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FOXD3 may be a new cellular target biomarker as a hypermethylation gene in human ovarian cancer.

AbstractBACKGROUND:
FOXD3 is aberrantly regulated in several tumors, but its underlying mechanisms in ovarian cancer (OC) remains largely unknown. The present study aimed to explore the role and associated mechanisms of FOXD3 in OC.
METHODS:
Microarray data from GEO was used to analyze differential CpG sites and differentially methylated regions (DMR) in tumor tissues and Illumina 450 genome-wide methylation data was employed. The FOXD3 expression level was determined through qRT-PCR and western blot analysis. Wound healing test, colony formation and flow cytometry assay were utilized to analyze cell migration, proliferation abilities, cell cycle and cell apoptosis, respectively. Finally, the effect of FOXD3 on tumor growth was investigated through in vivo xenograft experiments.
RESULTS:
GEO data analysis showed that FOXD3 was hypermethylated in OC tissues. Also, qRT-PCR revealed that FOXD3 was low expressed and methylation-specific PCR (MSP) confirmed that the methylation level of FOXD3 was hypermethylated. Combined treatment of 5-aza-2'-deoxycytidine (5-Aza-dC) could synergistically restored FOXD3 expression. Finally, in vitro and in vivo experiments showed that demethylated FOXD3 decreased cell proliferation and migration abilities, and increased the cell apoptosis. In vivo experiment detected that demethylated FOXD3 restrained tumor growth.
CONCLUSIONS:
FOXD3 could act as a tumor suppressor to inhibit cell proliferation, migration and promote cell apoptosis in OC cells.
AuthorsGui-Fang Luo, Chang-Ye Chen, Juan Wang, Hai-Yan Yue, Yong Tian, Ping Yang, Yu-Kun Li, Yan Li
JournalCancer cell international (Cancer Cell Int) Vol. 19 Pg. 44 ( 2019) ISSN: 1475-2867 [Print] England
PMID30858761 (Publication Type: Journal Article)

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