Innovative Analyses Support a Role for DNA Damage and an Aberrant Cell Cycle in Myelodysplastic Syndrome Pathogenesis

Author:

Head David R.1,Jacobberger James W.2,Mosse Claudio13,Jagasia Madan1,Dupont William1,Goodman Stacey13,Flye Leanne4ORCID,Shinar Andrew1,McClintock-Treep Sara1,Stelzer Greg4ORCID,Briggs Robert1,Shults Keith4

Affiliation:

1. Vanderbilt University Medical Center, Nashville, TN 37232-5310, USA

2. Case Comprehensive Cancer Center, Cleveland, OH 44106-5065, USA

3. Tennessee Valley Healthcare System, U.S. Department of Veterans Affairs, Nashville, TN 37212, USA

4. Esoterix Center for Innovation, Brentwood, TN, USA

Abstract

We used flow cytometry to analyze the cell cycle, DNA damage, and apoptosis in hematopoietic subsets in MDS marrow. Subsets were assigned using CD45, side scatter, CD34, and CD71. Cell cycle fractions were analyzed using DRAQ 5 (DNA content) and MPM-2 (mitoses). DNA damage was assessed using p-H2A.X, and apoptosis using Annexin V. Compared to controls, MDS patients demonstrated no increased mitoses in erythroid, myeloid, or CD34+ cells. Myeloid progenitors demonstrated increased G2 cells, which with no increased mitoses suggested delayed passage through G2. Myeloid progenitors demonstrated increased p-H2A.X, consistent with DNA damage causing this delay. Annexin V reactivity was equivalent in MDS and controls. Results for each parameter varied among hematopoietic compartments, demonstrating the need to analyze compartments separately. Our results suggest that peripheral cytopenias in MDS are due to delayed cell cycle passage of marrow progenitors and that this delayed passage and leukemic progression derive from excessive DNA damage.

Publisher

Hindawi Limited

Subject

Cell Biology,Hematology,Immunology

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