Anti-GAPDH antibody (ab8245), anti-PCNA antibody (ab29), anti-Akt antibody (ab8805), anti-p-Akt antibody (ab131443), anti-IκBα antibody (ab32518), anti-NF-κB p65 antibody (ab86299), anti-CCR7 antibody (ab32527), anti-p53 antibody [DO-1] (ab1101), anti-Bax antibody [E63] (ab32503), anti-Bcl-2 antibody [E17] (ab32124), anti-caspase-3 antibody (ab13847), anti-vimentin antibody [RV202] (ab8978), anti-N-cadherin antibody (ab18203), anti-E-cadherin antibody [HECD-1] (ab1416), and anti-keratin antibody [C-11] (ab118817) were obtained from Abcam (Cambridge, UK). Pyrrolidine dithiocarbamate (PDTC) was purchased from Calbiochem (San Diego, CA, USA).

Human lung cancer A549 cells were cultured in DMEM-F12 supplemented with 10% fetal bovine serum (FBS) (Gibco, Gaithersburg, MD, USA) and 1% penicillin in a humidified 5% CO₂ atmosphere at 37°C. Cells were seeded at 1×10⁴ cells/well into 96-well plates and allowed to attach overnight. Cell viability was assessed by the CKK-8 assay (Sigma-Aldrich, St. Louis, MO, USA). Briefly, cells were treated with 1, 10, 20, 50, 100 and 200 nM CCL21 (Peprotech, Rocky Hill, NJ, USA) for 24 h and then assayed.

Human CCR7-siRNA was obtained from Guangzhou RiboBio Co. Ltd., (Guangzhou, China) and the sequences were in accordance with a previous study (7). Cells were cultured in 6-well plates and grown to 30–50% confluence before transfection. The duplexes were diluted to give a final concentration of 30 nM. The siRNA was transfected into cells using Lipofectamine RNAiMAX reagent according to the manufacturer's instructions (Invitrogen Life Technologies, Carlsbad, CA, USA).

Total proteins from 10-cm dishes (10⁶-10⁷ cells) were extracted using protein extraction reagents (Thermo Fisher Scientific Inc., Waltham, MA, USA). The nuclear proteins from 10-cm dishes (10⁶-10⁷ cells) were extracted using a CelLytic™ NuCLEAR™ extraction kit (Sigma-Aldrich). Proteins samples were quantified using a BCA protein assay kit (Beyotime Institute of Biotechnology, Jiangsu, China) and denaturated with SDS-PAGE sample loading buffer (Beyotime). Proteins (30–50 µg) were separated by reducing SDS-PAGE electrophoresis. Then the proteins were transferred onto a PVDF membrane (Millipore, Billerica, MA, USA) and blocked with 5% non-fat milk in Tris-Tween buffered saline buffer for 1.5 h. The primary antibody was incubated overnight at 4°C and the HRP-conjugated secondary antibodies were subsequently incubated for 2 h at room temperature. Then the blots were developed on the membrane using Alpha Imager 2200 software (Alpha Innotech Corporation, San Leandro, CA, USA). We digitally quantified the resultant signals and normalized the data to GAPDH or PCNA abundance.

Inflammatory cytokines were quantitatively detected by real-time PCR. Approximately 1×10⁶ cells/ml from each group were collected from 6-well plates for real-time PCR detection. The gene sequences were used to design primers and were synthesized by Invitrogen Life Technologies (Table I). Double-distilled water was used instead of a template as a negative control. The number of β-actin transcripts was used as a reference of endogenous RNA, and the quantification of test genes for each sample was standardized relative to the number of β-actin transcripts. The 2^−∆∆Ct cycle threshold formula was used to calculate the relative abundance of the transcripts.

All data were analyzed by SPSS 17.0 software. Differences were assessed by Ducan's multiple comparison test. Data are expressed as the mean ± SEM. Values in the same row with different superscripts are significant (P<0.05).

CCL21 is a ligand of CCR7 and has been suggested to upregulate CCR7 expression (7). As shown in Fig. 1A, CCL21 increased cell viability in a dose-dependent manner. After exposure to 50, 100 and 200 nM of CCL21, cell proliferation was markedly promoted compared with that noted in the control group (P<0.05). A significant difference was observed at 50 nM, and was thus used to upregulate CCR7 expression (P<0.05) for the following analysis (Fig. 1B and C). A549 cells were transfected with CCR7-siRNA to inhibit CCR7 expression. The results revealed that CCL21 treatment markedly enhanced CCR7 expression, while CCR7-siRNA suppressed its expression (Fig. 1B and C).

To further investigate the mechanism of CCR7-mediated cell apoptosis, four apoptosis-related proteins (p53, Bax, Bcl-2 and caspase-3) were analyzed after CCR7 overexpression and inhibition in A549 cells. As shown in Fig. 2, CCR7 overexpression markedly inhibited p53 and caspase-3 expression (P<0.05), while CCR7-siRNA enhanced cellular abundance of p53, Bax, and caspase-3 (P<0.05). Meanwhile, the expression of Bcl-2, an anti-apoptotic protein, was significantly decreased after CCR7-siRNA transfection when compared with that in the control group (P<0.05).

Akt and NF-κB are widely associated with apoptosis. In this study, we found that CCR7 upregulation markedly activated Akt signaling as evidenced by the increased Akt phosphorylation (p<0.05) (Fig. 3A and B), while CCR7-siRNA failed to influence Akt (P>0.05).

Furthermore, CCR7 upregulation enhanced IκBα expression while CCR7-siRNA inhibited the expression of IκBα (P<0.05) (Fig. 3A and C), an inhibitory protein of the NF-κB pathway. Thus, we further determined nuclear NF-κB p65 abundance and the results revealed that CCR7-siRNA markedly increased the expression level of nuclear p65 (P<0.05) (Fig. 3A and D).

PDTC was used to inhibit NF-κB signaling in A549 cells. CCR7-siRNA markedly inhibited CCR7 expression and enhanced nuclear p65 abundance (P<0.05), while PDTC, a special antagonist of NF-κB, suppressed NF-κB activation induced by CCR7 inhibition (P<0.05) (Fig. 4A-C).

Inhibition of NF-κB via PDTC treatment markedly downregulated p53 and Bax when compared with the levels noted following CCR7-siRNA treatment (P<0.05) (Fig. 4D and E). Meanwhile, Bcl-2 abundance was significantly higher after PTDC exposure than that in the CCR7-siRNA group (P<0.05) (Fig. 4D and E).

NF-κB signaling has been widely demonstrated to regulate inflammatory cytokines. Thus cellular expression of IL-1β, IL-6, IL-10, IL-17 and TNF-α was determined via RT-PCR. The results revealed that CCL21 treatment markedly upregulated IL-1β and IL-10 expression (P<0.05) (Table II), suggesting that overexpression of CCR7 promoted the inflammatory response. However, CCR7-siRNA treatment significantly suppressed IL-1β and IL-10 expression (P<0.05) (Table II).

TGF-β1 (20 ng/ml) was used to induce EMT in A549 cells according to a previous study (8). Vimentin (a mesenchymal cell marker), CK (an epithelial cell marker), N-cadherin, and E-cadherin have been widely used to evaluate EMT (8,9). The results showed that TGF-β1 markedly induced cell EMT as evidenced by the increased vimentin and N-cadherin and decreased CK (P<0.05) (Fig. 5). Meanwhile, CCR7-siRNA treatment significantly alleviated TGF-β1-induced EMT in A549 cells via mediating vimentin and CK expression (P<0.05) (Fig. 5).

TGF-β1 treatment induced a cell inflammatory response via upregulation of IL-1β, IL-17, and TNF-α (P<0.05) (Table III), while CCR7-siRNA treatment significantly alleviated IL-1β and TNF-α expression after TGF-β1 exposure (P<0.05) (Table III).