Development of an Optimized LC-MS Method for the Detection of Specialized Pro-Resolving Mediators in Biological Samples

Kutzner, Laura; Rund, Katharina M.; Ostermann, Annika I.; Hartung, Nicole M.; Galano, Jean‐Marie; Balas, Laurence; Durand, Thierry; Balzer, Michael S.; David, Sascha; Schebb, Nils Helge

doi:10.3389/fphar.2019.00169

Cited by 67 publications

(85 citation statements)

References 74 publications

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“…In order to obtain the best results, they tried different compositions and gradients of the mobile phase [102]. Using a Zorbax Eclipse Plus C18 column with a diameter of particles less than 2 microns (150 × 2.1 mm, 1.8 µm; Agilent, Waldbronn, Germany) and an optimized gradient, Kutzner et al separated the maresin (Mar)1 and 7 (S)-Mar1 and protectin (N)PD1 and PDX stereoisomers from human serum and the results were comparable to those achieved by using a chiral column [103]. The high resolution power of approaches using these columns is usually used for separation of known isomers, not for identification of novel compounds.…”

Section: Chiral Chromatographymentioning

confidence: 88%

“…Various parameters such as source temperature (ST), collision energy (CE), declustering potential (DP), collision cell exit potential (CEP), collision activated dissociation (CAD), and gas pressure affect the signal intensity in the SRM mode. Simultaneously, caution should be taken with increasing the temperature of nebulizer gas as well as auxiliary gas, because the optimum temperature for some compounds may lead to the thermal degradation of others [103]. To obtain better detection limits and avoid interference from nearby isomers, at the last step of optimization, the most intense and specific fragments and transitions are usually chosen [101,103,163].…”

Section: Lc-ms/msmentioning

confidence: 99%

“…Simultaneously, caution should be taken with increasing the temperature of nebulizer gas as well as auxiliary gas, because the optimum temperature for some compounds may lead to the thermal degradation of others [103]. To obtain better detection limits and avoid interference from nearby isomers, at the last step of optimization, the most intense and specific fragments and transitions are usually chosen [101,103,163]. However, in the case of interference ions, it is better to select more characteristic rather than stronger fragmentation ions.…”

Section: Lc-ms/msmentioning

confidence: 99%

“…For example, when Yang et al developed a method for murine sera and BALF oxylipin profiling, for 8, 9 EET the weaker transition 319.2/123 was chosen, because the stronger transition 319.2/167 overlaps with the transition 319.2/167 for 11, 12 EET [101]. Also, to increase the sensibility of the MS method, the optimization of MS operating conditions should be carried out for each individual compound [15,69,103,131,164]. By the careful selection of transitions, it is possible to optimize sensitivity and selectivity so that the overall sensitivity will improve several times [85,101].…”

Section: Lc-ms/msmentioning

confidence: 99%

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Methods of the Analysis of Oxylipins in Biological Samples

et al. 2020

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Oxylipins are derivatives of polyunsaturated fatty acids and due to their important and diverse functions in the body, they have become a popular subject of studies. The main challenge for researchers is their low stability and often very low concentration in samples. Therefore, in recent years there have been developments in the extraction and analysis methods of oxylipins. New approaches in extraction methods were described in our previous review. In turn, the old analysis methods have been replaced by new approaches based on mass spectrometry (MS) coupled with liquid chromatography (LC) and gas chromatography (GC), and the best of these methods allow hundreds of oxylipins to be quantitatively identified. This review presents comparative and comprehensive information on the progress of various methods used by various authors to achieve the best results in the analysis of oxylipins in biological samples.

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Section: Chiral Chromatographymentioning

confidence: 88%

Section: Lc-ms/msmentioning

confidence: 99%

Section: Lc-ms/msmentioning

confidence: 99%

Section: Lc-ms/msmentioning

confidence: 99%

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Methods of the Analysis of Oxylipins in Biological Samples

et al. 2020

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“…Plasma concentrations of SAMPs, here SPM profiles, have also been measured using liquid chromatographytandem mass spectrometry (LC-MS) technology [49,50]. Of note, in a recently published evaluation of SPM profiles using an optimized LC-MS method for the detection of SPMs in biological samples, Kutzner et al [51] concluded, "SPMs were generally not detectable/quantifiable in plasma and serum of healthy individuals, while good recovery rates were found in spiked samples. These results strongly support findings that circulating levels of SPMs are very low, i.e., < 0.1 nM in healthy subjects.…”

Section: Plasma Concentration Of Hmgb1 S100 Proteins Circulating Dnmentioning

confidence: 99%

Use of DAMPs and SAMPs as Therapeutic Targets or Therapeutics: A Note of Caution

Land

2020

Mol Diagn Ther

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This opinion article discusses the increasing attention paid to the role of activating damage-associated molecular patterns (DAMPs) in initiation of inflammatory diseases and suppressing/inhibiting DAMPs (SAMPs) in resolution of inflammatory diseases and, consequently, to the future roles of these novel biomarkers as therapeutic targets and therapeutics. Since controlled production of DAMPs and SAMPs is needed to achieve full homeostatic restoration and repair from tissue injury, only their pathological, not their homeostatic, concentrations should be therapeutically tackled. Therefore, distinct caveats are proposed regarding choosing DAMPs and SAMPs for therapeutic purposes. For example, we discuss the need to a priori identify and define a context-dependent "homeostatic DAMP:SAMP ratio" in each case and a "homeostatic window" of DAMP and SAMP concentrations to guarantee a safe treatment modality to patients. Finally, a few clinical examples of how DAMPs and SAMPs might be used as therapeutic targets or therapeutics in the future are discussed, including inhibition of DAMPs in hyperinflammatory processes (e.g., systemic inflammatory response syndrome, as currently observed in , administration of SAMPs in chronic inflammatory diseases, inhibition of SAMPs in hyperresolving processes (e.g., compensatory antiinflammatory response syndrome), and administration/induction of DAMPs in vaccination procedures and anti-cancer therapy.

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