Hypoxia mediated KDM4A to induce ferroptosis resistance in CC cells. SiHa and Hela cell lines were transfected with shKDM4A, followed by 2-h normoxia or hypoxia treatment and 24-h incubation with Erastin. (A) The efficiency of shKDM4A transfection was detected by RT-qPCR; (B) The mRNA level of KDM4A was detected by RT-qPCR; (C) Cell viability was determined by MTT assay; (D-F) The intracellular iron concentration, MDA, and GSH levels were measured using colorimetry method. The experiments were conducted in 3 replicates independently. The data were expressed as mean ± standard deviation. One-way ANOVA was used for comparisons among groups with Tukey’s multiple comparisons test as the post hoc test; , & vs. the Normal + Erastin + shNC group, p <0.05; # vs. the Normal + Erastin + shKDM4A group, p <0.05.