Development of a Homogeneous Assay for Measurement of Small Dense LDL Cholesterol

被引:144
作者
Ito, Yasuki [1 ]
Fujimura, Miki
Ohta, Motoko
Hirano, Tsutomu [2 ]
机构
[1] Denka Seiken Co Ltd, Reagent R&D Dept, Chuo Ku, Tokyo 1030025, Japan
[2] Showa Univ, Sch Med, Dept Med, Div Endocrinol Diabet & Metab, Tokyo 142, Japan
关键词
ISCHEMIC-HEART-DISEASE; LIPOPROTEIN PARTICLES; RISK; SUBFRACTIONS; MEN; SPHINGOMYELIN; AGGREGATION; FUSION; SINGLE;
D O I
10.1373/clinchem.2010.149559
中图分类号
R446 [实验室诊断]; R-33 [实验医学、医学实验];
学科分类号
1001 ;
摘要
BACKGROUND: Plasma concentrations of small dense (sd)-LDL are associated with the prevalence of cardiovascular events. However, the special equipment and long assay times required for sd-LDL measurement have hindered its clinical application. Herein, we report development of a simple homogeneous assay for sd-LDL-cholesterol (C) adaptable to autoanalyzers. MATERIALS AND METHODS: We identified suitable surfactants and phospholipases by screening for those selective for the sd-LDL fraction (d 1.044-1.063 kg/L) and for the dissociation of other lipoproteins, including large buoyant LDL (lb-LDL). Principal characteristics of this assay were compared with ultracentrifugal isolation of LDL subfractions and with our previous heparin-magnesium precipitation assay for sd-LDL. We measured sd-LDL-C concentrations in 460 healthy, normolipidemic individuals. RESULTS: We used a polyoxyethylene benzylphenyl ether derivative to dissociate triglyceride-rich lipoproteins and HDLs, whereas sphingomyelinase proved most effective for dissociation of lb-LDL from LDL owing to the higher sphingomyelin content in the lb-LDL subfractions. A polyoxyethylene styrenephenyl ether derivative protected sd-LDL against the dissociative actions of sphingomyelinase and cholesterol oxidase/esterase during an initial incubation step. Next, polyoxyethylene alkyl ether dissociated sd-LDL-C and the cholesterol released from sd-LDL were subsequently measured by using cholesterol oxidase/esterase. The homogeneous method correlated excellently with ultracentrifugation for sd-LDL-C (y = 0.99x-0.09, R-2 = 0.91, n = 60) and exhibited within-run precision CVs <1.1%. The distribution of sd-LDL-C was skewed, and the central 95% of sd-LDL-C concentrations ranged from 0.24 to 0.88 mmol/L (9.4-34.0 mg/dL). CONCLUSIONS: The homogeneous assay allows reproducible measurement of sd-LDL-C within 10 min and appears promising in further investigations of the clinical significance of sd-LDL-C. (C) 2010 American Association for Clinical Chemistry
引用
收藏
页码:57 / 65
页数:9
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