| Literature DB >> 12942512 |
Chang Seok Lee1, Jik Hyon Han, Sang Mong Lee, Jae Sam Hwang, Seok Woo Kang, Bong Hee Lee, Hak R Kim.
Abstract
To identify and characterize the HDLp (high-density lipophorin) receptor from Galleria mellonella (LpRGm), we used techniques of ligand blotting. This method was, to our knowledge, first used to characterize the lipophorin receptor (LpR) in insects. LpRGm had an approximate molecular weight of 97 kDa under non-reducing conditions and bound the HDLp specifically. The time-course of lipophorin binding to their receptor protein was rapid. The binding of lipophorins to their receptors was saturable with a Kd of 34.33+/-4.67 microg/ml. Although Ca2+ was essentially required in the binding of HDLp to their receptors, interestingly increasing concentration of Ca2+ has shown to have a slight inhibitory effect. EDTA was used here as Ca2+ chelating reagent, because Mg2+ in the binding buffer did not affect the binding of HDLp to their receptors, and inhibited the binding of HDLp and LpRGm absolutely. Suramin (polysulfated polycyclic hydrocarbon), known to inhibit the binding of lipoproteins to their receptors, effectively abolished the binding of HDLp to their receptors. LpRGm showed the stage specific binding activity especially in day 1-3 last instar larval, prepupal, and day 1-3 adult stages. Copyright 2003 Wiley-Liss, Inc.Entities:
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Year: 2003 PMID: 12942512 DOI: 10.1002/arch.10095
Source DB: PubMed Journal: Arch Insect Biochem Physiol ISSN: 0739-4462 Impact factor: 1.698