The Development of Metabolomic Sampling Procedures for Pichia pastoris, and Baseline Metabolome Data

Tredwell, Gregory D.; Edwards-Jones, Bryn; Leak, David J.; Bundy, Jacob G.

doi:10.1371/journal.pone.0016286

Cited by 53 publications

(36 citation statements)

References 34 publications

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“…For each sample, NMR spectra were phased, baseline corrected, and a line broadening function of 0.5 Hz was applied, following recommended Chenomx protocols and previously reported metabolomics analysis methods (Sun et al ., 2012; Tredwell et al ., 2011; Weljie et al ., 2006; Wu et al ., 2010). For metabolite identification, the Chenomx small molecule library for 600-MHz ( 1 H Larmor frequency) magnetic field strength NMR spectrometers was used, and NMR spectral patterns were fitted for each sample independently.…”

Section: Methodsmentioning

confidence: 99%

Untargeted metabolomics studies employing NMR and LC–MS reveal metabolic coupling between Nanoarcheum equitans and its archaeal host Ignicoccus hospitalis

et al. 2014

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Interspecies interactions are the basis of microbial community formation and infectious diseases. Systems biology enables the construction of complex models describing such interactions, leading to a better understanding of disease states and communities. However, before interactions between complex organisms can be understood, metabolic and energetic implications of simpler real-world host-microbe systems must be worked out. To this effect, untargeted metabolomics experiments were conducted and integrated with proteomics data to characterize key molecular-level interactions between two hyperthermophilic microbial species, both of which have reduced genomes. Metabolic changes and transfer of metabolites between the archaea Ignicoccus hospitalis and Nanoarcheum equitans were investigated using integrated LC-MS and NMR metabolomics. The study of such a system is challenging, as no genetic tools are available, growth in the laboratory is challenging, and mechanisms by which they interact are unknown. Together with information about relative enzyme levels obtained from shotgun proteomics, the metabolomics data provided useful insights into metabolic pathways and cellular networks of I. hospitalis that are impacted by the presence of N. equitans, including arginine, isoleucine, and CTP biosynthesis. On the organismal level, the data indicate that N. equitans exploits metabolites generated by I. hospitalis to satisfy its own metabolic needs. This finding is based on N. equitans’s consumption of a significant fraction of the metabolite pool in I. hospitalis that cannot solely be attributed to increased biomass production for N. equitans. Combining LC-MS and NMR metabolomics datasets improved coverage of the metabolome and enhanced the identification and quantitation of cellular metabolites.

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Section: Methodsmentioning

confidence: 99%

Untargeted metabolomics studies employing NMR and LC–MS reveal metabolic coupling between Nanoarcheum equitans and its archaeal host Ignicoccus hospitalis

et al. 2014

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“…As a result buffer additives have been employed to reduce metabolite leakage. 11 The commonly employed buffer additives are HEPES, 10,12 AMBIC, 13,14 tricine, 10,12,15 or NaCl. 16 Although the influence of these buffer additives in preserving the membrane integrity and therefore in minimising metabolite leakage is well studied for bacteria, 11,12,[17][18][19] fungi 20 and yeast, 10,15,21,22 they have not been as rigorously studied in mammalian cells.…”

Section: Introductionmentioning

confidence: 99%

Influence of washing and quenching in profiling the metabolome of adherent mammalian cells: a case study with the metastatic breast cancer cell line MDA-MB-231

Kapoore

Coyle

Staton

et al. 2017

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Metabolome characterisation is a powerful tool in oncology. To obtain a valid description of the intracellular metabolome, two of the preparatory steps are crucial, namely washing and quenching. Washing must effectively remove the extracellular media components and quenching should stop the metabolic activities within the cell, without altering the membrane integrity of the cell. Therefore, it is important to evaluate the efficiency of the washing and quenching solvents. In this study, we employed two previously optimised protocols for simultaneous quenching and extraction, and investigated the effects of a number of washing steps/solvents and quenching solvent additives, on metabolite leakage from the adherent metastatic breast cancer cell line MDA-MB-231. We explored five washing protocols and five quenching protocols (including a control for each), and assessed for effectiveness by detecting ATP in the medium and cell morphology changes through scanning electron microscopy (SEM) analyses. Furthermore, we studied the overall recovery of eleven different metabolite classes using the GC-MS technique and compared the results with those obtained from the ATP assay and SEM analysis. Our data demonstrate that a single washing step with PBS and quenching with 60% methanol supplemented with 70 mM HEPES (−50°C) results in minimum leakage of intracellular metabolites. Little or no interference of PBS (used in washing) and methanol/HEPES (used in quenching) on the subsequent GC-MS analysis step was noted. Together, these findings provide for the first time a systematic study into the washing and quenching steps of the metabolomics workflow for studying adherent mammalian cells, which we believe will improve reliability in the application of metabolomics technology to study adherent mammalian cell metabolism. IntroductionMammalian metabolomics has received increased attention in recent years mainly because of its potential in the prognosis and diagnosis of cancer and for assessing treatment efficacy by analysing cells, fluids or tissues for specific biomarkers in experimental, translational and clinical studies. Adherent mammalian cell-lines are used extensively in oncology research as preclinical models but to date there is insufficient information on the application of metabolomics for the analysis of cultured mammalian cell lines.1,2 To obtain reliable metabolomics data for adherent cells, an optimised workflow must be identified which will provide maximum coverage for all classes of metabolites with minimum leakage. Breast cancer (BC) is a highly heterogeneous cancer for which morphologically and clinically distinct subgroups of cell lines have been established. 3 Triple negative breast cancer (TNBC) is characterised by the absence of estrogen receptor (ER), progesterone receptor (PR) and lack of overexpression of human epidermal growth factor receptor (HER-2). TNBC represents approximately 20% of all BC and is typically associated with poor prognosis. Moreover, due to its aggressive phenotype, TNBC only partially res...

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“…The applicable sampling methods for yeasts' metabolome analysis are depending on the organism to be explored [37]. Recently, studies were carried out to develop a better protocol to extract metabolites from yeasts cells through different types of methods [2,[4][5][6].…”

Section: Metabolomics Studies In Komagataella Pastorismentioning

confidence: 99%

“…Tredwell et al [2] performed intracellular metabolite extraction using 4 different concentrations of methanol quenching solutions and compared each of them with the boiling ethanol extraction method as refer to Gonzalez et al [38]. The extracted metabolites were investigated by using both GCMS and 1 HNMR techniques.…”

Section: Metabolomics Studies In Komagataella Pastorismentioning

confidence: 99%

Metabolomics Study in Methylotrophic Yeast: A Minireview

Fam¹,

Sabri²,

Baharum³

et al. 2017

JLS

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Abstract:Methylotrophic yeast has been used as a cost-effective and valuable host for expression of recombinant protein due to its unique methanol utilisation pathway. It has an AOX (alcohol oxidase) protein which has been characterised to be a strong and tightly methanol-inducible dependent promoter. Metabolomics is the systematic study and inclusive analysis of small molecules called metabolites in a biological system. Metabolomics plays an important part in connecting the phenotype and genotype gap because it magnifies the modifications in the proteome and provides a better phenotype representation of an organism. This quantitative study has provided a new perception on the metabolic burden derived from the overexpression of recombinant protein in methylotrophic yeast. In this review, we discuss the fundamental aspect of metabolomics in methylotrophic yeast followed by their latest developments.

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The Development of Metabolomic Sampling Procedures for Pichia pastoris, and Baseline Metabolome Data

Cited by 53 publications

References 34 publications

Untargeted metabolomics studies employing NMR and LC–MS reveal metabolic coupling between Nanoarcheum equitans and its archaeal host Ignicoccus hospitalis

Untargeted metabolomics studies employing NMR and LC–MS reveal metabolic coupling between Nanoarcheum equitans and its archaeal host Ignicoccus hospitalis

Influence of washing and quenching in profiling the metabolome of adherent mammalian cells: a case study with the metastatic breast cancer cell line MDA-MB-231

Metabolomics Study in Methylotrophic Yeast: A Minireview

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