A Pseudomonas putida Strain Genetically Engineered for 1,2,3-Trichloropropane Bioremediation

Samin, Ghufrana; Pavlová, Martina; Arif, Muhammad I.; Postema, Christiaan P.; Damborský, Jiřı́; Janssen, Dick B.

doi:10.1128/aem.01620-14

Cited by 46 publications

(35 citation statements)

References 51 publications

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“…The biodegradation activity of engineered P. putida in spiked soil (autoclaved soil and natural soil containing microbial flora) on oil biodegradation showed oil removal compared to wildtype group was increased statistically significant. In the recent study by Samin et al 2014 genetically engineered P. putida via cloning of dehalogenase gene (dhaA31) generated for evaluation the 1,2,3-Trichloropropane (TCP) degradation activity (36). Same to the findings of the present study PAH compound in oil and chlorinated hydrocarbon can effectively biocatalyst by GEMs.…”

Section: Discussionsupporting

confidence: 60%

Application of Genetically Engineered Dioxygenase Producing Pseudomonas putida on Decomposition of Oil from Spiked Soil

Mardani

Mahvi

Hashemzadeh‐Chaleshtori

et al. 2017

Jundishapur J Nat Pharm Prod

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Background: It is well known that bioremediation or using microorganism enzymes plays an important role in decomposition and changing of oil pollutants and PAH compounds into nonhazardous or less-hazardous substances. The genetically manipulated bacteria like Pseudomonas sp. can enhancement the natural biodegradation activity of polycyclic aromatic hydrocarbons (PAHs) in polluted cities. Pseudomonas putida (P. putida) is a saprotrophic soil bacterium that is found throughout various environments such as soil and freshwater environments. Oil and petroleum industries are important exposure of PAHs in environment that strongly associated with the development of human cancers. Objectives: In the present work, P. putida was genetically manipulated for the biodegradation of oil in spiked soil and its activity was measured using the high-performance liquid chromatography (HPLC) method. Methods: The catechol 2,3-dioxygenase (C23O) encoded gene (nahH) was cloned into pUC18 for generating pUC18-nahH. This recombinant vector was transferred into P. putida, successfully, and both wild type and genetically modified P. putida were inoculated in spiked soil with oil for pilot plan preparation. Then, biodegradation activity of this bacterium on the elimination of phenanthrene and pyrene as an oil indicator in spiked soil were evaluated by the HPLC measurement technique. Results:The results showed the biodegradation of these PAH compounds in oil-spiked soil by genetically manipulated P. putida in both groups (containing autoclaved soil and dish containing natural soil) comparing to the inoculated group by wild type of P. putida were statistically significant (P < 0.05). Finally, confirmatory tests (catalase, oxidase, and PCR) were accomplished on isolated bacteria from spiked soil and were indicated that engineered P. putida was alive and functional by producing the C23O enzyme for biodegradation activity of oil. Conclusions: These findings demonstrated a degradable strain of P. putida that was generated in this study by genetic engineering can be useful to assess biodegradation of PAHs compounds in oil and petrochemical pollutions.

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Section: Discussionsupporting

confidence: 60%

Application of Genetically Engineered Dioxygenase Producing Pseudomonas putida on Decomposition of Oil from Spiked Soil

Mardani

Mahvi

Hashemzadeh‐Chaleshtori

et al. 2017

Jundishapur J Nat Pharm Prod

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“…Given these abilities, it is no surprise that the solvent tolerant strains of the Pseudomonads are often used for the bioremediation of toxic organic solvents like 1,2,3 trichlorpropane (Samin et al, 2014) or biocatalytic transformations of aromatic hydrocarbons like the epoxidation of styrene (Volmer et al, 2014) (reviewed in (Poblete-Castro et al, 2012)). Strains of the Pseudomonads are also used for the de novo production of aromatic hydrocarbons like p-hydroxybenzoic acid (Verhoef et al, 2007) and p-coumarate (Nijkamp et al, 2007).…”

Section: Hydrocarbonsmentioning

confidence: 99%

Efflux systems in bacteria and their metabolic engineering applications

Jones

Lozada

Pfleger

2015

Appl Microbiol Biotechnol

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The production of valuable chemicals from metabolically engineered microbes can be limited by excretion from the cell. Efflux is often overlooked as a bottleneck in metabolic pathways, despite its impact on alleviating feedback inhibition and product toxicity. In the past, it has been assumed that endogenous efflux pumps and membrane porins can accommodate product efflux rates, however, there are an increasing number of examples wherein overexpressing efflux systems is required to improve metabolite production. In this review, we highlight specific examples from the literature where metabolite export has been studied to identify unknown transporters, increase tolerance to metabolites, and improve the production capabilities of engineered bacteria. The review focuses on the export of a broad spectrum of valuable chemicals including amino acids, sugars, flavins, biofuels and solvents. The combined set of examples supports the hypothesis that efflux systems can be identified and engineered to confer export capabilities on industrially relevant microbes.

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“…18 Consequently, the design of enzymes and pathways that would allow organisms to degrade or even recycle TCP was investigated by different groups, with results that convincingly showed that biodegradation can be achieved. 19,20 The results of this work provide insight in the causes of success and failure as well as provide indications for future directions.…”

Section: Introductionmentioning

confidence: 93%

“…The DhaA31 variant 57 was introduced in the 2,3-dichloro-1propanol degrader Pseudomonas MC4 61 using chromosomal integration instead of a plasmid and without co-introduction of an antibiotic resistance marker or plasmid mobilization genes. 20 Insertion into the chromosome looks more attractive for bioremediation applications, and should relieve concerns related to distribution in the environment of genes encoding engineered enzymes or antibiotic resistance proteins. The Pseudomonas MC4 host was obtained earlier by classical enrichment with 2,3-dichloro-1-propanol from a site in the Botlek area mentioned above.…”

Section: Engineering Tcp Degrading Enzymes and Organismsmentioning

confidence: 99%