In PR NSCLC cells, overexpression of miR-489-3p increased sensitivity to PTX and suppressed cell growth via inhibiting IGF1. (a and b) A combination of qRT-PCR and ELISA was used to quantify IGF1 expression. (c) The MTT assay was used to determine cellular proliferation. (d) The MTT test was used to calculate the IC50 values of DTX, DDP, and PTX. *.