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PDBsum entry 3hq2
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Contents |
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* Residue conservation analysis
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PDB id:
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Hydrolase
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Title:
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Bsucp crystal structure
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Structure:
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Bacillus subtilis m32 carboxypeptidase. Chain: a, b. Engineered: yes
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Source:
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Bacillus subtilis. Organism_taxid: 1423. Strain: 168. Gene: bsu22080, ypwa. Expressed in: escherichia coli. Expression_system_taxid: 562.
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Resolution:
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2.90Å
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R-factor:
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0.188
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R-free:
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0.251
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Authors:
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M.M.Lee,C.E.Isaza,J.D.White,R.P.-Y.Chen,G.F.-C.Liang,H.T.-F.He, S.I.Chan,M.K.Chan
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Key ref:
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M.M.Lee
et al.
(2009).
Insight into the substrate length restriction of M32 carboxypeptidases: Characterization of two distinct subfamilies.
Proteins,
77,
647-657.
PubMed id:
DOI:
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Date:
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05-Jun-09
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Release date:
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30-Jun-09
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PROCHECK
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Headers
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References
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P50848
(CBP1_BACSU) -
Carboxypeptidase 1 from Bacillus subtilis (strain 168)
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Seq:
Struc:
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501 a.a.
496 a.a.
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Key: |
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PfamA domain |
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Secondary structure |
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CATH domain |
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Enzyme class:
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E.C.3.4.17.19
- carboxypeptidase Taq.
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Reaction:
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Release of a C-terminal amino acid with broad specificity, except for -Pro.
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Cofactor:
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Zn(2+)
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DOI no:
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Proteins
77:647-657
(2009)
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PubMed id:
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Insight into the substrate length restriction of M32 carboxypeptidases: Characterization of two distinct subfamilies.
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M.M.Lee,
C.E.Isaza,
J.D.White,
R.P.Chen,
G.F.Liang,
H.T.He,
S.I.Chan,
M.K.Chan.
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ABSTRACT
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M32 carboxypeptidases are a distinct family of HEXXH metalloproteases whose
structures exhibit a narrow substrate groove that is blocked at one end.
Structural alignments with other HEXXH metalloprotease-peptide complexes
suggested an orientation in which the substrate is directed towards the back of
the groove. This led us to hypothesize, and subsequently confirm that the
maximum substrate length for M32 carboxypeptidases is restricted. Structural and
sequence analyses implicate a highly conserved Arg at the back of the groove as
being critical for this length restriction. However, the Thermus thermophilus
and Bacillus subtilis M32 members lack this conserved Arg. Herein, we present
the biochemical and structural characterization of these two proteins. Our
findings support the important role of the conserved Arg in maintaining the
length restriction, and reveal a proline-rich loop as an alternate blocking
strategy. Based on our results, we propose that M32 carboxypeptidases from
Bacilli belong to a separate subfamily. Proteins 2009. (c) 2009 Wiley-Liss, Inc.
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Selected figure(s)
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Figure 1.
Figure 1. Structural comparison of the subunit conformations of
PfuCP (open), TthCP (open) and BsuCP (closed). (A) Ribbons
diagram of PfuCP (PDB ID: 1KA2) colored in pink with the  -helices
of the subdomain associated with the groove closure in red. The
residues forming the metal active site are shown in ball and
stick. The bound Mg ion is colored in green and the remaining
ions in CPK. (B) Ribbons diagram of TthCP in the same
orientation colored in tan with the -helices
of the subdomain associated with the conformational change in
green. The residues forming the metal active site are shown in
ball and stick. (C) Ribbons diagram of BsuCP subunit colored in
cyan with the -helices
of the subdomain associated with the conformational change in
blue. The residues forming the zinc active site are shown in
ball and stick. The zinc ion is colored in orange and the
remaining ions in CPK. (D) Overlap of the TthCP (colored in tan
and green) and BsuCP (colored in cyan and blue) structures
aligned based on their common HEXXH motif. The subdomain
exhibiting the largest shift is colored in green and blue,
respectively. (E) Surface diagram of PfuCP showing the open
conformation of the groove. The green color indicates the
location of the metal active site. (F) Surface diagram of TthCP
showing the open conformation of the groove. (G) Surface diagram
of BsuCP showing closed groove conformation.
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Figure 3.
Figure 3. Comparison of the PfuCP/BsuCP active sites with ACE2
in the open and closed conformations. Ribbons diagram of protein
with side chains of key active site residues as stick drawings.
The metal ion is shown as a green sphere and its bonds to its
ligating residues are shown in stick. (A) PfuCP (PDB ID: 1KA4)
active site in open conformation with ribbons and carbons
colored in pink remaining elements in CPK. For this figure, the
ring of His A411 of PfuCP was rotated by 180° to be
consistent with the higher resolution TthCP structure and the
orientation of the conserved residue in the BsuCP structure. (B)
BsuCP active site in closed conformation with bound phosphate
ion with ribbons colored in cyan. (C) ACE2 (PDB ID: 1R42) active
site in open conformation in absence of bound substrate with
ribbons colored in yellow.[31] (D) ACE2 (PDB ID: 1R4L) active
site in closed conformation with ribbons colored in yellow and
carbons of bound MLN-4760 inhibitor colored in cyan and the
remaining atoms in CPK.[31] For panels (C) and (D), the ring of
His A505 was rotated by 180° to allow formation of a
hydrogen bond between its NE2 ring nitrogen and the Tyr A515
oxygen. The presence of this potential hydrogen bond was
predicted from their contact distance (  2.7
Å) in the 1R4L structure. This distance is long 3.3
Å in the 1R4L structure, but its His A505 was flipped as
well for consistency.
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The above figures are
reprinted
by permission from John Wiley & Sons, Inc.:
Proteins
(2009,
77,
647-657)
copyright 2009.
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Figures were
selected
by an automated process.
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Links
