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. 2019 Nov 19;2019:4851323. doi: 10.1155/2019/4851323

Table 2.

Mass spectrometric multiple reaction monitoring detection of protein glycation, oxidation, nitration, crosslinks, and branched-chain amino acids.

Analyte group Analyte R t (min) Parent ion (Da) Ion (Da) CE (eV) Neutral fragment loss (es) Internal standard and amount added
Glycation FL 28.5 291.0 84.3 31 H2CO2, fructosylamine [2H4]FL, 0.3 pmol
CML 28.5 204.9 130.1 12 NH2CH2CO2H [13C6]CML, 0.25 pmol
MG-H1 11.6 & 12.5 229.2 114.3 14 NH2CH(CO2H)CH2CH=CH2 [15N2]MG-H1, 1.25 pmol
Glucosepane 16.5 429.2 382.1 38 C2H5O [13C6]Glucosepane, 0.25 pmol
Pyrraline 17.9 255.2 84.3 23 2-CHO-5-HOCH2-pyrrole, H2CO2 [13C6,15N2]Pyrraline, 1.00 pmol

Oxidative damage Dityrosine 19.9 361.2 315.3 15 H2CO2 [2H6]DT, 0.25 pmol
GSA 32.2 114.0 68.0 15 H2CO2 [2H3]AAA, 2.5 pmol

Nitration damage 3-NT 23.2 227.1 181.2 13 H2CO2 [2H3]3-NT, 0.25 pmol

TG crosslink GEEK 9.3 276.1 147.1 12 NH2CH(CO2H)CH2CH=C=O Nε-(γ-[13C5]glutamyl) lysine, 2.5 pmol

BCAA Leu 27.6 132.3 86.2 10 H2CO2 [2H3]Leu, 250 pmol
Ile 31.5 132.3 86.2 10 H2CO2 [13C6]Ile, 250 pmol
Val 8.2 117.8 72.0 19 H2CO2 [2H8]Val, 250 pmol

For MG-H1, Rt values for the 2 epimers are given. LC-MS/MS was performed as described previously [25, 35] with chromatography using two Hypercarb™ (5 μm particle size, 0.2 × 50 mm and 0.2 × 250 mm) columns, column switching, and elution with 0.1% trifluoroacetic acid (TFA) in water and custom acetonitrile (MeCN) gradient. Different chromatography conditions were used for assay of GEEK: the column was Hypercarb™ (2 μm particle size, 0.2 × 150 mm) with isocratic elution at 0.2 ml/min with 3.75% MeCN and 0.1% TFA in water (solvent A) for 15 min. After each run the column was washed by elution with 50% tetrahydrofuran in 0.1% TFA in water for 20 min and reequilibrated by elution with solvent A at 0.4 ml/min for 15 min. Pentosidine was detected by in-line fluorimetry; excitation wavelength 320 nm, emission wavelength 365 nm [35].