The soil bacterium and platform strain Pseudomonas putida KT2440 has become the host of choice for metabolic engineering applications that require high levels of stress resistance and a robust, versatile metabolism (Nikel et al., ; Poblete‐Castro et al., ; Nikel and de Lorenzo, ). A dedicated synthetic biology toolbox is key to harness the full potential of this bacterium ― and strategies for tightly controlling gene expression are not only fundamental for understanding basic properties of the cell physiology and regulatory processes thereof, but they are also crucial for biotechnological applications (Gomez et al., ; Benedetti et al., ; Chavarría et al., ; Martínez‐García and de Lorenzo, ; Calero and Nikel, ). Gene expression systems offer the possibility to control when (and how much of) a target protein should be produced. Ideally, such systems should display two states (ON and OFF), enabling to temporally separate plasmid replication and maintenance (OFF) from an active state, when the gene of interest (GOI) is expressed and the encoded protein(s) is/are produced (ON) (Ter, ). In addition, since the accumulation of heterologous proteins is often accompanied by metabolic burden in the recombinant cells carrying the cognate gene construct (Wu et al., ), the ON and OFF states of the expression system should be clearly differentiated and externally controllable ― that is, the system should display very low levels (ideally, zero) of basal expression (leakiness) in the non‐induced, OFF state.

Transferring regulatory elements of gene expression devices across bacterial hosts is often accompanied by changes in the behaviour of the system, for example basal expression, fold change in expression levels between the induced and non‐induced state, and induction dynamics (Slusarczyk et al., ; Segall‐Shapiro et al., ). Expression systems traditionally used in the model host Escherichia coli (e.g. LacI^Q/P_trc), for instance, are known to display different characteristics when plugged‐in into a different bacterium ― with a much higher basal expression and lower induction fold in P. putida. Due to the versatile metabolism of Pseudomonas species, rich in degradation routes for alkane and aromatic compounds (Jiménez et al., ; Nikel et al., ,), several transcriptional regulators responsive to such substrates, along with the corresponding operator sites and other regulatory elements, have been sourced from these bacterial species. Transcriptional regulator/promoter pairs of this sort include, among many others, the (alkyl)benzoate(s)‐activated XylS/Pm system (de Lorenzo et al., ), the alkene(s)‐activated AlkS/P_alkB system (Panke et al., ), the xylene(s)‐responsive XylR/Pu system (Marqués and Ramos, ), the phenol‐inducible DmpR regulator (Shingler and Moore, ) and the salicylate‐activated NahR/P_sal system (Cebolla et al., ).

The XylS/Pm regulatory system originates from the catabolic megaplasmid pWW0 of P. putida mt‐2, where it controls the transcription of genes in the lower (meta) cleavage pathway for degradation of aromatic compounds (Ramos et al., ). Expression systems based on the XylS/Pm pair have been extensively adopted for both fundamental studies and metabolic engineering of Pseudomonas, because of its low basal expression, relatively high fold‐change induction, and the use of low‐cost inducers such as 3‐methylbenzoate (3‐mBz) and derivatives thereof (Gawin et al., ). In its native configuration, the XylS protein binds as a dimer to two operator sites (distal and proximal) closely upstream to the −35 motif of the Pm promoter, where it recruits the RNA polymerase with the σ³² or σ³⁸ factors (Marqués et al., ; González‐Pérez et al., ). The dimerization is promoted by 3‐mBz and related aromatic molecules, but it can also occur at high intracellular concentrations of XylS (Ruíz et al., ) ― albeit at a rate lower than that triggered by 3‐mBz. Furthermore, xylS is under control of a constitutive promoter and a xylene‐inducible promoter (Gallegos et al., ), ensuring synchronic expression of the long upper and lower TOL degradation pathway genes through a metabolic amplification motif (Silva‐Rocha et al., ). While this transcriptional wiring is beneficial in its natural context, it hampers its application in a heterologous milieu. Zwick et al. () showed that high xylS expression levels lead to increased basal Pm promoter activity and limited inducibility of the system by externally added effectors. Expression levels are likewise dependent on gene dosage: while the system is usually tightly controlled as a single‐copy genomic integration, basal expression dramatically increases with the copy number if the regulatory elements are plasmid‐borne. This situation helps explaining the significant discrepancies in the induction levels reported for the XylS/Pm system, ranging from ~10‐fold for medium copy number plasmids based on the origin of vegetative replication (oriV) pBBR1 in P. putida (Calero et al., ) to ~100‐fold for low copy number plasmids with oriV(RK2) in E. coli (Winther‐Larsen et al., ). The origins of replication commonly used in Pseudomonas display medium‐to‐high copy number levels [oriV(pBBR1) = 30 ± 7; oriV(RK2) = 20 ± 10; oriV(RSF1010) = 130 ± 40; and oriV(pRO1600/ColE1) ~30–40 (Jahn et al., ; Cook et al., )].

In order to enable better control of gene expression in Gram‐negative bacteria (and, in particular, in Pseudomonas species), in this study, we have re‐wired the functional elements of the XylS/Pm regulatory system (Fig. ) in combination with the recently described FENIX system for post‐translational control (Durante‐Rodríguez et al., ). By physically decoupling the xylS and Pm components, while rendering target protein(s) sensitive to conditional proteolysis, we have achieved a tightly controlled expression output of the system, with close‐to‐zero leakiness and in a plasmid copy number ― independent fashion.

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Scheme of tightly regulated expression systems for Pseudomonas based on physically decoupled XylS/Pm elements and conditional proteolysis.A. The trans‐module of the system, carrying the xylS regulator gene under transcriptional control of its native promoters, is flanked by the Tn7 recognitions sites borne by plasmid pTn7·xylS. The trans‐module is integrated into the host genome through the Tn7 transposase functions contained in the helper plasmid pTns2.B. Insertion of the cis‐module of the system into the vector of interest. The cis‐module is comprised of the distal and proximal XylS‐binding sites, followed by the −35 and −10 binding sites for the RNA polymerase. The whole module is 70‐bp long and can be easily introduced into any target vector through site‐directed mutagenesis PCR.C. A suitable plasmid carrying the cis‐module is delivered into a host Pseudomonas strain already containing the trans‐module integrated into the chromosome. The genomic integration of xylS in monocopy ensures low transcription levels of the regulator gene; upon addition of 3‐mBz as the inducer, XylS dimerizes and activates transcription from the Pm promoter.D. The trans‐module carrying the gene encoding the NIa protease under the transcriptional control of XylS/Pm is flanked by the Tn7 recognition sites borne by plasmid pTn7·X‐nia. This module is integrated into the host genome through the Tn7 transposase functions contained in the helper plasmid pTns2.E. Insertion of the Pm promoter and the 3′‐tag for conditional proteolysis to a gene of interest.F. The constructed plasmid (carrying the cis‐module) is delivered into a host Pseudomonas strain already containing the trans‐module in the chromosome. The inducer 3‐mBz promotes dimerization of XylS and, consequently, triggers transcription from the Pm promoter. Note that the Pm promoter drives the transcription of the gene of interest as well as that of nia. Only if both gene products are present in sufficient amounts, they will interact and the target protein is then relieved from the proteolysis tag – thereby enabling stable accumulation of the product. The abbreviations used in this scheme are as follows: 3‐mBz, 3‐methylbenzoate; GOI, gene of interest; NIa, nuclear inclusion protein A.

After observing high basal expression stemming from the XylS/Pm system in plasmid‐based systems, we set out to characterize this expression system on different standard vectors (i.e. carrying different oriV and hence displaying diverse copy numbers) to gain insight in the regulation of the transcriptional response. In order to investigate the consequences of copy number on the behaviour of the XylS/Pm system, plasmids with different copy numbers were constructed (Table ), containing the gene encoding msfGFP under the transcriptional control of XylS/Pm. Plasmids pS238·GFP and pS248·GFP were constructed following the Standard European Vector Architecture (SEVA; Silva‐Rocha et al., ; Martínez‐García et al., ) by amplification of msfGFP from pSEVA237M (Table ) with the primer pair gfp_RBS‐F and gfp‐R (Table ) and ligation of the DNA fragment into the SpeI and AvrII‐digested vectors pSEVA238 and pSEVA248. The msfGFP fluorescence (λ excitation = 485 nm, λ emission = 516 nm) was determined during cultivation of the cells in M9 minimal medium (Nikel et al., ,) supplemented with 0.2% (w/v) citrate at 30°C in a 96‐well plate (Synergy H1, BioTek). The expression strength of msfGFP was estimated from the change of fluorescence divided by the change of optical density at 600 nm.

Interestingly, higher copy number correlated with elevated maximum expression of msfGFP under the XylS/Pm system, but inducibility (i.e. the fold‐change difference between the induced and uninduced state) also decreased drastically. In particular, we observed a nine and threefold change in the ratio of induced/uninduced states when P. putida was expressing msfGFP from plasmid pS238·GFP or pS248·GFP respectively. This result is in accordance to the functional model of the XylS regulator proposed by Zwick et al. (), indicating that the formation of XylS dimers depends on inducer concentration at low XylS concentration, while at higher XylS availability, active regulator dimers can be formed even without inducer. Furthermore, this model points that the active XylS dimer concentration seems to be limited by its low solubility in the cell cytoplasm.

Against this background, and in order to uncouple the copy number of xylS (hence, the intracellular concentration of XylS) from msfGFP under the transcriptional control of Pm, xylS was integrated into the chromosome by using the Tn7‐bearing plasmid pTn7·xylS. For the construction of plasmid pTn7·xylS, the fragment contain xylS was amplified from plasmid pS238·nia with the primer pair xylS·pTn7‐F and xylS·pTn7‐R (Table ), and vector pTn7‐M was amplified with the primer pair pTn7·xylS‐F and pTn7·xylS‐R. These DNA fragments were then merged in a USER assembly reaction. Furthermore, plasmids pS23·Pm‐GFP and pS24·Pm‐GFP (which contain msfGFP under the control of Pm, but do not carry xylS) were constructed in parallel. This set of plasmids were obtained by site‐directed mutagenesis PCR of plasmids pSEVA237M and pSEVA247M with the primers Pm_ins‐F and Pm_ins‐R (Table ). A P. putida strain, carrying xylS integrated into the genome, and transformed with either plasmid pS23·Pm‐GFP (in which the oriV is pBBR1) or pS24·Pm‐GFP (in which the oriV is RO1600/ColE1) showed inducibility levels of 170 and 84‐fold when compared to control experiments without 3‐mBz respectively. In these uncoupled systems, the basal expression strength decreased more than the induced expression strength. On the other hand, it was observed that the maximum expression strength decreased, likely because XylS is produced at subsaturation concentrations with respect to activation of Pm. It is also possible that the basal expression of the GOI decreased due to a lower amount of available XylS (which would dimerize without inducer if its concentration reaches a certain threshold). Even though the uncoupling strategy led to a drastic improvement in the inducibility of the XylS/Pm expression system, some degree of basal (i.e. leaky) expression was still detected.

In order to reduce basal expression further, we set to design a system in which not only xylS and Pm copy numbers are controlled by physical uncoupling, but also expression of the GOI was further controlled by post‐translational degradation control. Plasmids pS23·Pm‐GFP* and pS24·Pm‐GFP* were constructed through site‐directed mutagenesis PCR using plasmids pS23·Pm‐GFP and pS24·Pm‐GFP respectively, as the template and primers ssr_nia_F and ssr_nia‐R (Table ). The msfGFP used in our experiments appears to be an excellent reporter for post‐translational control, as it is very stable and therefore tends to accumulate in the cells (Pedelacq et al., ). The gene encoding the nuclease NIa was integrated through the use of the plasmid pTn7·X‐nia. For the construction of plasmid pTn7·X‐nia, the fragment containing xylS/Pm→nia was amplified from plasmid pS238·NIa with the primer pair xylS·pTn7‐F and nia·pTn7‐R (Table ), and plasmid pTn7‐M was amplified with the primer pair pTn7·nia‐F and pTn7·xylS‐R. These fragments were then merged in a USER assembly reaction as indicated above.

The expression system employing transcriptional and post‐translational control over the expression of msfGFP showed lower expression levels when induced as compared with the expression system without post‐translational control (Fig. ). This phenomenon could be caused by the presence of additional XylS binding sites (in the Pm promoter of the integration), which recruit active XylS dimers and hence lowers the actual concentration of free XylS dimers, which can then bind to the plasmid‐borne XylS binding sites. Interestingly, no basal expression was observed with either plasmid, which leads to close‐to‐zero levels of leaky expression in the absence of 3‐mBz and, at the same time, yielded the highest (indicated as ∞ in Fig. B) inducibility of the system.

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Characterization of the tightly regulated expression systems for Pseudomonas based on physically decoupled XylS/Pm elements and conditional proteolysis.A. M9 minimal medium plates with 0.2% (w/v) citrate, containing 0 mM (left) or 1 mM (right) 3‐methylbenzoate (3‐mBz) were seeded with P. putida with an empty Tn7 module integrated into the chromosome and transformed with either vector pSEVA231 or vector pSEVA241, which served as negative controls (indicated as Empty in the figure). The same strain was transformed either with plasmid pS238·GFP or pS248·GFP carrying the XylS/Pm expression system in its original configuration (indicated as XylS/Pm in the figure). Strain KT·P, containing a chromosomal copy of xylS, was transformed either with plasmid pS23·Pm‐GFP or pS24·Pm‐GFP, in which the xylS/Pm system has been physically decoupled (indicated as DC in the figure). Strain KT·PN, containing a single xylS/Pm→nia integration in the chromosome, was transformed either with plasmid pS23·Pm‐GFP* or pS24·Pm‐GFP* harbouring the decoupled xylS/Pm system and equipped with conditional proteolytic control of GFP due to inducible nia expression (indicated as DC/NIa in the figure). Strains harbouring plasmids pS24x (x represents any of the variants described above) carrying the origin of vegetative replication (oriV) pRO1600/ColE1 were seeded in the upper part of the plate, while strains harbouring the plasmids pS23x, carrying oriV(pBBR1), were seeded in the lower part. Plates were incubated at 30°C for 18 h. The plates were visualized under blue light (Safe‐Imager, Invitrogen) and photographed.B. The increase in msfGFP fluorescence per unit of biomass (estimated as the optical density at 600 nm) relative to the negative control was measured during cultivation in M9 minimal medium containing 0.2% (w/v) citrate supplemented or not with 3‐mBz at 1 mM (upper part) and the resulting expression fold changes (lower part). Depicted in the diagram are the genetic elements either integrated into the single Tn7 integration site in the chromosome or plasmid‐borne. Bars represent the mean values of the corresponding parameter ± standard deviation (n ≥ 3 in all cases), and a Student t‐test revealed significant differences between all groups. Note that in some cases the level of msfGFP fluorescence of control experiments was below the limit of detection; in these experiments (DC/NIa), the ratio between induced and uninduced conditions is indicated with a ∞ symbol.

In this work, we have demonstrated how the repurposing of a classical gene expression system by means of the physical separation of xylS and Pm can lead to much higher induction fold changes compared with the systems carrying xylS and Pm on the same vector. The phenomenon underlying the results observed in our uncoupled system could be connected to the data reported by Goñi‐Moreno et al. (), indicating that the proximity of a source (i.e. XylS) and target (i.e. Pm promoter) elements dictates noise patterns of the expression system. Furthermore, the dual transcriptional and post‐translational control of the gene expression flow in our system reduced basal expression down to undetectable amounts of msfGFP caused by leaky expression of the GOI thereof. Since the expression of xylS might be too low to reach saturation of the Pm promoter by active XylS dimers upon addition of the chemical inducer, the final output of the system was lower than in the plasmid‐based counterpart. If stronger gene expression is desired, the system could be further improved through the implementation of engineered xylS and/or variants of the Pm promoter (Bakke et al., ; Vee Aune et al., ; Zwick et al., ). In any case, for applications where tight control over gene expression is crucial, the modular expression systems presented here offer a solid alternative that can be easily implemented into virtually any combination of vectors and GOIs (and Gram‐negative bacterial hosts). In particular, the synthetic systems discussed in this article constitute a valuable tool for maintaining low leaky expression of genes involved in pathways leading to toxic intermediates or products (a classical problem in metabolic engineering), and for the design of circuits in which the transcriptional output of a given system is ‘cascaded’ into another signal, thereby multiplying the tightness of the transcriptional regulation thereof.

We are indebted to Belén Calles (CNB‐CSIC, Madrid, Spain) for sharing research materials and fruitful discussions. The financial support from The Novo Nordisk Foundation (NNF10CC1016517) and from the European Union's Horizon2020 Research and Innovation Programme under grant agreement No. 814418 (SinFonia) to P.I.N. is gratefully acknowledged. J.T. and V.M. are the recipients of a fellowship from the Novo Nordisk Foundation as part of the Copenhagen Bioscience Ph.D. Programme, supported through grant NNF 18CC0033664. The responsibility of this article lies with the authors. The NNF and the European Union are not responsible for any use that may be made of the information contained therein.

None declared.