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Alcohol and Alcoholism Advance Access originally published online on October 3, 2005
Alcohol and Alcoholism 2006 41(1):18-23; doi:10.1093/alcalc/agh216
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© The Author 2005. Published by Oxford University Press on behalf of the Medical Council on Alcohol. All rights reserved

DEFECTIVE GLYCOSYLATION OF CHOLESTERYL ESTER TRANSFER PROTEIN IN PLASMA FROM ALCOHOL ABUSERS

M. JOHANNA LIINAMAA*, MINNA L. HANNUKSELA, MARIA E. RÄMET and MARKKU J. SAVOLAINEN

Department of Internal Medicine and Clinical Research Center, University of Oulu, Oulu, Finland

* Author to whom correspondence should be addressed at: Department of Internal Medicine, University of Oulu, PO Box 5000, 90014 Oulu, Finland. Tel: +358 8 573 6314; Fax +358 8 315 4543; E-mail: johanna.liinamaa{at}oulu.fi

(Received 16 November 2004; first review notified 20 January 2005; in revised form 13 June 2005; accepted 9 September 2005)

Aims: Alcohol consumption reduces the carbohydrate content of some glycoproteins, e.g. carbohydrate-deficient transferrin. The aim of this study was to investigate if there is such an alcohol-induced glycosylation defect in plasma cholesteryl ester transfer protein (CETP). A defect in the posttranslational glycosylation of CETP may affect its structure and electrical charge and may therefore affect its function. CETP activity is low in alcohol abusers. Methods: We studied the effect of alcohol consumption on CETP properties in 10 alcohol abusers and 10 control subjects. CETP was partially purified from lipoprotein-free plasma by FPLC using a Phenyl-Sepharose column. Isoelectric focusing, polyacrylamide gel electrophoresis, and western blotting were performed for partially purified CETP. Results: CETP had a lower molecular weight in the alcohol abusers than in the controls (range 50.6–84.0 kDa in the alcohol abusers vs 51.3–85.0 kDa in the controls). CETP purified from alcohol abusers had a higher isoelectric point, indicating a lower negative charge on the surface of the protein than in the controls' CETP. A similar effect was observed when control CETP was incubated with neuraminidase, an enzyme which is known to remove sialic acid from glycoproteins. Conclusions: We conclude that CETP from alcohol abusers may have a glycosylation defect due to defective sialylation caused posttranslationally by alcohol itself or its metabolite acetaldehyde. The defective glycosylation of CETP associated with altered binding to lipoproteins may lead to the low CETP activity observed previously in alcoholic subjects.


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