Selective Chemical Labeling Strategy for Oligonucleotides Determination: A First Application to Full-Range Profiling of Transfer RNA Modifications.

Anal Chem

State Key Laboratory of Quality Research in Chinese Medicines, Guangdong-Hong Kong-Macao Joint Laboratory of Respiratory Infectious Disease, Macau Institute for Applied Research in Medicine and Health, Macau University of Science and Technology, Macau 999078, People's Republic of China.

Published: January 2023

AI Article Synopsis

  • The current difficulties in mass spectrometry for analyzing nucleic acids stem from their high polarity and low signal intensity, hindering drug quality control and DNA/RNA studies.
  • A new labeling method using -(tert-butyldimethylsilyl)--methyl-trifluoroacetamide (MTBSTFA) enhances oligonucleotide detection by providing strong retention and clear data without harmful byproducts.
  • This method improves RNA analysis by effectively profiling tRNA and identifying modified bases, revealing significant findings related to nonalcoholic fatty liver disease in cell studies.

Article Abstract

To date, the extremely high polarity and poor signal intensity of macromolecular nucleic acids are greatly impeding the progress of mass spectrometry technology in the quality control of nucleic acid drugs and the characterization of DNA oxidation and RNA modifications. We recently described a general -(tert-butyldimethylsilyl)--methyl-trifluoroacetamide (MTBSTFA) labeling method for oligonucleotide determination and applied it to the full-range profiling of tRNA in vitro and in vivo studies for the first time. The primary advantages of this method include strong retention, no observable byproducts, predictable and easily interpreted MS data, and the circumvention of instrument harmful reagents that were necessary in previous methods. Selective labeling of -(tert-butyldimethylsilyl)--methyl-trifluoroacetamide to the terminal phosphate groups of oligonucleotides endows it broadly applicable for DNA/RNA profiling. Moreover, the improvement of sequence coverage was achieved in yeast tRNA analysis owing to this method's good detection capability of 1-12 nucleotides in length. We also extended this strategy to determine the abundance of modified bases and discover new modifications via digesting RNA into single-nucleotide products, promoting the comprehensive mapping of RNA. The easy availability of derivatization reagent and the simple, rapid one-step reaction render it easy to operate for researchers. When applied in characterizing tRNAs in HepG2 cells and rats with nonalcoholic fatty liver disease, a fragment of U[mG][mG], specific for tRNA in cells, was significantly upregulated, indicating a possible clue to nonalcoholic fatty liver disease pathogenesis.

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http://dx.doi.org/10.1021/acs.analchem.2c02302DOI Listing

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