Metabolic impact of an NADH-producing glucose-6-phosphate dehydrogenase in Escherichia coli

Olavarría, Karel; Ingeniis, Jessica De; Zielinski, Daniel C.; Fuentealba, Matías; Muñoz, Rodrigo A.A.; McCloskey, Douglas; Feist, Adam M.; Cabrera, Ricardo

doi:10.1099/mic.0.082180-0

Cited by 18 publications

(26 citation statements)

References 56 publications

(66 reference statements)

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“…It has been shown previously that disrupting the gnd gene resulted in non appreciable changes to growth rate, but induces major changes in fluxes through the PPP and TCA cycle [1][2][3] . Similar observations have also been made of zwf mutants 4,5 , which demonstrate that metabolic networks can rapidly adjust enzyme level and flux without an appreciable cost to growth rate.…”

Section: Introductionsupporting

confidence: 72%

Growth adaptation ofgndandsdhCB Escherichia colideletion strains diverges from a similar initial perturbation of the transcriptome

McCloskey

Sandberg

et al. 2018

Preprint

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Adaptive laboratory evolution (ALE) has emerged as a new approach with which to pursue fundamental biological inquiries and, in particular, new insights into the systemic function of a gene product. Two E. coli knockout strains were constructed: one that blocked the Pentose Phosphate Pathway (gnd KO) and one that decoupled the TCA cycle from electron transport (sdhCDAB KO). Despite major perturbations in central metabolism, minimal growth rate changes were found in the two knockout strains. More surprisingly, many similarities were found in their initial transcriptomic states that could be traced to similarly perturbed metabolites despite the differences in the network location of the gene perturbations and concomitant rerouting of pathway fluxes around these perturbations. However, following ALE, distinct metabolomic and transcriptomic states were realized. These included divergent flux and gene expression profiles in the gnd and sdhCDAB KOs to overcome imbalances in NADPH production and nitrogen/sulfur assimilation, respectively, that were not obvious limitations of growth in the unevolved knockouts. Therefore, this work demonstrates that ALE provides a productive approach to reveal novel insights of gene function at a systems level that cannot be found by observing the fresh knockout alone.All rights reserved. No reuse allowed without permission.(which was not peer-reviewed) is the author/funder, who has granted bioRxiv a license to display the preprint in perpetuity.The copyright holder for this preprint . http://dx

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Section: Introductionsupporting

confidence: 72%

Growth adaptation ofgndandsdhCB Escherichia colideletion strains diverges from a similar initial perturbation of the transcriptome

McCloskey

Sandberg

et al. 2018

Preprint

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“…Because the genes gnd and zwf-2 are in the same operon, the activity of 6phosphogluconate dehydrogenase (GND) could indirectly indicate the expression of the protein encoded by zwf-2, annotated as another G6PDH. 13 C-labeling experiments had shown that the oxidative branch of the pentose-phosphate pathway is operative in P. putida KT2440 when glucose is the sole carbon source [2], so we decided to measure the activity of GND in the crude cellular extracts ( Table 3). The registered GND activities together with the biased estimations of E (Fig.…”

Section: Pputg6pdh-1 Is Not the Only Form Of G6pdh Expressed During Tmentioning

confidence: 99%

Quantifying NAD(P)H production in the upper Entner–Doudoroff pathway from Pseudomonas putida KT2440

et al. 2015

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“…However, this analysis involved considerably shorter simulations (0.5 ps), not intended to evaluate the stability of protein-ligand binding. In addition, we previously reported MD simulations of the dual Lm G6PDH with NAD + and NADP + , based on its crystallographic complexes [ 11 ]. In this enzyme, the R46 residue is homologous to R50 of Ec G6PDH ( Fig 6 ) and has been shown to perform an equivalent function in the interaction with the 2’-phosphate of NADP + [ 8 ].…”

Section: Discussionmentioning

confidence: 99%

“…coli enzyme and is important for interacting with the 2’-phosphate and the ribose-3’-hydroxyl group of NADP + . Interestingly, in opposition to Ec G6PDH, the simulations of the Lm G6PDH-NAD + complex showed that the ribose-adenine region was stable in its pocket, mainly because of stable hydrogen bonding with the main chain atoms of T14 and R46, together with a stabilizing interaction with the side chains of Q47 and T14 [ 11 ].…”

Section: Discussionmentioning

confidence: 99%

“…Particularly, complexes of Lm G6PDH with NADP + (PDB ID 1H9A), NAD + (PDB ID 1H94), NADPH and D-glucose (PDB ID 1E7Y) have provided information about the residues modulating the preference for both dinucleotides, which have also been evaluated by site-directed mutations. We recently published the effect of the double mutant R46E-Q47E on the cofactor preference of Lm G6PDH [ 11 ]. In fact, we demonstrated that the mutant performed as a specific NADH-producer in vivo .…”

Section: Introductionmentioning

confidence: 99%

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Determinants of Cofactor Specificity for the Glucose-6-Phosphate Dehydrogenase from Escherichia coli: Simulation, Kinetics and Evolutionary Studies

et al. 2016

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Glucose 6-Phosphate Dehydrogenases (G6PDHs) from different sources show varying specificities towards NAD+ and NADP+ as cofactors. However, it is not known to what extent structural determinants of cofactor preference are conserved in the G6PDH family. In this work, molecular simulations, kinetic characterization of site-directed mutants and phylogenetic analyses were used to study the structural basis for the strong preference towards NADP+ shown by the G6PDH from Escherichia coli. Molecular Dynamics trajectories of homology models showed a highly favorable binding energy for residues K18 and R50 when interacting with the 2'-phosphate of NADP+, but the same residues formed no observable interactions in the case of NAD+. Alanine mutants of both residues were kinetically characterized and analyzed with respect to the binding energy of the transition state, according to the kcat/KM value determined for each cofactor. Whereas both residues contribute to the binding energy of NADP+, only R50 makes a contribution (about -1 kcal/mol) to NAD+ binding. In the absence of both positive charges the enzyme was unable to discriminate NADP+ from NAD+. Although kinetic data is sparse, the observed distribution of cofactor preferences within the phylogenetic tree is sufficient to rule out the possibility that the known NADP+-specific G6PDHs form a monophyletic group. While the β1-α1 loop shows no strict conservation of K18, (rather, S and T seem to be more frequent), in the case of the β2-α2 loop, different degrees of conservation are observed for R50. Noteworthy is the fact that a K18T mutant is indistinguishable from K18A in terms of cofactor preference. We conclude that the structural determinants for the strict discrimination against NAD+ in the case of the NADP+-specific enzymes have evolved independently through different means during the evolution of the G6PDH family. We further suggest that other regions in the cofactor binding pocket, besides the β1-α1 and β2-α2 loops, play a role in determining cofactor preference.

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Metabolic impact of an NADH-producing glucose-6-phosphate dehydrogenase in Escherichia coli

Cited by 18 publications

References 56 publications

Growth adaptation ofgndandsdhCB Escherichia colideletion strains diverges from a similar initial perturbation of the transcriptome

Growth adaptation ofgndandsdhCB Escherichia colideletion strains diverges from a similar initial perturbation of the transcriptome

Quantifying NAD(P)H production in the upper Entner–Doudoroff pathway from Pseudomonas putida KT2440

Determinants of Cofactor Specificity for the Glucose-6-Phosphate Dehydrogenase from Escherichia coli: Simulation, Kinetics and Evolutionary Studies

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