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Rapid analysis of fatty acids in plasma lipids
Authors:Akira Ohta  Michael C. Mayo  Nancy Kramer  William E. M. Lands
Affiliation:(1) Department of Biological Chemistry, University of Illinois at Chicago, 60680 Chicago, Illinois;(2) Department of Biological Chemistry, The University of Illinois at Chicago, 1853 West Polk Street, 60612 Chicago, IL;(3) Present address: Japan Tobacco Co., Ltd., Kanagawa, Japan;(4) Present address: DuPont Co., Wilmington, DE
Abstract:A rapid and convenient procedure for the quantitative determination of the fatty acid composition of plasma lipids is described. Human plasma was applied directly to the preadsorbent zones of thin-layer silica gel plates with added antioxidant, internal standards and carriers. The thin-layer chromatography (TLC) plates were partially developed with methanol followed by chloroform/methanol (1∶1, v/v), and then they were fully developed in hexane/diethyl ether/acetic acid (80∶20∶1, v/v/v) to separate the major classes of lipids. Silica gel from regions containing the separated lipids was scraped into screw-capped tubes and treated with boron trifluoride-methanol prior to gas chromatography. The method of direct application to TLC plates gave yields and compositions of fatty acids very similar to the method of applying extracted plasma lipids. This relatively simple method is suitable for analyzing the fatty acids in plasma lipids from a 50 microliter finger-tip blood samples from an individual, and it may be useful in wide-scale screening of different individuals to estimate the relative amounts of ingested polyunsaturated fatty acids. Pfizer Biomedical Research Awardee.
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