2003
DOI: 10.1074/jbc.m212393200
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Protection of Cap-dependent Protein Synthesisin Vivo and in Vitro with an eIF4G-1 Variant Highly Resistant to Cleavage by Coxsackievirus 2A Protease

Abstract: The shutoff of host protein synthesis by certain picornaviruses is mediated, at least in part, by proteolytic cleavage of eIF4G-1. Previously, we developed a cleavage site variant of eIF4G-1, termed eIF4G-1 SM , that was 100-fold more resistant to in vitro cleavage by Coxsackievirus 2A protease (2A Pro ) than wild-type eIF4G-1 (eIF4G-1 WT ), but it was still digested at high protease concentrations. Here we identified a secondary cleavage site upstream of the primary site. We changed Gly at the P1 -position of… Show more

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Cited by 14 publications
(13 citation statements)
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“…Expression and Purification of Recombinant Proteins-The expression and purification of two fragments of eIF4G-1 (NCBI accession number NP_886553) have been described previously; eIF4G(589 -1600) is aa residues 589 -1600 with an N-terminal tag consisting of thioredoxin, His 6 , and S-peptide (52), and eIF4G(1357-1600) is similar except with aa residues 1357-1600 (53). Recombinant human MNK1 and MNK2 were expressed from plasmids pET14-His 6 -Mnk1 and pET14-His 6 -Mnk2, respectively (54).…”
Section: Methodsmentioning
confidence: 99%
“…Expression and Purification of Recombinant Proteins-The expression and purification of two fragments of eIF4G-1 (NCBI accession number NP_886553) have been described previously; eIF4G(589 -1600) is aa residues 589 -1600 with an N-terminal tag consisting of thioredoxin, His 6 , and S-peptide (52), and eIF4G(1357-1600) is similar except with aa residues 1357-1600 (53). Recombinant human MNK1 and MNK2 were expressed from plasmids pET14-His 6 -Mnk1 and pET14-His 6 -Mnk2, respectively (54).…”
Section: Methodsmentioning
confidence: 99%
“…Moreover, this assay confirmed intrinsically higher IRES stimulation and accelerated eIF4GI cleavage with CBV3 versus PV 2A pro (Fig. 6A and B -mediated eIF4GI degradation in IRES stimulation, we followed a strategy first reported by Zhao et al (56). First, we constructed expression vectors encoding eIF4GI isoforms via initiation at two of the five authentic initiating AUGs: b (41), and e (197) (numbers in paretheses correspond to the amino acid numbers of eIF4GI-a) (Fig.…”
Section: Ires Stimulation By Ev Infection Coincides With Proteolytic mentioning
confidence: 99%
“…Furthermore, we constructed eIF4G-b and eIF4GI-e variants resistant to 2A pro cleavage (eIF4G-bR and eIF4GI-eR) by altering the primary (aa 682 to 683) and secondary (aa 674 to 675) eIF4GI cleavage sites (Fig. 7A) (56). HeLa cells were transfected with plasmids expressing eIF4GI-b-eIF4GI-bR or eIF4GI-e-eIF4GI-eR or with pcDNA3.1 vector DNA.…”
Section: Ires Stimulation By Ev Infection Coincides With Proteolytic mentioning
confidence: 99%
See 1 more Smart Citation
“…The enzymes were expressed (Wang et al 2002) and purified (Zhao et al 2003) as previously described. Capped 32 P-labled oligonucleotides were subjected to digestion with either wild-type or catalytically inactive GST-hDcp2 at 37°C…”
Section: Decapping Assaysmentioning
confidence: 99%