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MB Sample ID: SA205970

Local Sample ID:Jurkat_Control_5
Subject ID:SU002236
Subject Type:Cultured cells
Subject Species:Homo sapiens
Taxonomy ID:9606

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Combined analysis:

Analysis ID AN003520 AN003521
Analysis type MS MS
Chromatography type Reversed phase Reversed phase
Chromatography system Agilent 1290 Infinity II Agilent 1290 Infinity II
Column Agilent InfinityLab Poroshell 120 EC–C18, 3.0 × 5 mm, 2.7 μm Agilent InfinityLab Poroshell 120 EC–C18, 3.0 × 5 mm, 2.7 μm
MS Type ESI ESI
MS instrument type QTOF QTOF
MS instrument name Agilent 6546 QTOF Agilent 6546 QTOF
Ion Mode POSITIVE NEGATIVE
Units AREA AREA

MS:

MS ID:MS003278
Analysis ID:AN003520
Instrument Name:Agilent 6546 QTOF
Instrument Type:QTOF
MS Type:ESI
MS Comments:The Agilent 6545 QTOF mass spectrometer equipped with a dual AJS ESI ion source was set with the following parameters: 150 V fragmentor, 65 V skimmer, 3500 V capillary voltage, 750 V octopole radio frequency voltage, 10 L/min nebulizer gas flow, 200 °C gas temperature, 50 psi nebulizer gas pressure, 12 L/min sheath gas flow, and 300 °C sheath gas temperature. Data were collected in positive and negative ESI modes in separate runs, operated in full scan mode from 50 to 1800 m/z with a scan rate of 3 spectra/s. A solution consisting of two reference mass compounds were used throughout the whole analysis: purine (C5H4N4) at m/z 121.0509 for the positive and m/z 119.0363 for the negative ionization modes; and HP-0921 (C18H18O6N3P3F24) at m/z 922.0098 for the positive and m/z 980.0163 (HP-0921+acetate) for the negative ionization modes. These masses were continuously infused into the system through an Agilent 1260 Iso Pump at a 1 mL/min (split ratio 1:100) to provide a constant mass correction. Ten Iterative-MS/MS runs were performed for both ion modes at the end of the analytical run. They were operated with an MS and MS/MS scan rates of 3 spectra/s, 40–1800 m/z mass window, a narrow (∼ 1.3 amu) MS/MS isolation width, 3 precursors per cycle, and 5000 counts and 0.001% of MS/MS threshold. Five iterative-MS/MS runs were set with a collision energy of 20 eV, and the subsequent five runs were performed at 40 eV. References masses and contaminants detected in blank samples were excluded from the analysis to avoid inclusion in the iterative-MS/MS.
Ion Mode:POSITIVE
  
MS ID:MS003279
Analysis ID:AN003521
Instrument Name:Agilent 6546 QTOF
Instrument Type:QTOF
MS Type:ESI
MS Comments:The Agilent 6545 QTOF mass spectrometer equipped with a dual AJS ESI ion source was set with the following parameters: 150 V fragmentor, 65 V skimmer, 3500 V capillary voltage, 750 V octopole radio frequency voltage, 10 L/min nebulizer gas flow, 200 °C gas temperature, 50 psi nebulizer gas pressure, 12 L/min sheath gas flow, and 300 °C sheath gas temperature. Data were collected in positive and negative ESI modes in separate runs, operated in full scan mode from 50 to 1800 m/z with a scan rate of 3 spectra/s. A solution consisting of two reference mass compounds were used throughout the whole analysis: purine (C5H4N4) at m/z 121.0509 for the positive and m/z 119.0363 for the negative ionization modes; and HP-0921 (C18H18O6N3P3F24) at m/z 922.0098 for the positive and m/z 980.0163 (HP-0921+acetate) for the negative ionization modes. These masses were continuously infused into the system through an Agilent 1260 Iso Pump at a 1 mL/min (split ratio 1:100) to provide a constant mass correction. Ten Iterative-MS/MS runs were performed for both ion modes at the end of the analytical run. They were operated with an MS and MS/MS scan rates of 3 spectra/s, 40–1800 m/z mass window, a narrow (∼ 1.3 amu) MS/MS isolation width, 3 precursors per cycle, and 5000 counts and 0.001% of MS/MS threshold. Five iterative-MS/MS runs were set with a collision energy of 20 eV, and the subsequent five runs were performed at 40 eV. References masses and contaminants detected in blank samples were excluded from the analysis to avoid inclusion in the iterative-MS/MS.
Ion Mode:NEGATIVE
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