
pmid: 11448166
Two proteins (SaM35 and SaM50) isolated from head tissues of the aphid vector, Sitobion avenae, were identified as potential receptors for barley yellow dwarf virus MAV isolate (Luteoviridae) based on MAV virus overlay assays and immunoblots of urea SDS 2-D gels. An anti-idiotypic antibody (MAV4 anti-ID) that mimics an epitope on MAV virions and competes with MAV in antibody binding assays also bound to SaM50 and SaM35 and to six additional proteins including a GroEL homolog. No MAV-binding proteins were detected from the nonvector aphid, Rhopalosiphum maidis, although MAV4 anti-ID did react with four proteins from R. maidis. It is hypothesized that SaM35 and SaM50 may be MAV receptors involved in MAV transmission based on their high affinity for MAV and their unique association with the vector, S. avenae. The additional aphid proteins binding the MAV4 anti-ID may represent less specific virus-binding proteins facilitating transmission through different aphid tissues.
anti-idiotypic antibody, Sitobion avenae, virus overlay assays, Virus Replication, anti-idiotypes, virus receptor, Insect Vectors, Luteoviridae, Virology, Aphids, Luteovirus, Animals, Receptors, Virus, Rhopalosiphum maidis
anti-idiotypic antibody, Sitobion avenae, virus overlay assays, Virus Replication, anti-idiotypes, virus receptor, Insect Vectors, Luteoviridae, Virology, Aphids, Luteovirus, Animals, Receptors, Virus, Rhopalosiphum maidis
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