1999
DOI: 10.1042/bj3380591
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NMR structure and dynamics of monomeric neutrophil-activating peptide 2

Abstract: Neutrophil-activating peptide 2 (NAP-2), which demonstrates a range of proinflammatory activities, is a 72-residue protein belonging to the alpha-chemokine family. Although NAP-2, like other alpha-chemokines, is known to self-associate into dimers and tetramers, it has been shown that the monomeric form is physiologically active. Here we investigate the solution structure of monomeric NAP-2 by multi-dimensional 1H-NMR and 15N-NMR spectroscopy and computational modelling. The NAP-2 monomer consists of an amphip… Show more

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Cited by 15 publications
(15 citation statements)
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“…Further, NMR CSP-based methods have been shown to be extremely useful for describing residue-specific GAG interactions, as protein-GAG complexes are notoriously difficult to crystallize. The CXCL7 monomer chemical shift assignments were previously reported in the presence of 2-chloroethanol [16,57]. Our chemical shifts were similar, but not identical, and interestingly, our heteronuclear relaxation data of the monomer showed a structured 30s-loop, whereas previous studies carried out in the presence of chloroethanol showed substantial dynamics similar to those observed for terminal residues.…”
Section: Discussionsupporting
confidence: 83%
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“…Further, NMR CSP-based methods have been shown to be extremely useful for describing residue-specific GAG interactions, as protein-GAG complexes are notoriously difficult to crystallize. The CXCL7 monomer chemical shift assignments were previously reported in the presence of 2-chloroethanol [16,57]. Our chemical shifts were similar, but not identical, and interestingly, our heteronuclear relaxation data of the monomer showed a structured 30s-loop, whereas previous studies carried out in the presence of chloroethanol showed substantial dynamics similar to those observed for terminal residues.…”
Section: Discussionsupporting
confidence: 83%
“…Comparison of our data to the previously reported relaxation data of CXCL7 in the presence of chloroethanol shows striking differences for the 30s-loop residues. Heteronuclear NOE measurements in the presence of 2-chloroethanol indicate a highly dynamic 30s-loop, especially residues Q33, V34 and E35, showing very low NOE values observed for the very terminal residues, whereas our values are similar to those of structured residues [16,31,32]. These observations suggest that chloroethanol influences dynamic properties, and so, these data may not fully reflect the dynamics of the native protein.…”
Section: Resultsmentioning
confidence: 62%
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