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Characterisation of epitopes on barley mild mosaic virus coat protein recognised by a panel of novel monoclonal antibodies

Zugehörigkeit
Biological Research Center, Institute of Plant Biology, Hungary
Veliceasa, D.;
Zugehörigkeit
Institute of Physical Biology, Heinrich Heine University, Germany
Tauscher, G.;
Zugehörigkeit
Biological Research Center, Institute of Plant Biology, Hungary
Surányi, G.;
Zugehörigkeit
Biological Research Center, Institute of Plant Biology, Hungary
Kós, P.B.;
Zugehörigkeit
Biological Research Center, Institute of Plant Biology, Hungary
Likó, I.;
Zugehörigkeit
Institute of Physical Biology, Heinrich Heine University, Germany
Santore, U.;
Zugehörigkeit
Federal Centre for Breeding Research on Cultivated Plants, Institute of Resistance Research and Pathogen Diagnostics, Aschersleben, Germany
Proll, Eckhard;
GND
1058968181
Zugehörigkeit
Federal Centre for Breeding Research on Cultivated Plants, Institute of Resistance Research and Pathogen Diagnostics, Aschersleben, Germany
Ehrig, Fred;
Zugehörigkeit
Research Group of Peptide Chemistry, Eötvös Loránd University, Hungary
Uray, K.;
Zugehörigkeit
Research Group of Peptide Chemistry, Eötvös Loránd University, Hungary
Hudecz, F.;
GND
105894021X
Zugehörigkeit
Federal Centre for Breeding Research on Cultivated Plants, Institute of Resistance Research and Pathogen Diagnostics, Aschersleben, Germany
Kühne, Thomas;
Zugehörigkeit
Biological Research Center, Institute of Plant Biology, Hungary
Lukács, N.

Barley mild mosaic virus (BaMMV), a member of the family Potyviridae, genus Bymovirus, is involved in the economically important yellow mosaic disease of winter barley in East Asia and Europe. We investigated serological properties of bacterially expressed BaMMV coat protein (CP) of a German isolate. Ten mouse monoclonal antibodies were produced using purified E. coli expressed BaMMV-CP as immunogen. The reactivity of MAbs with different strains of BaMMV was analysed by several immunological methods that are frequently used in diagnostic virology: enzyme-linked immunosorbent assay (ELISA), dot-blot, Western-blotting (WB), direct tissue blotting immunoassay (DTBIA) and immunoelectron microscopy (IEM). The amino acids involved in the formation of epitopes recognised by several MAbs were mapped by using synthetic pin-bound peptides and the localisation of epitopes in assembled virus particles was determined by electron microscope studies. MAbs V29 and M1 decorated the whole virion indicating that their epitopes ⁶PDPI⁹ and ⁹⁶ITDDEK ¹⁰¹, respectively, are exposed on the surface. The MAbs V6 and V14 both interacted with ⁴⁴LPEPKM⁴⁹, which seems to be accessible at only one end of the virus particle. The MAbs V6, V14, V29 and M1 detected epitopes common to a wide range of BaMMV isolates and can therefore be used effectively in routine diagnostic tests for BaMMV from barley leaves. We suggest that MAbs M1, V6, V14 and V29 are most suitable for use in TAS-ELISA, V6, V14 and V29 for Western blotting and V29 and M1 for electron microscope serology. © Springer-Verlag 2005.

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