Mechanism and Physiologic Significance of the Suppression of Cholesterol Esterification in Human Interstitial Fluid

被引:7
作者
Miller, Norman E. [1 ]
Olszewski, Waldemar L. [2 ]
Miller, Irina P. [3 ]
Nanjee, Mahmud N. [4 ]
机构
[1] Univ Oxford, Magdalen Coll, Oxford, England
[2] Polish Acad Sci, Med Res Ctr, Dept Surg Res & Transpiantol, Warsaw, Poland
[3] Queen Mary Univ London, Dept Cardiovasc Biochem, London, England
[4] Univ Utah, Sch Med, Cardiovasc Genet Unit, Salt Lake City, UT USA
来源
FRONTIERS IN PHARMACOLOGY | 2016年 / 7卷
基金
英国惠康基金;
关键词
apolipoprotein Al; lecithin:cholesterol acyltransferase; high density lipoproteins; lymph; interstitial fluid; HIGH-DENSITY-LIPOPROTEINS; APOLIPOPROTEIN-A-I; HUMAN PERIPHERAL LYMPH; ESTER TRANSFER PROTEIN; LECITHINCHOLESTEROL ACYLTRANSFERASE; PLASMA-LIPOPROTEINS; FAMILIAL LECITHIN; SIZE SUBCLASSES; LCAT DEFICIENCY; TRANSGENIC MICE;
D O I
10.3389/fphar.2016.00216
中图分类号
R9 [药学];
学科分类号
1007 ;
摘要
Cholesterol esterification in high density lipoproteins (HDLs) by lecithin:cholesterol acyltransferase (LCAT) promotes unesterified cholesterol (UC) transfer from red cell membranes to plasma in vitro. However, it does not explain the transfer of UC from most peripheral cells to interstitial fluid in vivo, as HDLs in afferent peripheral lymph are enriched in UC. Having already reported that the endogenous cholesterol esterification rate (ECER) in lymph is only 5% of that in plasma, we have now explored the underlying mechanism. In peripheral lymph from 20 healthy men, LCAT concentration, LCAT activity (assayed using an optimized substrate), and LCAT specific activity averaged, respectively, 11.8, 10.3, and 84.9% of plasma values. When recombinant human LCAT was added to lymph, the increments in enzyme activity were similar to those when LCAT was added to plasma. Addition of apolipoprotein Al (apo Al), fatty acid-free albumin, Intralipid, or the d < 1.006 g/ml plasma fraction had no effect on ECER. During incubation of lymph plus plasma, the ECER was similar to that observed with buffer plus plasma. When lymph was added to heat-inactivated plasma, the ECER was 11-fold greater than with lymph plus buffer. Addition of discoidal proteoliposomes of apo Al and phosphatidycholine (PC) to lymph increased ECER 10-fold, while addition of apo AI/PC/UC disks did so by only six-fold. We conclude that the low ECER in lymph is due to a property of the HDLs, seemingly substrate inhibition of LCAT by excess cell-derived UC. This is reversed when lymph enters plasma, consequent upon redistribution of UC from lymph HDLs to plasma lipoproteins.
引用
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页数:8
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