Abstract:
A reversed-phase high-performance liquid chromatography method for the
determination of creatinine in human serum samples has been developed. Results
from measurements of by a high-performance liquid chromatography on 232
serum samples were compared with enzymatic and Jaffé methods. The serum
samples were deproteinized with ethanol. For the separation, a column MAG 1,
250 mm x 4.6 mm, Labiospher PSI 100 C18, 5 :m, was used. The mixture of
ethanol and 25 mmol l–1 sodium hydrogenphosphate (3:97 v/v), pH 6.5 was used
as a mobile phase. The analytical performance of this method is satisfactory: the
intra-assay and inter-assay coefficients of variation were below 6 %. Quantitative
recoveries of spiked serum samples were between 101.8 and 106.0 %. The limit of
quantification was 10.0 :mol l–1. The results obtained by chromatographic method
correlated well with Jaffé assays. Enzymatic method gave at average significantly
higher values depending on a group of patients. The presented high-performance liquid chromatographic assay is useful for the analysis of samples where the
classical Jaffé or enzymatic methods do not give reliable results and can be a
candidate for reference method.
