Positively regulated bacterial expression systems

Brautaset, Trygve; Lale, Rahmi; Valla, Svein

doi:10.1111/j.1751-7915.2008.00048.x

Cited by 73 publications

(66 citation statements)

References 133 publications

(254 reference statements)

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“…Moreover, in E. coli, the regulatory system of the rhaB promoter comprising RhaS, RhaR, and CRP is applied to the heterologous expression system, in which the expression of the target gene situated downstream of the rhaB promoter is capable of being strictly controlled by the addition of rhamnose or glucose (53). Similarly to this, it is possible that, in the cells of B. subtilis and related species, the expression of the introduced gene under the control of the rhaEW promoter can be finely regulated by RhaR and CcpA in the presence of rhamnose or glucose.…”

Section: Discussionmentioning

confidence: 99%

Regulation of the rhaEWRBMA Operon Involved in l -Rhamnose Catabolism through Two Transcriptional Factors, RhaR and CcpA, in Bacillus subtilis

et al. 2016

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The Bacillus subtilis rhaEWRBMA (formerly yuxG-yulBCDE) operon consists of four genes encoding enzymes for L-rhamnose catabolism and the rhaR gene encoding a DeoR-type transcriptional regulator. DNase I footprinting analysis showed that the RhaR protein specifically binds to the regulatory region upstream of the rhaEW gene, in which two imperfect direct repeats are included. Gel retardation analysis revealed that the direct repeat farther upstream is essential for the high-affinity binding of RhaR and that the DNA binding of RhaR was effectively inhibited by L-rhamnulose-1-phosphate, an intermediate of L-rhamnose catabolism. Moreover, it was demonstrated that the CcpA/P-Ser-HPr complex, primarily governing the carbon catabolite control in B. subtilis, binds to the catabolite-responsive element, which overlaps the RhaR binding site. In vivo analysis of the rhaEW promoter-lacZ fusion in the background of ccpA deletion showed that the L-rhamnose-responsive induction of the rhaEW promoter was negated by the disruption of rhaA or rhaB but not rhaEW or rhaM, whereas rhaR disruption resulted in constitutive rhaEW promoter activity. These in vitro and in vivo results clearly indicate that RhaR represses the operon by binding to the operator site, which is detached by L-rhamnulose-1-phosphate formed from L-rhamnose through a sequence of isomerization by RhaA and phosphorylation by RhaB, leading to the derepression of the operon. In addition, the lacZ reporter analysis using the strains with or without the ccpA deletion under the background of rhaR disruption supported the involvement of CcpA in the carbon catabolite repression of the operon. IMPORTANCESince L-rhamnose is a component of various plant-derived compounds, it is a potential carbon source for plant-associating bacteria. Moreover, it is suggested that L-rhamnose catabolism plays a significant role in some bacteria-plant interactions, e.g., invasion of plant pathogens and nodulation of rhizobia. Despite the physiological importance of L-rhamnose catabolism for various bacterial species, the transcriptional regulation of the relevant genes has been poorly understood, except for the regulatory system of Escherichia coli. In this study, we show that, in Bacillus subtilis, one of the plant growth-promoting rhizobacteria, the rhaEWRBMA operon for L-rhamnose catabolism is controlled by RhaR and CcpA. This regulatory system can be another standard model for better understanding the regulatory mechanisms of L-rhamnose catabolism in other bacterial species. Bacillus subtilis is a soil-dwelling bacterium that has been extensively and closely studied as a Gram-positive model bacterium. B. subtilis species have often been isolated from the rhizosphere of various terrestrial plants; many of them have been shown to be plant growth-promoting rhizobacteria whose association with the plant roots enhances the adaptive potential of plants and increases their growth (1). Interestingly, B. subtilis is also a saprophytic bacterium that secretes various degrading enzymes, incl...

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Section: Discussionmentioning

confidence: 99%

Regulation of the rhaEWRBMA Operon Involved in l -Rhamnose Catabolism through Two Transcriptional Factors, RhaR and CcpA, in Bacillus subtilis

et al. 2016

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“…Furthermore, the extent of expression from the lactate dehydrogenase (ldhA) promoter used in these examples is influenced by the redox conditions associated with the transition from aerobic to anaerobic growth, which may not be universally useful (Bartosiak-Jentys et al, 2012). Positively regulated protein expression systems in bacteria are common and rely on gene expression controlled by inducible promoters (Brautaset et al, 2009). Such promoters give tractable expression when induced with specific agents or conditions (e.g.…”

Section: Introductionmentioning

confidence: 99%

Modular system for assessment of glycosyl hydrolase secretion in Geobacillus thermoglucosidasius

et al. 2013

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“…The bottom line is that in the very competitive environments where these bacteria thrive, expression of extra genes must be tightly controlled for being triggered only when and where they are needed. This scenario is thus an excellent ground in which to mine pairs of transcriptional factors (TFs)/cognate chemical inducers which can be reformatted for creating new conditional expression systems (98). This approach is helping to overcome the dearth of alternative inducible devices for synthetic biology circuits (Fig.…”

Section: Expression Systemsmentioning

confidence: 99%

Mining Environmental Plasmids for Synthetic Biology Parts and Devices

2015

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The scientific and technical ambition of contemporary synthetic biology is the engineering of biological objects with a degree of predictability comparable to those made through electric and industrial manufacturing. To this end, biological parts with given specifications are sequence-edited, standardized, and combined into devices, which are assembled into complete systems. This goal, however, faces the customary context dependency of biological ingredients and their amenability to mutation. Biological orthogonality (i.e., the ability to run a function in a fashion minimally influenced by the host) is thus a desirable trait in any deeply engineered construct. Promiscuous conjugative plasmids found in environmental bacteria have evolved precisely to autonomously deploy their encoded activities in a variety of hosts, and thus they become excellent sources of basic building blocks for genetic and metabolic circuits. In this article we review a number of such reusable functions that originated in environmental plasmids and keep their properties and functional parameters in a variety of hosts. The properties encoded in the corresponding sequences include inter alia origins of replication, DNA transfer machineries, toxin-antitoxin systems, antibiotic selection markers, site-specific recombinases, effector-dependent transcriptional regulators (with their cognate promoters), and metabolic genes and operons. Several of these sequences have been standardized as BioBricks and/or as components of the SEVA (Standard European Vector Architecture) collection. Such formatting facilitates their physical composability, which is aimed at designing and deploying complex genetic constructs with new-to-nature properties.

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Positively regulated bacterial expression systems

Cited by 73 publications

References 133 publications

Regulation of the rhaEWRBMA Operon Involved in l -Rhamnose Catabolism through Two Transcriptional Factors, RhaR and CcpA, in Bacillus subtilis

Regulation of the rhaEWRBMA Operon Involved in l -Rhamnose Catabolism through Two Transcriptional Factors, RhaR and CcpA, in Bacillus subtilis

Modular system for assessment of glycosyl hydrolase secretion in Geobacillus thermoglucosidasius

Mining Environmental Plasmids for Synthetic Biology Parts and Devices

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