Literature DB >> 34559515

High-Resolution Mapping of Amino Acid Residues in DNA-Protein Cross-Links Enabled by Ribonucleotide-Containing DNA.

Jin Tang1, Wenxin Zhao1, Nathan G Hendricks2, Linlin Zhao1,3.   

Abstract

DNA-protein cross-links have broad applications in mapping DNA-protein interactions and provide structural insights into macromolecular structures. However, high-resolution mapping of DNA-interacting amino acid residues with tandem mass spectrometry remains challenging due to difficulties in sample preparation and data analysis. Herein, we developed a method for identifying cross-linking amino residues in DNA-protein cross-links at single amino acid resolution. We leveraged the alkaline lability of ribonucleotides and designed ribonucleotide-containing DNA to produce structurally defined nucleic acid-peptide cross-links under our optimized ribonucleotide cleavage conditions. The structurally defined oligonucleotide-peptide heteroconjugates improved ionization, reduced the database search space, and facilitated the identification of cross-linking residues in peptides. We applied the workflow to identifying abasic (AP) site-interacting residues in human mitochondrial transcription factor A (TFAM)-DNA cross-links. With sub-nmol sample input, we obtained high-quality fragmentation spectra for nucleic acid-peptide cross-links and identified 14 cross-linked lysine residues with the home-built AP_CrosslinkFinder program. Semi-quantification based on integrated peak areas revealed that K186 of TFAM is the major cross-linking residue, consistent with K186 being the closest (to the AP modification) lysine residue in solved TFAM:DNA crystal structures. Additional cross-linking lysine residues (K69, K76, K136, K154) support the dynamic characteristics of TFAM:DNA complexes. Overall, our combined workflow using ribonucleotide as a chemically cleavable DNA modification together with optimized sample preparation and data analysis offers a simple yet powerful approach for mapping cross-linking sites in DNA-protein cross-links. The method is amendable to other chemical or photo-cross-linking systems and can be extended to complex biological samples.

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Year:  2021        PMID: 34559515      PMCID: PMC8772389          DOI: 10.1021/acs.analchem.1c03481

Source DB:  PubMed          Journal:  Anal Chem        ISSN: 0003-2700            Impact factor:   8.008


  44 in total

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Journal:  Nat Commun       Date:  2012       Impact factor: 14.919

5.  Direct DNA crosslinking with CAP-C uncovers transcription-dependent chromatin organization at high resolution.

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Authors:  David J López; José A Rodríguez; Sonia Bañuelos
Journal:  Int J Mol Sci       Date:  2021-06-11       Impact factor: 5.923

7.  The mitochondrial transcription and packaging factor Tfam imposes a U-turn on mitochondrial DNA.

Authors:  Huu B Ngo; Jens T Kaiser; David C Chan
Journal:  Nat Struct Mol Biol       Date:  2011-10-30       Impact factor: 15.369

8.  Capturing snapshots of APE1 processing DNA damage.

Authors:  Bret D Freudenthal; William A Beard; Matthew J Cuneo; Nadezhda S Dyrkheeva; Samuel H Wilson
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9.  Photo-cross-linking and high-resolution mass spectrometry for assignment of RNA-binding sites in RNA-binding proteins.

Authors:  Katharina Kramer; Timo Sachsenberg; Benedikt M Beckmann; Saadia Qamar; Kum-Loong Boon; Matthias W Hentze; Oliver Kohlbacher; Henning Urlaub
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10.  Atomic-resolution mapping of transcription factor-DNA interactions by femtosecond laser crosslinking and mass spectrometry.

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Journal:  Nat Commun       Date:  2020-06-15       Impact factor: 14.919

View more
  1 in total

1.  Facile preparation of model DNA interstrand cross-link repair intermediates using ribonucleotide-containing DNA.

Authors:  Jin Tang; Feng Tang; Linlin Zhao
Journal:  DNA Repair (Amst)       Date:  2022-01-31
  1 in total

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