Difference between revisions of "MFQL library"

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(MFQL used in [3] for identification of Lipids in human blood plasma)
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E. coli total lipid extract was purchased from Avanti Polar Lipids (Alabaster, AL, USA) and analyzed on the LTQ Orbitrap XL instrument in negative ion mode. A solution of the total lipid concentration of 2.5 μg/ml in 7.5 mM ammonium acetate in choloroform/methanol/2-propanol (1/2/4, v/v/v) was infused into the mass spectrometer by TriVersa robotic ion source using a chip with the diameter of spraying nozzles of 4.1 μm. To produce the spectra dataset, the extract was analyzed in several independent experiments: experiment I, eight acquisitions under the unit mass resolution (R) settings using ion trap (IT) to acquire both MS and MS/MS spectra; experiment II, six acquisitions with R = 7,500 for MS spectra (Orbitrap) and unit resolution for MS/MS spectra (IT); experiment III, four acquisitions with R = 30,000 for MS spectra (Orbitrap) and unit resolution for MS/MS spectra (IT); experiment IV, four acquisitions with R = 100,000 for MS spectra (Orbitrap) and unit resolution for MS/MS spectra (IT); experiment V, seven acquisitions with R = 100,000 for MS spectra (Orbitrap) and R = 15,000 for MS/MS spectra (Orbitrap). MS/MS experiments were performed using Pulsed Q Collision Induced Dissociation(PQD).
 
E. coli total lipid extract was purchased from Avanti Polar Lipids (Alabaster, AL, USA) and analyzed on the LTQ Orbitrap XL instrument in negative ion mode. A solution of the total lipid concentration of 2.5 μg/ml in 7.5 mM ammonium acetate in choloroform/methanol/2-propanol (1/2/4, v/v/v) was infused into the mass spectrometer by TriVersa robotic ion source using a chip with the diameter of spraying nozzles of 4.1 μm. To produce the spectra dataset, the extract was analyzed in several independent experiments: experiment I, eight acquisitions under the unit mass resolution (R) settings using ion trap (IT) to acquire both MS and MS/MS spectra; experiment II, six acquisitions with R = 7,500 for MS spectra (Orbitrap) and unit resolution for MS/MS spectra (IT); experiment III, four acquisitions with R = 30,000 for MS spectra (Orbitrap) and unit resolution for MS/MS spectra (IT); experiment IV, four acquisitions with R = 100,000 for MS spectra (Orbitrap) and unit resolution for MS/MS spectra (IT); experiment V, seven acquisitions with R = 100,000 for MS spectra (Orbitrap) and R = 15,000 for MS/MS spectra (Orbitrap). MS/MS experiments were performed using Pulsed Q Collision Induced Dissociation(PQD).
  
The below listed MFQL files can be applied for all mass spectrometric settings. The mass spectrometric settings are saved in the *ini file utilized for the import of a dataset.[[File:lpdX_benchmark.txt]] ('''IMPORTANT:''' for usage in LipidXplorer please rename file to lpdX_benchmark.ini)
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The below listed MFQL files can be applied for all mass spectrometric settings. The mass spectrometric settings are saved in the *ini file utilized for the import of a dataset.[[media:lpdX_benchmark.txt]] ('''IMPORTANT:''' for usage in LipidXplorer please rename file to lpdX_benchmark.ini)
  
* Phosphatidylethanolamine in negative mode: [[File:PE_negative_FAS.mfql]]
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* Phosphatidylethanolamine in negative mode: [[media:PE_negative_FAS.mfql|PE_negative_FAS.mfql]]
* Lyso-Phosphatidylethanolamine in negative mode: [[File:LPE_negative_FAS.mfql]]
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* Lyso-Phosphatidylethanolamine in negative mode: [[media:LPE_negative_FAS.mfql|LPE_negative_FAS.mfql]]
* Phosphatidylglycerol in negative mode: [[File:PG_negative_FAS.mfql]]
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* Phosphatidylglycerol in negative mode: [[media:PG_negative_FAS.mfql|PG_negative_FAS.mfql]]
* Phosphatidylinositol in negative mode: [[File:PI_negative_FAS.mfql]]
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* Phosphatidylinositol in negative mode: [[media:PI_negative_FAS.mfql|PI_negative_FAS.mfql]]
* Phosphatidylserine in negative mode: [[File:PS_negative_FAS.mfql]]
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* Phosphatidylserine in negative mode: [[media:PS_negative_FAS.mfql|PS_negative_FAS.mfql]]
* Phosphatic acid in negative mode: [[File:PA_negative_FAS.mfql]]
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* Phosphatic acid in negative mode: [[media:PA_negative_FAS.mfql|PA_negative_FAS.mfql]]
  
 
===MFQL used in '''[1]''' for lipid identification in bovine heart===
 
===MFQL used in '''[1]''' for lipid identification in bovine heart===
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Total lipid extract of bovine heart (Avanti Polar Lipids) was analyzed in six technical replicates on a LTQ-Orbitrap XL mass spectrometer using a target resolution of 100,000 for MS spectra (Orbitrap) and unit resolution for MS/MS (IT) in negative ion mode. Six replicates were acquired, each consisting of 31 MS and 310 MS/MS spectra.  
 
Total lipid extract of bovine heart (Avanti Polar Lipids) was analyzed in six technical replicates on a LTQ-Orbitrap XL mass spectrometer using a target resolution of 100,000 for MS spectra (Orbitrap) and unit resolution for MS/MS (IT) in negative ion mode. Six replicates were acquired, each consisting of 31 MS and 310 MS/MS spectra.  
  
* Phosphatidylethanolamine in negative mode: [[File:neg_bovine_heart_PE.mfql]]
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* Phosphatidylethanolamine in negative mode: [[media:neg_bovine_heart_PE.mfql|neg_bovine_heart_PE.mfql]]
* Lyso-Phosphatidylethanolamine in negative mode: [[File:neg_bovine_heart_LPE.mfql]]
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* Lyso-Phosphatidylethanolamine in negative mode: [[media:neg_bovine_heart_LPE.mfql|neg_bovine_heart_LPE.mfql]]
* Phosphatidylethanolamine ether in negative mode: [[File:neg_bovine_heart_PEO.mfql]]
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* Phosphatidylethanolamine ether in negative mode: [[media:neg_bovine_heart_PEO.mfql|neg_bovine_heart_PEO.mfql]]
* Phosphatidylcholine in negative mode: [[File:neg_bovine_heart_PC.mfql]]
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* Phosphatidylcholine in negative mode: [[media:neg_bovine_heart_PC.mfql|neg_bovine_heart_PC.mfql]]
* Lyso-Phosphatidylcholine in negative mode: [[File:neg_bovine_heart_LPC.mfql]]
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* Lyso-Phosphatidylcholine in negative mode: [[media:neg_bovine_heart_LPC.mfql|neg_bovine_heart_LPC.mfql]]
* Phosphatidylcholine ether in negative mode: [[File:neg_bovine_heart_PCO.mfql]]
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* Phosphatidylcholine ether in negative mode: [[media:neg_bovine_heart_PCO.mfql|neg_bovine_heart_PCO.mfql]]
* Phosphatic acid in negative mode: [[File:neg_bovine_heart_PA.mfql]]
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* Phosphatic acid in negative mode: [[media:neg_bovine_heart_PA.mfql|neg_bovine_heart_PA.mfql]]
* Lyso-Phosphatic acid in negative mode: [[File:neg_bovine_heart_LPA.mfql]]
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* Lyso-Phosphatic acid in negative mode: [[media:neg_bovine_heart_LPA.mfql|neg_bovine_heart_LPA.mfql]]
* Phosphatidylglycerol in negative mode: [[File:neg_bovine_heart_PG.mfql]]
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* Phosphatidylglycerol in negative mode: [[media:neg_bovine_heart_PG.mfql|neg_bovine_heart_PG.mfql]]
* Lyso-Phosphatidylglycerol in negative mode: [[File:neg_bovine_heart_LPG.mfql]]
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* Lyso-Phosphatidylglycerol in negative mode: [[media:neg_bovine_heart_LPG.mfql|neg_bovine_heart_LPG.mfql]]
* Phosphatidylinositol in negative mode: [[File:neg_bovine_heart_PI.mfql]]
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* Phosphatidylinositol in negative mode: [[media:neg_bovine_heart_PI.mfql|neg_bovine_heart_PI.mfql]]
* Lyso-Phosphatidylinositol in negative mode: [[File:neg_bovine_heart_LPI.mfql]]
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* Lyso-Phosphatidylinositol in negative mode: [[media:neg_bovine_heart_LPI.mfql|neg_bovine_heart_LPI.mfql]]
* Sphingomylien in negative mode: [[File:neg_bovine_heart_LPI.mfql]]
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* Sphingomylien in negative mode: [[media:neg_bovine_heart_LPI.mfql|neg_bovine_heart_LPI.mfql]]
* Ceramide in negative mode: [[File:neg_bovine_heart_DAG.mfql]]
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* Ceramide in negative mode: [[media:neg_bovine_heart_DAG.mfql|]neg_bovine_heart_DAG.mfql]
* Diacylglycerol in negative mode: [[File:neg_bovine_heart_DAG.mfql]]
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* Diacylglycerol in negative mode: [[media:neg_bovine_heart_DAG.mfql|neg_bovine_heart_DAG.mfql]]
* Triacylglycerol in negative mode: [[File:neg_bovine_heart_TAG.mfql]]
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* Triacylglycerol in negative mode: [[media:neg_bovine_heart_TAG.mfql|neg_bovine_heart_TAG.mfql]]
* Cardiolipin in negative mode: [[File:neg_bovine_heart_CL.mfql]]
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* Cardiolipin in negative mode: [[media:neg_bovine_heart_CL.mfql|neg_bovine_heart_CL.mfql]]
  
 
===MFQL used in '''[2]''' for identification of Maradolipids in Dauer Larva in Caenorhabditis elegans===
 
===MFQL used in '''[2]''' for identification of Maradolipids in Dauer Larva in Caenorhabditis elegans===
  
* Maradolipids in negative ion mode: [[File:Maradolipid.mfql]]
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* Maradolipids in negative ion mode: [[media:Maradolipid.mfql|Maradolipid.mfql]]
  
 
===MFQL used in '''[3]''' for identification of Lipids in human blood plasma===
 
===MFQL used in '''[3]''' for identification of Lipids in human blood plasma===
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Spectra acquired within 28 s to 120 s from the start of sample infusion (timing required to stabilize the analyte flow and electrospray, as was judged by total ion current (TIC) trace) were averaged and recalibrated using m/z of synthetic standards SM 35:1 and PC –O 20:0/-O 20:0 as references. Only peaks detected at the signal-to-noise ratio above the factor of 5 and recognized in more than 20% of all spectra were further considered. Identification of lipid species relied on accurately determined masses considering a mass accuracy of better than 4 ppm and a retrieval rate of 90% for all plasma samples.
 
Spectra acquired within 28 s to 120 s from the start of sample infusion (timing required to stabilize the analyte flow and electrospray, as was judged by total ion current (TIC) trace) were averaged and recalibrated using m/z of synthetic standards SM 35:1 and PC –O 20:0/-O 20:0 as references. Only peaks detected at the signal-to-noise ratio above the factor of 5 and recognized in more than 20% of all spectra were further considered. Identification of lipid species relied on accurately determined masses considering a mass accuracy of better than 4 ppm and a retrieval rate of 90% for all plasma samples.
  
In this zip file: [[File:Mfql_screens_MS-only_positive.zip‎|Positive MS only screens]] the following queries can be found which were used in '''[3]''':
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In this zip file: [[media:Mfql_screens_MS-only_positive.zip|Positive MS only screens]] the following queries can be found which were used in '''[3]''':
 
* Ceramide
 
* Ceramide
 
* Cholesterylester
 
* Cholesterylester

Revision as of 10:37, 31 March 2011

MFQL used in [1] for lipid identification in E.coli

E. coli total lipid extract was purchased from Avanti Polar Lipids (Alabaster, AL, USA) and analyzed on the LTQ Orbitrap XL instrument in negative ion mode. A solution of the total lipid concentration of 2.5 μg/ml in 7.5 mM ammonium acetate in choloroform/methanol/2-propanol (1/2/4, v/v/v) was infused into the mass spectrometer by TriVersa robotic ion source using a chip with the diameter of spraying nozzles of 4.1 μm. To produce the spectra dataset, the extract was analyzed in several independent experiments: experiment I, eight acquisitions under the unit mass resolution (R) settings using ion trap (IT) to acquire both MS and MS/MS spectra; experiment II, six acquisitions with R = 7,500 for MS spectra (Orbitrap) and unit resolution for MS/MS spectra (IT); experiment III, four acquisitions with R = 30,000 for MS spectra (Orbitrap) and unit resolution for MS/MS spectra (IT); experiment IV, four acquisitions with R = 100,000 for MS spectra (Orbitrap) and unit resolution for MS/MS spectra (IT); experiment V, seven acquisitions with R = 100,000 for MS spectra (Orbitrap) and R = 15,000 for MS/MS spectra (Orbitrap). MS/MS experiments were performed using Pulsed Q Collision Induced Dissociation(PQD).

The below listed MFQL files can be applied for all mass spectrometric settings. The mass spectrometric settings are saved in the *ini file utilized for the import of a dataset.media:lpdX_benchmark.txt (IMPORTANT: for usage in LipidXplorer please rename file to lpdX_benchmark.ini)

MFQL used in [1] for lipid identification in bovine heart

Total lipid extract of bovine heart (Avanti Polar Lipids) was analyzed in six technical replicates on a LTQ-Orbitrap XL mass spectrometer using a target resolution of 100,000 for MS spectra (Orbitrap) and unit resolution for MS/MS (IT) in negative ion mode. Six replicates were acquired, each consisting of 31 MS and 310 MS/MS spectra.

MFQL used in [2] for identification of Maradolipids in Dauer Larva in Caenorhabditis elegans

MFQL used in [3] for identification of Lipids in human blood plasma

Mass spectrometric analysis was performed on a hybrid LTQ Orbitrap mass spectrometer (Thermo Fisher Scientific, Bremen, Germany) equipped with a robotic nanoflow ion source TriVersa (Advion BioSciences Ltd, Ithaca NY) using chips with 4.1 µm nozzle diameter. The ion source was controlled by Chipsoft 6.4. software (Advion BioSciences) and operated at the ionization voltage of 0.95 kV and gas pressure 1.25 psi. Plates with lipid extracts were chilled down to 12°C. MS survey scans were acquired in positive ion mode using the Orbitrap analyzer operated under the target mass resolution of 100,000 (Full Width at Half Maximum, FWHM), defined at m/z 400 under automatic gain control set to 1.0×106 as the target value. Spectra acquired within 28 s to 120 s from the start of sample infusion (timing required to stabilize the analyte flow and electrospray, as was judged by total ion current (TIC) trace) were averaged and recalibrated using m/z of synthetic standards SM 35:1 and PC –O 20:0/-O 20:0 as references. Only peaks detected at the signal-to-noise ratio above the factor of 5 and recognized in more than 20% of all spectra were further considered. Identification of lipid species relied on accurately determined masses considering a mass accuracy of better than 4 ppm and a retrieval rate of 90% for all plasma samples.

In this zip file: Positive MS only screens the following queries can be found which were used in [3]:

  • Ceramide
  • Cholesterylester
  • Diacylglycerols
  • Glucosylceramide
  • GPL-diether
  • Lysophosphatidylcholine (LPC)
  • Lysophosphatidylethanolamine (LPE)
  • Phosphatidylcholine (PC)
  • Phosphatidylcholine ether (PC-O)
  • Phosphatidylethanolamine (PE)
  • Phosphatidylethanolamine ether (PE-O)
  • Phosphatidylinositol (PI)
  • Phosphatidylserine (PS)
  • Sphingomyline (SM)
  • Triacylglycerols (TAG)

References

[1] Herzog, R., Schwudke, D., Schuhmann, K., Sampaio, J.L., Bornstein, S.R., Schroeder, M., and Shevchenko, A. 2011. A novel informatics concept for high-throughput shotgun lipidomics based on the molecular fragmentation query language. Genome Biol 12(1): R8.

[2]Penkov S, Mende F, Zagoriy V, Erkut C, Martin R, Pässler U, Schuhmann K, Schwudke D, Gruner M, Mäntler J, Reichert-Müller T, Shevchenko A, Knölker HJ, Kurzchalia TV. 2010. Maradolipids: diacyltrehalose glycolipids specific to dauer larva in Caenorhabditis elegans. Angew Chem Int Ed Engl. 49(49):9430-5.

[3] Graessler J, Schwudke D, Schwarz PE, Herzog R, Shevchenko A, Bornstein SR: Top-down lipidomics reveals ether lipid deficiency in blood plasma of hypertensive patients. PLoS One 2009, 4:e6261.