2001
DOI: 10.1074/jbc.m007176200
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Site-directed Mutagenesis of Human Ceruloplasmin

Abstract: A fully active recombinant human ceruloplasmin was obtained, and it was mutated to produce a ceruloplasmin stable to proteolysis. The stable ceruloplasmin was further mutated to perturb the environment of copper at the type 1 copper sites in two different domains. The wild type and the mutated ceruloplasmin were produced in the yeast Pichia pastoris and characterized. The mutations R481A, R701A, and K887A were at the proteolytic sites, did not alter the enzymatic activity, and were all necessary to protect cer… Show more

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Cited by 22 publications
(10 citation statements)
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“…The gradual disjunction of the fragments diminish, and ultimately interrupts the electron transfer between the copper ions of the catalytic center in Cp. Copper ions acting independently are likely to acquire prooxidant features observed in the cleaved Cp, in contrast to the intact protein [41]. Thus, Cp-Mpo interaction favors the antioxidant activity of Cp.…”
Section: Discussionmentioning
confidence: 99%
“…The gradual disjunction of the fragments diminish, and ultimately interrupts the electron transfer between the copper ions of the catalytic center in Cp. Copper ions acting independently are likely to acquire prooxidant features observed in the cleaved Cp, in contrast to the intact protein [41]. Thus, Cp-Mpo interaction favors the antioxidant activity of Cp.…”
Section: Discussionmentioning
confidence: 99%
“…This would naturally happen when expressing membrane-bound Cp-GPI, but it could also occur with secreted Cp. In fact, although Fet3p is firmly bound to the plasma membrane, it has been reported that a fraction of Fet3p can be released into the medium by spontaneous limited proteolysis (14), and this was shown to happen also in the strain expressing recombinant Cp (9). The FLAG-tagged Cp-GPI isoform produced in yeast could be easily purified (supplemental Fig.…”
Section: Expression Of Recombinant Cp In a P Pastoris Fet3⌬ Strain-mentioning
confidence: 99%
“…The limited proteolysis with trypsin affords the same fragments; i.e., the cleavage always proceeds at the particular peptide bonds located after R481, R701, and K887 [13,15]. The replacement of these amino-acid residues by site-directed mutagenesis produced human CP resistant to proteolysis [28].…”
Section: Resultsmentioning
confidence: 98%