An expanded CRISPRi toolbox for tunable control of gene expression in <i>Pseudomonas putida</i>

Batianis, Christos; Kozaeva, Ekaterina; Damalas, Stamatios G.; Martín-Pascual, María; Volke, Daniel C.; Nikel, Pablo I.; Santos, Vítor A. P. Martins dos

doi:10.1111/1751-7915.13533

Cited by 51 publications

(49 citation statements)

References 78 publications

(99 reference statements)

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“…Furthermore, a dynamic regulation approach can be employed to balance the biochemical activities based on metabolite concentrations: CRISPR-interference [159][160][161] as well as conditional proteolysis systems [162] have been implemented in Pseudomonas and can be used to down-regulate biochemical functions leading up to the toxic intermediate (e.g. by coupling the output to a suitable expression system, biosensor or riboswitch).…”

Section: Engineering Of Optimal Flux In Cell Factories With Novel Pathwaysmentioning

confidence: 99%

Towards robust Pseudomonas cell factories to harbour novel biosynthetic pathways

Bitzenhofer

Kruse

Thies

et al. 2021

Essays in Biochemistry

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Biotechnological production in bacteria enables access to numerous valuable chemical compounds. Nowadays, advanced molecular genetic toolsets, enzyme engineering as well as the combinatorial use of biocatalysts, pathways, and circuits even bring new-to-nature compounds within reach. However, the associated substrates and biosynthetic products often cause severe chemical stress to the bacterial hosts. Species of the Pseudomonas clade thus represent especially valuable chassis as they are endowed with multiple stress response mechanisms, which allow them to cope with a variety of harmful chemicals. A built-in cell envelope stress response enables fast adaptations that sustain membrane integrity under adverse conditions. Further, effective export machineries can prevent intracellular accumulation of diverse harmful compounds. Finally, toxic chemicals such as reactive aldehydes can be eliminated by oxidation and stress-induced damage can be recovered. Exploiting and engineering these features will be essential to support an effective production of natural compounds and new chemicals. In this article, we therefore discuss major resistance strategies of Pseudomonads along with approaches pursued for their targeted exploitation and engineering in a biotechnological context. We further highlight strategies for the identification of yet unknown tolerance-associated genes and their utilisation for engineering next-generation chassis and finally discuss effective measures for pathway fine-tuning to establish stable cell factories for the effective production of natural compounds and novel biochemicals.

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Section: Engineering Of Optimal Flux In Cell Factories With Novel Pathwaysmentioning

confidence: 99%

Towards robust Pseudomonas cell factories to harbour novel biosynthetic pathways

Bitzenhofer

Kruse

Thies

et al. 2021

Essays in Biochemistry

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“… TF Promoter Inducer(s) Reported pros, cons and main applications in P. putida Ref. (s) Positively regulated induction systems XylS Pm m -toluate and derivatives + High expression levels + Extensively characterized + Cheap inducers − Catabolite repression − Dose-dependent response in absence of inducer metabolization pathways − Bimodal response − Leaky expression 28 , 49 , 63 , 130 – 139 Applications: Expression of I- sceI , dCas9 , trfA , the λ red operon, and recombinases in genome engineering tools; expression of toxic genes for controlled autolysis; production of recombinant antibody fragments and p -coumaric acid RhaRS P rhaB l -rhamnose + No catabolite repression + No metabolization of rhamnose: dose-dependent response + Tight regulation + Non-toxic inducer − Inhomogeneous response at intermediate inducer levels − Expensive inducers 132 , 138 , 140 , 141 Applications: Expression of dCas9 for CRISPRi and Cre for genomic deletions; production of p -coumaric acid AraC P BAD l -arabinose + Characterization + No catabolite repression + No metabolization of arabinose: dose-dependent response + Tight regulation + Non-toxic inducer − Inhomogeneous response at intermediate inducer levels − Poor arabinose uptake without AraE transporter − Expensive inducers 132 , 142 , 143 Applications: Production of p -coumaric acid Negatively regulated induction systems LacI Plac, PlacUV5, Ptac, Ptrc Lactose, isopropyl β...…”

Section: Constructing Novel Genetic Circuits: the Sum Is More Than Itmentioning

confidence: 99%

“…In some applications, the lack of a suitable repressor can be substituted by CRISPR interference (CRISPRi) technology 39 . This technology enables the simultaneous, tunable, and transient repression of multiple genes by expression of gene-specific sgRNAs and a single nuclease-deficient Cas9 (dCas9) and has been successfully applied in P. putida 49 , M. smegmatis 50 , K. pneumoniae 51 , B. subtilis 51 , and L. lactis 52 with up to 98% repression. Although this technique offers great potential, one must note that its efficiency and efficacy remains dependent on (1) the presence of a PAM sequence within or near the promoter region for efficient transcriptional repression, (2) the strengths and weaknesses of the expression system used for dCas9 expression, (3) the burden imposed by accumulation of a large heterologous protein (dCas9), and (4) polar effects such as the repression of downstream operons.…”

Section: Constructing Novel Genetic Circuits: the Sum Is More Than Itmentioning

confidence: 99%

Exploring the synthetic biology potential of bacteriophages for engineering non-model bacteria

2020

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Non-model bacteria like Pseudomonas putida, Lactococcus lactis and other species have unique and versatile metabolisms, offering unique opportunities for Synthetic Biology (SynBio). However, key genome editing and recombineering tools require optimization and large-scale multiplexing to unlock the full SynBio potential of these bacteria. In addition, the limited availability of a set of characterized, species-specific biological parts hampers the construction of reliable genetic circuitry. Mining of currently available, diverse bacteriophages could complete the SynBio toolbox, as they constitute an unexplored treasure trove for fully adapted metabolic modulators and orthogonally-functioning parts, driven by the longstanding co-evolution between phage and host.

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“…More recent innovative developments deal with recombineering methods, such as RecET-based markerless recombineering system for deletion and integration of large-sized genes and clusters (Choi and Lee 2020 ), efficient single-stranded recombineering by using a thermoinducible system (Aparicio et al 2020a ), as well as CRISPR/Cas9 technologies. The latter was utilized for efficient curing of helper plasmids (Wirth et al 2020 ), counterselection of infrequent mutations created through recombineering (Aparicio et al 2018 ), metabolic engineering for PHA bioconversion from ferulic acid (Zhou et al 2020 ), as well as CRISPR interference-mediated gene regulation (Batianis et al 2020 ; Kim et al 2020 ). The incredible pace of development of new tools leaves no doubt that there will be precise CRISPR-based technologies soon, speeding up genomic manipulations even further.…”

Section: Recent Advances In Genetic Engineeringmentioning

confidence: 99%

Industrial biotechnology of Pseudomonas putida: advances and prospects

Weimer

Kohlstedt

Volke

et al. 2020

Appl Microbiol Biotechnol

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136

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Pseudomonas putida is a Gram-negative, rod-shaped bacterium that can be encountered in diverse ecological habitats. This ubiquity is traced to its remarkably versatile metabolism, adapted to withstand physicochemical stress, and the capacity to thrive in harsh environments. Owing to these characteristics, there is a growing interest in this microbe for industrial use, and the corresponding research has made rapid progress in recent years. Hereby, strong drivers are the exploitation of cheap renewable feedstocks and waste streams to produce value-added chemicals and the steady progress in genetic strain engineering and systems biology understanding of this bacterium. Here, we summarize the recent advances and prospects in genetic engineering, systems and synthetic biology, and applications of P. putida as a cell factory. Key points • Pseudomonas putida advances to a global industrial cell factory. • Novel tools enable system-wide understanding and streamlined genomic engineering. • Applications of P. putida range from bioeconomy chemicals to biosynthetic drugs. Electronic supplementary material The online version of this article (10.1007/s00253-020-10811-9) contains supplementary material, which is available to authorized users.

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An expanded CRISPRi toolbox for tunable control of gene expression in Pseudomonas putida

Cited by 51 publications

References 78 publications

Towards robust Pseudomonas cell factories to harbour novel biosynthetic pathways

Towards robust Pseudomonas cell factories to harbour novel biosynthetic pathways

Exploring the synthetic biology potential of bacteriophages for engineering non-model bacteria

Industrial biotechnology of Pseudomonas putida: advances and prospects

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