesis – it has been possible to enhance the titer by 85-fold through mutation (Ziemons et al, 2017). There are several such examples in industry, but only a few in microbes of agricultural importance.…”

Section: Discussionmentioning

confidence: 99%

A Novel Seed-Dressing Formulation Based on an Improved Mutant Strain of Trichoderma virens, and Its Field Evaluation

et al. 2019

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Using gamma-ray-induced mutagenesis, we have developed a mutant (named G2) of Trichoderma virens that produced two- to three-fold excesses of secondary metabolites, including viridin, viridiol, and some yet-to-be identified compounds. Consequently, this mutant had improved antibiosis against the oomycete test pathogen Pythium aphanidermatum . A transcriptome analysis of the mutant vis-à-vis the wild-type strain showed upregulation of several secondary-metabolism-related genes. In addition, many genes predicted to be involved in mycoparasitism and plant interactions were also upregulated. We used tamarind seeds as a mass multiplication medium in solid-state fermentation and, using talcum powder as a carrier, developed a novel seed dressing formulation. A comparative evaluation of the wild type and the mutant in greenhouse under high disease pressure (using the test pathogen Sclerotium rolfsii ) revealed superiority of the mutant over wild type in protecting chickpea ( Cicer arietinum ) seeds and seedlings from infection. We then undertook extensive field evaluation (replicated micro-plot trials, on-farm demonstration trials, and large-scale trials in farmers’ fields) of our mutant-based formulation (named TrichoBARC) for management of collar rot ( S. rolfsii ) in chickpea and lentil ( Lens culinaris ) over multiple locations in India. In certain experiments, other available formulations were included for comparison. This formulation consistently, over multiple locations and years, improved seed germination, reduced seedling mortality, and improved plant growth and yield. We also noticed growth promotion, improved pod bearing, and early flowering (7–10 days) in TrichoBARC-treated chickpea and lentil plants under field conditions. In toxicological studies in animal models, this formulation exhibited no toxicity to mammals, birds, or fish.

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“…Thus, identification of new enzymes of this type might open new production routes. Interesting in this respect is the conversion of phenylacetonitrile to phenylacetic acid, which is used among others for the production of penicillin G (Ziemons et al 2017). The new insights obtained by identification and analysis of Nit09 contribute to the understanding of the sequence function relationship of arylacetonitrilases and thus to the development of better or novel nitrilase biocatalysts.…”

Section: A Novel and Stable Arylacetonitrilasementioning

confidence: 99%

From sequence to function: a new workflow for nitrilase identification

Egelkamp

Friedrich

Hertel

et al. 2020

Appl Microbiol Biotechnol

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Nitrilases are industrially important biocatalysts due to their ability to degrade nitriles to carboxylic acids and ammonia. In this study, a workflow for simple and fast recovery of nitrilase candidates from metagenomes is presented. For identification of active enzymes, a NADH-coupled high-throughput assay was established. Purification of enzymes could be omitted as the assay is based on crude extract containing the expressed putative nitrilases. In addition, long incubation times were avoided by combining nitrile and NADH conversion in a single reaction. This allowed the direct measurement of nitrile degradation and provided not only insights into substrate spectrum and specificity but also in degradation efficiency. The novel assay was used for investigation of candidate nitrilase-encoding genes. Seventy putative nitrilase-encoding gene and the corresponding deduced protein sequences identified during sequence-based screens of metagenomes derived from nitrile-treated microbial communities were analyzed. Subsequently, the assay was applied to 13 selected candidate genes and proteins. Six of the generated corresponding Escherichia coli clones produced nitrilases that showed activity and one unusual nitrilase was purified and analyzed. The activity of the novel arylacetonitrilase Nit09 exhibited a broad pH range and a high long-term stability. The enzyme showed high activity for arylacetonitriles with a K M of 1.29 mM and a V max of 13.85 U/mg protein for phenylacetonitrile. In conclusion, we provided a setup for simple and rapid analysis of putative nitrilase-encoding genes from sequence to function. The suitability was demonstrated by identification, isolation, and characterization of the arylacetonitrilase. Key points • A simple and fast high-throughput nitrilase screening was developed. • A set of putative nitrilases was successfully screened with the assay. • A novel arylacetonitrilase was identified, purified, and characterized in detail.

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Penicillin production in industrial strain Penicillium chrysogenum P2niaD18 is not dependent on the copy number of biosynthesis genes

Cited by 36 publications

References 48 publications

Comparative genomics of Alexander Fleming’s original Penicillium isolate (IMI 15378) reveals sequence divergence of penicillin synthesis genes

Comparative genomics of Alexander Fleming’s original Penicillium isolate (IMI 15378) reveals sequence divergence of penicillin synthesis genes

A Novel Seed-Dressing Formulation Based on an Improved Mutant Strain of Trichoderma virens, and Its Field Evaluation

From sequence to function: a new workflow for nitrilase identification

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