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PDBsum entry 6mjs
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Electron transport
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PDB id
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6mjs
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PDB id:
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| Name: |
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Electron transport
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Title:
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Azurin 122w/124w/126re
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Structure:
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Azurin. Chain: a, b, c, d. Engineered: yes. Mutation: yes
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Source:
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Pseudomonas aeruginosa (strain atcc 15692 / dsm 22644 / cip 104116 / jcm 14847 / lmg 12228 / 1c / prs 101 / pao1). Organism_taxid: 208964. Strain: atcc 15692 / dsm 22644 / cip 104116 / jcm 14847 / lmg 12228 / 1c / prs 101 / pao1. Gene: azu, pa4922. Expressed in: escherichia coli bl21(de3). Expression_system_taxid: 469008
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Resolution:
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1.85Å
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R-factor:
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0.170
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R-free:
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0.198
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Authors:
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K.Takematsu,S.Zalis,H.B.Gray,A.Vlcek,J.R.Winkler,H.Williamson, J.T.Kaiser,J.Heyda,D.Hollas
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Key ref:
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K.Takematsu
et al.
(2019).
Two Tryptophans Are Better Than One in Accelerating Electron Flow through a Protein.
ACS Cent Sci,
5,
192-200.
PubMed id:
DOI:
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Date:
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21-Sep-18
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Release date:
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20-Feb-19
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PROCHECK
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Headers
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References
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P00282
(AZUR_PSEAE) -
Azurin from Pseudomonas aeruginosa (strain ATCC 15692 / DSM 22644 / CIP 104116 / JCM 14847 / LMG 12228 / 1C / PRS 101 / PAO1)
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Seq:
Struc:
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148 a.a.
128 a.a.*
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Key: |
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PfamA domain |
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Secondary structure |
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*
PDB and UniProt seqs differ
at 7 residue positions (black
crosses)
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DOI no:
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ACS Cent Sci
5:192-200
(2019)
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PubMed id:
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Two Tryptophans Are Better Than One in Accelerating Electron Flow through a Protein.
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K.Takematsu,
H.R.Williamson,
P.Nikolovski,
J.T.Kaiser,
Y.Sheng,
P.Pospíšil,
M.Towrie,
J.Heyda,
D.Hollas,
S.Záliš,
H.B.Gray,
A.Vlček,
J.R.Winkler.
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ABSTRACT
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We have constructed and structurally characterized a Pseudomonas
aeruginosa azurin mutant Re126WWCuI , where two adjacent
tryptophan residues (W124 and W122, indole separation 3.6-4.1 Å) are inserted
between the CuI center and a Re photosensitizer coordinated to the
imidazole of H126
(ReI(H126)(CO)3(4,7-dimethyl-1,10-phenanthroline)+).
CuI oxidation by the photoexcited Re label (*Re) 22.9 Å away
proceeds with a ∼70 ns time constant, similar to that of a single-tryptophan
mutant (∼40 ns) with a 19.4 Å Re-Cu distance. Time-resolved spectroscopy
(luminescence, visible and IR absorption) revealed two rapid reversible electron
transfer steps, W124 → *Re (400-475 ps, K1 ≅ 3.5-4) and
W122 → W124•+ (7-9 ns, K2 ≅ 0.55-0.75),
followed by a rate-determining (70-90 ns) CuI oxidation by
W122•+ ca. 11 Å away. The photocycle is completed by 120 μs
recombination. No photochemical CuI oxidation was observed in
Re126FWCuI , whereas in Re126WFCuI , the
photocycle is restricted to the ReH126W124 unit and CuI remains
isolated. QM/MM/MD simulations of Re126WWCuI indicate that
indole solvation changes through the hopping process and W124 → *Re electron
transfer is accompanied by water fluctuations that tighten W124 solvation. Our
finding that multistep tunneling (hopping) confers a ∼9000-fold advantage over
single-step tunneling in the double-tryptophan protein supports the proposal
that hole-hopping through tryptophan/tyrosine chains protects enzymes from
oxidative damage.
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