期刊
JOURNAL OF VIROLOGY
卷 74, 期 13, 页码 5880-5885出版社
AMER SOC MICROBIOLOGY
DOI: 10.1128/JVI.74.13.5880-5885.2000
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资金
- NIAID NIH HHS [AI20181, R01 AI012464, AI12464, R01 AI020181, R37 AI012464] Funding Source: Medline
The M2 gene of respiratory syncytial (RS) virus has two open reading frames (ORFs), ORF1 encodes a 22-kDa protein termed M2-1, The M2-1 protein contains a Cys(3)-His(1) motif (C-X-7-C-X-5-C-X-3-A) near the amino terminus. This motif is conserved in all human, bovine, and ovine strains of RS virus. A similar motif found in the mammalian transcription factor Nup475 has been shown to bind zinc, The M2-1 protein of human RS virus functions as a transcription factor which increases polymerase processivity, and it enhances readthrough of intergenic junctions during RS virus transcription, thereby acting as a transcription antiterminator, The M2-1 protein also interacts with the nucleocapsid protein. We examined the effects of mutations of cysteine and histidine residues predicted to coordinate zinc in the Cys(3)-His(1) motif on transcription antitermination and N protein binding. We found that mutating the predicted zinc-coordinating residues, the cysteine residues at amino acid positions 7 and 15 and the histidine residue at position 25, prevented M2-1 from enhancing transcriptional readthrough, In contrast, mutations of amino acids within this motif not predicted to coordinate zinc had no effect. Mutations of the predicted zinc-coordinating residues in the Cys(3)-His(1) motif also prevented M2-1 from interacting with the nucleocapsid protein. One mutation of a noncoordinating residue in the motif which did not affect readthrough during transcription, E10G, prevented interaction with the nucleocapsid protein. This suggests that M2-1 does not require interaction with the nucleocapsid protein in order to function during transcription. Analysis of the M2-1 protein in reducing sodium dodecyl sulfate-polyacrylamide gels revealed two major forms distinguished by their mobilities. The slower migrating form was shown to be phosphorylated, whereas the faster migrating form was not. Mutations in the Cys(3)-His(1) motif caused a change in distribution of the M2-1 protein from the slower to the faster migrating form. The data presented here shaw that the Cys(3)-His(1) motif of M2-1 is essential for maintaining the functional integrity of the protein.
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