1989
DOI: 10.1016/0042-6822(89)90132-3
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Characterization of the catalytic residues of the tobacco etch virus 49-kDa proteinase

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Cited by 132 publications
(84 citation statements)
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“…The 151 amino acid deletion of ASX protease rendered it inactive at all cleavage sites analysed, as did the Gin or Leu substitutions for His 239. As a Tyr for His 234 substitution had been previously shown to render the TEV 49K protease inactive for its autocatalytic processing (Dougherty et al, 1989b), our results support the previous identification of this His residue as part of the catalytic triad of the potyviral protease (Dougherty et al, 1989b). Dougherty et al (1989b) also reported that substituting Glu for Asp at position 269 of the TEV 49K protease resulted in an anomalous proteolytic activity capable of cutting at the 49K N-terminal cleavage site but not at the C-terminal one.…”
Section: Discussionsupporting
confidence: 80%
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“…The 151 amino acid deletion of ASX protease rendered it inactive at all cleavage sites analysed, as did the Gin or Leu substitutions for His 239. As a Tyr for His 234 substitution had been previously shown to render the TEV 49K protease inactive for its autocatalytic processing (Dougherty et al, 1989b), our results support the previous identification of this His residue as part of the catalytic triad of the potyviral protease (Dougherty et al, 1989b). Dougherty et al (1989b) also reported that substituting Glu for Asp at position 269 of the TEV 49K protease resulted in an anomalous proteolytic activity capable of cutting at the 49K N-terminal cleavage site but not at the C-terminal one.…”
Section: Discussionsupporting
confidence: 80%
“…As a Tyr for His 234 substitution had been previously shown to render the TEV 49K protease inactive for its autocatalytic processing (Dougherty et al, 1989b), our results support the previous identification of this His residue as part of the catalytic triad of the potyviral protease (Dougherty et al, 1989b). Dougherty et al (1989b) also reported that substituting Glu for Asp at position 269 of the TEV 49K protease resulted in an anomalous proteolytic activity capable of cutting at the 49K N-terminal cleavage site but not at the C-terminal one. Interestingly, the effect of the replacement of the Asp 274 of PPV NIa, which corresponds to Asp 269 of TEV (Garcia et al, 1989a), by Glu also depended on the cleavage site analysed: D274E NIa protease cleaved at the NIb-CP junction almost as efficiently as the wildtype protease and at the CI-6K site with low efficiency, whereas cleavage at the C terminus of the NIa protease was undetectable in our system (Fig.…”
Section: Discussionsupporting
confidence: 80%
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