DNA Adductomics by mass tag prelabeling

Poguang Wang; Elisabeth Roider; Michael E Coulter; Christopher A Walsh; Caitlin S Kramer; Penny J Beuning; Roger W Giese

doi:10.1002/rcm.9095

DNA Adductomics by mass tag prelabeling

Rapid Commun Mass Spectrom. 2021 Jul 15;35(13):e9095. doi: 10.1002/rcm.9095.

Authors

Poguang Wang¹, Elisabeth Roider², Michael E Coulter³, Christopher A Walsh⁴, Caitlin S Kramer⁵, Penny J Beuning⁵, Roger W Giese¹

Affiliations

¹ Department of Pharmaceutical Sciences, Northeastern University, Boston, MA, USA.
² Cutaneous Biology Research Center, Massachusetts General Hospital, Harvard Medical School, Boston, MA, USA.
³ Center for Integrative Neuroscience, UCSF, San Francisco, CA, USA.
⁴ Division of Genetics and Genomics, Boston Children's Hospital, Center for Life Sciences, Harvard Medical School, Boston, MA, USA.
⁵ Department of Chemistry and Chemical Biology, Northeastern University, Boston, MA, USA.

Abstract

Rationale: As a new approach to DNA adductomics, we directly reacted intact, double-stranded (ds)-DNA under warm conditions with an alkylating mass tag followed by analysis by liquid chromatography/mass spectrometry. This method is based on the tendency of adducted nucleobases to locally disrupt the DNA structure (forming a "DNA bubble") potentially increasing exposure of their nucleophilic (including active hydrogen) sites for preferential alkylation. Also encouraging this strategy is that the scope of nucleotide excision repair is very broad, and this system primarily recognizes DNA bubbles.

Methods: A cationic xylyl (CAX) mass tag with limited nonpolarity was selected to increase the retention of polar adducts in reversed-phase high-performance liquid chromatography (HPLC) for more detectability while maintaining resolution. We thereby detected a diversity of DNA adducts (mostly polar) by the following sequence of steps: (1) react DNA at 45°C for 2 h under aqueous conditions with CAX-B (has a benzyl bromide functional group to label active hydrogen sites) in the presence of triethylamine; (2) remove residual reagents by precipitating and washing the DNA (a convenient step); (3) digest the DNA enzymatically to nucleotides and remove unlabeled nucleotides by nonpolar solid-phase extraction (also a convenient step); and (4) detect CAX-labeled, adducted nucleotides by LC/MS² or a matrix-assisted laser desorption/ionization (MALDI)-MS technique.

Results: Examples of the 42 DNA or RNA adducts detected, or tentatively so based on accurate mass and fragmentation data, are as follows: 8-oxo-dGMP, ethyl-dGMP, hydroxyethyl-dGMP (four isomers, all HPLC-resolved), uracil-glycol, apurinic/apyrimidinic sites, benzo[a]pyrene-dGMP, and, for the first time, benzoquinone-hydroxymethyl-dCMP. Importantly, these adducts are detected in a single procedure under a single set of conditions. Sensitivity, however, is only defined in a preliminary way, namely the latter adduct seems to be detected at a level of about 4 adducts in 10⁹ nucleotides (S/N ~30).

Conclusions: CAX-Prelabeling is an emerging new technique for DNA adductomics, providing polar DNA adductomics in a practical way for the first time. Further study of the method is encouraged to better characterize and extend its performance, especially in scope and sensitivity.

MeSH terms

Animals
Benzo(a)pyrene / analysis
Benzyl Compounds
Cations
Cattle
Chromatography, High Pressure Liquid
DNA Adducts / analysis*
DNA Adducts / chemistry
DNA Adducts / metabolism
Ethylamines
Guanine / analogs & derivatives
Guanine / analysis
Humans
Nucleotides / metabolism
Phosphorus Radioisotopes
Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization
Uracil / analogs & derivatives
Uracil / analysis

Substances

Benzyl Compounds
Cations
DNA Adducts
Ethylamines
Nucleotides
Phosphorus Radioisotopes
benzo(a)pyrene-DNA adduct
uracil glycol
Benzo(a)pyrene
8-hydroxyguanine
Uracil
Guanine
Phosphorus-32
triethylamine
benzyl bromide

Abstract

MeSH terms

Substances

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