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J. Biol. Chem., Vol. 261, Issue 17, 7941-7951, Jun, 1986
PK Weech, R Camato, RW Milne and YL Marcel
We have produced five hybridomas which secreted monoclonal antibodies that
reacted with human plasma apolipoprotein D. On analysis by polyacrylamide
gel electrophoresis (PAGE) high density lipoproteins and
lecithin:cholesterol acyltransferase (EC 2.3.1.43)-enriched fractions of
plasma contained many protein bands that reacted with the antibodies.
Purified apolipoprotein D had the lowest Mr (29,000), the lowest pI
(4.8-5.2), and the greatest migration on alkaline urea-PAGE of all the
immunoreactive bands. These characteristics agreed with those described for
apolipoprotein D in the literature. The other immunoreactive proteins had
apparent Mr from about 39,000 to 98,000, they migrated more slowly than
apolipoprotein D on alkaline urea-PAGE, and there were 10 polymorphs on
isoelectric focusing. These cross- reacting proteins were present in the
high density lipoproteins of each of four individuals sampled on several
occasions and in pooled plasma. All of the monoclonal antibodies reacted
both with apo-D and the higher Mr cross-reacting proteins. Each of our five
monoclonal antibodies bound to one of two distinct antigenic sites on
apo-D, determined by antibody competition immunoassays. Neither of these
two sites was composed of carbohydrate, but expression of both sites seemed
to be influenced by thiol-reducing agents: site 5G10 gained but 4E11 either
lost immunoreactivity or was unchanged by reduction according to the
conditions. We conclude that apolipoprotein D is only one of several plasma
proteins, which contain two homologous polypeptide antigenic sites,
recognized by monoclonal antibodies and also by a specific goat antiserum.
Apolipoprotein D had the least Mr of these proteins.
Apolipoprotein D and cross-reacting human plasma apolipoproteins identified using monoclonal antibodies
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