PDBsum entry 1sp4

Hydrolase/hydrolase inhibitor

PDB id

1sp4

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Contents

			Protein chains

					48 a.a. *


					205 a.a. *

			Ligands

					EP2

			Waters ×176

* Residue conservation analysis

PDB id:

1sp4

Links

Name:

Hydrolase/hydrolase inhibitor

Title:

Crystal structure of ns-134 in complex with bovine cathepsin b: a two headed epoxysuccinyl inhibitor extends along the whole active site cleft

Structure:

Cathepsin b. Chain: a. Fragment: light chain. Cathepsin b. Chain: b. Fragment: heavy chain. Ec: 3.4.22.1

Source:

Bos taurus. Cattle. Organism_taxid: 9913. Tissue: kidney. Tissue: kidney

Biol. unit:

Trimer (from PQS)

Resolution:

2.20Å

R-factor:

0.194

Authors:

I.Stern,N.Schaschke,L.Moroder,D.Turk

Key ref:

I.Stern et al. (2004). Crystal structure of NS-134 in complex with bovine cathepsin B: a two-headed epoxysuccinyl inhibitor extends along the entire active-site cleft. Biochem J, 381, 511-517. PubMed id: 15084146

Date:

16-Mar-04

Release date:

04-May-04

PROCHECK

	Headers

	References

Protein chain

P07688 (CATB_BOVIN) - Cathepsin B from Bos taurus

Seq: Struc:					335 a.a. 48 a.a.

Protein chain

P07688 (CATB_BOVIN) - Cathepsin B from Bos taurus

Seq: Struc:					335 a.a. 205 a.a.*

Key:

PfamA domain

Secondary structure

CATH domain

* PDB and UniProt seqs differ at 1 residue position (black cross)



		Enzyme reactions

Enzyme class:

Chains A, B: E.C.3.4.22.1 - cathepsin B.

[IntEnz] [ExPASy] [KEGG] [BRENDA]

Reaction:

Hydrolysis of proteins with broad specificity for peptide bonds. Preferentially cleaves -Arg-Arg-|-Xaa bonds in small molecule substrates (thus differing from cathepsin L). In addition to being an endopeptidase, shows peptidyl-dipeptidase activity, liberating C-terminal dipeptides.

	Biochem J 381:511-517 (2004)
PubMed id: 15084146

Crystal structure of NS-134 in complex with bovine cathepsin B: a two-headed epoxysuccinyl inhibitor extends along the entire active-site cleft.
I.Stern, N.Schaschke, L.Moroder, D.Turk.

ABSTRACT

The crystal structure of the inhibitor NS-134 in complex with bovine cathepsin B reveals that functional groups attached to both sides of the epoxysuccinyl reactive group bind to the part of active-site cleft as predicted. The -Leu-Pro-OH side binds to the primed binding sites interacting with the His110 and His111 residues with its C-terminal carboxy group, whereas the -Leu-Gly-Meu (-Leu-Gly-Gly-OMe) part (Meu, methoxycarbonylmethyl) binds along the non-primed binding sites. Comparison with the propeptide structures of cathepsins revealed that the binding of the latter part is least similar to the procathepsin B structure; this result, together with the two-residue shift in positioning of the Leu-Gly-Gly part, suggests that the propeptide structures of the cognate enzymes may not be the best starting point for the design of reverse binding inhibitors.

Literature references that cite this PDB file's key reference

PubMed id

Reference

19020347

M.Andrejasic, J.Praaenikar, and D.Turk (2008).
PURY: a database of geometric restraints of hetero compounds for refinement in complexes with macromolecular structures.

Acta Crystallogr D Biol Crystallogr, 64, 1093-1109.

15776409

S.H.Verhelst, and M.Bogyo (2005).
Solid-phase synthesis of double-headed epoxysuccinyl activity-based probes for selective targeting of papain family cysteine proteases.

Chembiochem, 6, 824-827.

The most recent references are shown first. Citation data come partly from CiteXplore and partly from an automated harvesting procedure. Note that this is likely to be only a partial list as not all journals are covered by either method. However, we are continually building up the citation data so more and more references will be included with time.