Cell type-specific MxA-mediated inhibition of measles virus transcription in human brain cells.

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J Virol. 1994 November; 68(11): 6910-6917

Cell type-specific MxA-mediated inhibition of measles virus transcription in human brain cells.

S Schneider-Schaulies, J Schneider-Schaulies, A Schuster, M Bayer, J Pavlovic and V ter Meulen

Institute for Virology and Immunobiology, Würzburg, Germany.

ABSTRACT

Measles virus (MV)-specific transcription in human brain cellsis characterized by particularly low abundances of the distalmRNAs encoding the MV envelope proteins. Similar transcriptionalrestrictions of the closely related vesicular stomatitis virushave been observed in mouse fibroblasts constitutively expressingthe interferon-inducible MxA protein (P. Staeheli and J. Pavlovic,J. Virol. 65:4498-4501, 1991). We found that MV infection ofhuman brain cells is accompanied by rapid induction and high-levelexpression of endogenous MxA proteins. After stable transfectionof MxA, human glioblastoma cells (U-87-MxA) released 50- to100-fold less infectious virus and expression of viral proteinswas highly restricted. The overall MV-specific transcriptionlevels were reduced by up to 90%, accompanied by low relativefrequencies of the distal MV-specific mRNAs. These restrictionswere linked to an inhibition of viral RNA synthesis and notto a decreased stability of the viral RNAs. Our results indicatethat expression of MxA is associated with transcriptional attenuationof MV in brain cells, thus probably contributing to the establishmentof persistent MV central nervous system infections. In addition,the mechanism of MxA-dependent resistance against MV infection,in contrast to that of vesicular stomatitis virus, is cell typespecific, because an inhibition of MV glycoprotein synthesisindependent of transcriptional alterations was observed in MxA-transfectedhuman monocytes (J. J. Schnorr, S. Schneider-Schaulies, A. Simon-Jödicke,J. Pavlovic, M. A. Horisberger, and V. ter Meulen, J. Virol.67: 4760-4768, 1993).

J Virol. 1994 November; 68(11): 6910-6917

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