Combined Solution and Crystal Methods Reveal the Electrostatic Tethers That Provide a Flexible Platform for Replication Activities in the Bacteriophage T7 Replisome

Foster, Brittni M.; Rosenberg, Daniel; Salvo, Henry; Stephens, Kasie L.; Bintz, Brittania J.; Hammel, Michal; Ellenberger, Tom; Gainey, Maria D.; Wallen, Jamie R.

doi:10.1021/acs.biochem.9b00525

Cited by 10 publications

(5 citation statements)

References 52 publications

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“…The scattering vector is defined as q = 4π sin θ/λ, where 2θ is the scattering angle. All experiments were performed at 20 °C and data was collected and processed as previously described . A SAXS flow cell was directly coupled with an online Agilent 1260 Infinity HPLC system using a Shodex KW803 column.…”

Section: Methodsmentioning

confidence: 99%

“…All experiments were performed at 20 °C and data was collected and processed as previously described. 24 A SAXS flow cell was directly coupled with an online Agilent 1260 Infinity HPLC system using a Shodex KW803 column. The column was equilibrated with a running buffer (20 mM Tris pH 7.0, 100 mM NaCl, 1 mM DTT) with a flow rate of 0.6 mL/min.…”

Section: ■ Experimental Sectionmentioning

confidence: 99%

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Structural Characterization of Sphingomonas sp. KT-1 PahZ1-Catalyzed Biodegradation of Thermally Synthesized Poly(aspartic acid)

Brambley

Bolay

Salvo

et al. 2020

ACS Sustainable Chem. Eng.

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Poly(aspartic acid) (PAA) is a green alternative to nonbiodegradable poly(carboxylates) and has applications in both industrial and biomedical settings. PAA is synthesized by heating monomeric aspartic acid to yield a polysuccinamide that can be ring-opened to yield thermal PAA composed of 30% α-amide and 70% β-amide linkages. Here, we report the first X-ray crystal structure of a PAA hydrolase from the bacteria Sphingomonas sp. KT-1 (PahZ1 KT-1 ) which functions to degrade synthetic PAA to oligo(aspartic acid) by selective cleavage of β-amide linkages. The structure was solved to 2.45 Å and shows a dimeric assembly where each monomer maintains an α/β hydrolase fold with a prominent, positively lined trough responsible for binding the anionic polymeric substrate. The putative catalytic sites of each monomer lie at the surface of the enzyme on opposite faces. The dimeric interface, as supported by small-angle X-ray scattering/multi-angle light scattering data, is primarily hydrophobic and is further stabilized by flanking hydrogen bonds. Molecular dynamics simulations support the previously determined specific cleavage of only the β-amide linkage through a conformational change that aligns the substrate with the active site Ser. These data provide a scaffold for further understanding the mechanism of PAA hydrolysis and opens the opportunity for using protein engineering to catalyze the biodegradation of other xenobiotics.

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Section: Methodsmentioning

confidence: 99%

Section: ■ Experimental Sectionmentioning

confidence: 99%

Structural Characterization of Sphingomonas sp. KT-1 PahZ1-Catalyzed Biodegradation of Thermally Synthesized Poly(aspartic acid)

Brambley

Bolay

Salvo

et al. 2020

ACS Sustainable Chem. Eng.

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“…Magnesium ions are shown as green spheres in the exonuclease and polymerase active sites. The structure was drawn using Pymol from PDBID: 6p7e ( 41 ). …”

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confidence: 99%

Conformational dynamics during high-fidelity DNA replication and translocation defined using a DNA polymerase with a fluorescent artificial amino acid

Dangerfield

Johnson²

2021

Journal of Biological Chemistry

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We address the role of enzyme conformational dynamics in specificity for a high-fidelity DNA polymerase responsible for genome replication. We present the complete characterization of the conformational dynamics during the correct nucleotide incorporation forward and reverse reactions using stopped-flow and rapid-quench methods with a T7 DNA polymerase variant containing a fluorescent unnatural amino acid, (7-hydroxy-4-coumarin-yl) ethylglycine, which provides a signal for enzyme conformational changes. We show that the forward conformational change (>6000 s −1 ) is much faster than chemistry (300 s −1 ) while the enzyme opening to allow release of bound nucleotide (1.7 s −1 ) is much slower than chemistry. These parameters show that the conformational change selects a correct nucleotide for incorporation through an induced-fit mechanism. We also measured conformational changes occurring after chemistry and during pyrophosphorolysis, providing new insights into processive polymerization. Pyrophosphorolysis occurs via a conformational selection mechanism as the pyrophosphate binds to a rare pretranslocation state of the enzyme–DNA complex. Global data fitting was achieved by including experiments in the forward and reverse directions to correlate conformational changes with chemical reaction steps. This analysis provided well-constrained values for nine rate constants to establish a complete free-energy profile including the rates of DNA translocation during processive synthesis. Translocation does not follow Brownian ratchet or power stroke models invoking nucleotide binding as the driving force. Rather, translocation is rapid and thermodynamically favorable after enzyme opening and pyrophosphate release, and it appears to limit the rate of processive synthesis at 4 °C.

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“…Other than vvUNG, the only known DNA polymerase processivity factor not belonging to the clamp superfamily is thioredoxin, a bacterial protein adopted as a processivity subunit by bacteriophage T7 DNA polymerase. Thioredoxin, however, does not seem to contact DNA directly but rather stabilizes a long polymerase loop that tracks along DNA [69][70][71][72]. Additionally, single-strand binding proteins, although not considered processivity subunits in a strict sense, often enhance the processivity of DNA polymerases and have been used toward this end in fusion constructs [73,74].…”

Section: Discussionmentioning

confidence: 99%

Correlated Target Search by Vaccinia Virus Uracil–DNA Glycosylase, a DNA Repair Enzyme and a Processivity Factor of Viral Replication Machinery

Diatlova

Mechetin

Yudkina

et al. 2023

IJMS

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The protein encoded by the vaccinia virus D4R gene has base excision repair uracil–DNA N-glycosylase (vvUNG) activity and also acts as a processivity factor in the viral replication complex. The use of a protein unlike PolN/PCNA sliding clamps is a unique feature of orthopoxviral replication, providing an attractive target for drug design. However, the intrinsic processivity of vvUNG has never been estimated, leaving open the question whether it is sufficient to impart processivity to the viral polymerase. Here, we use the correlated cleavage assay to characterize the translocation of vvUNG along DNA between two uracil residues. The salt dependence of the correlated cleavage, together with the similar affinity of vvUNG for damaged and undamaged DNA, support the one-dimensional diffusion mechanism of lesion search. Unlike short gaps, covalent adducts partly block vvUNG translocation. Kinetic experiments show that once a lesion is found it is excised with a probability ~0.76. Varying the distance between two uracils, we use a random walk model to estimate the mean number of steps per association with DNA at ~4200, which is consistent with vvUNG playing a role as a processivity factor. Finally, we show that inhibitors carrying a tetrahydro-2,4,6-trioxopyrimidinylidene moiety can suppress the processivity of vvUNG.

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Combined Solution and Crystal Methods Reveal the Electrostatic Tethers That Provide a Flexible Platform for Replication Activities in the Bacteriophage T7 Replisome

Cited by 10 publications

References 52 publications

Structural Characterization of Sphingomonas sp. KT-1 PahZ1-Catalyzed Biodegradation of Thermally Synthesized Poly(aspartic acid)

Structural Characterization of Sphingomonas sp. KT-1 PahZ1-Catalyzed Biodegradation of Thermally Synthesized Poly(aspartic acid)

Conformational dynamics during high-fidelity DNA replication and translocation defined using a DNA polymerase with a fluorescent artificial amino acid

Correlated Target Search by Vaccinia Virus Uracil–DNA Glycosylase, a DNA Repair Enzyme and a Processivity Factor of Viral Replication Machinery

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