The Structure of the Staphylococcus aureus Sortase-Substrate Complex Reveals How the Universally Conserved LPXTG Sorting Signal Is Recognized

Suree, Nuttee; Liew, Chu Kong; Villareal, Valerie A.; Thieu, William; Fadeev, Evgeny A.; Clemens, Jeremy J.; Jung, Michael E.; Clubb, Robert T.

doi:10.1074/jbc.m109.022624

Cited by 175 publications

(404 citation statements)

References 68 publications

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“…Inhibitor, calcium, and the mutation site for Tby are shown as red sticks, a white sphere, and an orange sphere, respectively. The ligand and calcium coordinates were taken from the PDB files 2MLM 18 and 2KID, 20 respectively. The observed chemical shift changes can be described by eq 1: (Figure 3C), in close agreement with the value determined by ITC measurement.…”

Section: ■ Resultsmentioning

confidence: 99%

O-tert-Butyltyrosine, an NMR Tag for High-Molecular-Weight Systems and Measurements of Submicromolar Ligand Binding Affinities

Chen

Kuppan

Lee³

et al. 2015

J. Am. Chem. Soc.

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O-tert-Butyltyrosine (Tby) is an unnatural amino acid that can be site-specifically incorporated into proteins using established orthogonal aminoacyl-tRNA synthetase/tRNA systems. Here we show that the tert-butyl group presents an outstanding NMR tag that can readily be observed in one-dimensional 1 H NMR spectra without any isotope labeling. Owing to rapid bond rotations and the chemical equivalence of the protons of a solvent-exposed tert-butyl group from Tby, the singlet resonance from the tert-butyl group generates an easily detectable narrow signal in a spectral region with limited overlap with other methyl resonances. The potential of the tert-butyl 1 H NMR signal in protein research is illustrated by the observation and assignment of two resonances in the Bacillus stearothermophilus DnaB hexamer (320 kDa), demonstrating that this protein preferentially assumes a 3-fold rather than 6-fold symmetry in solution, and by the quantitative measurement of the submicromolar dissociation constant K d (0.2 μM) of the complex between glutamate and the Escherichia coli aspartate/ glutamate binding protein (DEBP, 32 kDa). The outstanding signal height of the 1 H NMR signal of the Tby tert-butyl group allows K d measurements using less concentrated protein solutions than usual, providing access to K d values 1 order of magnitude lower than established NMR methods that employ direct protein detection for K d measurements.

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Section: ■ Resultsmentioning

confidence: 99%

O-tert-Butyltyrosine, an NMR Tag for High-Molecular-Weight Systems and Measurements of Submicromolar Ligand Binding Affinities

Chen

Kuppan

Lee³

et al. 2015

J. Am. Chem. Soc.

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show abstract

“…These results are consistent with mapping of the GGG-binding region proposed by NMR amide backbone chemical shift data. The chemical shifts of the visible amide hydrogen resonances for residues 92-97 and 165 were among the most perturbed upon binding of a Gly 3 peptide (29). Because of the absence of a high-resolution structure of the srtA-Gly 3 complex at this time, it is difficult to rationalize in more detail the basis of altered K m GGG among evolved mutants.…”

Section: Directed Evolution Of Sortase a Enzymes With Improved Catalyticmentioning

confidence: 92%

“…The effects of the individual mutations on LPETG substrate recognition can be rationalized in light of the reported solution structure of WT S. aureus srtA covalently bound to an LPAT peptide substrate (29). The mutated residues are all located at the surface of the enzyme, near the LPAT-binding groove (Fig.…”

Section: Directed Evolution Of Sortase a Enzymes With Improved Catalyticmentioning

confidence: 99%

A general strategy for the evolution of bond-forming enzymes using yeast display

Chen

Dorr

Liu

2011

Proc. Natl. Acad. Sci. U.S.A.

503

584

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The ability to routinely generate efficient protein catalysts of bondforming reactions chosen by researchers, rather than nature, is a long-standing goal of the molecular life sciences. Here, we describe a directed evolution strategy for enzymes that catalyze, in principle, any bond-forming reaction. The system integrates yeast display, enzyme-mediated bioconjugation, and fluorescence-activated cell sorting to isolate cells expressing proteins that catalyze the coupling of two substrates chosen by the researcher. We validated the system using model screens for Staphylococcus aureus sortase A-catalyzed transpeptidation activity, resulting in enrichment factors of 6,000-fold after a single round of screening. We applied the system to evolve sortase A for improved catalytic activity. After eight rounds of screening, we isolated variants of sortase A with up to a 140-fold increase in LPETG-coupling activity compared with the starting wild-type enzyme. An evolved sortase variant enabled much more efficient labeling of LPETG-tagged human CD154 expressed on the surface of HeLa cells compared with wild-type sortase. Because the method developed here does not rely on any particular screenable or selectable property of the substrates or product, it represents a powerful alternative to existing enzyme evolution methods.

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“…We used the structural coordinates from the SrtA substrate complex [SrtA/LPAT*; Protein Data Bank (PDB) ID code 2KID] to model the enzyme active site as a target for computational screening (14). The scaffold of topsentin A, a natural product that inhibits sortase A in vitro (15), Significance Antiinfectives, drugs that inhibit virulence strategies of microbial pathogens without affecting bacterial growth, may prevent hospital-acquired infections caused by antibiotic-resistant Staphylococcus aureus.…”

Section: Resultsmentioning

confidence: 99%

Antiinfective therapy with a small molecule inhibitor of Staphylococcus aureus sortase

Zhang

Liu

Zhu

et al. 2014

Proc. Natl. Acad. Sci. U.S.A.

133

145

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Methicillin-resistant Staphylococcus aureus (MRSA) is the most frequent cause of hospital-acquired infection, which manifests as surgical site infections, bacteremia, and sepsis. Due to drug-resistance, prophylaxis of MRSA infection with antibiotics frequently fails or incites nosocomial diseases such as Clostridium difficile infection. Sortase A is a transpeptidase that anchors surface proteins in the envelope of S. aureus, and sortase mutants are unable to cause bacteremia or sepsis in mice. Here we used virtual screening and optimization of inhibitor structure to identify 3-(4-pyridinyl)-6-(2-sodiumsulfonatephenyl) [1,2,4]

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The Structure of the Staphylococcus aureus Sortase-Substrate Complex Reveals How the Universally Conserved LPXTG Sorting Signal Is Recognized

Cited by 175 publications

References 68 publications

O-tert-Butyltyrosine, an NMR Tag for High-Molecular-Weight Systems and Measurements of Submicromolar Ligand Binding Affinities

O-tert-Butyltyrosine, an NMR Tag for High-Molecular-Weight Systems and Measurements of Submicromolar Ligand Binding Affinities

A general strategy for the evolution of bond-forming enzymes using yeast display

Antiinfective therapy with a small molecule inhibitor of Staphylococcus aureus sortase

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