Quantification of Histone H1 Subtypes Using Targeted Proteomics

Lurdes Zamora, Alicia Roque*, Marta Andrés, Jordi López-Gómez, Inma Ponte, Marta Vilaseca, Laura Villarreal, Blanca Xicoy

*Corresponding author for this work

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Abstract

Histone H1 is involved in the regulation of chromatin structure. Human somatic cells express up to seven subtypes. The variability in the proportions of somatic H1s (H1 complement) is one piece of evidence supporting their functional specificity. Alterations in the protein levels of different H1 subtypes have been observed in cancer, suggesting their potential as biomarkers and that they might play a role in disease development. We have developed a mass spectrometry-based (MS) parallel reaction monitoring (PRM) assay suitable for the quantification of H1 subtypes. Our PRM method is based on the quantification of unique peptides for each subtype, providing high specificity. Evaluation of the PRM performance on three human cell lines, HeLa, K562, and T47D, showed high reproducibility and sensitivity. Quantification values agreed with the electrophoretic and Western blot data, indicating the accuracy of the method. We used PRM to quantify the H1 complement in peripheral blood samples of healthy individuals and chronic myeloid leukemia (CML) patients. In CML, the first line of therapy is a tyrosine kinase inhibitor, imatinib. Our preliminary data revealed differences in the H1 complement in CML patients between imatinib responders and non-responders. These results support further research to determine if the H1 content or subtype composition could help predict imatinib response.

Original languageEnglish
Article number1221
Number of pages18
JournalBiomolecules
Volume14
Issue number10
DOIs
Publication statusPublished - 27 Sept 2024

Keywords

  • histone H1
  • functional differentiation
  • parallel reaction monitoring
  • imatinib resistance
  • chronic myeloid leukemia
  • cancer biomarker

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