A Set of Active Promoters with Different Activity Profiles for Superexpressing <i>Rhodococcus</i> Strain

Shemyakina, A. O.; Grechishnikova, Elena G.; Novikov, A. D.; Asachenko, Andrey F.; Kalinina, Tatyana I; Lavrov, K. V.; Yanenko, A. S.

doi:10.1021/acssynbio.0c00508

Cited by 6 publications

(4 citation statements)

References 72 publications

(128 reference statements)

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“…Two growth phases were examined, as promoter activity can vary significantly with growth phase. 47 Of the tested promoters, P M6 , P tet , and P T1 were the strongest, although P M6 yielded ∼2.5−3 times greater fluorescence than the other two. We had identified P M6 previously and developed P T1 as a derivative.…”

Section: ■ Results and Discussionmentioning

confidence: 87%

“…Integrative promoter constructs were transformed into RHA1, and promoter activity was determined in mid exponential and early stationary phase by using fluorescence normalized to OD 600 as a readout (Figure C and D). Two growth phases were examined, as promoter activity can vary significantly with growth phase . Of the tested promoters, P M6 , P tet , and P T1 were the strongest, although P M6 yielded ∼2.5–3 times greater fluorescence than the other two.…”

Section: Results and Discussionmentioning

confidence: 99%

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An Integrative Toolbox for Synthetic Biology in Rhodococcus

2021

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The development of microbial cell factories requires robust synthetic biology tools to reduce design uncertainty and accelerate the design-build-test-learn process. Herein, we developed a suite of integrative genetic tools to facilitate the engineering of Rhodococcus, a genus of bacteria with considerable biocatalytic potential. We first created pRIME, a modular, copy-controlled integrative-vector, to provide a robust platform for strain engineering and characterizing genetic parts. This vector was then employed to benchmark a series of strong promoters. We found P M6 to be the strongest constitutive rhodococcal promoter, 2.5-to 3-fold stronger than the next in our study, while overall promoter activities ranged 23-fold between the weakest and strongest promoters during exponential growth. Next, we used an optimized variant of P M6 to develop hybrid-promoters and integrative vectors to allow for tetracycline-inducible gene expression in Rhodococcus. The best of the resulting hybrid-promoters maintained a maximal activity of ∼50% of P M6 and displayed an induction factor of ∼40-fold. Finally, we developed and implemented a uLoop-derived Golden Gate assembly strategy for high-throughput DNA assembly in Rhodococcus. To demonstrate the utility of our approaches, pRIME was used to engineer Rhodococcus jostii RHA1 to grow on vanillin at concentrations 10-fold higher than what the wild-type strain tolerated. Overall, this study provides a suite of tools that will accelerate the engineering of Rhodococcus for various biocatalytic applications, including the sustainable production of chemicals from lignin-derived aromatics.

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Section: ■ Results and Discussionmentioning

confidence: 87%

Section: Results and Discussionmentioning

confidence: 99%

An Integrative Toolbox for Synthetic Biology in Rhodococcus

2021

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“…Recently, a review on the advances in genetic toolkits and methods for engineering Rhodococcus has been published, and, in parallel, a set of Rhodococcus promoter-RBS combinations with fine-tuning of different activity levels have been built and compiled [35,45]. The Rhodococcus promoter regions described here can contribute to enrich the set of genetic parts for gene expression control in this strain.…”

Section: Promoter Cloning and Characterizationmentioning

confidence: 99%

“…The studies done with a series of R. ruber mutants (∆kshB and single, double and triple ∆kshA mutants) have probed that KshA2 isoform is needed for the degradation of steroid substrates with short side chain; KshA3 works on those molecules with longer side chains and KshA1 acts as a more versatile enzyme related to the cholic acid (ACHO) catabolism and collaborating with KshA2 or KshA3 activities [31]. Although these enzymes are important within the steroid catabolism, there are not many studies done on genetic regulation of these activities, just for KstD promoters [32], a partial study on Ksh2 in Rhodococcus erythropolis strain SQ1 [33] and general studies on Rhodococcus gene promoters [34,35]. The findings of how the steroid clusters are regulated could be useful in metabolic engineering of Rhodococcus strains.…”

Section: Introductionmentioning

confidence: 99%

Further Studies on the 3-Ketosteroid 9α-Hydroxylase of Rhodococcus ruber Chol-4, a Rieske Oxygenase of the Steroid Degradation Pathway

2021

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The biochemistry and genetics of the bacterial steroid catabolism have been extensively studied during the last years and their findings have been essential to the development of biotechnological applications. For instance, metabolic engineering of the steroid-eater strains has allowed to obtain intermediaries of industrial value. However, there are still some drawbacks that must be overcome, such as the redundancy of the steroid catabolism genes in the genome and a better knowledge of its genetic regulation. KshABs and KstDs are key enzymes involved in the aerobic breakage of the steroid nucleus. Rhodococcus ruber Chol-4 contains three kshAs genes, a single kshB gene and three kstDs genes within its genome. In the present work, the growth of R. ruber ΔkshA strains was evaluated on different steroids substrates; the promoter regions of these genes were analyzed; and their expression was followed by qRT-PCR in both wild type and ksh mutants. Additionally, the transcription level of the kstDs genes was studied in the ksh mutants. The results show that KshA2B and KshA1B are involved in AD metabolism, while KshA3B and KshA1B contribute to the cholesterol metabolism in R. ruber. In the kshA single mutants, expression of the remaining kshA and kstD genes is re-organized to survive on the steroid substrate. These data give insight into the fine regulation of steroid genes when several isoforms are present.

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