Mutational analysis of the cellular receptor for poliovirus

Author:

Freistadt M S1,Racaniello V R1

Affiliation:

1. Department of Microbiology, Columbia University College of Physicians and Surgeons, New York, New York 10032.

Abstract

To identify sequences of the cellular poliovirus receptor (PVR) involved in viral infection, mutant PVR cDNAs were constructed and assayed for biological activity in mouse L cells. To confirm that mutant PVRs reached the cell surface, an immunological tag, consisting of part of CH3 from human immunoglobulin G1, was engineered into the PVR. Deletion of PVR amino acids 256 to 320 or 385 to the carboxy terminus yielded receptors that were able to support poliovirus infection. PVRs lacking amino acids 40 to 136 or 137 to 256 were expressed at the cell surface but were not active as receptors for poliovirus. The results show that immunoglobulin-type domain 3 and the extreme carboxy terminus of the PVR are not required for viral receptor function, but sequences within the two amino-terminal domains contribute to the initiation of poliovirus infection.

Publisher

American Society for Microbiology

Subject

Virology,Insect Science,Immunology,Microbiology

Reference23 articles.

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3. Segmental flexibility and complement fixation of genetically engineered chimeric human, rabbit and mouse antibodies;Dangl J. L.;EMBO J.,1988

4. Epstein-Barr virus receptor on human B Iymphocytes is the C3d receptor CR2;Fingeroth J.;Proc. Natl. Acad. Sci. USA,1984

5. Heterogeneous expression of poliovirus receptor-related proteins in human cells and tissues;Freistadt M. F.;Mol. Cell. Biol.,1990

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