K. Hermann et D. Abeck, Determination of histidine and urocanic acid isomers in the human skin by high-performance capillary electrophoresis, J CHROMAT B, 749(1), 2000, pp. 41-47
Histidine was baseline separated from histamine, 1-methylhistamine and cis-
and trans-urocanic acid using high-performance capillary electrophoresis (
HPCE) on a fused-silica column (50 cm X 75 mum) with 0.05 M NaH2PO4 buffer,
pH 5.0, and 12 kV. The detection Limit of histidine, trans- and cis-urocan
ic acid was 10(-6) M at a wavelength of 214 nm. The detection limit of the
urocanic acid isomers was slightly enhanced to 5.10(-7) M at 267 nm. The tr
ansformation of the trans-urocanic acid standard in vitro into the cis-isom
er was dependent on the time of exposure and the energy of the Light source
. WE light induced a significantly faster conversion than WA light. The HPC
E method was used for the characterization and measurement of histidine and
urocanic acid in human skin eluates. The concentrations of histidine, tran
s- or cis-urocanic acid in ethanol washes from the skin of healthy, non-all
ergic volunteers were 2.22+/-0.40.10(-5), 0.96+/-0.26-10(-5) and 1.04+/-0.3
0.10(-5) M,respectively, (mean+/-SEM, n=8). The results obtained by HPCE co
rrelated well with data obtained by HPLC. Correlation coefficients of r(2)=
0.981, r(2)=0.814 and r(2)=0.956 were found for histidine, trans- and cis-u
rocanic acid, respectively. (C) 2000 Elsevier Science B.V. All rights reser
ved.