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Naji, M. |
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Motta, Antonella |
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Aletan, Dirar |
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Mohamed, Tarek |
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Ertürk, Emre |
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Taccardi, Nicola |
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Kononenko, Denys |
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Petrov, R. H. | Madrid |
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Alshaaer, Mazen | Brussels |
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Bih, L. |
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Casati, R. |
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Muller, Hermance |
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Kočí, Jan | Prague |
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Šuljagić, Marija |
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Kalteremidou, Kalliopi-Artemi | Brussels |
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Azam, Siraj |
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Ospanova, Alyiya |
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Blanpain, Bart |
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Ali, M. A. |
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Popa, V. |
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Rančić, M. |
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Ollier, Nadège |
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Azevedo, Nuno Monteiro |
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Landes, Michael |
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Rignanese, Gian-Marco |
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Li, Nan
in Cooperation with on an Cooperation-Score of 37%
Topics
Publications (11/11 displayed)
- 2024The modified boundary layer mechanism for the release between polyimide film and poly(ether ketone ketone) thermoplasticscitations
- 2024Alloying effects on deformation induced microstructure evolution in coppercitations
- 2022Interface effect of Fe and Fe<sub>2</sub>O<sub>3</sub> on the distributions of ion induced defectscitations
- 2021High temperature nanoindentation of Cu-TiN nanolaminatescitations
- 2019High-Throughput Nanomechanical Screening of Phase-Specific and Temperature-Dependent Hardness in AlxFeCrNiMn High-Entropy Alloyscitations
- 2019One-step polymeric phononic crystal manufacture.
- 2018Oxide Morphology of C26M at 300 - 600 °C
- 2017Oxide Morphology of a FeCrAl Alloy, Kanthal APMT, following Extended Aging at 300-600C
- 2017Mechanical behavior of rare‐earth orthophosphates near the monazite/xenotime boundary characterized by nanoindentationcitations
- 2013Proofreading exonuclease on a tethercitations
- 2013Catalyst composition and impurity-dependent kinetics of nanowire heteroepitaxy.
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article
Proofreading exonuclease on a tether
Abstract
<p>A complex of the three (αεθ) core subunits and the β<sub>2</sub> sliding clamp is responsible for DNA synthesis by Pol III, the Escherichia coli chromosomal DNA replicase. The 1.7 Å crystal structure of a complex between the PHP domain of α (polymerase) and the C-terminal segment of ε (proofreading exonuclease) subunits shows that ε is attached to α at a site far from the polymerase active site. Both α and ε contain clamp-binding motifs (CBMs) that interact simultaneously with β<sub>2</sub> in the polymerization mode of DNA replication by Pol III. Strengthening of both CBMs enables isolation of stable αεθ:β<sub>2</sub> complexes. Nuclear magnetic resonance experiments with reconstituted αεθ:β<sub>2</sub> demonstrate retention of high mobility of a segment of 22 residues in the linker that connects the exonuclease domain of ε with its α-binding segment. In spite of this, small-angle X-ray scattering data show that the isolated complex with strengthened CBMs has a compact, but still flexible, structure. Photo-crosslinking with p-benzoyl-L-phenylalanine incorporated at different sites in the α-PHP domain confirm the conformational variability of the tether. Structural models of the αεθ:β<sub>2</sub> replicase complex with primer-template DNA combine all available structural data.</p>