R. Beaud scite author profile

R. Beaud

3Publications

51Citation Statements Received

75Citation Statements Given

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104

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Affiliations

Institut Jacques Monod, Institut Pasteur, Inserm

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Preferential virosomal location of underphosphorylated H5R protein synthesized in vaccinia virus-infected cells.

Beaud

Beaud²

1997

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The phosphorylation state of vaccinia virus (VV) protein H5R synthesized in infected cells was investigated by two-dimensional gel electrophoresis. Most of the H5R protein was underphosphorylated (pI 5n9 to 6n8) and, on centrifugation of cell lysates, was associated with virosomes sedimenting with nuclei. However, about a quarter of the H5R protein synthesized was highly phosphorylated (pI 5n5), and this was the major form of the H5R protein present in cytoplasmic extracts. Immunofluorescence of VVinfected cells in the absence of DNA replication

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Étude des Salmonella possédant les facteurs antigéniques 6,7:c:1,5

Minor

Beaud

Laurent

et al. 1985

Annales de l'Institut Pasteur / Microbiologie

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Vaccinia virus gene H5R encodes a protein that is phosphorylated by the multisubstrate vaccinia virus B1R protein kinase

Beaud

Leader

1995

J Virol

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Vaccinia virus gene B1R encodes a protein kinase, the previously identified substrates of which include the proteins S2 and Sa of 40S ribosomal subunits. This work characterizes another substrate of the B1R kinase: a 36-kDa protein induced at the early stage of infection. Partially purified 36-kDa protein, eluted from a single-stranded DNA-cellulose column by 0.5 M NaCl, was separated by two-dimensional gel electrophoresis. Phosphorylation in vitro yielded multiple forms of the 36-kDa protein with approximate isoelectric points (pI) of 5.5, 5.7, 5.9, and 6.3, in addition to the apparently unphosphorylated form with a pI of approximately 6.8. The tryptic peptides derived from 36-kDa proteins with pI values of 5.7, 5.9, and 6.3 yielded almost identical high-pressure liquid chromatography profiles, strongly suggesting that the 36-kDa protein was modified by the phosphorylation of at least four sites, which were characterized as threonine residues. The amino acid sequence of several tryptic peptides derived from the 36-kDa protein showed that the 36-kDa protein was encoded by gene H5R of vaccinia virus. Consistent with this, the B1R kinase-either expressed in Escherichia coli or highly purified from HeLa cells-phosphorylated a recombinant trpE-H5R fusion protein in vitro. Fingerprints of the trpE-H5R and 36-kDa proteins phosphorylated by recombinant B1R kinase revealed common sites of phosphorylation, although some tryptic peptides were specific to either protein. Comparison was made of fingerprints of tryptic phosphopeptides derived from 36-kDa single-stranded DNA-binding protein labelled in vivo or in vitro. A common subset of peptides was observed, suggesting that some sites on H5R protein are phosphorylated by the B1R kinase in infected cells. These results suggest that some of the multiple threonine sites in the H5R protein are phosphorylated in vivo by the B1R protein kinase.

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R. Beaud

Preferential virosomal location of underphosphorylated H5R protein synthesized in vaccinia virus-infected cells.

Étude des Salmonella possédant les facteurs antigéniques 6,7:c:1,5

Vaccinia virus gene H5R encodes a protein that is phosphorylated by the multisubstrate vaccinia virus B1R protein kinase

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