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Solution structure of the N-terminal zinc binding domain of HIV-1 integrase

Mengli Cai
Ronglan Zheng
Angela M. Gronenborn
Research01 Jul 1997
Nature Structural Biology

Volume: 4, P: 567-577
Refined solution structure of the oligomerization domain of the tumour suppressor p53

G. Marius Clore
James Ernst
Angela M. Gronenborn
Research01 Apr 1995
Nature Structural Biology

Volume: 2, P: 321-333
The solution structure of a specific GAGA factor–DNA complex reveals a modular binding mode

James G. Omichinski
Paolo V. Pedone
G. Marius Clore
Research01 Feb 1997
Nature Structural Biology

Volume: 4, P: 122-132
The solution structure of an HMG-I(Y)–DNA complex defines a new architectural minor groove binding motif

Jeffrey R. Huth
Carole A. Bewley
G. Marius Clore
Research01 Aug 1997
Nature Structural Biology

Volume: 4, P: 657-665
Comparison of four independently determined structures of human recombinant interleukin–4

Lorna J. Smith
Christina Redfield
Alexander Wlodawer
Research01 May 1994
Nature Structural Biology

Volume: 1, P: 301-310
Use of dipolar ¹H–¹⁵N and ¹H–¹³C couplings in the structure determination of magnetically oriented macromolecules in solution

Nico Tjandra
James G. Omichinski
Ad Bax
Research01 Sept 1997
Nature Structural Biology

Volume: 4, P: 732-738
Defining long range order in NMR structure determination from the dependence of heteronuclear relaxation times on rotational diffusion anisotropy

Nico Tjandra
Daniel S. Garrett
G. Marius Clore
Research01 Jun 1997
Nature Structural Biology

Volume: 4, P: 443-449
Three-dimensional NMR spectroscopy of a protein in solution

Hartmut Oschkinat
Christian Griesinger
G. Marius Clore
Research24 Mar 1988
Nature

Volume: 332, P: 374-376
The solution structure of HIV-1 Nef reveals an unexpected fold and permits delineation of the binding surface for the SH3 domain of Hck tyrosine protein kinase

Stephan Grzesiek
Ad Bax
Paul T Wingfield
Research01 Apr 1996
Nature Structural Biology

Volume: 3, P: 340-345
Solvent isotope effect and protein stability

George I. Makhatadze
G. Marius Clore
Angela M. Gronenborn
Research01 Oct 1995
Nature Structural Biology

Volume: 2, P: 852-855
Solution structure of the 40,000 M_r phosphoryl transfer complex between the N-terminal domain of enzyme I and HPr

Daniel S. Garrett
Yeong-Jae Seok
G. Marius Clore
Research01 Feb 1999
Nature Structural Biology

Volume: 6, P: 166-173
Solution structure of cyanovirin-N, a potent HIV-inactivating protein

Carole A. Bewley
Kirk R. Gustafson
Angela M. Gronenborn
Research01 Jul 1998
Nature Structural Biology

Volume: 5, P: 571-578
Atomic-resolution dynamics on the surface of amyloid-β protofibrils probed by solution NMR

Nicolas L. Fawzi
Jinfa Ying
G. Marius Clore
Research30 Oct 2011
Nature

Volume: 480, P: 268-272
Probing exchange kinetics and atomic resolution dynamics in high-molecular-weight complexes using dark-state exchange saturation transfer NMR spectroscopy

Nicolas L Fawzi
Jinfa Ying
G Marius Clore
Protocols19 Jul 2012
Nature Protocols

Volume: 7, P: 1523-1533
Solution structure of the cellular factor BAF responsible for protecting retroviral DNA from autointegration

Mengli Cai
Ying Huang
G. Marius Clore
Research01 Oct 1998
Nature Structural Biology

Volume: 5, P: 903-909
Structure and dynamics of KH domains from FBP bound to single-stranded DNA

Demetrios T. Braddock
John M. Louis
G. Marius Clore
Research28 Feb 2002
Nature

Volume: 415, P: 1051-1056
Detecting transient intermediates in macromolecular binding by paramagnetic NMR

Nuclear magnetic resonance spectroscopy was used to detect transient intermediates that occurred when the HOXD9 homeodomain was searching for its target sequence in a short DNA duplex, and determined that this transcription factor binds to non-cognate DNA sites to enhance the rate of specific association.

Junji Iwahara
G. Marius Clore
Research27 Apr 2006
Nature

Volume: 440, P: 1227-1230
Visualization of transient encounter complexes in protein–protein association

Nuclear magnetic resonance spectroscopy is used to visualize directly an ensemble of transient, non-specific 'encounter' complexes for the first binary complex in the bacterial phosphotransferase system (the N-terminal domain of enzyme I and the phosphocarrier protein HPr). An atomic probability distribution map suggests that long-range electrostatic interactions facilitate the formation of the final protein–protein complex by reducing the dimensionality of the search process.

Chun Tang
Junji Iwahara
G. Marius Clore
Research15 Oct 2006
Nature

Volume: 444, P: 383-386
Large interdomain rearrangement triggered by suppression of micro- to millisecond dynamics in bacterial Enzyme I

Enzyme I (EI)—a component of the bacterial phosphotransferase signal transduction system—undergoes large conformational rearrangements upon substrate binding. Here the authors show that the EI open-to-closed conformational switch occurs through suppression of micro- to millisecond dynamics of C-terminal domain.

Vincenzo Venditti
Vitali Tugarinov
G. Marius Clore
Research12 Jan 2015
Nature Communications

Volume: 6, P: 1-9
Autoprocessing of HIV-1 protease is tightly coupled to protein folding

John M. Louis
G. Marius Clore
Angela M. Gronenborn
Research01 Sept 1999
Nature Structural Biology

Volume: 6, P: 868-875
Open-to-closed transition in apo maltose-binding protein observed by paramagnetic NMR

It is well known that large-scale rearrangements of domains of a protein can play an important role in ligand binding and recognition, catalysis, and regulation. Though X-ray crystal structures can provide a static picture of the apo (usually open) and holo (usually closed) states of a protein, it is not usually clear whether the apo state exists as a single species where the closed state is energetically inaccessible and interdomain rearrangement is induced by ligand or substrate binding or whether the predominantly open form already co-exists in rapid equilibrium with a minor closed species. In this paper, the authors obtained paramagnetic relaxation enhancement data that indicate that there is a rapidly exchanging mixture of a predominantly open form of the maltose-binding protein and a minor (partially-closed) form of the protein. Ensemble simulated annealing refinement was used to determine an ensemble average structure of the minor apo species and demonstrate that it is distinct from the sugar-bound state.

Chun Tang
Charles D. Schwieters
G. Marius Clore
Research25 Oct 2007
Nature

Volume: 449, P: 1078-1082
Visualizing transient events in amino-terminal autoprocessing of HIV-1 protease

HIV-1 protease processes the Gag and Gag-Pol polyproteins into mature structural and functional proteins. The mature protease is only active as a dimer, with catalytic residues contributed by each subunit. The precursor of the active protease undergoes 'maturation' via the intramolecular cleavage of a dimeric species, but it is not clear how this cleavage reaction occurs. The early events in N-terminal auto-processing were visualized using NMR spectroscopy, and it was determined that the precursor forms transient, lowly populated dimeric encounter complexes that occupy a wide range of orientations relative to the mature dimer. The N-terminal region makes transient intra- and intersubunit contacts with the substrate binding site, enabling auto-cleavage to occur when the correct dimer orientation is sampled by the encounter complex ensemble.

Chun Tang
John M. Louis
G. Marius Clore
Research02 Oct 2008
Nature

Volume: 455, P: 693-696

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