Atomic Resolution Structure of a Protein Prepared by Non-Enzymatic His-Tag Removal. Crystallographic and NMR Study of GmSPI-2 Inhibitor

Purification of suitable quantity of homogenous protein is very often the bottleneck in protein structural studies. Overexpression of a desired gene and attachment of enzymatically cleavable affinity tags to the protein of interest made a breakthrough in this field. Here we describe the structure of...

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Autores principales: Kopera, Edyta, Bal, Wojciech, Lenarčič Živkovič, Martina, Dvornyk, Angela, Kludkiewicz, Barbara, Grzelak, Krystyna, Zhukov, Igor, Zagórski-Ostoja, Włodzimierz, Jaskolski, Mariusz, Krzywda, Szymon
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2014
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Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4169406/
https://www.ncbi.nlm.nih.gov/pubmed/25233114
http://dx.doi.org/10.1371/journal.pone.0106936
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author Kopera, Edyta
Bal, Wojciech
Lenarčič Živkovič, Martina
Dvornyk, Angela
Kludkiewicz, Barbara
Grzelak, Krystyna
Zhukov, Igor
Zagórski-Ostoja, Włodzimierz
Jaskolski, Mariusz
Krzywda, Szymon
author_facet Kopera, Edyta
Bal, Wojciech
Lenarčič Živkovič, Martina
Dvornyk, Angela
Kludkiewicz, Barbara
Grzelak, Krystyna
Zhukov, Igor
Zagórski-Ostoja, Włodzimierz
Jaskolski, Mariusz
Krzywda, Szymon
author_sort Kopera, Edyta
collection PubMed
description Purification of suitable quantity of homogenous protein is very often the bottleneck in protein structural studies. Overexpression of a desired gene and attachment of enzymatically cleavable affinity tags to the protein of interest made a breakthrough in this field. Here we describe the structure of Galleria mellonella silk proteinase inhibitor 2 (GmSPI-2) determined both by X-ray diffraction and NMR spectroscopy methods. GmSPI-2 was purified using a new method consisting in non-enzymatic His-tag removal based on a highly specific peptide bond cleavage reaction assisted by Ni(II) ions. The X-ray crystal structure of GmSPI-2 was refined against diffraction data extending to 0.98 Å resolution measured at 100 K using synchrotron radiation. Anisotropic refinement with the removal of stereochemical restraints for the well-ordered parts of the structure converged with R factor of 10.57% and R (free) of 12.91%. The 3D structure of GmSPI-2 protein in solution was solved on the basis of 503 distance constraints, 10 hydrogen bonds and 26 torsion angle restraints. It exhibits good geometry and side-chain packing parameters. The models of the protein structure obtained by X-ray diffraction and NMR spectroscopy are very similar to each other and reveal the same β(2)αβ fold characteristic for Kazal-family serine proteinase inhibitors.
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spelling pubmed-41694062014-09-22 Atomic Resolution Structure of a Protein Prepared by Non-Enzymatic His-Tag Removal. Crystallographic and NMR Study of GmSPI-2 Inhibitor Kopera, Edyta Bal, Wojciech Lenarčič Živkovič, Martina Dvornyk, Angela Kludkiewicz, Barbara Grzelak, Krystyna Zhukov, Igor Zagórski-Ostoja, Włodzimierz Jaskolski, Mariusz Krzywda, Szymon PLoS One Research Article Purification of suitable quantity of homogenous protein is very often the bottleneck in protein structural studies. Overexpression of a desired gene and attachment of enzymatically cleavable affinity tags to the protein of interest made a breakthrough in this field. Here we describe the structure of Galleria mellonella silk proteinase inhibitor 2 (GmSPI-2) determined both by X-ray diffraction and NMR spectroscopy methods. GmSPI-2 was purified using a new method consisting in non-enzymatic His-tag removal based on a highly specific peptide bond cleavage reaction assisted by Ni(II) ions. The X-ray crystal structure of GmSPI-2 was refined against diffraction data extending to 0.98 Å resolution measured at 100 K using synchrotron radiation. Anisotropic refinement with the removal of stereochemical restraints for the well-ordered parts of the structure converged with R factor of 10.57% and R (free) of 12.91%. The 3D structure of GmSPI-2 protein in solution was solved on the basis of 503 distance constraints, 10 hydrogen bonds and 26 torsion angle restraints. It exhibits good geometry and side-chain packing parameters. The models of the protein structure obtained by X-ray diffraction and NMR spectroscopy are very similar to each other and reveal the same β(2)αβ fold characteristic for Kazal-family serine proteinase inhibitors. Public Library of Science 2014-09-18 /pmc/articles/PMC4169406/ /pubmed/25233114 http://dx.doi.org/10.1371/journal.pone.0106936 Text en © 2014 Kopera et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Kopera, Edyta
Bal, Wojciech
Lenarčič Živkovič, Martina
Dvornyk, Angela
Kludkiewicz, Barbara
Grzelak, Krystyna
Zhukov, Igor
Zagórski-Ostoja, Włodzimierz
Jaskolski, Mariusz
Krzywda, Szymon
Atomic Resolution Structure of a Protein Prepared by Non-Enzymatic His-Tag Removal. Crystallographic and NMR Study of GmSPI-2 Inhibitor
title Atomic Resolution Structure of a Protein Prepared by Non-Enzymatic His-Tag Removal. Crystallographic and NMR Study of GmSPI-2 Inhibitor
title_full Atomic Resolution Structure of a Protein Prepared by Non-Enzymatic His-Tag Removal. Crystallographic and NMR Study of GmSPI-2 Inhibitor
title_fullStr Atomic Resolution Structure of a Protein Prepared by Non-Enzymatic His-Tag Removal. Crystallographic and NMR Study of GmSPI-2 Inhibitor
title_full_unstemmed Atomic Resolution Structure of a Protein Prepared by Non-Enzymatic His-Tag Removal. Crystallographic and NMR Study of GmSPI-2 Inhibitor
title_short Atomic Resolution Structure of a Protein Prepared by Non-Enzymatic His-Tag Removal. Crystallographic and NMR Study of GmSPI-2 Inhibitor
title_sort atomic resolution structure of a protein prepared by non-enzymatic his-tag removal. crystallographic and nmr study of gmspi-2 inhibitor
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4169406/
https://www.ncbi.nlm.nih.gov/pubmed/25233114
http://dx.doi.org/10.1371/journal.pone.0106936
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