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Conformational transitions of proteins engaged in dna double-strand break repair, analysed by trytophan flourescence emission and fret

We analysed protein–DNA and protein–protein interactions relevant to the repair of DNA DSBs (double-strand breaks) by NHEJ (non-homologous end-joining). Conformational transitions in mammalian DNA ligases III (LigIII) and IV (LigIV), as well as in PARP-1 [poly(ADP-ribose) polymerase-1], were analyse...

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Main Authors: Stankova, Katia, Ivanova, Katia, Mladenov, Emil, Rosidi, Bustanur, Sharma, Aparna, Boteva, Rayna, Iliakis, George
Format: Article
Published: Biochemical Society 2012
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TP Chemical technology
Online Access:http://eprints.utm.my/id/eprint/46731/
http://dx.doi.org/10.1042/BJ20112151
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spelling my.utm.467312019-03-05T02:03:18Z http://eprints.utm.my/id/eprint/46731/ Conformational transitions of proteins engaged in dna double-strand break repair, analysed by trytophan flourescence emission and fret Stankova, Katia Ivanova, Katia Mladenov, Emil Rosidi, Bustanur Sharma, Aparna Boteva, Rayna Iliakis, George TP Chemical technology We analysed protein–DNA and protein–protein interactions relevant to the repair of DNA DSBs (double-strand breaks) by NHEJ (non-homologous end-joining). Conformational transitions in mammalian DNA ligases III (LigIII) and IV (LigIV), as well as in PARP-1 [poly(ADP-ribose) polymerase-1], were analysed upon binding to double-stranded DNA by changes in tryptophan emission and FRET (Förster resonance energy transfer) from tryptophan to DNA-conjugated Alexa Fluor® 532. For LigIII, two non-equivalent high- and low-affinity DNA-binding sites are detected interacting sequentially with DNA. PARP-1 displays a single high-affinity DNA-binding site and can displace bound DNA fragments from the low-affinity site of LigIII, consistent with its mediator role in LigIII–DNA interactions. For the LX [LigIV–XRCC4 (X-ray cross-complementation group 4)] complex, a single DNA-binding site is detected. Binding of Ku to DNA was accompanied by conformational changes in the protein and intermolecular FRET from dansyl chromophores of the labelled Ku to the Alexa Fluor® chromophores of Alexa Fluor® 532-conjugated DNA. The average distance of 5.7 nm calculated from FRET data is consistent with a location of Ku at the very end of the DNA molecule. Binding of LX to Ku–DNA complexes is associated with conformational changes in Ku, translocating the protein further towards the DNA ends. The protein–protein and protein–DNA interactions detected and analysed generate a framework for the characterization of molecular interactions fundamental to the function of NHEJ pathways in higher eukaryotes. Biochemical Society 2012 Article PeerReviewed Stankova, Katia and Ivanova, Katia and Mladenov, Emil and Rosidi, Bustanur and Sharma, Aparna and Boteva, Rayna and Iliakis, George (2012) Conformational transitions of proteins engaged in dna double-strand break repair, analysed by trytophan flourescence emission and fret. Biochemical Journal, 44 (3). pp. 701-709. ISSN 0264-6021 http://dx.doi.org/10.1042/BJ20112151 DOI:10.1042/BJ20112151
institution Universiti Teknologi Malaysia
building UTM Library
collection Institutional Repository
continent Asia
country Malaysia
content_provider Universiti Teknologi Malaysia
content_source UTM Institutional Repository
url_provider http://eprints.utm.my/
topic TP Chemical technology
spellingShingle TP Chemical technology
Stankova, Katia
Ivanova, Katia
Mladenov, Emil
Rosidi, Bustanur
Sharma, Aparna
Boteva, Rayna
Iliakis, George
Conformational transitions of proteins engaged in dna double-strand break repair, analysed by trytophan flourescence emission and fret
description We analysed protein–DNA and protein–protein interactions relevant to the repair of DNA DSBs (double-strand breaks) by NHEJ (non-homologous end-joining). Conformational transitions in mammalian DNA ligases III (LigIII) and IV (LigIV), as well as in PARP-1 [poly(ADP-ribose) polymerase-1], were analysed upon binding to double-stranded DNA by changes in tryptophan emission and FRET (Förster resonance energy transfer) from tryptophan to DNA-conjugated Alexa Fluor® 532. For LigIII, two non-equivalent high- and low-affinity DNA-binding sites are detected interacting sequentially with DNA. PARP-1 displays a single high-affinity DNA-binding site and can displace bound DNA fragments from the low-affinity site of LigIII, consistent with its mediator role in LigIII–DNA interactions. For the LX [LigIV–XRCC4 (X-ray cross-complementation group 4)] complex, a single DNA-binding site is detected. Binding of Ku to DNA was accompanied by conformational changes in the protein and intermolecular FRET from dansyl chromophores of the labelled Ku to the Alexa Fluor® chromophores of Alexa Fluor® 532-conjugated DNA. The average distance of 5.7 nm calculated from FRET data is consistent with a location of Ku at the very end of the DNA molecule. Binding of LX to Ku–DNA complexes is associated with conformational changes in Ku, translocating the protein further towards the DNA ends. The protein–protein and protein–DNA interactions detected and analysed generate a framework for the characterization of molecular interactions fundamental to the function of NHEJ pathways in higher eukaryotes.
format Article
author Stankova, Katia
Ivanova, Katia
Mladenov, Emil
Rosidi, Bustanur
Sharma, Aparna
Boteva, Rayna
Iliakis, George
author_facet Stankova, Katia
Ivanova, Katia
Mladenov, Emil
Rosidi, Bustanur
Sharma, Aparna
Boteva, Rayna
Iliakis, George
author_sort Stankova, Katia
title Conformational transitions of proteins engaged in dna double-strand break repair, analysed by trytophan flourescence emission and fret
title_short Conformational transitions of proteins engaged in dna double-strand break repair, analysed by trytophan flourescence emission and fret
title_full Conformational transitions of proteins engaged in dna double-strand break repair, analysed by trytophan flourescence emission and fret
title_fullStr Conformational transitions of proteins engaged in dna double-strand break repair, analysed by trytophan flourescence emission and fret
title_full_unstemmed Conformational transitions of proteins engaged in dna double-strand break repair, analysed by trytophan flourescence emission and fret
title_sort conformational transitions of proteins engaged in dna double-strand break repair, analysed by trytophan flourescence emission and fret
publisher Biochemical Society
publishDate 2012
url http://eprints.utm.my/id/eprint/46731/
http://dx.doi.org/10.1042/BJ20112151
_version_ 1643652123586461696
score 13.160551

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