PDBsum entry 6pha

Hydrolase

PDB id

6pha

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Contents

			Protein chain

					297 a.a.

			Ligands

					VO4


					GOL ×5


					ACT ×3

			Waters ×152

PDB id:

6pha

Links

Name:

Hydrolase

Title:

Protein tyrosine phosphatase 1b (1-301), f182a mutant, vanadate bound state

Structure:

Tyrosine-protein phosphatase non-receptor type 1. Chain: a. Synonym: protein-tyrosine phosphatase 1b,ptp-1b. Engineered: yes. Mutation: yes

Source:

Homo sapiens. Human. Organism_taxid: 9606. Gene: ptpn1, ptp1b. Expressed in: escherichia coli bl21(de3). Expression_system_taxid: 469008.

Resolution:

2.30Å

R-factor:

0.227

R-free:

0.277

Authors:

D.S.Cui,J.M.Lipchock,J.P.Loria

Key ref:

D.S.Cui et al. (2019). Uncovering the Molecular Interactions in the Catalytic Loop That Modulate the Conformational Dynamics in Protein Tyrosine Phosphatase 1B. J Am Chem Soc, 141, 12634-12647. PubMed id: 31339043 DOI: 10.1021/jacs.9b04470

Date:

25-Jun-19

Release date:

07-Aug-19

PROCHECK

	Headers

	References

Protein chain

P18031 (PTN1_HUMAN) - Tyrosine-protein phosphatase non-receptor type 1 from Homo sapiens

Seq: Struc:					435 a.a. 297 a.a.*

Key:

PfamA domain

Secondary structure

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



		Enzyme reactions

Enzyme class:

E.C.3.1.3.48 - protein-tyrosine-phosphatase.

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

Reaction:

O-phospho-L-tyrosyl-[protein] + H2O = L-tyrosyl-[protein] + phosphate

O-phospho-L-tyrosyl-[protein]	+	H2O	=	L-tyrosyl-[protein]	+	phosphate

Molecule diagrams generated from .mol files obtained from the KEGG ftp site

Key reference

DOI no: 10.1021/jacs.9b04470	J Am Chem Soc 141:12634-12647 (2019)
PubMed id: 31339043

Uncovering the Molecular Interactions in the Catalytic Loop That Modulate the Conformational Dynamics in Protein Tyrosine Phosphatase 1B.
D.S.Cui, J.M.Lipchock, D.Brookner, J.P.Loria.

ABSTRACT

Active-site loops are integral to the function of numerous enzymes. They enable substrate and product binding and release, sequester reaction intermediates, and recruit catalytic groups. Here, we examine the catalytic loop in the enzyme protein tyrosine phosphatase 1B (PTP1B). PTP1B has a mobile so-called WPD loop (named for its three N-terminal residues) that initiates the dephosphorylation of phosphor-tyrosine substrates upon loop closure. We have combined X-ray crystallography, solution NMR, and pre-steady-state kinetics experiments on wild-type and five WPD loop mutants to identify the relationships between the loop structure, dynamics, and function. The motions of the WPD loop are modulated by the formation of weak molecular interactions, where perturbations of these interactions modulate the conformational equilibrium landscape. The point mutants in the WPD loop alter the loop equilibrium position from a predominantly open state (P185A) to 50:50 (F182A), 35:65 (P188A), and predominantly closed states (T177A and P188A). Surprisingly, there is no correlation between the observed catalytic rates in the loop mutants and changes to the WPD loop equilibrium position. Rather, we observe a strong correlation between the rate of dephosphorylation of the phosphocysteine enzyme intermediate and uniform millisecond motions, not only within the loop but also in the adjacent α-helical domain of PTP1B. Thus, the control of loop motion and thereby catalytic activity is dispersed and resides within not only the loop sequence but also the surrounding protein architecture. This has broad implications for the general mechanistic understanding of enzyme reactions and the role that flexible loops play in the catalytic cycle.