Increased production of L-serine in Escherichia coli through Adaptive Laboratory Evolution

Mundhada, Hemanshu; Seoane, Jose Miguel; Schneider, Konstantin; Koza, Anna; Christensen, Hanne Bjerre; Klein, Tobias; Phaneuf, Patrick V.; Herrgård, Markus J.; Feist, Adam M.; Nielsen, Alex Toftgaard

doi:10.1016/j.ymben.2016.11.008

Cited by 121 publications

(144 citation statements)

References 52 publications

(74 reference statements)

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“…), but that it was due to a change in membrane tension that activated a mechanosensitive glutamate efflux pump encoded by a gene called NCgl1221 (a homologue of the E. coli yggB gene, now known as mscS, the mechanosensitive channel of small conductance) [84][85][86][87][88][89]. Similar efflux pumps are now known to be involved in the export of product during a variety of other amino acid fermentations [79,90], such as those for lysine [91][92][93][94][95], isoleucine [96,97], serine [98], threonine [99][100][101][102], cysteine [103], methionine [104], alanine [105] and others [103,106,107]. Thus, the general role of product exporters in enhancing fermentation yields (as per Figure 1) is clear [2,103,108].…”

Section: Role Of Efflux Transporters In Metabolic Flux Controlmentioning

confidence: 99%

Control of metabolite efflux in microbial cell factories: current advances and future prospects

Kell¹

2018

Preprint

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The yield and ease of purification of biotechnological products are typically greatly enhanced if they can be secreted into the external medium. Although not universally appreciated, however, small molecule biotechnological products do not ‘float across’ the phospholipid bilayer portion of biological membranes, and thus they need transporters to assist their passage into the extramembrane and extracellular spaces. Some of these transporters may be reversible, equilibrative transporters that might more normally be used for uptake, while others may have an efflux directionality imposed on them via suitable energy coupling mechanisms. Despite the energetic costs of small molecule synthesis, natural evolution does in fact provide a number of mechanisms by which the secretion of such products can actually enhance fitness. Where available these provide useful starting points, and assaying for such activities is crucial. In particular, in a systems biology approach, we first need to identify such/suitable activities before we can seek to increase them. They may then be improved through promoter engineering, via manipulation of control elements, or by directed evolution of the transporter proteins themselves. Modern methods of synthetic biology provide enormous opportunities for all kinds of efflux transporter engineering; they are just beginning to be realised.

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Section: Role Of Efflux Transporters In Metabolic Flux Controlmentioning

confidence: 99%

Control of metabolite efflux in microbial cell factories: current advances and future prospects

Kell¹

2018

Preprint

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“…Nowadays, methods for generation of sequence-variant libraries often include custom-designed DNA oligo library pools, multiplexed oligo assembly, or more or less randomized mutagenesis of template DNA fragments (Mutalik et al, 2013;Plesa et al, 2018;Yang et al, 2017). Screening and selection assays based on conditional growth, genetically-encoded biosensors, and reporter gene activities, has recently been applied to complement the efficiency of library generation Mundhada et al, 2016;Raman et al, 2014;Skjoedt et al, 2016). Irrespective of the origin of input library and the screening assays applied, when aiming to infer functional consequences of regulatory or genic DNA variants, it is important to acknowledge the impact of gene dosage and the genomic context of the gene encoding the protein of interest, as both overexpression and epigenetic regulation can impact downstream regulation arising from genetic variants when expressed from non-native plasmid-based cassettes or when using heterologous promoters (Gibson et al, 2013).…”

Section: Introductionmentioning

confidence: 99%

CasPER, a method for directed evolution in genomic contexts using mutagenesis and CRISPR/Cas9

Jakočiūnas

Pedersen

Lis

et al. 2018

Metabolic Engineering

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“…ALE has been applied to increasing chemical tolerance (Atsumi et al, 2010; Horinouchi et al, 2010; Mundhada et al, 2017; Reyes et al, 2012), rates of growth on diverse substrates (Cordova et al, 2016; Herring et al, 2006; Lee and Palsson, 2010; Sandberg et al, 2017), and gaining general insight into microbial responses to environmental or genetic perturbations (Charusanti et al, 2010; Fong and Palsson, 2004; Tenaillon et al, 2012). Following an ALE experiment, the resulting strains are sequenced to identify genetic mutations (Herring et al, 2006).…”

Section: Introductionmentioning

confidence: 99%

Fast growth phenotype of E. coli K-12 from adaptive laboratory evolution does not require intracellular flux rewiring

Long

Gonzalez

Feist

et al. 2017

Metabolic Engineering

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Adaptive laboratory evolution (ALE) is a widely-used method for improving the fitness of microorganisms in selected environmental conditions. It has been applied previously to Escherichia coli K-12 MG1655 during aerobic exponential growth on glucose minimal media, a frequently used model organism and growth condition, to probe the limits of E. coli growth rate and gain insights into fast growth phenotypes. Previous studies have described up to 1.6-fold increases in growth rate following ALE, and have identified key causal genetic mutations and changes in transcriptional patterns. Here, we report for the first time intracellular metabolic fluxes for six such adaptively evolved strains, as determined by high-resolution 13C-metabolic flux analysis. Interestingly, we found that intracellular metabolic pathway usage changed very little following adaptive evolution. Instead, at the level of central carbon metabolism the faster growth was facilitated by proportional increases in glucose uptake and all intracellular rates. Of the six evolved strains studied here, only one strain showed a small degree of flux rewiring, and this was also the strain with unique genetic mutations. A comparison of fluxes with two other wild-type (unevolved) E. coli strains, BW25113 and BL21, showed that inter-strain differences are greater than differences between the parental and evolved strains. Principal component analysis highlighted that nearly all flux differences (95%) between the nine strains were captured by only two principal components. The distance between measured and flux balance analysis predicted fluxes was also investigated. It suggested a relatively wide range of similar stoichiometric optima, which opens new questions about the path-dependency of adaptive evolution.

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Increased production of L-serine in Escherichia coli through Adaptive Laboratory Evolution

Cited by 121 publications

References 52 publications

Control of metabolite efflux in microbial cell factories: current advances and future prospects

Control of metabolite efflux in microbial cell factories: current advances and future prospects

CasPER, a method for directed evolution in genomic contexts using mutagenesis and CRISPR/Cas9

Fast growth phenotype of E. coli K-12 from adaptive laboratory evolution does not require intracellular flux rewiring

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