Accumulation of High-Density Lipoprotein-Derived Estradiol-17β Fatty Acid Esters in Low-Density Lipoprotein Particles1
Author(s) -
H. Helisten,
Anna Höckerstedt,
Kristiina Wähälä,
Aila Tiitinen,
Herman Adlercreutz,
Matti Jauhiainen,
Matti J. Tikkanen
Publication year - 2001
Publication title -
the journal of clinical endocrinology and metabolism
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.206
H-Index - 353
eISSN - 1945-7197
pISSN - 0021-972X
DOI - 10.1210/jcem.86.3.7292
Subject(s) - chemistry , lipoprotein , endocrinology , medicine , intermediate density lipoprotein , high density lipoprotein , low density lipoprotein , in vivo , dtnb , lipophilicity , cholesterol , biochemistry , fatty acid , estrogen , very low density lipoprotein , enzyme , glutathione , biology , microbiology and biotechnology
Estrogens are known to be powerful antioxidants in lipid-aqueous systems, as demonstrated by their inhibition of low-density lipoprotein (LDL) oxidation in vitro. Studies reporting that endogenous human estrogens could be rendered fat-soluble by esterification with fatty acids in vivo, and the subsequent detection of such esters in blood and fat tissue suggested a possible mechanism explaining how estrogens might protect LDL. Because of their lipophilicity, esterified estrogens may become incorporated in the lipoprotein structure, providing antioxidant potential for the particles. We incubated labeled 17beta-estradiol with ovarian follicular fluid and with plasma in the absence and presence of the LCAT inhibitor DTNB. This was followed by ultracentrifugal isolation of LDL and high-density lipoprotein and analysis of the radioactive label in the "ester" and "free" fractions purified from these lipoproteins. The results indicated that LCAT-mediated synthesis of esterified 17beta-estradiol occurred in high-density lipoprotein particles, and suggested a novel cholesterol ester transfer protein-mediated mechanism for their transfer to LDL particles.
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