AI Article Synopsis

  • A new strategy for identifying covalent modification sites, particularly acetylation and methylation of histone H3 from chicken erythrocytes, has been developed using low enzyme ratios and short digestion times alongside advanced mass spectrometry techniques.
  • High-accuracy MALDI-TOF mass measurements have successfully differentiated between methylated and acetylated peptides, pinpointing specific lysines on histone H3 that are modified.
  • Notably, the method has revealed a new methylation site at lysine 79, and offers a faster and more efficient alternative to traditional protein analysis techniques like sequencing and Western blotting, promising advancements in chromosome research.

Article Abstract

A new strategy has been employed for the identification of the covalent modification sites (mainly acetylation and methylation) of histone H3 from chicken erythrocytes using low enzyme/substrate ratios and short digestion times (trypsin used as the protease) with analysis by HPLC separation, matrix-assisted laser desorption ionization-time-of-flight (MALDI-TOF), matrix-assisted laser desorption ionization-postsource decay, and tandem mass spectrometric techniques. High-accuracy MALDI-TOF mass measurements with representative immonium ions (126 for acetylated lysine, 98 for monomethylated lysine, and 84 for di-, tri-, and unmethylated lysine) have been effectively used for differentiating methylated peptides from acetylated peptides. Our results demonstrate that lysines 4, 9, 14, 27, and 36 of the N-terminal of H3 are methylated, while lysines 14, 18, and 23 are acetylated. Surprisingly, a non-N-terminal residue, lysine 79, in the loop region hooking up to the bound DNA, was newly found to be methylated (un-, mono-, and dimethylated isoforms coexist). The reported mass spectrometric method has the advantages of speed, directness, sensitivity, and ease over protein sequencing and Western-blotting methods and holds the promise of an improved method for determining the status of histone modifications in the field of chromosome research.

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http://dx.doi.org/10.1006/abio.2002.5719DOI Listing

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