Abstract
In recent years, the anticancer properties of metabolites from halophilic microorganisms have received a lot of attention. Twenty-nine halophilic bacterial strains were selected from a culture collection to test the effects of their supernatant metabolites on stem cell-like properties of six human cancer cell lines. Human fibroblasts were used as normal control. Sphere and colony formation assay were done to assess the stem cell-like properties. invasion and migration assay, and tumor development in mice model were done to assess the anti-tumorigenesis effect in vitro and in vivo. The metabolites from Salinivenus iranica demonstrated the most potent cytotoxic effect on breast cancer cell lines (IC50 = 100 µg/mL) among all strains, with no effect on normal cells. In MDA-MB-231 cells, the supernatant metabolites enhanced both early and late apoptosis (approximately 9.5% and 48.8%, respectively) and decreased the sphere and colony formation ability of breast cancer cells. Furthermore, after intratumor injection of metabolites, tumors developed in the mice models reduced dramatically, associated with increased pro-apoptotic caspase-3 expression. The purified cytotoxic molecule, a phenol amine with a molecular weight of 1961.73 Dalton (IC50 = 1 µg/mL), downregulated pluripotency gene SRY-Box Transcription Factor 2 (SOX-2) expression in breast cancer cells which is associated with resistance to conventional anticancer treatment. In conclusion, we suggested that the phenol amine molecule from Salinivenus iranica could be a potential anti-breast cancer component.
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Introduction
Cancer stem cells are small populations in tumor cells responsible for cancer complications like drug resistance and metastasis1,2,3. Cancer stem cell targeting is an intelligent approach for increasing the survival rate in cancer treatment4,5. Several investigations have screened natural products for their inhibitory effects on cancer stem cells6. Among these natural products, Salinomycin, a metabolite generated from the soil bacterium Streptomyces albus, is one of the natural products that directly kills and inhibits cancer stem cells and is on the verge of being approved by the Food and Drug Administration (FDA) as an effective anti-cancer drug with few side effects7. This evidence supports the idea that microorganisms can be used in cancer stem cell targeting.
Halophiles are a group of extremophile microorganisms that live in high salt concentrations8. Recent scientific research has emphasized the significance of metabolites derived from halophilic microorganisms for treating cancer. Specifically, two metabolites known as 8-O-Methyltetrangulol and Naphthomycin A were isolated from the halophilic strain Streptomyces sp. WH26 and have shown promising cytotoxic activity against various types of cancer cell lines. These include human lung cancer cells (A549), human cervical cancer cells (HeLa), human hepatocellular carcinoma cells (BEL-7402), and human colorectal adenocarcinoma cells (HT-29)9. In another study, researchers found that five of forty moderately halophilic bacterial strains reduced the viability of human hepatocellular carcinoma Bel 7402 cells to 50% when tested at 40 µg/mL10. In 2019 Neelam et al., reported that metabolites from Piscibacillus sp. C12A1 isolated from Sambhar Lake in India decreased the viability of the MDA-MB-231 breast cancer cell line with downregulation of Bcl-xL and CDK-2 expression in these cells. Also, these metabolites inhibited cell migration and colony formation of MDA-MB-231 cancer cells11.
Despite the abovementioned evidence, no research has been done on the effect of metabolites from halophiles or extremophiles on cancer stem cells; therefore, studies in this regard are necessary. This study screened the cytotoxic effect of supernatant metabolites (SM) from twenty-nine native halophilic and halotolerant strains obtained from the Iranian biological resource center (IBRC) on six distinct cancer cell lines, including lung (A549), prostate (DU145, LNCaP, PC3), breast (MCF-7, MDA-MB-468), and human fibroblasts as the normal control. It is important to note that the cancer cell lines used in this study are heterogeneous and include only a small subset of stem cells. The mechanism of action and tumorigenicity of strains that selectively reduced viability only on cancer cells and stem cell-like properties of cancer cells and not normal cells were assessed through in vitro and mouse models. In vitro assays, such as colony formation and sphere formation, were used to demonstrate the stem cell-like characteristics of these cancer cells. As the selected SMs showed potential anticancer effects on breast cancer cells, the MDA-MB-231 breast cancer cell line was added to the study and used alongside the other two breast cancer cell lines. Furthermore, the effector molecule of the supernatant metabolite was purified, and its structure was partially elucidated.
Results
Screening and finding the most cytotoxic strains against different cancer lines
Twenty-nine halophilic and halotolerant bacterial strains were obtained from the Iranian biological resource center (IBRC) microorganisms bank, all of which were type strains of the species (Table 1). To screen the anti-cancer effect of the selected strains, three cancer types were chosen; prostate cancer (DU145, LNCaP, PC3), breast cancer (MDA-MB-468, MCF-7), and lung carcinoma (A549). Human fibroblasts (HFF-5) were used as normal cells. All cells were treated with different concentrations of Supernatant Metabolites (SM) of those selected strains. As shown in Table 1, the SM of eleven strains like Alloactinosynnema iranicum, Alteribacillus persepolensis, Bacillus iranensis, Bacillus persicus, Cyclobacterium halophilum, Limimonas halophila, Oceanobacillus limi, Pseudomonas salegens, Salinicoccus iranensis, Salinivibrio proteolyticus, and Thalassobacillus cyri did not have any cytotoxic effect on fibroblasts and cancer cells.
However, Salinivenus lutea was cytotoxic on normal fibroblasts even at a 200 µg/mL dose. Aliicoccus persicus and Aquibacillus albus did not have any effect at a 100 µg/mL dose on cell viability in all cells. Meanwhile, they were heavily toxic for both normal fibroblast and cancer cells at 400 µg/mL and 800 µg/mL. Twelve strains were not toxic for fibroblasts and only affected cell viability of one or two tumor types but at 400 µg/mL and 800 µg/mL. Among twenty-nine selected strains, we found Salinibacter ruber and Salinivenus iranica with an anti-cancer effect on all breast cancer cell lines (MCF7, MDA-MB-231, MDA-MB-468) at 100 µg/mL and without any effect on normal fibroblasts (Table 1). The SM of both strains significantly reduced the viability of cells to 50% 48h post-treatment, and their effect was stable for an extra 48h when the SM was removed from culture media (Fig. 1a,b). Hence, these strains were selected for further experiments.
Salinivenus iranica, Salinibacter ruber, and the cancer stem cell-like properties of breast cancer cell lines
Sphere and colony formation determine the self-renewal potential of cancer cells12,13. Therefore, we evaluated the effect of Salinibacter ruber and Salinivenus iranica SMs on sphere and colony formation ability of MDA-MB-231, MDA-MB-468, and MCF-7 cells. Prior to treatment, all three human breast cancer cell lines exhibited stem-like properties, as evidenced by their ability to form colonies and large spheres. These characteristics are indicative of the presence of stem-like cells in the cell lines. Our results indicated that cells in all treated groups with both SMs lost their repopulation and could not form large spheres. Salinivenus iranica and Salinibacter ruber reduced the spheroid formation ability to about 3.5, 8.4, and 2.7 folds in MDA-MB-231, MDA-MB-468, and MCF-7 cells, respectively (p < 0.001). In addition, Salinivenus iranica and Salinibacter ruber SMs significantly decreased the size of spheres about 1.4-fold in MDA-MB-231 cells, 2.2 folds in MDA-MB-468, and 1.5-fold in MCF-7 cells (Fig. 2a,1–6). The results of the colony formation test were a bit different as Salinivenus iranica reduced the percentage and size of colonies in all treated cells significantly in MDA-MB-231, MDA-MB-468, and MCF-7 cells, (p < 0.001). While Salinibacter ruber only declined colonies in MCF-7 cells (1.8-fold, p < 0.001) with no reduction in the size of colonies (Fig. 2a,7–12). The type of colonies also is a determinative factor for the presence of stem-like cells in a cell population as the higher number of holoclones (compact colonies with distinct margins) means that cancer stem cells were higher in the cell pools. The results exhibited that the number of holoclones reduced in Salinivenus iranica treated cells from 24.50 and 31.12 to 5.50 and 12.62 in MDA-MB-231 and MCF-7, respectively (p < 0.001) along with the reduction in meroclones (loose colonies) and paraclones (colonies with both compact and loose cells) in MDA-MB-468 cells. Salinibacter ruber only reduced the number of holoclones in MCF-7 cells from 31.12 to 16.75 (p < 0.001). However, it significantly enhanced the number of paraclones in MDA-MB-231 cells with no significant effect on the number of meroclones (Fig. 2b).
Our study found that treatment with Salinibacter ruber resulted in a significant decrease in the migration of breast cancer cells (p < 0.001). However, the invasion of MDA-MB-231 and MCF-7 cells was reduced by 60% (p < 0.001) and 77.5% (p < 0.001), respectively, while the invasion of MDA-MB-468 cells was increased by 89.1% (p < 0.001). Notably, the invasion index dramatically increased in cells treated with Salinibacter ruber, from 0.15 to 0.56 (p < 0.001) in MDA-MB-231 cells, from 0.04 to 0.60 (p < 0.001) in MDA-MB-468 cells, and from 0.74 to 6.00 (p < 0.001) in MCF-7 cells. Conversely, treatment with Salinivenus iranica had different effects on the invasion and migration of breast cancer cells. The migration of MDA-MB-231 and MDA-MB-468 cells increased by approximately two-fold (p < 0.001), while the migration of MCF-7 cells decreased by approximately 75% (p < 0.001). Specifically, Salinivenus iranica reduced the invasion of MDA-MB-231 and MCF-7 cells by 85.0% (p < 0.001) and 53.1% (p < 0.01), respectively, but did not significantly affect the invasion potential of MDA-MB-468 cells. Furthermore, Salinivenus iranica reduced the invasion index of MDA-MB-231 treated cells from 0.16 to 0.01 (p < 0.001). However, it significantly (p < 0.01) enhanced the invasion potential of MCF-7 by approximately two-fold, with no significant change in the invasion index of MDA-MB-468 cells (Fig. 2c). As the decrease in invasion index is an indicator of stem-like cells in cancer cell populations, and its reduction showed the reduction of cancer stem cells14, the results from Salinivenus iranica were better in reducing the cancer stem cells.
Overall, because of the more desirable results of Salinivenus iranica SM on inhibiting cancer stem cells (sphere and colony formation and invasion index), this strain was selected for future experiments.
Salinivenus iranica’s supernatant metabolites induce late apoptosis and S phase inhibition in breast cancer cells
The apoptosis assay was done on treated and untreated breast cancer cell lines to find the effect of Salinivenus iranica SM on the induction of apoptosis. As shown in Fig. 3a, the percentage of both early and late apoptosis was extremely enhanced in all treated cells, which were associated with overexpression of pro-apoptotic caspase-3 (CASP3) (a marker of late apoptosis) (p < 0.001). Resistance to traditional anticancer therapy is related to SOX2 expression. Therefore, inhibiting SOX2 expression may decrease the malignant characteristics associated with breast cancer, such as invasion, migration, proliferation, stemness, and chemoresistance15. As a result, SOX2 expression was monitored. Expression of the SOX2 gene was significantly down-regulated in MDA-MB-231 and MDA-MB-468 cells (p < 0.001, Fig. 3a).
Cell cycle analysis showed that the percentage of cells in the S phase of the cell cycle significantly reduced in MDA-MB-231 (16.49% vs. 12.11%, p < 0.05) and MCF-7 cells (36.66% vs. 16.65%, p < 0.001) post-treatment, while no significant change was observed in MDA-MB-468. On the other hand, after treatment, the percentage of cells in the G1 and G2 phase was up-regulated significantly in MDA-MB-468 cells (50.95% vs. 56.45%, p < 0.01) and (14.10% vs. 19.16%, p < 0.01), respectively. Also, the percentage of cells in the G1 phase was up-regulated significantly in MCF-7 cells (58.21% vs. 74.18%, p < 0.001). In G1/G2 and G2 phase no significant changes were observed in MDA-MB-231 and MCF-7 cells, respectively (Fig. 3b).
Salinivenus iranica inhibits breast tumor growth in vivo
We injected 1.25 × 106 of 4T1 cells (mice breast cancer cell line) subcutaneously to develop breast cancer tumors in BALB/c mice. When the tumor size reached 50–60 mm3 (about three days post cellular injection), Salinivenus iranica SM at a dose of 17.5 mg/kg (Equivalent to 100 µg/mL in vitro) was injected intratumorally, just for one time. Interestingly, the size of injected tumors was smaller than controls post seven days of SM injection (181.60 mm3 vs. 661.74 mm3). The expression of ki67 and sox2 (markers of cell proliferation and pluripotency) was downregulated. However, cdh1 (migration-related gene) was significantly upregulated in injected tumors (p < 0.01, Fig. 3c).
A phenol Amine molecule acts as the effective part of Salinivenus iranica metabolites
To find the effective part of Salinivenus iranica's SM, the crude metabolite was fractionated by four solvents: hexane, ethyl acetate, butanol, and water. It was separated into thirty-one fractions. A solution containing 100 µg/mL of separately fraction was prepared, and the viability of three human breast cancer cell lines was evaluated in their presence. Fraction number 6 of hexane had decreased the viability of all cell lines to 1% after 48 h, while the other 30 fractions did not exhibit any significant effect on cell lines viability (Fig. 4a). As the fraction had only one visible peak, the effective anticancer metabolite was purified in this phase. The mass spectrophotometry defined that this molecule's molecular weight (MW) was about 1961.78 Da (Fig. 4b). In Fourier Transform Infrared Spectroscopy (FT-IR) analysis, three types of functional groups were observed in this molecule (Fig. 4c). 1: In 2950 – 2850 cm−1, Alkyl C-H Stretch was distinguished, which are generally less useful in defining structure as a consequence of fairly ubiquitination. 2: In 3500—3300 cm−1, Amine N–H Stretch was detected, which is a primary amine, as Primary amines produce two N–H stretch absorptions, secondary amides only one, and tertiary none. 3: In 3550–3200 cm−1, Alcohol/Phenol O–H Stretch was detected. These results exhibited that the effective part of Salinivenus iranica metabolites was a phenol amine molecule with a molecular weight of 1961.78 Da.
To determine the anticancer activity of purified phenol amine molecule, MDA-MB-231, MDA-MB-468, and MCF-7 breast cancer cell lines and one normal human fibroblast cell line (HFF-5) were subjected to treatment by different concentrations of this molecule. After 48 h, none of the concentrations had a cytotoxic effect on fibroblasts, while the 1 µg/mL of the phenol amine molecule significantly reduced the viability of all breast cancer cells to 50% (Fig. 5a). Also, this molecule significantly downregulated the expression of the pluripotency gene, SOX2 (p < 0.001), and caused the overexpression of CASP3 (a marker of late apoptosis) (p < 0.01, Fig. 5b) in all breast cancer cells.
Discussion
Using natural compounds to target cancer stem cells could help decrease the severe side effects of chemotherapy and provide a potential anti-cancer response8,10,16. Therefore, in the present study, we screened supernatant metabolites (SM) of at least twenty-nine strains of halophilic bacteria isolated from different hypersaline lakes of Iran to find the effective anti-cancer strain that could potentially target most cancer cell lines, including breast (MDA-MB-468 and MCF-7), lung (A549) and prostate (DU145, PC3, and LNCaP) cancer cells. Our initial screening indicated that the SM of Salinibacter ruber and Salinivenus iranica reduced the viability of breast cancer cell lines at lower concentrations while it was ineffective on normal cells (HFF-5). At higher concentrations, these bacteria were able to decrease the viability of all selected cancer cell lines. This suggested that their effects might be dose-dependent. SMs enhanced the percentage of early and late apoptosis and the expression level of CASP3 in breast cancer cells. Sagar et al. observed that halophilic bacterial extracts were toxic at the dose of 200 and/or 500 µg/mL on HeLa, MCF-7, and DU145 cells17 and induced apoptosis in cancer cells18. Apoptotic cell death is induced by caspase-3, which is an executioner caspase and a crucial mediator of intrinsic and extrinsic pathway-activated apoptosis. Upon activation of pro-apoptotic proteins, caspase-3 cleaves proteins such as cell cycle proteins, and DNase proteins and leads to apoptotic cell death19. More so, caspase-3, recognized as an important early biomarker for evaluating chemotherapy-induced cell death, is mainly responsible for tumor cells' response to chemotherapy via the cell apoptosis pathway and activation20. Furthermore, the molecule, PPDHMP, from Staphylococcus sp. strain MB30 (a marine bacterium) induces apoptosis in the lung (A549) and cervical (HeLa) cancer cells through increases in the expression of CASP321. Moreover, the number of cells in the cell cycle's S phase (synthesis phase) significantly reduced in MDA-MB-231 and MCF-7 cells post-treatment with Salinivenus iranica. Therefore, Salinivenus iranica could inhibit the synthesis phase in breast cancer cells.
Interestingly, Salinivenus iranica SMs significantly reduced the number and size of spheres and colonies in all breast cancer cell lines, which were associated with the downregulation of SOX2 as a pluripotency gene. SOX2 is an essential gene in breast cancer cells that plays an early role in breast carcinogenesis and induces the metastatic potential in these cells22, and its inhibition could prevent tumor initiation of human breast cancer23. In contrast, Salinibacter ruber SMs potentially reduced the number and size of spheres and had no reduction effect on colony formation ability of all breast cancer cell lines. Both sphere and colony formation can indicate the presence of cancer stem cells in breast cancer cell lines12,24. More so, holoclones, which are compact colonies with specific borders, are an important marker of cancer stem cells24. Salinivenus iranica reduces the number of holoclones in MDA-MB-231 and MCF-7 cells. In contrast, the Salinibacter ruber reduced these numbers only in MCF-7 and enhanced the number of paraclones in MDA-MB-231, which is a pattern of induction of differentiation. Moreover, cancer stem cells are assumed as metastasis inducers in breast cancer16, and the invasion index is an exhibitor of invasion in cancer cells. Our results indicated that the Salinibacter ruber significantly increased this index in all breast cancer cells, but Salinivenus iranica reduced this index in MDA-MB-231 cells. Therefore, we suggested that Salinivenus iranica is a more reliable strain for inhibiting cancer stem cells. In vivo examinations showed that the tumor size decreased in the presence of Salinivenus iranica SM. Halophilic bacterial extracts exhibited tumor growth inhibition ability in previous studies. It was reported that Streptomyces sp. ANAM-5 and AIAH-10 in their co-culture produced some metabolites which had decreased tumor growth in Ehrlich Ascites Carcinoma cell-bearing albino mice25. The expression of ki67 was significantly down-regulated in treated tumors compared to the untreated ones. As ki67 is the marker of proliferation26, this revealed the role of the SM in the proliferation inhibition of breast cancer cells. Also, the expression of sox2 (a pluripotency gene) was reduced in treated tumors, which approved the in vitro studies. The upregulation of gene cdh1, which encodes E-cadherin, is important in inhibiting metastasis in the breast cancer tumor cells because the inhibition of cdh1 causes the initiation of epithelial-mesenchymal transition and metastasis27. The expression of cdh1 was enhanced in mouse breast cancer tumors after Salinivenus iranica treatment, and it was similar to the effect of Salinomycin on mouse breast cancer stem cells28. This showed the similarities between Salinomycin and Salinivenus iranica SM in inhibiting breast cancer stem cells. Moreover, the purified phenol amine molecule reduced the viability of breast cancer cells at a lower concentration with a significant decrease in SOX-2 expression. This revealed that the purified phenol amine was the effective molecule that performed the principal role in inhibiting breast cancer stem cells in Salinivenus iranica SM.
Conclusions
This is the first study to investigate the anti-cancer stem cell effects of halophilic bacterial metabolites. The findings revealed that metabolites produced from Salinivenus iranica have significant anti-cancer and anti-cancer stem cell activities. Furthermore, the anti-cancer stem cell ability of the purified phenol amine molecule was discovered in this study. The apoptosis was induced by overexpression of CASP3, and the pluripotency was reduced by the downregulation of SOX2. In addition, the SM decreased the invasion index of breast cancer cell lines and demonstrated these results in tumors of the mouse model.
Methods
Bacterial culture, supernatant isolation, and metabolite extraction
Twenty-nine halophilic strains were selected from the Iranian Biological Resources Center (IBRC) microorganism’s bank. All strains cultured in Sea Water Nutrient (SWN) medium with the total salt of 3% or 7% or in Modified Growth Medium (MGM) with 23% total salt or Yeast Malt Agar (YM Agar or ISPII medium, Table 1). All the materials and reagents were purchased from Merck (E. Merck, Darmstadt, Germany). One loopful of agar slant culture of each strain for metabolite production was inoculated into 25 mL of proper medium. The inoculated medium was incubated at 34 or 40 °C for 12 h on a rotary shaker at 150 rpm and then transferred into a 225 mL medium to cultivate at the same temperature for 3 or 7 days. The culture was taken and centrifuged at 4000 g for 40 min. The cell-free supernatant was filtered with Whatman no.1 filter paper. An equal volume of ethyl acetate was added to the upper layer with the ratio of 1:1 and was shaken well for 2 h at room temperature, and was allowed to settle overnight at 4 °C. The upper organic layer containing supernatant metabolites was collected in a clean, dry bottle and then evaporated by BUCHI Rotavapor R_114 (Switzerland) until 1 mL of total volume remained in the rotary balloon. The remaining volume was transferred to a sterile vial with identified weight and evaporated again to dry completely. The vial which contained the dried metabolite was weighted, and the pure weight of the metabolite was calculated. The SM was dissolved in DMSO (Merck, Germany), serving as a stock solution, which was later diluted to a final solvent concentration. The SM was tested as the weight of total SM/volume9. The SM of each inoculated medium was isolated and used as a control negative.
Human cell culture
HFF-5 (Human Foreskin Fibroblast) cells were obtained from the Royan Institute cell bank (Tehran, Iran). Prostate cancer cell lines of PC3, LNCaP, and DU145 were obtained from the national cell bank of Iran (Pasteur Institute of Iran, Tehran, Iran). Lung cancer cell line, A549 (IBRC C10080) and breast cancer cell lines, MDA-MB-468 (IBRC C 10095), MDA-MB-231(IBRC C10684), MCF-7 (IBRC C10082), and 4T1 (IBRC C10056) were obtained from the cell bank of Iranian Biological Resource Center, Tehran, Iran. The monolayer of Breast cancer cell lines was grown in DMEM high glucose (GIBCO; Germany) medium, and other cell lines were grown as a monolayer in RPMI 1640 (GIBCO; Germany) medium. All cells were grown in media supplemented with 10% (v/v) Fetal Bovine Serum (FBS), 1.0 mM sodium pyruvate and 2 mM L-glutamine, 100 U/mL penicillin, and 100 μg/mL streptomycin (all from GIBCO; Germany) at 37 °C in a humidified atmosphere of 95% air and 5% CO229.
MTT assay
The effect of SMs on cell viability was evaluated using the MTT-assay by 3-(4,5-Dimethylthiazol-2-yl)-2,5-diphenyl tetrazolium bromide (MTT, Biosera, Austria), and the results were expressed as viable cell percentages compared to the control. A 96-well plate was seeded with approximately 5000 cells per well and allowed to adhere for 24 h. Three replicates of each plate were incubated with different concentrations of metabolite extracts (0, 10, 100, 200, 400, and 800 µg/mL) or purified molecules (100, 50, 25, 10, 5, 2.5, 1, 0.5, 0.25, and 0.1 µg/mL), and viability was measured after 48 h30. The final concentration of DMSO was 1mM which was not cytotoxic for our cell lines (data have not been shown). After treatment, 10 μL of 5 mg/mL solution of MTT in PBS was added to each well. The plate was then incubated for 3 h at 37 °C. Finally, the medium was removed, and 100 μL of the DMSO was added to each well to solubilize the blue formazan. Dye absorbance was measured at 560 nm. One chamber of each 96 well plate contained only DMSO, and its OD560 was assumed blank. The resulting ODs (control and treated groups) from each plate were first subtracted from the blank of the same plate, and then the mean of OD560 for control and treated groups was calculated. The percentage of viable cells was calculated via mean OD560 (Treated group)/ mean OD560 (Control group) × 100. The effect of SM from inoculated mediums was also measured in the same way, and no significant changes were observed (data have not been shown).
Sphere formation assay
Sphere formation capacities were assessed after 48 h of SM pretreatment. To perform this assessment, cells were seeded at a density of 106 cells/well in 6-well plates and allowed to adhere for 24 h. Then the cells were treated with bacterial metabolite at 0 (as control) and 100 µg/mL (IC50 dose). After 48 h, cells were harvested for sphere formation assay. To create a single-cell suspension for sphere formation, the single-cell suspension was prepared by enzymatic (1 × Trypsin–EDTA, Sigma Aldrich) and manual disaggregation (25-gauge needle). Cells were seeded in culture dishes coated with (2-hydroxyethyl methacrylate) (poly-HEMA, Sigma) and cultivated in serum-free DMEM supplemented with B27 (GIBCO, Karlsruhe, Germany), 20 ng/ml EGF and bFGF (Royan Institute, Tehran, Iran), and PenStrep. Cells were grown for 7 days and maintained in a humidified incubator at 37 °C and an atmospheric pressure of 5% (v/v) carbon dioxide/air. After 7 days, the spheres with a diameter of > 50 µm were counted using an eyepiece graticule. The percentage of spheres pre-and post-treatment was calculated by dividing the number of spheroids by the number of seeding number × 100 and is referred to as the percentage of sphere formation. Values were expressed as means ± SD of at least three independent experiments.
Colony formation assay
Colony formation capacities were assessed after 48 h of SM pretreatment. The numbers of 200 cells from pretreated and un-pretreated (Control) groups were plated in each well of six-well plates in DMEM medium supplemented with 10% (v/v) FBS and allowed to grow for 12 days. After this, the upper media was removed, and the chamber was washed twice with PBS. Then the colonies were fixed with paraformaldehyde 4% and stained with crystal violet. The colonies were counted under light microscopy, and the percentage of colonies pre-and post-treatment was calculated by dividing the number of colonies by the number of seeding number × 100, which is referred to as the percentage of colony formation. Values were expressed as means ± SD of at least three independent experiments.
Invasion and migration assay
Invasion and migration assays were done after 48 h of SM pretreatment. To assess migration, 125 × 103 were seeded in the serum-free medium into the upper chamber of the transwell filter (pore size 8 µm, Corning; Germany). The bottom of the wells (24-well plate) was filled with DMEM medium supplemented with 20% (v/v) FBS. To assess invasion, the same procedure was done with only one difference: Transwell filters were coated with 0.5 mg/mL of Matrigel overnight later, before seeding. For both migration and invasion assay, the media and remaining cells in the upper chamber were removed 12 h after seeding, and the lower side of the filters was washed twice with PBS and fixed with paraformaldehyde 4%, then they were colored with crystal violet. The number of migrated and invaded cells was counted and compared between treated and untreated (Control) cells. The invasion index was calculated as the number of invaded cells/numbers of migrated cells.
Quantitative real-time RT-PCR (qRT-PCR)
Total mRNA was isolated from treated and control cell lines after 48 h using TRIzol reagent (Invitrogen) according to the manufacturer’s instruction. cDNA was synthesized using the RevertAid H Minus First Strand cDNA Synthesis Kit (Fermentas, Waltham, Massachusetts, USA). SYBR Premix Ex Taq II (Tli RNase H Plus) (Takara, Berkeley, California, USA) was utilized to perform quantitative real-time reverse transcription-PCR (RT-PCR) using Rotor-Gene 6000 (Corbett). The GAPDH and gapdh gene transcripts were measured as a normalizer to determine the other gene relative transcripts (2−ΔΔCt)30. The sequences of primers are GAPDH: 5′ GTG GTC TCC TCT GAC TTC AAC 3′, 5′ AGG GTC TCT CTC TTC CTC TTG 3′, SOX2: 5′ CAA GAT GGC CCA GGA GAA C 3′, 5′ TCA TGT AGG TCT GCG AGC TG 3′, CASP3: 5′ AAG CGA ATC AAT GGA CTC TGG 3′, 5′ CAA GTT TCT GAA TGT TTC CCT GAG 3′, gapdh: 5′ CAA GGA GTA AGA AAC CCTG 3′, 5′ TCT GGG ATG GAA ATT GTG AG 3′, ki67: 5′ AGA GCC TTA GCA ATA GCA ACG 3′, 5′ GTC TCC CGC GAT TCC TCT G 3′, sox2: 5′ GCT GGG AGA AAG AAG AGG AG 3′, 5′ ATC TGG CGG AGA ATA GTT GG 3′, cdh1: 5′ TCG GAA GAC TCC CGA TTC AAA 3′, 5′ CGG ACG AGG AAA CTG GTC TC 3′.
Apoptosis test
The apoptotic effects of SM on treated and control cells were measured using the annexin-V/PI Staining Kit (Sigma) according to the manufacturer’s instruction. Annexin-V binding to phosphatidylserine suggests early apoptosis, whereas binding to annexin-V and PI indicates late apoptosis31.
Cell cycle test
Cell cycle analysis was measured by flow cytometry. After 48 h of treatment, treated and untreated (control) cells were fixed in cold 70% alcohol at 4 °C overnight. The fixed cells were then treated with 0.25% Triton X-100 for 5 min in an ice bath and stained in propidium iodide (PI) solution (50 μg/mL, Sigma; USA) which contained 0.1 mg/mL RNase for 1 h in a dark room at 37 °C. Cell cycle analysis used by FACScan flow cytometer (BD Biosciences, Bedford, MA).
Mouse tumorigenicity assay
The suspension of 1.2 × 106 cells (4T1 cells) was prepared in 20 µL of Matrigel (0.34 mg/mL, BD Biosciences, San Jose, CA, USA). Six BALB/c female mice were aged 4–6 weeks (were purchased from Pasteur Institute of Iran and maintained in a clean area). Animals were allowed to acclimate for two weeks prior to experimentation. All mice were injected with the 1.2 × 106 cells subcutaneously, with one injection on the flank of each animal. Once tumors got palpable (about 4 days post-injection), tumor volumes were calculated using the formula: (L × W2)/2 which L and W indicated length and width, respectively. The length and width were measured with a caliper 2,4,5 and 7 days after intratumor metabolite injection30. To find the proper dose of SM intra-tumor injection, we considered the 100 µg/mL dose of in vitro injection as 100 mg/kg32,33. Because the minimum weight of our mice was 17.5 g, we injected 1.75 mg of SM intratumorally in each mouse in the treated group. We select the minimum dose to avoid the death of mice. The SM was dissolved in DMSO (total volume 70 µL), and then an intra-tumor injection was done. Three tumors were injected with only DMSO (70 µL) as the control. Mice were sacrificed in a humane manner when the tumor size exceeds 25 mm in diameter in either direction. This study was carried out in accordance with the recommendations of the animal care committee of the Chancellor for Royan Institute. The protocol was approved by the animal care committee of Royan Institute (Tehran, Iran, approval number 931119) and was performed in accordance with the ethical standards. All authors complied with the ARRIVE guidelines. Human data are not involved in this study.
High-performance liquid chromatography
The chromatography experiments were performed by Knauer HPLC pump model S 1000 and controller, autosampler model S 3900, and photodiode array detector model S 2800. The Eurospher C18 column 250 × 4.6 mm with precolumn, 100 A°- 5µm, was used. The Bacterial SM was analyzed by gradient method using water/methanol as a mobile phase with the following gradient program: 0 min- 90% water, 5 min- 57% water, 11 min- 30% water, 16 min- 0% water, 21 min- 0% water, 26 min- 90 water. The flow rate was 1 mL/min, and the injection volume was 100 μL.
Mass spectrometry
The ESI–MS/MS system, ThermoFisher Scientific (Bremen, Germany) ion trap mass spectrometer (model LCQ, mass range m/z 10–2000), was used to identify fraction number 6. The Xcalibur software was used to conduct instrument control, data acquisition, and processing. Typical positive ESI–MS conditions were: capillary voltage + 46 kV; spray voltage + 5 kV; tube lens: − 60 kV and capillary temperature: 300 °C.
Fourier transform infrared spectroscopy (FT-IR)
To identify the functional groups of extracted compounds, IR spectra were recorded at 5 cm−1 resolutions with 60 scans using Bruker Tensor 27 spectrometer (USA).
Statistical analysis
The one-way ANOVA test was used to determine the statistical significance of the differences between the treated and the control groups. All of the experiments were performed in triplicates or more, and the data obtained were expressed as means ± SD. p < 0.05 were considered statistically significant.
Data availability
All data generated or analysed during this study are included in this published article.
References
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Acknowledgements
We gratefully thank Mr. Mostafa Shahnani for his help in HPLC analysis and Seyedehsaba Nateghi for language editing. Atefeh Safarpour has received research support from the Iran National Science Foundation (INSF Grant Number 97011205) for the purification of phenol amine molecule and its anticancer activity.Effective molecule purification part of this study presented at 12th international conference on halophilic microorganisms and can be accessed at http://studia.ubbcluj.ro/download/pdf/1230.pdf.
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All authors contributed to the study's conception and design. M.A. and A.S. performed the microbiological part. M.E. and A.S. performed the cancer part. A.S. performed the experiments and A.S, M.E., and S.A.S.F. analyzed and interpreted the data. M.E. and A.S. discussed the paper and A.S. drafted the manuscript. All authors critically revised the manuscript. All authors read and approved the final manuscript.
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Safarpour, A., Ebrahimi, M., Fazeli, S.A.S. et al. A phenol amine molecule from Salinivenus iranica acts as the inhibitor of cancer stem cells in breast cancer cell lines. Sci Rep 13, 12669 (2023). https://doi.org/10.1038/s41598-023-39736-9
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DOI: https://doi.org/10.1038/s41598-023-39736-9
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