A Two-Enzyme Adaptive Unit within Bacterial Folate Metabolism

Schober, Andrew F; Mathis, Andrew D.; Ingle, Christine; Park, Junyoung O.; Chen, Li; Rabinowitz, Joshua D.; Junier, Ivan; Rivoire, Olivier; Reynolds, Kimberly A.

doi:10.1016/j.celrep.2019.05.030

Cited by 33 publications

(24 citation statements)

References 68 publications

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“…Perhaps not surprisingly, we found that pathways of adaptation to genetic inactivation of an antibiotic target provide a route to high levels of resistance. Likewise, a recent study also reported that E. coli cells challenged with increasing concentrations of trimethoprim in the presence of thymidine repeatedly evolved high levels of resistance by thyA loss-of-function mutations besides acquisition of commonly observed resistant mutations in DHFR (Schober et al, 2019). Strikingly, mutations in thyA are also known to confer trimethoprim resistance in bacterial clinical isolates of S. aureus (Chatterjee et al, 2008; Kriegeskorte et al, 2014), and H. influenza (Rodríguez-Arce et al, 2017), which emphasizes the need of laboratory studies of microbial adaptation as useful models to tackle serious global threat.…”

Section: Discussionmentioning

confidence: 93%

“…The most crucial factor in determining the fate of D27 mutant evolution appears to be the higher accessibility of mutational routes for inactivating thyA that lead to their fixation very early in the evolution experiment. Thymidylate synthase is the only known enzyme in E. coli able to synthetize dTMP de novo from dUMP, and inactivation of thyA inevitably commits the cell to thymine auxothrophy; reversion of DHFR function on the thyA - background is not expected to change this phenotype, as it is known that folA + thyA - strains are thymine-dependent (Bertino and Stacey, 1966; Schober et al, 2019). Competition between DHFR reversion and thyA inactivation thus appears to be decisive in determining the evolutionary solution.…”

Section: Discussionmentioning

confidence: 99%

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Adaptation to mutational inactivation of an essential gene converges to an accessible suboptimal fitness peak

Rodrigues

Shakhnovich

2019

eLife

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The mechanisms of adaptation to inactivation of essential genes remain unknown. Here we inactivate E. coli dihydrofolate reductase (DHFR) by introducing D27G,N,F chromosomal mutations in a key catalytic residue with subsequent adaptation by an automated serial transfer protocol. The partial reversal G27- > C occurred in three evolutionary trajectories. Conversely, in one trajectory for D27G and in all trajectories for D27F,N strains adapted to grow at very low metabolic supplement (folAmix) concentrations but did not escape entirely from supplement auxotrophy. Major global shifts in metabolome and proteome occurred upon DHFR inactivation, which were partially reversed in adapted strains. Loss-of-function mutations in two genes, thyA and deoB, ensured adaptation to low folAmix by rerouting the 2-Deoxy-D-ribose-phosphate metabolism from glycolysis towards synthesis of dTMP. Multiple evolutionary pathways of adaptation converged to a suboptimal solution due to the high accessibility to loss-of-function mutations that block the path to the highest, yet least accessible, fitness peak.

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Section: Discussionmentioning

confidence: 93%

Section: Discussionmentioning

confidence: 99%

Adaptation to mutational inactivation of an essential gene converges to an accessible suboptimal fitness peak

Rodrigues

Shakhnovich

2019

eLife

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“…Because DHFR 56 is known to progress through multiple conformational states during catalysis (Boehr, McElheny, 57 Dyson, & Wright, 2006;Sawaya & Kraut, 1997) (Figure S1), we expected the mutational 58 landscape of DHFR to be constrained by the requirement to adopt these different conformations. 59Moreover, prior work had suggested DHFR is impacted by cellular constraints such as protein 60 quality control (Bershtein, Mu, Serohijos, Zhou, & Shakhnovich, 2013) and the build-up of a 61 toxic metabolic intermediate (Schober et al, 2019). We hence expected deep mutational scanning 62 to reveal a highly constrained mutational landscape for DHFR that would contrast with the 63 mutational tolerance observed in other systems.…”

mentioning

confidence: 95%

“…Moreover, prior work had suggested DHFR is impacted by cellular constraints such as protein 60 quality control (Bershtein, Mu, Serohijos, Zhou, & Shakhnovich, 2013) and the build-up of a 61 toxic metabolic intermediate (Schober et al, 2019). We hence expected deep mutational scanning 62 to reveal a highly constrained mutational landscape for DHFR that would contrast with the 63 mutational tolerance observed in other systems.…”

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confidence: 95%

Modulating the cellular context broadly reshapes the mutational landscape of a model enzyme

Thompson

Zhang

Ingle

et al. 2019

Preprint

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20Protein mutational landscapes are shaped by the cellular environment, but key factors and their 21 quantitative effects are often unknown. Here we show that Lon, a quality control protease 22 naturally absent in common E. coli expression strains, drastically reshapes the mutational 23 landscape of the metabolic enzyme dihydrofolate reductase (DHFR). Selection under conditions 24 that resolve highly active mutants reveals that 23.3% of all single point mutations in DHFR are 25 advantageous in the absence of Lon, but advantageous mutations are largely suppressed when 26Lon is reintroduced. Protein stability measurements demonstrate extensive activity-stability 27 tradeoffs for the advantageous mutants and provide a mechanistic explanation for Lon's 28 widespread impact. Our findings suggest possibilities for tuning mutational landscapes by 29 modulating the cellular environment, with implications for protein design and combatting 30 antibiotic resistance. 31 & Ranganathan, 2011), we aimed first to measure a mutational landscape for DHFR and then to 55 determine how a change to the cellular environment might affect the landscape. Because DHFR 56 is known to progress through multiple conformational states during catalysis (Boehr, McElheny, 57 Dyson, & Wright, 2006;Sawaya & Kraut, 1997) (Figure S1), we expected the mutational 58 landscape of DHFR to be constrained by the requirement to adopt these different conformations. 59Moreover, prior work had suggested DHFR is impacted by cellular constraints such as protein 60 quality control (Bershtein, Mu, Serohijos, Zhou, & Shakhnovich, 2013) and the build-up of a 61 toxic metabolic intermediate (Schober et al., 2019). We hence expected deep mutational scanning 62 to reveal a highly constrained mutational landscape for DHFR that would contrast with the 63 mutational tolerance observed in other systems. 64 65 Results 66As the basis for our studies, we first sought to establish highly sensitive selection conditions for 67 DHFR function that would be calibrated to DHFR activity and capable of resolving mutants with 68 turnover rates near-to or faster-than wild-type. We anticipated that we would need to control 69 DHFR expression because two prior studies that modified the chromosomal DHFR gene had 70 reported an overall high mutational tolerance under permissive selection conditions that revealed 71 determinants of antibiotic resistance (Garst et al., 2017) and that DHFR expression can be 72 reduced to ~30% without a growth impact (Bershtein et al., 2013). We used an E. coli strain 73 derived from ER2566 with the genes for DHFR and a downstream enzyme, thymidylate 74 synthase, deleted in the genome and complemented on a pACYC-DUET plasmid with a weak 75 ribosome binding site (see Methods). To tightly control growth conditions, we performed 76 selections in a turbidostat to maintain the culture in early Log phase growth (Figure 1A, Figure 77

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“…DHFR also acts closely with TYMS-1 to recycle DHF back to THF. Notably, DHFR1 and TYMS1 are intimately linked as bifunctional enzymes in parasites, and copurify in plants, and together represent the rate-limiting enzymes for one carbon metabolism 15–17…”

Section: Resultsmentioning

confidence: 99%

Regulation of the one carbon folate cycle as a shared metabolic signature of longevity

Annibal

Tharyan

Schonewolff

et al. 2020

Preprint

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AbstractThe metabolome represents a complex network of biological events that reflects the physiologic state of the organism in heath and disease. Additionally, specific metabolites and metabolic signaling pathways have been shown to modulate animal ageing, but whether there are convergent mechanisms uniting these processes remains elusive. Here, we used high resolution mass spectrometry to obtain the metabolomic profiles of canonical longevity pathways in C. elegans and identify metabolites regulating life span. By leveraging the metabolomic profiles across pathways, we found that one carbon metabolism and the folate cycle were pervasively regulated in common. We observed similar changes in long lived mouse models of reduced insulin/IGF signaling. Genetic manipulation of pathway enzymes and supplementation with one carbon metabolites reveal that regulation of the folate cycle represents a shared causal mechanism of longevity and proteoprotection.

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A Two-Enzyme Adaptive Unit within Bacterial Folate Metabolism

Cited by 33 publications

References 68 publications

Adaptation to mutational inactivation of an essential gene converges to an accessible suboptimal fitness peak

Adaptation to mutational inactivation of an essential gene converges to an accessible suboptimal fitness peak

Modulating the cellular context broadly reshapes the mutational landscape of a model enzyme

Regulation of the one carbon folate cycle as a shared metabolic signature of longevity

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