Fresh Water Cyanobacteria Geitlerinema sp. CCC728 and Arthrospira sp. CCC729 as an Anticancer Drug Resource

An increasing number of cancer patients worldwide, especially in third world countries, have raised concern to explore natural drug resources, such as the less explored fresh water filamentous cyanobacteria. Six strains of cyanobacteria (Phormidium sp. CCC727, Geitlerinema sp. CCC728, Arthrospira sp. CCC729, Phormidium sp. CCC731, Phormidium sp. CCC730, and Leptolyngbya sp. CCC732) were isolated (paddy fields and ponds in the Banaras Hindu University, campus) and five strains screened for anticancer potential using human colon adenocarcinoma (HT29) and human kidney adenocarcinoma (A498) cancer cell lines. Geitlerinema sp. CCC728 and Arthrospira sp. CCC729 were the most potent as determined by examination of morphological features and by inhibition of growth by graded concentrations of crude extracts and thin-layer chromatography (TLC) eluates. Cell cycle analysis and multiplex assays using cancer biomarkers also confirmed Geitlerinema sp. CCC728 and Arthrospira sp. CCC729 as cancer drug resources. Apoptotic studies in the cells of A498 (cancer) and MCF-10A (normal human epithelial) exposed to crude extracts and TLC fractions revealed no significant impact on MCF-10A cells emphasizing its importance in the development of anticancer drug. Identification of biomolecules from these extracts are in progress.


Introduction
More than 60% of the world's total cancer cases (14 million new cases per year) occur in Africa, Asia, and Central and South America, and these regions account for~70% of cancer deaths in the world (13 million per year) [1]. A number of chemotherapeutic agents (60% of the approved drugs) for cancer are sourced from natural compounds [2]. da Rocha et al. have reviewed the importance of natural drug resources, including microbes [3]. Cyanobacteria, the photosynthetic oxygen-evolving prokaryotes that originated~2.8 billion years ago [4], faced many stresses during evolution and thus, seem to have been endowed with the ability to synthesize a huge diversity of antimicrobial, anticancer, and anti-inflammatory agents [5][6][7][8][9][10][11]. Recently, green carbon nanotags (G-Tags) from harmful cyanobacteria have been synthesized for use in cancer therapy because of their high solubility, excellent photostability, low cytotoxicity, and ability to induce death in multiple cancer cell lines, including human hepatocellular liver carcinoma (Hep-G2) and human breast adenocarcinoma (MCF-7) [12]. Due to increase in the number of cancer patients and limitations of available drugs, problems with drug safety, narrow spectrum of activity and effectiveness, the development of newer broad-spectrum anticancer molecules from the less explored freshwater cyanobacteria is desirable.
Some earlier studies have shown that filamentous marine cyanobacteria are important sources of biomolecules for preventing cancer proliferation, neurodegenerative disorders and infectious diseases [8]. Noticeably, marine cyanobacteria produce a wide range of compounds with pro-apoptotic properties [13]. Cell shrinkage, membrane budding, and apoptosis were observed in human promyelocytic leukemia (HL-60) cells exposed to the aqueous extracts of unicellular marine strains of Synechocystis and Synechococcus [14]. Therefore we intend to screen fresh water cyanobacteria for anticancer properties on selected cell lines.
In the present communication, we have screened five freshwater, non-heterocystous, filamentous cyanobacterial strains (Phormidium sp. CCC727, Geitlerinema sp. CCC728, Arthrospira sp. CCC729, Phormidium sp. CCC731 and Leptolyngbya sp. CCC732) for their anticancer potential by using human colon adenocarcinoma (HT29) and human kidney adenocarcinoma (A498) cancer cell lines, along with normal rat-kidney cells (NRK52E) as a control. We have used the Bio-Plex Pro human cancer biomarker panel, cell cycle analysis, and a calcein-based cell viability assay for this purpose.

Isolation and culture of cyanobacterial strains
Cyanobacterial strains were isolated from local freshwater habitats, such as paddy fields and ponds, at the Banaras Hindu University, Varanasi, India. Samples were washed multiple times with sterile water and cultured in BG11 medium [15]. Unialgal population of strains were procured by picking up clonal population from algal medium agar plate obtained by serially diluting the source inocula. The purity of culture was routinely checked by streaking such culture on nutrient agar plates containing 0.5% of the glucose (w/v). These should be incubated and observation made after 24h. If there is a bacterial growth, they will appear, the incubation of plates for more than 6 days, may have fungal contaminants [16]. Cyanobacteria were identified based on the morphological features described by Desikachary [17] as well as 16S rRNA amplification [18] and strains were deposited in Centre for conservation and Utilization of blue green algae, Indian Agriculture Research Institute, New Delhi, India. Strain no. given as Phormidium sp. CCC727; Geitlerinema sp. CCC728; Arthrospira sp. CCC729; Phormidium sp. CCC731; and Leptolyngbya sp. CCC732. Culture were plated on agar plate (2%) and individual cultures were grown in Erlenmeyer flasks (1 L) at 28 ± 2°C with a light intensity of 14.40 Wm -2 provided by a cool white fluorescent tungsten light and a light/dark cycle of 18/6 h. The culture media and glassware were sterilized at 1.0546 kg cm -2 (15 lb) at 121°C for 15 min. All manipulations were done aseptically under a laminar flow hood (INSTECH, New Delhi, India).
DNA isolation and PCR amplification of 16S rRNA genes DNA from cyanobacteria was isolated using the method designed by Sambrook and Russell [19]. Cyanobacterial cultures were centrifuged at 6,800 g for 10 min, and the pellet was broken in liquid nitrogen. The pellet was suspended and vortexed in 1 mL TE buffer (pH 8.0, 10 mM Tris HCl, 1 mM EDTA) for 15 seconds. Thereafter, 30 μL sodium dodecyl sulfate (SDS, 10% w/ v) was added, followed by 5 μL proteinase-K (100 μgÁmL -1 ), mixed gently, and incubated at 37°C for 2 h. Subsequently, 100 μL NaCl (5 M) was added, vortexed for 15 seconds, and incubated at 65°C after adding 80 μL cetryltrimethyl ammonium bromide (CTAB, 10% w/v). The lysate was extracted with a chloroform: isoamyl alcohol mixture (24:1), and the aqueous phase was collected after centrifugation (6,800 g for 10 min). This was followed by extraction with a Tris-saturated phenol, chloroform, and isoamyl alcohol mixture (25:24:1). The aqueous phase obtained was added with 2 μL RNAse (~30 μgÁmL -1 ) and incubated at 37°C for 30 min. An equal volume of isopropanol was added to precipitate the DNA, followed by centrifugation (6,800 g for 10 min). The DNA pellet was washed twice with chilled ethanol (70%), resuspended in Milli-Q water (30 μL), and stored at 4°C. Genomic DNA was quantified with a NanoDrop spectrophotometer (NanoVue Plus, GE Health Care, Uppsala, Sweden).
The 16S rRNA genes of the cyanobacterial DNA were polymerase chain reaction (PCR)amplified using the cyanobacterium specific primer set: CYA106 F-5 0 CGG ACG GGT GAG TAA CGC GTG A 3 0 and 781R (a)-5 0 GAC TAC TGG GGT ATC TAA TCC CAT T 3 0 [18]. PCR was performed in a 25 μL final volume of reaction mixture containing 100 ng/ μL DNA, 2.5 μL of 10× PCR buffer with 15 mM MgCl 2 , 0.5 μL of 2.5 pmol dNTPs, 0.75 μL of 10 pmol of each primer, and 0.05 U Taq DNA Polymerase (Bangalore Genei, Bangalore, India) in a Thermal Cycler (Eppendorf, Germany). The thermal cycling profile was as follows: 3 min initial denaturation at 94°C, followed by 35 amplification cycles each consisting of 1 min denaturation at 94°C, 1 min annealing at 59.5°C, and 2 min elongation at 72°C, with a final 7 min elongation at 72°C. The PCR product was sequenced using an ABI 3130 Genetic Analyzer, Foster City, USA.

Phylogenetic analysis
Phylogenetic tree of amplified sequences of 16S rRNA genes from target cyanobacterial strains was constructed using MEGA5 with neighbor joining algorithm.

Preparation of cyanobacterial crude extracts
Extraction was performed adopting 40-45 d old batch cultures according to the method reported by Doan et al. [20]. The harvested biomass of each cyanobacterial species was lyophilized (Christ Alpha 1-2, Germany), and 1 g dry weight was extracted twice with 60 mL followed by 40 mL methanol (100%). The extract was concentrated in a rotary vacuum evaporator (Perfit, Ambala, India) at 40°C, and dried residues were dissolved in 3 mL of dimethyl sulfoxide (DMSO) for storage at 4°C until further use.
bands on the plates were designated as A, B, C, D, and E and were dissolved in methanol (1 mL). In the second step, each eluate was subjected to TLC purification using hexane: ethyl acetate (1:1). Only the potent designated bands of the first step were subjected to the second step. Ultimately, the bands separated in the second TLC step were monitored for anticancer potential against HT29 and A498 cancer call lines. All experiments were performed in triplicate.

Screening for anticancer activity
Cells were seeded in 96-well plates at 3 × 10 4 cellsÁmL -1 and 2 × 10 5 cellsÁmL -1 in 24-well plates. The cells were allowed to adhere for 48 h under optimum culture conditions. The cells were then treated for 72 h with 200 μgÁmL -1 , 50 μgÁmL -1 , or 12.5 μgÁmL -1 crude extracts of Phormidium sp. CCC727, Geitlerinema sp. CCC728, Arthrospira sp. CCC729, Phormidium sp. CCC731, Phormidium sp. CCC730, and Leptolyngbya sp. CCC732, containing 1, 0.5, 0.25 and 0.0625% DMSO respectively which act as negative controls. After 72 h, the medium from each well of the 96-well plates was removed, and the wells were washed with 1× PBS (pH 7.4). Calcein (2 μM, 200 μL) was added to each well, and the plates were incubated in the dark at 37°C for 30 min. Calcein is cleaved by intracellular esterase in viable cells to generate a green fluorescent protein under UV light. Fluorescent images of the cells stained with Calcein were obtained using a fluorescent microscope (Leica DM IL Wetzlar, Germany) and the fluorescence was quantified using a fluorometer (FLUOstar Omega BMG Labtech Mornington,Victoria, Australia). Phase contrast images were obtained at different magnifications using a phase contrast microscope (NIKON Eclipse Ti-S, Nikon Instruction Inc., Chicago, Illinois, USA).

Flow cytometry analysis
Cell cycle analysis was performed by flow cytometry using Propidium iodide (PI) staining. Treated cells were trypsinized and resuspended in FBS-supplemented DMEM/F-12 medium. Following centrifugation at 300 g for 10 min, the cell pellet was washed with 1× PBS and further resuspended and fixed in 50% ethanol. The suspension was stored overnight in the dark at 4°C. The fixed cells were harvested by centrifugation at 800 g for 10 min and resuspended in staining buffer (0.1% Triton X-100, 0.2 mgÁmL -1 RNase A, 20 μgÁmL -1 PI) prepared in Milli-Q water. The resuspended cells were incubated at 37°C for 45 min. The cells were then analyzed for their DNA content in an Influx C7 sorter (BD Biosciences, Franklin lakes, New Jersey, United States). Cells were gated and analyzed for doublet discrimination. A population of single cells was acquired at excitation (490 nm) and emission (630 nm) wavelengths. Data analysis was performed using BD FACS Software (BD Biosciences) to identify the percentage of cells in different phases of the cell cycle.
Apoptosis analysis in MCF-10A and A498 Cells were done by apoptosis detection kit (BD Biosciences, San Jose, CA, USA) according to the manufacturer's protocol. Cells (5x10 4 cellsÁmL -1 ) were plated on 24-well culture plate up to 24 h. These cells were exposed to C4, C5, D3 and D4 TLC fractions (12.5 μgÁmL -1 ) for 72 h. These cells were harvested, washed with PBS, resuspended in 100 μL of binding buffer containing 5μL of Annexin V and Propidium Iodide (PI) and incubated for 10 min at room temperature in the dark. Subsequent to the incubation, samples were diluted by adding 400 μL of binding buffer and analyzed using BD FACS Canto II flow cytometer equipped with FACS Diva software, version 6.1.2 (BD Biosciences, San Jose, CA, USA). The results were expressed as Annexin V-FITC+ and PI-cells identified as apoptotic cells, Annexin V-FITC+ and PI+ cells as late apoptotic cells, Annexin V-FITC-and PI+ cells as necrotic cells and Annexin V-FITC-and PI-as healthy cells.

Multiplex analysis for cancer biomarkers
Frozen supernatants of the control and treated samples were centrifuged at !12000 g for 10 min at 4°C. The Bio-Plex Pro Human Cancer Biomarker Panel 1 Assay Kit (Bio-Rad Laboratories, Hercules, CA) was used for quantification of cancer biomarkers using Bio-Plex MAGPIX Multiplex Reader (Bio-Rad Laboratories). The cancer biomarker panel quantifies the expression of 16 proteins known to have a role in progression of different human cancers using a bead-based suspension phase assay. Supernatants obtained from the samples were incubated with antibody-coated beads and then washed and incubated with biotinylated detection antibody. The beads were further washed and incubated with streptavidin-phycoerythrin (PE) conjugate. Biomarkers were quantified using PE fluorescence intensity on the MAGPIX system. The results were expressed as mean fluorescence intensity (MFI) or as pgÁmL -1 of protein.

Statistical analysis
To find out the significant differences in anticancer activity of crude extracts and TLC fractions, one way analysis of variance (F test) followed by Post Hoc (Student Newman Keuls) test was used to find out paiwaise significant differences between the mean values. Student t-test was used to find out the significant mean difference for variables between cancer marker proteins and crude extracts of target cyanobacteria. All statistical analysis has been performed with SPSS 16.0 trial version.

Phylogeny of PCR amplified 16S rRNA of target cyanobacterial strains
The 16S rRNA genes of Phormidium sp. CCC727, Geitlerinema sp. CCC728, Arthrospira sp. CCC729, Phormidium sp. CCC730, Phormidium sp. CCC731 and Leptolyngbya sp. CCC732 were amplified. These amplified sequences were further compared with the reported organisms available in NCBI database, and were found to be closely related as represented in S1 Table, showing very close identity and query coverage area with the similar genera with the different accession number, confirmed our findings. Phylogenetic relationship clearly demonstrated that Arthrospira sp. CCC729, Phormidium sp. CCC730 and Phormidium sp. CCC731 in the different cluster, while Phormidium sp. CCC727, Geitlerinema sp. CCC728, Leptolyngbya sp. CCC732 clustered together (Fig 1). Therefore we have selected only one Phormidium sp. CCC731 from one cluster and another Phormidium sp. CCC727 from different cluster (Fig 1.). Based on this preliminary screening for anticancer activity, we selected Geitlerinema sp. CCC728 and Arthrospira sp. CCC729 for further screening. The crude extracts were purified by a two-step TLC as described. The designated bands (A, B, C, D, E, and F) from the first TLC (Fig 2A and 2C) purification of cyanobacterial crude extracts were screened against A498 cells (S12-S14 Figs). Fraction C of Geitlerinema sp. CCC728 (Rf = 0.44) and fraction D of Arthrospira sp. CCC729 (Rf = 0.42) were selected for further purification by a second TLC step (Fig 2B  and 2D).

Anticancer activity of crude extracts and TLC fractions
The presence of more than one UV-illuminated band indicated a mixture of compounds. The bands separated in the second step, C2, C3, C4, and C5 from Geitlerinema sp. CCC728 ( Fig 2B) and D1, D2, D3, and D4 from Arthrospira sp. CCC729 (Fig 2D), were examined further for anticancer potential by using the calcein fluorescence assay. The quantitative measurement of the anticancer activity of the bands from Geitlerinema sp. CCC728 (C) and Arthrospira sp. CCC729 (D) at a low concentration (12.5 μgÁmL -1 ) was compared with that of the cyanobacterial crude extracts (100 μgÁmL -1 ). It is interesting to note that the crude extracts of Geitlerinema sp. CCC728 and Arthrospira sp. CCC729 showed 53% and 27.78% reduction in fluorescence measurements (Fig 3A), respectively. However, the C4 and C5 bands of Geitlerinema CCC728 resulted only in 19.95% and 23.07% reduction, respectively, while the C2 and C3 bands did not alter the fluorescence intensity of cancer cells compared with the control (Fig  3B). Similarly, the potent bands from Arthrospira sp. CCC729 (D3 and D4) at 12.5 μgÁmL -1 showed only 12.77% and 14.87% reduction in fluorescence intensity, while the D1 and D2 eluates reduced the fluorescence intensity only marginally (average 3.19%; Fig 3C). Statistical analysis of Calcein fluorescence assay for A498 cell lines indicated that Mean Fluorescence Intensity (MFI) varied significantly due to crude extracts of Geitlerinema sp. CCC728 and Arthrospira sp. CCC729 (F 2,6 = 187.896, p < 0.001), TLC fractions of Geitlerinema sp. CCC728 Post hoc SNK test revealed significant differences in MFI at p < 0.001 for crude extracts of Geitlerinema sp. CCC728 and Arthrospira sp. CCC729 (Fig 3A), TLC fractions of Geitlerinema sp. CCC728 (Fig 3B) and TLC fractions of Arthrospira sp. CCC729 (Fig 3C).
To confirm that these extracts have activity only in cancer cell lines, we used a normal rat kidney epithelial cell (NRK52E) and a non-tumorigenic epithelial cell line of human breast (MCF-10A). Fig 4A and 4B show the impact of the crude extract and TLC-purified fractions (C2, C3, C4 and C5) of Geitlerinema sp. and Arthrospira sp. on NRK52E cells. Both crude extracts and the TLC fractions did not show any significant activity against NRK52E cells. Lack of activity in NRK52E cells clearly indicated that these cyanobacterial strain could act as a resource of anticancer biomolecule (s) that do not significantly affect normal kidney cells. Statistical analysis of NRK52E cell lines measured by Calcein fluorescence assay indicated that Mean Fluorescence Intensity (MFI) varied significantly due to crude extract with TLC fractions of Geitlerinema sp. CCC728 (F 5,18 = 174, p<0.001) and crude extract with TLC fractions of Arthrospira sp. CCC729 (F 5,18 = 3.09, p< 0.001) (Fig 4A and 4B). Mean fluorescence intensity of crude and TLC fractions C2, C4 and C5 of Geitlerinema sp. CCC728 was 11.05% lower to that of control. C3 fraction showed 19.94% reduction in mean fluorescence intensity. Mean fluorescence intensity of crude from Arthrospira sp. CCC729 showed 21.49% reduction over control. Interestingly, TLC fractions D1, D2, D3 and D4 of Arthrospira sp. CCC729 showed increase in the mean fluorescence intensity of NRK52E cells by 19.52%. This indicated that TLC fractions of Arthrospira sp. CCC729 supported growth of NRK52E cells in contrast to former where C2, C3, C4 and C5 reduced mean fluorescence intensity, although at low level.
for PI fluorescence intensity to quantify the amount of DNA per cell. Significant changes in the cell cycle profile were observed in all cases. For the C4 and C5 fractions of Geitlerinema sp. CCC728, significant cell cycle arrest was seen in the S and G2/M phases, suggesting inhibition of cell cycle progression and growth. Similar results were seen with the D3 extract of Arthrospira sp. CCC729. However, with the D4 extract of Arthrospira sp. CCC729, cells were arrested in the S phase of the cell cycle. Overall, the crude extracts showed significant levels of cancer cell inhibitory activity dependent on the perturbation of cell cycle checkpoints (Fig 6).
A498 as well as MCF-10A cells were exposed to TLC fractions C4 and C5 (Geitlerinema sp. CCC728), D3 and D4 (Arthrospira sp. CCC729). The apoptotic analysis of these cells were done using annexin assay kit and data is represented in S15 and S16 Figs respectively. Statistical analysis of A498 cell lines under treatment showed significant impact on cancer cells (F 4, 10 = 106.582, p<0.001) (Fig 7A). As far as MCF-10A cells were concerned they were not significantly affected by fractions selected in experiment (F 4, 10 = 2.588, p> 0.05) (Fig 7B). Thus, population of A498 cells clearly undergone increased in apoptosis with exposure to C4, C5, D3 and D4 fractions in comparison to MCF-10A cells.

Assessment of cancer biomarkers
To ascertain the anticancer potentials of Geitlerinema sp. CCC728 and Arthrospira sp. CCC729, a multiplex assay was also applied for cancer protein biomarkers. This assay was based on monitoring the levels of established cancer biomarkers in A498 cancer cells after treatment with crude extracts at 100 μgÁmL -1 . The crude extract of Arthrospira sp. CCC729 showed reduction in expression in the cells for ten cancer marker proteins: soluble human epidermal growth factor receptor 2 (sHER-2/neu), follistatin, granulocyte colony stimulating Fresh Water Cyanobacteria as Anticancer Drug Resource factor (G-CSF), prolactin, soluble epidermal growth factor receptor (sEGFR), soluble Tie2 receptor (sTIE-2), soluble vascular endothelial growth factor receptor 1 (sVEGFR-1), and platelet derived growth factor, a dimeric glycoprotein composed of two A (-AA) or two B (-BB) chains (PDGF-AB/BB; Fig 8A), as well as osteopontin ( Fig 8B) and hepatocyte growth factor (HGF; Fig 8C). Of the 16 cancer marker proteins used in the multiplex assay, six proteins, basic fibroblast growth factor (FGF-basic), leptin, platelet endothelial cell adhesion molecule (PECAM-1), sVEGFR-2, soluble interleukin-6 receptor alpha (sIL-6Rα), and stem cell factor (SCF) (Fig 9), did not show reduction in expression after treatment with Arthrospira sp. CCC729. Multiplex analysis in the case of Arthrospira sp. CCC729, the "t" test indicated that the expression of crude varied significantly with their respective controls at p< 0.05 (Figs 8A, 8B, 8C and 9), except for PECAM-1 and sIL-6Rα, expression were not statistically significant (p > 0.05) (Fig 9).

Discussion
Phylogenetic relationship based on 16S rRNA among five different Oscillatorialean members collected from local fresh waters showed Arthrospira sp. CCC729 and Geitlerinema sp. CCC728 Fresh Water Cyanobacteria as Anticancer Drug Resource different clusters (Fig 1), Geitlerinema sp. CCC728 is in close association with Leptolyngbya sp. CCC732, and Phormidium sp. CCC727. Similar species of cyanobacteria were clustered with Limnothrix / Geitlerinema-like cyanobacterium, together in a phylogenetic study based on 16S rRNA [21]. They have also shown that Geitlerinema sp. AC0243 extract was toxic but unlike that of other known cyanotoxins owing probably intragenomic variations as well as 16S rRNA  Fresh Water Cyanobacteria as Anticancer Drug Resource heterogeneity in the filamentous cyanobacterium as evident in Leptolyngbya sp. [22] Arthrospira / Spirulina on the other hand a healthfood and known to possess antioxidative property, rich source of carotenoids, polyunsaturated fatty acid [23; 24]. Therefore, response of crude extracts and TLC fractions of these two cyanobacteria differed towards cancer cell lines and this difference was also reflected in sensitivity towards NRK52E cells. To date, marine filamentous cyanobacteria [13], with the exception of unicellular strains such as Synechocystis sp. and Synechococcus sp. [14], have been screened for their promising anticancer properties and active biomolecules, but the specific targets and mechanisms behind their action are not well understood. Phromidium sp. has been earlier shown to have anticancer activity using HT29 and HeLa cells [25]. Oscillatoria sp. and Leptolyngbya sp. were identified as sources of largamide A-H [26] and coibamide A [27], respectively. These compounds could induce apoptosis in A549 lung carcinoma, HT29 colon carcinoma cells and rat aorta 10 cells [28][29]. Geitlerinema sp., which is the source for ankaraholide A, shows anticancer activity against NCI-H460 lung tumor, MDA-MB-435 breast carcinoma, KB oral epidermoid and Lo Vo colon cancer cells [30]. In addition, crude extracts of selected cyanobacteria showed concentration-dependent and species-specific inhibition of growth of A498 and HT29 cancer cells. Further, the cyanobacterial crude extracts caused shrinkage in cancer cells as well as dispersion of aggregated HT29 cells but not A498 cells, indicating their response when compared with cells with DMSO only (see S1-S11 Figs). Thus, our results are in accordance with earlier studies in which cancer cells treated with anticancer agents showed typical morphological markers of apoptosis such as shrinkage and surface budding [31]. In addition to the use of morphological markers in screening for apoptotic cells, some other cellular and molecular alterations/ biomarkers associated with the death of cancer cells can also be monitored. The crude extracts of the tested cyanobacteria are mixtures of various native biomolecules; therefore, the probable anticancer biomolecules must be separated and identified for their structural identities. Based on our observations against selected cancer lines, Geitlerinema sp. CCC728 and Arthrospira sp. CCC729 proved to be potent anticancer drug sources. We adopted 12.5 μgÁmL -1 as the concentration of the potent band eluates, compared with 100 μgÁmL -1 of the crude extracts, in anticipation of increased effectiveness after separation from the crude materials. The purified fractions also had anticancer potential, although with lower impact (Fig 3A, 3B and 3C). Fresh Water Cyanobacteria as Anticancer Drug Resource Similar results were reported by Chu et al, while investigating the protective effect of aqueous extract from Spirulina platensis against cell death induced by free radicals and concluded that a mixture of compounds was more active than a single pure one [24]. The negligible impact on NRK52E and MCF-10A cells by purified TLC fractions emphasized the significance of such natural resources to be explored for biomolecules with anticancer activity (Figs 4 and 5). This difference in activity may be ascribed to be species specific as described earlier. Impact of crude extracts in both the cases may be attributed to presence of other than bioactive compounds.
Cell cycle analysis provided critical insights into the mechanisms of action of these extracts. Some extracts inhibited the cell cycle in the S and G2/M phases, while others inhibited the cell cycle at the G1 phase which can be one of the mechanisms for genomic instability seen in cancer cells (Fig 6). Similarly, in addition to the antiproliferative effect of Spirulina extract on hepatic stellate cell (HSC), the flow cytometric analysis on cell growth and cell cycle arrest revealed that aqueous extract of Spirulina could inhibit cell proliferation by inducing G2/M arrest in HSCs through regulating the G2 check point [24]. Likewise our data on cell cycle analysis indicated that Geitlerinema sp. CCC728 and Arthrospira sp. possess the potential for amelioration of selected cancer cells. We have also validated anticancer potential by apoptotic study, where increase in the mean percentage population of A498 cells under apoptosis was recorded after exposure to TLC purified fractions from both the cyanobacteria (Fig 7A and S15  Fig). Interestingly, none of the fractions in the investigation could induce apoptosis in MCF-10A cells (Fig 7B and S16 Fig) suggesting these cyanobacteria can act as an ideal natural anticancer resource.
In vitro multiplex assays yield a composite profile of clinically relevant protein biomarkers. Therefore, multiplex assays identifying different cancer biomarker proteins also confirmed the anticancer potential of Geitlerinema sp. CCC728 and Arthrospira sp. CCC729 in A498 cancer cell lines. Biomarker's expression vary with the type of cancers. We have compiled the data in two groups, (a) group of biomarkers whose expressions were inhibited (downregulated) as Figs 8 and 10 for Arthrospira CCC729 and Geitlerinema CCC728. (b) Figs 9 and 11 are group of biomarkers whose expressions were upregulated (over expressed). Downregulation and upregulation of biomarkers might have resulted because of their interactions with certain biomolecules present in the crude extract. We observed an overall reduction in the concentration of many of these cancer related proteins following treatment of the cells with the extracts. The multiplex assays thereby verified the claim that Geitlerinema sp. CCC728 and Arthrospira sp. CCC729 are potent anticancer drug sources (Figs 8 and 10). However, some of the biomarkers showed increased expression following treatment (Figs 9 and 11). This observation indicated specificity in biomolecules interaction with protein biomarker expression. Further identification and characterization of the active biomolecules are in progress.

Conclusions
Cancer cell lines adopted (HT29 and A498) showed deformities, cell disaggregation in morphological features after exposure to crude as well as TLC purified fractions of Geitlerinema sp. CCC728 and Arthrospira sp. CCC729. On comparison with normal rat kidney (NRK52E) and normal human epithelial (MCF-10A) cells, the crude extracts and TLC fractions of these cyanobacteria indicated a possible source of anticancer molecules. Flow cytometric analysis also showed cell cycle arrest in S and G2/M phase, suggesting of antiproliferative nature of such crude extracts and TLC fractions. Apoptotic analysis of A498 and MCF-10A cells (normal human epithelial) after exposure to TLC fractions clearly demonstrated that these fractions induced apoptosis in A498 in contrast to MCF-10A cells. Bio-plex Pro human cancer biomarker assay indicated presence of anticancer biomolecules by observing the down/ up regulation of marker proteins. These screening processes are recommended prior to isolation and identification of biomolecules for anticancer properties in little explored fresh water filamentous cyanobacteria.  Table. A comparison of 16S r RNA amplified sequences from target cyanobacteria with homologous organism available in NCBI database. (TIF)