Identification and Expression of Human Cytomegalovirus Transcription Units Coding for Two Distinct Fcγ Receptor Homologs

Author:

Atalay Ramazan1,Zimmermann Albert1,Wagner Markus2,Borst Eva2,Benz Christine2,Messerle Martin2,Hengel Hartmut1

Affiliation:

1. Robert Koch-Institut, Fachgebiet Virale Infektionen, 13353 Berlin

2. Max von Pettenkofer-Institut, Lehrstuhl Virologie, 81377 München, Germany

Abstract

ABSTRACT Cellular receptors for the Fc domain of immunoglobulin G (IgG) (FcγRs) comprise a family of surface receptors on immune cells connecting humoral and cellular immune responses. Several herpesviruses induce FcγR activities in infected cells. Here we identify two distinct human cytomegalovirus (HCMV)-encoded vFcγR glycoproteins of 34 and 68 kDa. A panel of HCMV strains exhibited a slight molecular microheterogeneity between Fcγ-binding proteins, suggesting their viral origin. To locate the responsible genes within the HCMV genome, a large set of targeted HCMV deletion mutants was constructed. The mutant analysis allowed the identification of a spliced UL119-UL118 mRNA to encode vFcγR gp68 and TRL11/IRL11 to encode vFcγR gp34. Both vFcγRs are surface resident type I transmembrane glycoproteins. Significant relatedness of sequences in the extracellular chain of gpUL119-118 and gpTRL11 with particular immunoglobulin supergene family domains present in FcγR I and FcγRs II/III, respectively, indicates a different ancestry and function of gpUL119-118 and gpTRL11. The HCMV-encoded vFcγRs highlight an impressive diversification and redundancy of FcγR structures.

Publisher

American Society for Microbiology

Subject

Virology,Insect Science,Immunology,Microbiology

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