Effect of phospholipase A2 digestion on the conformation and lysine/fibrinogen binding properties of human lipoprotein[a]

Gunther M. Fless; Elliot W. Kirk; Olga Klezovitch; José Y. Santiago; Celina Edelstein; Jane Hoover-Plow; Angelo M. Scanu

Journal of Lipid Research (Apr 1999)

Effect of phospholipase A2 digestion on the conformation and lysine/fibrinogen binding properties of human lipoprotein[a]

Gunther M. Fless,
Elliot W. Kirk,
Olga Klezovitch,
José Y. Santiago,
Celina Edelstein,
Jane Hoover-Plow,
Angelo M. Scanu

Affiliations

Gunther M. Fless: To whom correspondence should be addressed.; Department of Medicine University of Chicago, 5841 South Maryland Avenue, Chicago, IL 60637
Elliot W. Kirk: Department of Medicine University of Chicago, 5841 South Maryland Avenue, Chicago, IL 60637
Olga Klezovitch: Department of Medicine University of Chicago, 5841 South Maryland Avenue, Chicago, IL 60637
José Y. Santiago: Department of Medicine University of Chicago, 5841 South Maryland Avenue, Chicago, IL 60637
Celina Edelstein: Department of Medicine University of Chicago, 5841 South Maryland Avenue, Chicago, IL 60637
Jane Hoover-Plow: Department of Molecular Cardiology, Joseph J. Jacobs Center for Thrombosis and Vascular Biology/FF20, Cleveland Clinic Foundation, 9500 Euclid Avenue, Cleveland, OH 44195
Angelo M. Scanu: Department of Medicine University of Chicago, 5841 South Maryland Avenue, Chicago, IL 60637; Department of Biochemistry and Molecular Biology, University of Chicago, 5841 South Maryland Avenue, Chicago, IL 60637

Journal volume & issue: Vol. 40, no. 4
pp. 583 – 592

Abstract

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In vitro hydrolysis of human lipoprotein[a] (Lp[a]) by phospholipase A2 (PLA2) decreased the phosphatidylcholine (PC) content by 85%, but increased nonesterified fatty acids 3.2-fold and lysoPC 12.9-fold. PLA2-treated Lp[a] had a decreased molecular weight, increased density, and greater electronegativity on agarose gels. In solution, PLA2-Lp[a] was a monomer, and when assessed by sedimentation velocity it behaved like untreated Lp[a], in that it remained compact in NaCl solutions but assumed the extended form in the presence of 6-amino hexanoic acid, which was shown previously to have an affinity for the apo[a] lysine binding site II (LBS II) comprising kringles IV5–8. We interpreted our findings to indicate that PLA2 digestion had no effect on the reactivity of this site. This conclusion was supported by the results obtained from lysine Sepharose and fibrinogen binding experiments, in the presence and absence of Tween 20, showing that phospholipolysis had no effect on the reactivity of the LBS-II domain. A comparable binding behavior was also exhibited by the free apo[a] derived from each of the two forms of Lp[a]. We did observe a small increase in affinity of PLA2-Lp[a] to lysine Sepharose and attributed it to changes in reactivity of the LBS I domain (kringle IV10) induced by phospholipolysis. In conclusion, the extensive modification of Lp[a] caused by PLA2 digestion had no significant influence on the reactivity of LBS II, which is the domain involved in the binding of apo[a] to fibrinogen and apoB-100. These results also suggest that phospholipids do not play an important role in these interactions.—Fless, G. M., E. W. Kirk, O. Klezovitch, J. Y. Santiago, C. Edelstein, J. Hoover-Plow, and A. M. Scanu. Effect of phospholipase A2 digestion on the conformation and lysine/fibrinogen binding properties of human lipoprotein[a]. J. Lipid Res. 1999. 40: 583–592.

Published in Journal of Lipid Research

ISSN: 0022-2275 (Print); 1539-7262 (Online)
Publisher: Elsevier
Country of publisher: United States
LCC subjects: Science: Chemistry: Organic chemistry: Biochemistry
Website: https://www.journals.elsevier.com/journal-of-lipid-research

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