Cell culture and gene manipulation

All the selected human breast cell lines were purchased from the American Type Culture Collection (ATCC, USA) and grown in the recommended media, including normal breast epithelial cell line (MCF-10A), ER-positive BCa cell lines (MCF-7 and T47D), and TNBC cell lines (MDA-MB-231 and BT549). RelB was ectopically expressed in ER-positive cells with low constitutive RelB. Conversely, RelB was knocked out from the TNBC cells using CRISPR-Cas9 approach. Briefly, several gRNAs were designed using the Optimized CRISPR Design Tool [27]. Double-strand oligo DNA for each gRNA was cloned into the EcoRIsite in pGL3-U6 SPsgRNA vector. The construct was co-transfected with 331-sp cas9 plasmid into MDA-MB-231 and BT549 cells. Single-cell colonies were selected using puromycin and neomycin, and further validated by western blots. DNA was extracted from the candidate clones and confirmed by DNA sequencing prior to T7EN1 digestion.

Cell proliferation

Cell proliferation was determined using cell counting and colony formation assay, respectively. BCa cells were seeded into 96-well plates at 10³ cells/well and treated with CCK-8 reagent (Dojindo Mol. Tech., Japan), and cell viability was measured as the optical density at 450nm. For colony formation assay, BCa cells were seeded into 6-well plates at 200 cells/well and cultured for 2–3weeks. The cells were fixed in 4% paraformaldehyde for 30min, stained with 0.5% crystal violet (Beyotime Biotech., China) for 1h. After rinsing three times with 1xPBS, the cell colonies were photographed and counted.

Flow cytometry

Flow cytometry was used to analyze apoptosis and cell cycle. For apoptotic cell qualification, 2×10⁵ cells were seeded in 6-well plates and cultured for 48h. The cells were collected and washed three times with cold PBS and then stained with 5μM annexin V-FITC and 2.5μM PI (Dojindo Mol. Tech.) in a supplied binding buffer for 15min at room temperature and dark condition. Apoptotic cells were counted using a BD FACSCalibur flow cytometer (BD Biosciences, USA) and the percentage of apoptotic cells was calculated by the number of preapoptotic and apoptotic cells divided by the amount of total cells. For cell cycle analysis, the cultured cells were detached, washed and fixed with 70% ethanol overnight at 4°C. The cells were then washed 2 times with cold PBS and treated with 400μl propidium iodide (BD Biosciences, USA) for 15min. The cell cycling phases were determined by Flow cytometry.

Cell motility

Cell movability was analyzed using wound healing assay and transwell assay, respectively. BCa cells were plated into 6-well plates at 3×10⁵ cells/well with serum-free DMEM for 12h. After rinsing with 1×PBS three times, the cultured cells were separated using pipette tips to create three parallel wounds. The wells were then washed several times with PBS to remove floating cells. The cells were continuatively cultured in the completed media. The wound closure was monitored at 24 and 48h using a microscope and the wound surface area was quantified. In addition, transwell assay (Corning, USA) was used to quantify cell migration and invasion abilities. For migration assay, the cells were plated into the upper chambers without coated membrane at 5×10⁴ cells/well. For invasion assay, the chamber inserts were coated with 50μl serum-free medium mixed with matrigels (BD Biosci., USA) and solidified at 37°C for 3h. The cells were placed into the upper chamber at 10⁵ cells/well. In both assays, the cells were plated in 200μl serum-free medium in the upper chambers, and 500μl medium supplemented with 20% FBS was placed into the lower chambers. After culturing the cells for 24h, the invaded cells on the lower surface were fixed in 4% paraformaldehyde, stained with crystal violet and counted using a microscope.

RNA sequencing

Total RNA was isolated from BCa cells using a total RNA isolation kit (Invitrogen). mRNA was converted to cDNA libraries and added adapters for sequencing. The procedure of NGS sequencing on Illumina HiSeq platform was conducted by Vazyme Biotech Co., Ltd. (Nanjing, China).

Chromatin Immunoprecipitation (ChIP)

A ChIP-IT system (Active Motif, USA) was used to quantify RelB binding to the NF-κB enhancer element located at the 5′-flanking region of the human MMP1 gene. Briefly, chromatin isolated from BCa cells were pulled down using a RelB antibody (Cell Signaling, USA). Unprecipitated chromatin was used as input control and chromatin pulled down by an IgG antibody served as a negative antibody control. The pulled down the enhancer fragment was quantified using a quantitative PCR with the gene-specific primers.

Western blotting

Cytosolic and nuclear proteins were extracted from cells and tumor tissues using a RIPA lysis buffer containing PMSF and then quantified using a BCA assay kit (KeyGen Biotech., China). The extracted proteins (50–100μg) were separated on SDS-PAGE gels and then transferred to PVDF membranes. The membranes were subsequently incubated overnight at 4°C with the primary antibodies against RelB, Bcl-2, Cyclin D1 and β-actin (Santa Cruz Biotech., USA); against ER, E-cadherin, Vimentin, Snail 1, Slug, Twist 1 (Cell Signaling Tech., USA). Thereafter, the membranes were washed three times with TBST buffer and incubated at room temperature for 2h with HRP-conjugated secondary antibody (Santa Cruze Biotech.). The immunoblots were visualized using an enhanced chemiluminescence detection system (Bio-Rad, USA). The intensities of blots were quantified using Quantity One software and protein expression was normalized by loading controls such as β-actin and GAPDH.

Animal experiment

The effects of RelB on tumorigenesis and metastasis were validated using BCa cells bearing mouse xenograft tumor experimental models. All animal studies were conducted according to the Institutional Animal Care and Use approved by the Research Committee of Nanjing Medical University (No. IACUC-1711030). Five-week-old female BALB/c athymic nude mice (Beijing Vital River Lab Animal Tech. Co., Ltd., China) were used for studying tumor growth and five-week-old female SCID mice (Nanjing Medical University, China) were used for studying tumor metastasis, respectively. For the tumor growth experiment, 5×10⁶ BCa cells were subcutaneously implanted into the right axilla of mice. Tumor volume was measured using digital calipers every other day and calculated using a standard formula (V=0.52×AB², A and B represent the diagonal tumor lengths). The mice were executed when tumor volume reached to 2000mm³ and tumor tissues were removed. For tumor metastasis study, 10⁶ BCa cells were injected into mice through tail vein and assessed for lung metastasis. The mice were sacrificed at 6weeks and the number of metastatic lung nodules was counted.

Usage of TCGA database

The TCGA BCa dataset was analyzed to assess the association of RelA or RelB expression with BCa occurrence and the correlation between the mRNA level of RelA or RelB and ER-negative BCa patient survival rate.

RelB promotes BCa cell proliferation

To investigate the potential mechanism by which RelB regulates downstream gene expression involved in BCa progression, RelB was ectopically expressed into MCF-7 and T47D cells with low levels of constitutive RelB (Fig. 3a). In parallel, RelB was knocked out from TNBC cells (MDA-MB-231 and BT549) using a CRISPR-Cas9 gene edition system (Additional file 3, Figure S1; Fig. 3b). The NF-κB activity was slightly elevated in the RelB-overexpressed ER-negative cells, but significantly reduced in RelB-knocked out TNBC cells (Fig. 3c and d). Consistently, the elevated RelB in ER-positive cells led to increased cell colony number and the cell proliferation rate (Fig. 3e, g and i). Conversely, cell colony formation and the cell proliferation rate significantly decreased in RelB-knocked out TNBC cells (Fig. 3f, h and j).

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Fig. 3

Determination of RelB-enhanced BCa cell survival and growth. a RelB was ectopically expressed in ER-positive BCa cells by stably transfected a human RelB cDNA construct. b RelB was knocked out in TNBC cells using a CRISPR-Cas9 gene edition system. c, d The relative NF-κB activity was quantified in RelB-manipulated BCa cells. e, f The survival rates in the RelB-manipulated BCa cells were examined by colony formation assay. g-j The proliferation rates in the RelB-manipulated BCa cells were quantified by CCK-8 assay. Mean±SD was representative of three independent experiments carried out in duplication. *(P <0.05), **(P <0.01) show the significances between two groups as indicated

RelB promotes G1/S transition and inhibits apoptosis

To elucidate the role of RelB in BCa cell proliferation, the cell cycling process and the cell apoptotic rate were analyzed by flow cytometry. The enforced expression of RelB in MCF-7 cells resulted in decreasing G1 phase but increasing S and G2/M phases, which enhances the acceleration of cell division (Fig. 4a). In contrast, knock out of RelB in MDA-MB-231 cells led to an increasing G1 phase but decreasing S phase (Fig. 4b). Furthermore, apoptosis was examined in the RelB-manipulated BCa cells. Although the elevated RelB in MCF-7 cells unlikely changed the cell apoptotic rate, the depletion of RelB in MDA-MB-231 cells obviously increased apoptotic cell rates (Fig. 4c and d). Consistently, the overexpression of RelB in MCF-7 cells resulted in upregulation of Cyclin D1, but no effect on Bcl-2 expression (Fig. 4e). Additionally, knock out of RelB in MDA-MB-231 cells led to suppression of Cyclin D1 and Bcl-2, suggesting that RelB sustains TNBC cell growth via activation of prosurvival and antiapoptotic pathways (Fig. 4f). Moreover, RelB depletion led to increases in p21 and p27, but decreases in c-Myc, Cyclin E1 and Bcl-xL (Additional file 4, Table S2; Additional file 5, Figure S2).

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Fig. 4

The effect of RelB on cell cycle and apoptosis. a, b The cell cycling process in RelB-manipulated BCa cells was analyzed using flow cytometry. c, d Preapoptotic and apoptotic cells in the RelB-manipulated BCa cells were quantified by flow cytometry. e, f The levels of Bcl-2 and Cyclin D1 proteins were measured by western blots. Statistical significance between two groups as described in Fig. 3

RelB enhances BCa cell mobility by enhancing EMT

It has been widely recognized that BCa progression is generally through the ER-dependent phenotype to ER-independent malignancy. Importantly, emerging evidence demonstrated the inverse relationship between ER and NF-κB in BCa cells [28]. Consistently, the expression of RelB appeared to be inversely correlated to ER levels in the tested cell lines (Additional file 6, Figure S3a). Furthermore, ER elements-driven luciferase reporter gene expression construct was constructed to examine whether RelB is able to regulate the ER response. Expectedly, the ER-reporter response was remarkably reduced due to the increased RelB in MCF-7 cells, suggesting that RelB negatively regulates ER signaling (Additional file 6, Figure S3b).

Furthermore, to testify whether RelB contributes to estrogen-deprived BCa progression, the effect of RelB on the metastatic ability of BCa cells was examined. Since the EMT process has been well documented in BCa metastasis, several EMT markers were measured in our panel of BCa cell lines. The elevated RelB in ER-positive cells led to decreasing E-cadherin but increasing Snail I, Slug I, Twist I and Vimentin (Fig. 5a). In parallel, knock out of RelB in TNBC cells resulted in decreasing those EMT markers, while E-cadherin was not detectable in TNBC cells (Fig. 5b). Accordingly, the effect of RelB on the cell motility was analyzed by quantifying cell capacities of wound healing, migration and invasion. As expected, the enforced expression of RelB in MCF-7 cells significantly enhanced the cell capacity for wound recovery compared to a vehicle control (Fig. 5c). Consistently, the elevated RelB in MCF-7 cells also resulted in enhancing cell migration and invasion (Fig. 5e). Subsequently, knock out of RelB in MDA-MB-231 cells led to decreases in those capacities (Fig. 5d and f). These results suggest that RelB promotes ER-independent BCa progression mainly through activating EMT process.

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Fig. 5

The effect of RelB on EMT. a, b The EMT-associated markers in RelB-manipulated BCa cells were measured by western blots. c, d The cell wound healing abilities were analyzed. e, f The cell a migration and invasion capacities were examined using a transwell assay. Statistical significance between two groups as described in Fig. 3

RelB upregulates bone metastasis associated protein, MMP1

To identify the important RelB-regulated genes involved in BCa metastasis, we applied RNA-Seq analysis using total RNA isolated from RelB-knocked out MDA-MB-231 cells vs. the parent cells. The results indicated that the mRNA expression profiles of numerous genes were altered in the RelB-knocked out cells (Fig. 6a and b). Importantly, multiple genes relating to metastatic signaling pathways were downregulated (Fig. 6c and Table 1). Among of them, MMP1, an activator in BCa bone metastasis [29], was highly related to the level of RelB. To assess the effect of RelB on MMP1 expression, we verified the expression level of MMP1 increased in RelB-overexpressed MCF-7 cells, but decreased in RelB-knocked out MDA-MB-231 cells, suggesting that RelB may directly regulate the MMP1 gene (Fig. 6d).

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Fig. 6

RelB-mediated transcriptional regulation. mRNA expression profiles in the RelB-knocked out MDA-MB-231 cell vs. the parent cell were examined using a RNA-Seq platform. a The distribution of mRNA profiles in the RelB-deprived cell was illustrated. b Cluster analysis of RNA-Seq data indicates up/down-regulated mRNA profiles (heatmap). c KEGG pathway enrichment analysis was performed to assess EMT/metastasis relating mRNA profiles. d The protein level of MMP1 was quantified in the RelB-manipulated BCa cells. e A 5′-flanking region of the human MMP1 gene (5’MMP1) containing the NF-κB element (underline) and the core promoter region was cloned in pGL4 vector to drive the luciferase reporter gene expression as illustrated. The enhancer activity modulated by RelB in BCa cells was estimated by normalized reporter responses. f A small DNA fragment containing the NF-κB element was pulled down from chromatins using a RelB antibody and then quantified by PCR. IgG serves as a negative antibody control. Statistical significance between two groups as described in Fig. 3

To elucidate how RelB regulates MMP1 expression, we identified a putative NF-κB element located in the 5′-finking region of the human MMP1 gene. For verifying this NF-κB element functional response to transcriptional activation by RelB, a 5′-flanking region containing the NF-κB enhancer element and the core promoter in the human MMP1 gene was cloned into a pGL4 vector to drive the luciferase reporter gene expression. Compared to the basic vector control, the reporter gene response driven by the MMP1 enhancer highly increased in RelB-overexpressed MCF-7 cells, but significantly decreased in RelB-knocked out MDA-MB-231 cells (Fig. 6e). Moreover, to confirm that RelB-mediated transcriptional activation through binding to the NF-κB enhancer element located at the 5′-flanking region of the MMP1 gene, a 240-bp fragment containing the NF-κB enhancer element was pulled down using a specific RelB antibody and amplified using PCR. The amount of pulled-down DNA fragment from MCF-7 cell chromatin was less than the level from MDA-MB-231 cell chromatin (Fig. 6f).

Furthermore, to validate whether the increased MMP1 can further promote EMT, MMP1 was manipulated by overexpressing in MCF-7 cells but silencing in MDA-MB-231 cells. The elevated MMP1 in MCF-7 cells led to a slight decrease in E-cadherin but increases in Snail 1, Twist1 and Vimentin. In contrast, the silence of MMP1 in MDA-MB-231 cells resulted in decreasing Snail 1, Twist 1, Slug and Vimentin, regardless of the undetectable of E-cadherin in the cells (Additional file 7, Figure S4a). In addition, to determine the functional contribution of MMP1 to EMT under the RelB regulation, MMP1 was either ectopically expressed in RelB-knocked out MBA-MB-231 cells or was silenced in RelB-overexpressed MCF-7 cells. Intriguingly, the elevated MMP1 in RelB-knocked out MBA-MB-231cells resulted in partially restored the EMT proteins, while the silence of MMP1 in RelB-overexpressed MCF-7 cells was able to abrogate the elevated EMT proteins except for no effect on Twist 1 expression (Additional file 7, Figure S4b).

We thank Dr. Daret K. St. Clair, University of Kentucky Markey Cancer Center for her kind suggestions. We are grateful to Dr. Xingxu Huang, School of Life Science and Technology, Shanghai-Tech University, China, for providing a CRISPR/Cas9 system used in this study to knock-out RelB in BCa cells.