Chromatin damage generated by DNA intercalators leads to degradation of RNA Polymerase II

Author:

Espinoza Jaime A1ORCID,Kanellis Dimitris C1ORCID,Saproo Sheetanshu1ORCID,Leal Karla1ORCID,Martinez Johana Fernandez1,Bartek Jiri12ORCID,Lindström Mikael S1ORCID

Affiliation:

1. Science for Life Laboratory, Division of Genome Biology, Department of Medical Biochemistry and Biophysics, Karolinska Institutet , S-171 21 Stockholm , Sweden

2. Danish Cancer Society Research Center , DK-2100 Copenhagen , Denmark

Abstract

Abstract In cancer therapy, DNA intercalators are mainly known for their capacity to kill cells by inducing DNA damage. Recently, several DNA intercalators have attracted much interest given their ability to inhibit RNA Polymerase I transcription (BMH-21), evict histones (Aclarubicin) or induce chromatin trapping of FACT (Curaxin CBL0137). Interestingly, these DNA intercalators lack the capacity to induce DNA damage while still retaining cytotoxic effects and stabilize p53. Herein, we report that these DNA intercalators impact chromatin biology by interfering with the chromatin stability of RNA polymerases I, II and III. These three compounds have the capacity to induce degradation of RNA polymerase II and they simultaneously enable the trapping of Topoisomerases TOP2A and TOP2B on the chromatin. In addition, BMH-21 also acts as a catalytic inhibitor of Topoisomerase II, resembling Aclarubicin. Moreover, BMH-21 induces chromatin trapping of the histone chaperone FACT and propels accumulation of Z-DNA and histone eviction, similarly to Aclarubicin and CBL0137. These DNA intercalators have a cumulative impact on general transcription machinery by inducing accumulation of topological defects and impacting nuclear chromatin. Therefore, their cytotoxic capabilities may be the result of compounding deleterious effects on chromatin homeostasis.

Funder

Cancerfonden

Vetenskapsrådet

Radiumhemmets forskningsfonder

Swedish Research Council

Publisher

Oxford University Press (OUP)

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