2008
DOI: 10.1016/j.ab.2008.06.022
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An Escherichia coli expression system for glutamyl endopeptidases optimized by complete suppression of autodegradation

Abstract: V8 protease (GluV8), a member of the glutamyl endopeptidase I family, isolated from the V8 strain of Staphylococcus aureus, is widely utilized for proteome analysis because of its unique substrate specificity and resistance to detergents. We recently developed an Escherichia coli expression system for the production of GluV8 based on a technique that suppresses the auto-proteolysis: the use of the prosequence of its homolog (GluSE) from Staphylococcus epidermidis as a chimeric form or the introduction of 4 sub… Show more

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Cited by 6 publications
(3 citation statements)
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“…This part might be accidentally tagged as a result of a T-to-G mutation from the stop codon (TGA) into Gly 711 (GGA) in the PeDPP7 gene. Similarly, a glutamic acid-specific V8 protease, GluV8, belonging to the S46 family was found to be tagged with the C-terminal 48 amino acid residues, which have been shown to be non-essential for the activity [35] , [36] . The characteristic GluV8 tag is 12 repeats of the triplet Pro-Asp/Asn-Asn [37] .…”
Section: Discussionmentioning
confidence: 99%
“…This part might be accidentally tagged as a result of a T-to-G mutation from the stop codon (TGA) into Gly 711 (GGA) in the PeDPP7 gene. Similarly, a glutamic acid-specific V8 protease, GluV8, belonging to the S46 family was found to be tagged with the C-terminal 48 amino acid residues, which have been shown to be non-essential for the activity [35] , [36] . The characteristic GluV8 tag is 12 repeats of the triplet Pro-Asp/Asn-Asn [37] .…”
Section: Discussionmentioning
confidence: 99%
“…The N-terminal Ser of the active SprE was numbered as the first amino acid residue (Ser1). In vitro mutagenesis was performed as reported previously [30] by PCR with mutated primer(s) to substitute 3 amino acids in the prosequence (Glu -15 Ser, Glu -14 Lys, Glu -8 Ile, designated as SprE-mut), 4 amino acids in the mature region (Glu11Gln, Glu6Gln, Ser1Thr/Ala/Val and Leu2Val), and an essential Ser 180 to Ala. All mutations were confirmed by DNA sequencing.…”
Section: Amino Acid Numbering and In Vitro Mutagenesismentioning
confidence: 99%
“…The autodegradation of Staphylococcal glutamyl endopeptidases occurring within the proseuqence region was efficiently suppressed by the substitution of Glu and Asp in the proseqquences, to Gln, Asn or other amino acids [25,30]. Here, this strategy was introduced at the N-terminal region of mature SprE.…”
Section: Suppression Of Auto-degradation Of Mature Sprementioning
confidence: 99%