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J Biol Chem, Vol. 274, Issue 18, 12898-12904, April 30, 1999
Megalin (gp330) Is an Endocytic Receptor for Thyroglobulin on
Cultured Fisher Rat Thyroid Cells
Michele
Marinò,
Gang
Zheng, and
Robert T.
McCluskey
From the Pathology Research Laboratory, Massachusetts General
Hospital, Harvard Medical School,
Charlestown, Massachusetts 02129
We recently reported that megalin (gp330), an
endocytic receptor found on the apical surface of thyroid cells, binds
thyroglobulin (Tg) with high affinity in solid phase assays.
Megalin-bound Tg was releasable by heparin. Here we show that Fisher
rat thyroid (FRTL-5) cells, a differentiated rat thyroid cell line, can
bind and endocytose Tg via megalin. We first demonstrated that FRTL-5 cells express megalin in a thyroid-stimulating
hormone-dependent manner. Evidence of Tg binding to megalin
on FRTL-5 cells and on an immortalized rat renal proximal tubule cell
line (IRPT cells), was obtained by incubating the cells with
125I-Tg, followed by chemical cross-linking and
immunoprecipitation of 125I-Tg with antibodies against
megalin. To investigate cell binding further, we developed an assay in
which cells were incubated with unlabeled Tg at 4 °C, followed by
incubation with heparin, which released almost all of the cell-bound Tg
into the medium. In solid phase experiments designed to illuminate the
mechanism of heparin release, we demonstrated that Tg is a
heparin-binding protein, as are several megalin ligands. The amount of
Tg released by heparin from FRTL-5 and IRPT cells, measured by
enzyme-linked immunosorbent assay (ELISA), was markedly reduced by two
megalin competitors, receptor-associated protein (RAP) and 1H2
(monoclonal antibody against megalin), indicating that much of the Tg
released by heparin had been bound to megalin (~60-80%). The amount
inhibited by RAP was considered to represent specific binding to
megalin, which was saturable and of high affinity
(Kd~11.2 nM). Tg endocytosis by
FRTL-5 and IRPT cells was demonstrated in experiments in which cells
were incubated with unlabeled Tg at 37 °C, followed by heparin to
remove cell-bound Tg. The amount of Tg internalized (measured by ELISA
in the cell lysates) was reduced by RAP and 1H2, indicating that Tg
endocytosis is partially mediated by megalin.
Copyright © 1999 by The American Society for Biochemistry and Molecular Biology, Inc.

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Copyright © 1999 by the American Society for Biochemistry and Molecular Biology.
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