Abstract
Macrophage scavenger receptors exhibit unusually broad, but circumscribed, polyanionic ligand-binding specificity. For example, the polyribonucleotides poly(I) and poly(G) are ligands but poly(A) and poly(C) are not. To further investigate the molecular basis of this polynucleotide-binding specificity, we tested the capacity of various oligodeoxyribonucleic acids to inhibit the scavenger receptor-mediated degradation of 125I-labeled acetylated low density lipoprotein by Chinese hamster ovary cells expressing the type I bovine scavenger receptor. A series of short oligodeoxyriboguanines (dGn, where 5 < or = n < or = 37) were effective inhibitors. The dG6, dG12, and dA5G37 members of this series were shown by circular dichroism and UV spectroscopy to be assembled into four-stranded helices stabilized by G-quartets. [32P]dA5G37 bound directly to scavenger receptors. Partial or complete denaturation of the quadruplex structures of these oligonucleotides by boiling destroyed their inhibitory activity. Receptor activity was also inhibited by d(T4G4)4, a telomere-like oligonucleotide which forms an intramolecular quadruplex. In addition, conversion of the four-stranded potassium salt of poly(I) to the single-stranded lithium salt dramatically reduced its inhibitory activity. Addition of KCl to the Li+ salt resulted in the reformation of poly(I)'s quadruplex structure and restoration of its inhibitory activity. A variety of single-stranded and double-stranded oligo- and polydeoxyribonucleotides (e.g. dA37, HaeIII restriction fragments of phi X174) exhibited very little or no inhibitory activity. Thus, a base-quartet-stabilized four-stranded helix appears to be a necessary structural determinant for polynucleotide binding to and inhibition of scavenger receptors. This conformational requirement accounts for the previously unexplained polyribonucleotide-binding specificity of scavenger receptors. The spatial distribution of the negatively charged phosphates in polynucleotide quadruplexes may form a charged surface which is complementary to the positively charged surface of the collagenous ligand-binding domain of the scavenger receptor.
Highlights
Macrophage scavenger receptors exhibit unusually broad, but circumscribed, polyanionic ligand-binding specificity
Two classes of macrophage scavenger receptors have been cloned from bovine, murine, human, and rabbitcDNA libraries (4-6, 8, 9).’
All of the quadruplex-forming oligonucleotide and polyribonucleotide molecules described above aggregated into heterogeneous higher order structures as determined by FPLC analysis
Summary
2 shows that thisoligonucleotide inhibited scavenger receptor plus uptake of [32P]dA5G3(7open triangles),which was calcuactivity, as measured by the degradation of lZ51-Ac-LDLby lated by subtracting the valuesfor thetotalbindingplus. The relationships of the structures of several dG, compounds to their inhibitory activitieswere assessed using CD spectroscopy at 37 “C and denaturatiobyn boiling in deionized ima near 241 nm, and distinctive shoulders nea2r30 nm (Fig. 5A). The spectra of these untreated oligo dG,’s were similar to previously reported spectra of quadruplex polynucleotides, including dGs (48), dGs (50),and dG12 (38), poly(G) (23), poly(dG) (48), and telomeric (34-36)4.5, and model telomeric sequences (32, 54).
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