Abstract
Melanotransferrin, also called p97, is a cell surface glycoprotein which was first described as a marker antigen for human melanoma cells. Although p97 has a striking structural similarity to human serum transferrin and lactoferrin, its function has not yet been determined. One feature that distinguishes p97 from the other members of the transferrin family is the presence of a stretch of 24 hydrophobic amino acids at the C terminus, previously assumed to form a proteinacious transmembrane domain. In this study, sensitivity to bacterial phosphatidylinositol-specific phospholipase C, biosynthetic labeling with [3H]ethanolamine, and partitioning in Triton X-114 are used to establish that p97 is expressed at the cell surface as a glycosylphosphatidylinositol-anchored protein. In addition, to gain insight into the intracellular transport of p97, biosynthetic transport studies were performed on a melanoma cell line. These studies resulted in the identification of an additional form of p97 which is found in the medium and which likely does not originate from an alternatively spliced form of the p97 mRNA. These findings, together with our recent observation of the co-localization of p97 and the transferrin receptor in brain capillary endothelium (W. A. Jefferies, M. R. Food, R. Gabathuler, S. Rothenberger, T. Yamada, and P. L. McGeer, manuscript submitted) raise important questions about the function of the two forms of p97 detected and the possible involvement of this protein in a cellular iron uptake mechanism that is independent from the transferrin/transferrin receptor system.
Highlights
Plasma membrane-associated proteins are imbedded in the membranveia a n a-helical transmembrane polypeptide segment
Melanotransferrin, known as the humanmelanoma-as- cursors of these proteins usually contain a segment which is sociated antigen p97, was one of the firstcell surface markers likely too short to act as a transmembrane anchor
Characterization of theGPI-anchored p97"Studies have shown that bacterial PI-PLC can cleave GPI anchors and release the proteins in a soluble form from intact cells
Summary
Membrane DAtatnaacsnphodmret nt of p97 from the American Type Culture Collection (ATCC) These lines were maintained in Dulbecco'smodified Eagle'smedium(DMEM) supplemented with 10% fetal bovine serum, 20 m HEPES, 100 unitdml penicillin, 100&mIstreptomycin, and 2 m L-glutamine.The Chinese hamster ovary (CHO) celline WTB was obtained from Dr F. The cells were washed several times in DMEM, divided into two samples that were incubated for 60 min at 6 "C in the presence or absence of PI-PLC(1.7 unit/106 cells), respectively, when treated with PI-PLC. Both the cell supernatant and the cell pellet were subsequently processed. Immunoprecipitated material was digested with 5 m of endoglycosidaseH (Endo H) (Boehringer Mannheim) for 20 h at 37 "C prior to analysis
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