Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Pivot Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Target Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Query: EC:3.1.27.4 (
ribonuclease
)
6,621
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
It has been shown previously that
CaBP2
, the rat analog of the murine protein ERp72, and CaBP1, the rat analogue of the hamster protein P5, represent members of the protein disulfide isomerase (PDI) family and are able to catalyze the reduction of insulin in the presence of various reductants (Nguyen Van et al., 1993). We have now examined the abilities of
CaBP2
and CaBP1 to catalyze the renaturation of denatured reduced model proteins. Both
CaBP2
and CaBP1 catalyzed the reappearance of the biological activity of the denatured reduced Fab fragment of a monoclonal anti-human creatine phosphokinase antibody. The reaction rate was positively correlated with the amount of
CaBP2
or CaBP1 and dependent on the GSH/GSSG ratio (maximum at GSH/GSSG = 1). Peptide prolyl-cis,trans-isomerase (PPI), which catalyzed some renaturation on its own, showed synergistic effects with PDI,
CaBP2
, and CaBP1. No synergistic effects could be observed when the combinations
CaBP2
+ PDI, CaBP1 + PDI, or
CaBP2
+ CaBP1 were tested. Variation of [Ca2+] between 0 and 1 mM did not have any effect on the rate or amount of renaturation catalyzed by
CaBP2
, CaBP1, or PDI, nor were these parameters affected by the simultaneous presence of BiP or grp94. Both
CaBP2
and CaBP1 catalyzed also the renaturation of denatured reduced
ribonuclease
AIII in a way that depended on the amounts of
CaBP2
or CaBP1 and on the redox potential of the redox system used (GSH/GSSG or CSH/CSSC). PPI alone had no effect on the rate of RNase AIII renaturation and did not significantly affect renaturation catalyzed by PDI,
CaBP2
, or CaBP1. PDI showed a moderate but significant synergism with
CaBP2
, and a strong synergism with CaBP1. The results indicate that both
CaBP2
and CaBP1 can catalyze the formation of disulfide bonds and protein disulfide isomerization and may thus be involved in the folding of nascent proteins in the secretory pathway. This does not exclude the possibility of additional functions of these proteins in the pre-Golgi compartments.
...
PMID:Effects of CaBP2, the rat analog of ERp72, and of CaBP1 on the refolding of denatured reduced proteins. Comparison with protein disulfide isomerase. 830 May 76
The rat luminal endoplasmic-recticulum calcium-binding proteins 1 and 2 (CaBP1 and
CaBP2
respectively) are members of the protein disulphide-isomerase (PDI) family. They contain two and three thioredoxin boxes (Cys-Gly-His-Cys) respectively and, like PDI, may be involved in the folding of nascent proteins. We demonstrate here that CaBP1, similar to PDI and
CaBP2
, can complement the lethal phenotype of the disrupted Saccharomyces cerevisiae PDI gene, provided that the natural C-terminal Lys-Asp-Glu-Leu sequence is replaced by His-Asp-Glu-Leu. Both the in vitro RNase AIII-re-activation assays and in vivo pro-(carboxypeptidase Y) processing assays using CaBP1 and
CaBP2
thioredoxin (trx)-box mutants revealed that, whereas the three trx boxes in
CaBP2
seem to be functionally equivalent, the first trx box of CaBP1 is significantly more active than the second trx box. Furthermore, only about 65% re-activation of denatured reduced RNase AIII could be obtained with CaBP1 or
CaBP2
compared with PDI, and the yield of PDI-catalysed reactions was significantly reduced in the presence of either CaBP1 or
CaBP2
. In contrast with PDI, neither CaBP1 nor
CaBP2
could catalyse the renaturation of denatured glyceraldehyde-3-phosphate dehydrogenase (GAPDH), which is a redox-independent process, and neither protein had any effect on the PDI-catalysed refolding of GAPDH. Furthermore, although PDI can bind peptides via its b' domain, a property it shares with PDIp, the pancreas-specific PDI homologue, and although PDI can bind malfolded proteins such as 'scrambled'
ribonuclease
, no such interactions could be detected for
CaBP2
. We conclude that: (1) both
CaBP2
and CaBP1 lack peptide-binding activity for GAPDH attributed to the C-terminal region of the a' domain of PDI; (2)
CaBP2
lacks the general peptide-binding activity attributed to the b' domain of PDI; (3) interaction of
CaBP2
with substrate (RNase AIII) is different from that of PDI and substrate; and (4) both
CaBP2
and CaBP1 may promote oxidative folding by different kinetic pathways.
...
PMID:Functional roles and efficiencies of the thioredoxin boxes of calcium-binding proteins 1 and 2 in protein folding. 1141 39
