The role of cell-free DNA in fibrinolysis for intraventricular hemorrhage

Fangke Xie; Qiang Tan; Anyong Yu; Peiwen Guo; Ling Wang; Zongwei Zeng; Liang Liang; Jishu Xian; Hua Feng; Zhi Chen

doi:10.3171/2020.7.JNS201429

The role of cell-free DNA in fibrinolysis for intraventricular hemorrhage

J Neurosurg. 2021 Jan 8;135(4):1105-1112. doi: 10.3171/2020.7.JNS201429.

Authors

Fangke Xie¹, Qiang Tan², Anyong Yu¹, Peiwen Guo², Ling Wang², Zongwei Zeng², Liang Liang², Jishu Xian², Hua Feng², Zhi Chen²

Affiliations

¹ 1Department of Emergency, Affiliated Hospital of Zunyi Medical University, Zunyi; and.
² 2Department of Neurosurgery, Southwest Hospital, Third Military Medical University (Army Medical University), Chongqing, China.

PMID: 33418533
DOI: 10.3171/2020.7.JNS201429

Abstract

Objective: Tissue plasminogen activator (tPA) fibrinolysis did not improve functional outcomes of patients with intraventricular hemorrhage (IVH), largely because of the unsatisfactory clot clearance. The presence of neutrophil extracellular traps (NETs) within the clot has been confirmed to impair tPA fibrinolysis, but the mechanism has been unclear. The authors hypothesized that cell-free DNA (cfDNA), the main framework of NETs, might be the important reason for the fibrinolysis resistance, and they validated the hypothesis, hoping to provide a new target to promote intraventricular fibrinolysis.

Methods: First, cfDNA was detected in IVH clots by immunofluorescence staining in a rat model of IVH. Second, after blood (with or without exogenous cfDNA) intraventricular injection, IVH rats were given intraventricular infusion of 2 μl of saline, tPA, or tPA + DNase1 randomly. Then, the ventricular volume, animal behavior, and reactive astrocyte proliferation were assessed. Third, the IVH clots were collected for fibrinolysis assay in vitro. Finally, the effects of exogenous cfDNA in IVH were evaluated.

Results: The presence of cfDNA in clots was observed as early as 1 hour after IVH. Compared with the whole-blood model, blood + cfDNA caused more severe ventricular dilation (day 7: blood 32.47 ± 2.096 mm3 vs blood + DNA 40.09 ± 2.787 mm3, p < 0.05), increased fibrinolysis resistance to tPA (day 7: tPA + DNA 26.04 ± 1.318 mm3 vs tPA 22.15 ± 1.706 mm3, p < 0.05), and further deteriorated the functional defects in rats (blood vs blood + DNA, p < 0.05). Degradation of cfDNA by DNase1 further enhanced the fibrinolysis effects on relieving the ventricular dilation (day 7: tPA + DNase1 11.67 ± 2.023 mm3 vs tPA, p < 0.05), improving the functional outcome (tPA vs tPA + DNase1, p < 0.05) and reducing periventricular astrocyte proliferation.

Conclusions: cfDNA impaired tPA fibrinolysis for IVH, and degradation of cfDNA may be a new target to improve this condition.

Keywords: cell-free DNA; fibrinolysis; intraventricular hemorrhage; neutrophil extracellular traps; tissue plasminogen activator; vascular disorders.