Cytotoxic Potential of Bioactive Compounds from Aspergillus flavus, an Endophytic Fungus Isolated from Cynodon dactylon, against Breast Cancer: Experimental and Computational Approach

Endophytic fungi are a diverse group of microorganisms that colonize the inter- or intracellular spaces of plants and exhibit mutual benefits. Their interactions with the host plant and other microbiomes are multidimensional and play a crucial role in the production of secondary metabolites. We screened bioactive compounds present in the extracts of Aspergillus flavus, an endophytic fungus isolated from the roots of the medicinal grass Cynodon dactylon, for its anticancer potential. An in vitro analysis of the Ethyl acetate extract from A. flavus showed significant cytostatic effects (IC50: 16.25 μg/mL) against breast cancer cells (MCF-7). A morphological analysis of the cells and a flow cytometry of the cells with annexin V/Propidium Iodide suggested that the extract induced apoptosis in the MCF-7 cells. The extract of A. flavus increased reactive oxygen species (ROS) generation and caused a loss of mitochondrial membrane potential in MCF-7 cells. To identify the metabolites that might be responsible for the anticancer effect, the extract was subjected to a gas chromatography-mass spectrometry (GC-MS) analysis. Interestingly, nine phytochemicals that induced cytotoxicity in the breast cancer cell line were found in the extract. The in silico molecular docking and molecular dynamics simulation studies revealed that two compounds, 2,4,7-trinitrofluorenone and 3α, 5 α-cyclo-ergosta-7,9(11), 22t-triene-6beta-ol exhibited significant binding affinities (−9.20, and −9.50 Kcal/mol, respectively) against Bcl-2, along with binding stability and intermolecular interactions of its ligand-Bcl-2 complexes. Overall, the study found that the endophytic A. flavus from C. dactylon contains plant-like bioactive compounds that have a promising effect in breast cancer.


Introduction
Cancer is one of the most devastating diseases worldwide, responsible for approximately 10 million deaths in 2020, or about one in every six deaths. It has been estimated Cynodon dactylon, often known as "Durva Grass", "Bermuda grass", "Dog's Tooth grass", "Bahama grass", "Devil's grass", "Couch grass", "Indian Doab", "Scutch grass", "Dhub", and "Arugampul", is a plant of immense religious significance that is reportedly used in the Ayurvedic, Siddha, Unani, Nepalese, and Chinese medical systems [25]. C. dactylon extract has been successfully tested in preclinical studies for its antitumor activity. For example, in vivo studies of C. dactylon root extract in diethyl nitrosamine (DEN) induced liver cancer in mice have shown its significant anticancer activity [26]. As we know that C. dactylon is home endophytic fungi that can be a source of unique substances, the present study is aimed at investigating the potential antitumor properties of the bioactive compounds from endophytic fungi in the in vitro breast cancer model.

Cell Lines and Culture Media
The MCF-7 cell line (human breast cancer epithelial cells) was obtained from the National Centre for Cell Science, Pune, India. For the culture maintenance and in vitro cytotoxicity experiment, MCF-7 cells were cultured in a culture flask or on plates (Falcon, Sigma-Aldrich, Bengaluru, India) in DMEM, supplemented with 20% heat inactivated FBS, 1% penicillin, streptomycin, and amphotericin B in stable conditions of 37 • C and 5% CO 2 in a humidified atmosphere. A passage no higher than 20 was used (P18 in most of the experiments). The cells were frequently tested against mycoplasma according to the laboratory protocol [27].

Collection of Plant and Isolation of Endophytic Fungus
Nourishing free growth C. dactylon plants were gathered from Sundarapandiam village, Virudhunagar Dist., Tamil Nadu, India (latitude 9.59721 • N, longitude 77.67405 • E). The location is characterized by a high level of vegetation development and a large variety of plants, including several species of grass. Immediately after collecting the grass, the samples were transported to the laboratory and carefully cleansed with distilled water. On the collection day, fungal endophytes were isolated as described by Tapfuma et al. [28]. The C. dactylon plant root was chopped into tiny (1 cm) pieces under sterile conditions. These were washed using running tap water for 2-5 min to remove dirt particles and undesired debris, followed by rinsing with deionized water. The chopped plant roots were then sterilized by soaking in 70% ethanol for 1 min, followed by 1% sodium hypochlorite for 6 min. The root sample was then cleaned again for 1 min in 70% ethanol before being rinsed with sterile deionized water. The sterilized root sample was coarsely crushed and serially diluted in sterile water using a sterile mortar and pestle. Dilutions ranging from 10 −2 to 10 −6 were plated on potato dextrose agar (PDA, pH = 5.6) and incubated at 27 • C for 4-7 days. The plates were examined after 48 h for the formation of fungal colonies. The morphology, texture, and color of the colonies were recorded. Lactophenol cotton blue (LCB) wet mount was used to observe the microscopic morphology of the fungi.

Molecular Identification of Endophytic Fungi
The endophytic fungus isolated from C. dactylon was identified using molecular gene sequencing according to the methods used by Sette et al. 2006 [29]. The 200 mg of fungal mycelial mat were mashed with a pestle and mortar in 500 µL of extraction buffer (200-mM Tris-HCl (pH = 8.0), 25-mM EDTA (pH = 8.0), 250-M NaCl, 10% CTAB) according to the Cetyltrimethyl ammonium bromide (CTAB)-phenol-chloroform-isoamyl alcohol technique (CTABPCI). The mashed fungal mycelia was then transferred to a new tube, where 3 µL proteinase K and 3 µL RNase were added, vortexed, and incubated at 37 • C for 1 h. After incubation, the tubes were placed in a 65 • C water bath for 10 min. After adding one volume of phenol, chloroform, and isoamyl alcohol (25:24:1), the solution was well mixed for 5 min before being centrifuged at 12,000 rpm for 5 min. The clear aqueous phase was collected and combined with one volume of chloroform: isoamyl alcohol (24:1) mixture before centrifugation at 12,000 rpm for 5 min to recover the aqueous phase. One volume of ice-cold isopropanol was added and the mixture was held overnight at −20 • C for DNA precipitation. The DNA was precipitated with 100% ethanol after being centrifuged at 10,000 rpm for 5 min and was then washed twice with 1 mL of 70% ethanol before being resuspended in 200 µL of deionized water or 1× TE (200 mM Tris-HCl (pH = 8.0), 20 mM EDTA (pH = 8.0)) buffer. A portion of the eluted fungal DNA was electrophoresed on a 0.8% agarose-EtBr gel, and the concentration was calculated using Qubit 3.0.
PCR with universal primers recognizing the internal transcribed spacer (ITS) region of the fungal DNA, ITS 5 (TCCTCCGCTTATTGATATGC) forward and ITS 4 (GGAAG-TAAAAGTCGTAACAAGG) reverse, was used to identify the species of isolated fungi. Amplified DNA fragments were validated and purified with a GeneJET PCR purification kit (Thermo Scientific, EU-Lithuania, Vilnius, Lithuania) to exclude primer dimer and other carryover contaminants. Using a 2% agarose gel and a 100-bp DNA ladder as a size reference, the product's quality was evaluated and determined to be acceptable for sequencing. The Big Dye ® Terminator 3.1 sequence kit was used to purify and prepare the PCR-amplified products for sequencing (Applied Biosystems, Foster City, CA, USA). According to the manufacturer's instructions, the denatured products were sequenced in both the forward and reverse directions using a Genetic Analyzer 3500 (Life Technologies Corporation, Applied Biosystems ® , Carlsbad, CA, USA). To validate the species, the sequences were aligned and modified using Mega software version 10. The annotated ITS rDNA contig was submitted to GenBank and assigned an entry number.

MTT Assay
The cytotoxic properties of the endophytic fungal extract were assessed using metabolic MTT assay in MCF-7 cells. Briefly, MCF-7 cells were seeded into 96-well microtiter plates and cultured at 37 • C with 5% CO 2 for 24 h to reach confluency. The cells were further treated with various concentrations of the endophytic fungal extract (100, 50, 25, 12.5, 6.25, 3.125 µg/mL). After 48 h, MTT assay was performed according to the standard procedure [30]. Untreated cells served as control. The absorbance was measured at 570 nm using a microplate reader (Bio-Rad, Hercules, CA, USA). The percentage of viability was calculated using the following formula: Cell viability (%)* = (A (mean absorbance of extract-treated cells) /A (control cells) ) × 100; *n = 3 where n is the number of independent experiments.

Detection of Cytotoxicity Using Dual Staining Assay
The MCF-7 cells were cultured in 24-well microtiter plates and treated with the IC 50 concentration of the endophytic fungal extract for 48 h. After 48 h of treatment, the cells were rinsed in ice-cold 1× PBS (phosphate buffered saline) and then stained with two fluorescent DNA binding stains [(10 µg/mL) (Acridine orange and Ethidium bromide)] [31]. After 30 min of incubation, the cells were observed for apoptosis under a fluorescent microscope (Labomed TCM 400 Inverted Binocular Microscope, USA, using Image aR Pro software) at 40× magnification. The untreated cells served as a control for the study. The percentage of the apoptotic cells was calculated using the following formula: (Total number of apoptotic cells/Total number of normal cells) × 100.

Apoptosis Analysis Using Flow Cytometry
MCF-7 cells were seeded on 24-well microtiter plates and cultivated overnight at 37 • C in a CO 2 incubator. The cells were then treated with the IC 50 concentration of the fungal extract for 48 h. Following incubation, the cells were washed in PBS and centrifuged for 5 min at 500× g in 4 • C. The supernatant was then removed, and the cell pellets combined to a concentration of 1 × 10 5 mL −1 in an ice-cold 1× binding buffer. Next, 1 µL of annexin V-fluorescein isothiocyanate reagent and 1 µL of propidium iodide (PI) were added to the tubes on ice. The tubes were then kept on ice and incubated in the dark for 15 min, and 400 µL of ice-cold 1× binding buffer were meticulously mixed in. Within 30 min, a flow cytometry analysis was performed (BD FACS calibur-Becton Dickinson, CytExpert v 1.2.11.0) [32].

Assessment of Mitochondrial Transmembrane Potential
The mitochondrial transmembrane potential was determined by using a lipophilic dye, Rhodamine-123 [33]. MCF-7 cells were seeded in the 24-well plate and maintained for 24 h in 5% CO 2 , 37 • C conditions to reach the exponential growth phase. Then, the cells were exposed to IC 50 of the fungal extract. After 48 h of incubation, the cells were stained with Rhodamine-123 dye for 30 min. Subsequently, they were washed with PBS and fixed with paraformaldehyde (4%) for 30 min. The morphological alterations and the permeability of the membrane were examined under the fluorescent microscope. The untreated cells served as a control.

Nuclear Integrity Measurement
MCF-7 cells were treated with the endophytic fungal extract for 48 h in a 24-well flat bottom microplate as described in the previous sections. Then, the cells were washed with PBS and fixed in paraformaldehyde (4%) for 30 min. After this, the cells were washed in Triton X100 (0.4%) for 20 min and washed in PBS. Next, the cells were stained with DAPI (0.5 µg mL −1 ) in the dark for 1 min and washed with PBS. A fluorescent microscope with an appropriate filter was used to capture images of the cells [30].

Determination of Reactive Oxygen Species (ROS)
The level of intracellular ROS was measured using 2 ,7 -dichlorofluorescein diacetate. The MCF-7 cells were cultured for 24 and 48 h after being exposed to 10% FBS and the IC 50 concentration of the endophytic fungal extract. The cells were then washed twice with PBS before being tagged with 10 M H 2 DCF-DA according to the manufacturer's protocol [32]. The fluorescence intensity was measured using a fluorescence spectrophotometer (Spectra-maxM2 fluorescence spectrophotometer, Molecular devices, San Jose, CA, USA) at 475 nm (λ ex ) and 525 nm (λ em ).

Gas Chromatography-Mass Spectrum (GC-MS) Analysis
We used sonication to lyse and homogenize fungal mycelia for the extraction of secondary compounds [34]. Around 500 mg of fungi (pure mycelial culture) were taken and dispersed in 10 mL of an 80% ethyl acetate solution. The contents were subjected for sonication in the ultrasonic bath sonicator (Elma Ultrasonic Cleaner S100H, Mumbai, India) at a 80 W cm 2 intensity for 0.5 pulse cycles at a temperature of 40 • C. After the process of sonication, the contents were filtered using a Whatman No. 1 paper filter to eliminate the mycelia, and the remaining filter was centrifuged at 2500 rpm. The liquid containing the secondary metabolic compounds of the endophytic fungi was determined by GC-MS analysis. A Shimadzu Make QP-2010 on a non-polar 60 M RTX 5MS column was used for the GC-MS analysis, with helium as the carrier gas, containing 15 psi as constant pressure.

In Silico Molecular Docking
The GC-MS spectrum provided a list of biologically active phytochemicals contained in the isolated endophytic fungal metabolic extract. The compounds were utilized for molecular docking studies against the overexpressed anti-apoptotic protein receptor (Bcl-2, PDB id: 6O0K, Resolution: 1.62 Å) of breast cancer. The three-dimensional molecular structure of compounds (ligands) from the endophytic fungal extract was created using Chemsketch software. The Chemistry at Harvard Molecular Mechanics (CHARMm) force field was used to optimize the ligands and minimize energy. The generated ligand structures were converted into the ".pdb" file format using BIOVIA|Discovery Studio Visualizer v20.1.0.19295 software (Accelrys Software Inc., San Diego, CA, USA). The target protein model was retrieved from the RCSB's protein data repository [35].

Molecular Dynamics (MD) Simulation
MD simulation studies were performed to investigate the binding stability of the top scored compounds of the endophytic fungal extract with the anti-apoptotic protein receptor (Bcl-2) of breast cancer [36]. Using the Desmond dynamic package 2017 in Schrodinger (Academic version) in a Linux environment, the time-dependent change of the complexes was calculated over 200 ns [36]. The complex of the identified phytocompounds with the Bcl-2 receptor was created using the OPLS (optimal potentials for liquid simulations)-2005 force field [37]. Additionally, a water model was created using the established SPC water model at distances of 10 Å units from an orthorhombic periodic boundary [38]. Further, the electric charges were neutralized by adding the required number of counter ions, and, before the MD simulation process started, the system decreased its energies through heating and equilibrium processes. The Nose-Hoover approach with the NPT (isothermal-isobaric ensemble) was used to apply a 300 K temperature and one atmospheric pressure (1.01325 bar) throughout the system's final manufacturing stage, which lasted up to 200 ns [39,40]. The best confirmations were chosen with regard to the complex's interactions and dynamical characteristics.

Statistical Analysis
SPSS Statistics version 20.0 was used for all statistical analyses. A one-way ANOVA followed by Dunnett's multiple comparisons post hoc test was used, with the significance level set at p < 0.05 or lower. Representative results of at least three independent repeats are shown in each experiment [41].

Isolation of Fungi and Microscopic Examination
C. dactylon roots served as the source of the fungi. Four endophytic fungi were selected for the study based on the morphology of the colonies and the antioxidant potentials of their extracts. In potato dextrose agar, the fungi colony looks powdery and has an olive-green conidial appearance. Later, the chosen fungus was sub-cultured and purified for further analysis. Figure 1a depicts the colony morphology of the endophytic fungi, and Figure 1b illustrates the microscopic view of the mycelia and the fungal spores using the lactophenol cotton blue mounting (LCB) technique.

Phylogenetic Analysis
Through the systematic selection of isolates from the fungal culture, all of the colonies were categorized according to their morphological parameters, such as the shape and color of the colony, and their reverse media color. Each fungal colony was purified by transplanting sequential hyphal ends over 2-3 passes. One of the four isolates, CD02, showed higher antioxidant activity and was chosen for further investigation. The selected fungal isolate was identified using PCR with ITS4 and ITS5 as forward and reverse primers, respectively. The BLASTn analysis revealed that the strain CD02 belongs to the genus Aspergillus, and the species was identified as Aspergillus flavus (Genbank No: ON509999.1). The rRNA sequence of the isolate, CD02, has a 96% identity with Aspergillus flavus. The 18S rRNA sequence of these fungal isolates was aligned with reference strains from GenBank, and this formation was used to build a phylogenetic tree (

Phylogenetic Analysis
Through the systematic selection of isolates from the fungal culture, all of the colonies were categorized according to their morphological parameters, such as the shape and color of the colony, and their reverse media color. Each fungal colony was purified by transplanting sequential hyphal ends over 2-3 passes. One of the four isolates, CD02, showed higher antioxidant activity and was chosen for further investigation. The selected fungal isolate was identified using PCR with ITS4 and ITS5 as forward and reverse primers, respectively. The BLASTn analysis revealed that the strain CD02 belongs to the genus Aspergillus, and the species was identified as Aspergillus flavus (Genbank No: ON509999.1). The rRNA sequence of the isolate, CD02, has a 96% identity with Aspergillus flavus. The 18S rRNA sequence of these fungal isolates was aligned with reference strains from GenBank, and this formation was used to build a phylogenetic tree ( Figure 2) showing the relations of the newly identified fungal strain with other members of the genus Aspergillus. The neighbor joining tree demonstrated a tight link between the strains recovered in this investigation and Aspergillus flavus MT584825.

Cytotoxicity Assay
The cytotoxic efficacy of the A. flavus extract against MCF-7 cells was assessed using metabolic MTT assay, a viability test directly measuring the cellular redox potential in a population of cells. The IC50 value of the fungal extract was found to be at 16.25 μg/mL. Figure 3a illustrates the percentage of the viability of the cells at various concentrations

Cytotoxicity Assay
The cytotoxic efficacy of the A. flavus extract against MCF-7 cells was assessed using metabolic MTT assay, a viability test directly measuring the cellular redox potential in a population of cells. The IC 50 value of the fungal extract was found to be at 16.25 µg/mL. Figure 3a illustrates the percentage of the viability of the cells at various concentrations (µg/mL), and Figure 3b,c shows the untreated control cells (Figure 3b) and changes in morphology of the MCF-7 cells after being treated with A. flavus extract (Figure 3c). The IC 50 concentration of the A. flavus extract (16.25 µg/mL) was then selected for further analysis. Doxorubicin (0.25 µM) served as a positive control for this experiment [42]. The statistical data are presented in Supplementary Table S1.

Assessment of Apoptosis by Flow Cytometer
Apoptosis was also studied using annexin V and PI staining. Figure 5 shows the results of the flow cytometry analysis of the A. flavus extract in MCF-7 cells treated with 16.25 μg/mL of extract for 48 h. Early apoptosis was observed in 14% of treated cells, which was significantly higher than in the control cells (0.89%). The percentage of cells in late

Assessment of Apoptosis by Flow Cytometer
Apoptosis was also studied using annexin V and PI staining. Figure 5 shows t results of the flow cytometry analysis of the A. flavus extract in MCF-7 cells treated w 16.25 μg/mL of extract for 48 h. Early apoptosis was observed in 14% of treated cells, whi was significantly higher than in the control cells (0.89%). The percentage of cells in l apoptosis induced by A. flavus extract was also significantly higher (38.9%) compared

Assessment of Apoptosis by Flow Cytometer
Apoptosis was also studied using annexin V and PI staining. Figure 5 shows the results of the flow cytometry analysis of the A. flavus extract in MCF-7 cells treated with 16.25 µg/mL of extract for 48 h. Early apoptosis was observed in 14% of treated cells, which was significantly higher than in the control cells (0.89%). The percentage of cells in late apoptosis induced by A. flavus extract was also significantly higher (38.9%) compared to the control cells (5.52%). Table 1 displays the percentages of live, early apoptosis, late apoptosis, and dead cells.

Measurement of Mitochondrial Transmembrane Potential
The changes in mitochondrial membrane potential were examined using rhodami 123 dye in MCF-7 cells with and without treatment with the A. flavus extract for 48 h (IC After 24 h, the mitochondrial membrane potential in the MCF-7 cells treated with the flavus extract was significantly reduced (Figure 6a,b). Some morphological changes in A. flavus extract-treated cells and their mitochondria can also be observed.

Measurement of Mitochondrial Transmembrane Potential
The changes in mitochondrial membrane potential were examined using rhodamine-123 dye in MCF-7 cells with and without treatment with the A. flavus extract for 48 h (IC 50 ). After 24 h, the mitochondrial membrane potential in the MCF-7 cells treated with the A. flavus extract was significantly reduced (Figure 6a,b). Some morphological changes in the A. flavus extract-treated cells and their mitochondria can also be observed.

Measurement of Mitochondrial Transmembrane Potential
The changes in mitochondrial membrane potential were examined using rhodamine-123 dye in MCF-7 cells with and without treatment with the A. flavus extract for 48 h (IC50). After 24 h, the mitochondrial membrane potential in the MCF-7 cells treated with the A. flavus extract was significantly reduced (Figure 6a,b). Some morphological changes in the A. flavus extract-treated cells and their mitochondria can also be observed.

Assessment of Nuclear Integrity by DAPI Staining
As the A. flavus extract was found to induce apoptosis in MCF-7 cells, the morphological changes of the cellular nuclei were analyzed using DAPI staining ( Figure  7). DAPI stain binds to the adenine and thymine regions of the nuclear DNA and produces

Assessment of Nuclear Integrity by DAPI Staining
As the A. flavus extract was found to induce apoptosis in MCF-7 cells, the morphological changes of the cellular nuclei were analyzed using DAPI staining (Figure 7). DAPI stain binds to the adenine and thymine regions of the nuclear DNA and produces a blue fluorescence. After a 48 h treatment of the cells with A. flavus extract, we observed shrinkage of the cells, condensation of the chromatin, and damage to the nuclear DNA (Figure 7). In addition, compared to the control, the A. flavus extract-treated MCF-7 cells showed a decreased intensity of blue fluorescence. All of these phenomena confirm the apoptotic nature of the cell death induced by the A. flavus extract [43].    Table S2.
μg/mL of extract chromatin. Condensation and fragmentation (indicated by arrow), nucleus shrinkage, and blebbing were also observed.

Assessment of Intracellular Reactive Oxygen Species
An important factor in the development and biology of cancer is the imbalance between the levels of reactive oxygen species and antioxidants. Figure 8a displays the results of the induction of ROS by the A. flavus extract in MCF-7 cells, using the H2DCF-DA staining method. Increased green fluorescence was seen in the cells treated with 16.25 μg/mL of the A. flavus extract as compared to the control (Figure 8b,c), indicating the onset of apoptosis in the MCF-7 cells. The statistical data are presented in Table S2.

Molecular Dynamics Simulation
The molecular dynamic simulation was carried out for 3α,5α-cyclo-ergosta-7,9(11),22ttriene-6β-ol, 2,4,7-trinitrofluorenone, and standard Venetoclax complexed with Bcl-2 protein for 200 ns. The molecular dynamic simulation trajectory events of Apo protein Bcl-2 showed fluctuation to 3.2 Å and retained its stability to 3 Å throughout the simulation period, with an average RMSD of 2.851 Å. The phytoconstituent 3α, 5α-cyclo-ergosta-7,9(11),22t-triene-6β-ol, 2,4,7-trinitrofluorenone complex showed fluctuation initially up to 3 Å and retain its stability thereafter until the end, with 2.8 Å throughout the simulation period with an average RMSD of 2.14 Å, while the other selected phytoconstituent, 2,4,7-Trinitrofluorenone, showed 2.98 Å and retained its stability to 2.6 Å throughout the simulation period with an average of 2.278 Å. The Venetoclax complex showed the fluctuation of 2.8 Å and retained its stability to 2.4 Å throughout the simulation period, with an average RMSD of 2.368 Å ( Figure 11). An RMSF analysis of all complexes shows no major fluctuation due the binding of amino acids with the key functional groups of ligands ( Figure 12).

Discussion
Despite the progress being made in cancer treatment, new approaches are still needed to overcome tricky situations that can affect the current therapies, such as the development of drug resistance, relapse, secondary cancers, and adverse effects of the therapeutic procedures. A potent source of new compounds for cancer treatment can be found in the greatest chemical laboratory on earth-nature. Sustainable drug discovery programs to find new therapeutic phytocompounds with anticancer potentials are run in parallel to the chemical engineering of drug molecules [44]. In recent years, the use of phytomedicines for cancer treatment has noticeably increased [45]. Phytomedicines are already used for the successful treatment of many diseases and overcome many harmful adverse effects of the standard methods [46]. Plant derived medicines are also used more and more often in combination therapy with other medicines to reduce adverse effects and to increase the effectiveness of the treatment [47,48]. Almost 60% of the anticancer drugs currently being used for anticancer therapy are obtained from natural sources [49,50]. In this study, we found highly effective phytocompounds with anticancer potential that come from a fungus, A. flavus, which is found in medicinal plants.
Interestingly, in recent years, materials and products with considerable medicinal values have been found to be produced by the microorganisms associated with plants, rather than by the actual plants [51]. The endophytic bacteria and fungi that thrive in apparently healthy internal plant tissues are either facultative or obligate symbiotic microbes [52]. As mentioned earlier, the Aspergillus species are an important source of novel active phytochemicals with potential therapeutic values [53]. The biggest advantages of endophytic fungi are their fast renewal, relatively easy cultivation, costeffectiveness, and environmental safety [54]. Numerous bioactive substances with a wide range of activities have been found in endophytic fungi over the last 20 years [55]. These bioactive compounds could be classified as flavonoids, alkaloids, terpenoids, diterpenes, sesquiterpenes, polyphenols, phenolic acids, indole derivatives, aliphatic compounds, pyridine, pyrazolidine, pyrimidine, thiazole derivatives, etc. In this study, the bioactive compounds present in the endophytic fungi A. flavus, isolated from the root of C. dactylon,

Discussion
Despite the progress being made in cancer treatment, new approaches are still needed to overcome tricky situations that can affect the current therapies, such as the development of drug resistance, relapse, secondary cancers, and adverse effects of the therapeutic procedures. A potent source of new compounds for cancer treatment can be found in the greatest chemical laboratory on earth-nature. Sustainable drug discovery programs to find new therapeutic phytocompounds with anticancer potentials are run in parallel to the chemical engineering of drug molecules [44]. In recent years, the use of phytomedicines for cancer treatment has noticeably increased [45]. Phytomedicines are already used for the successful treatment of many diseases and overcome many harmful adverse effects of the standard methods [46]. Plant derived medicines are also used more and more often in combination therapy with other medicines to reduce adverse effects and to increase the effectiveness of the treatment [47,48]. Almost 60% of the anticancer drugs currently being used for anticancer therapy are obtained from natural sources [49,50]. In this study, we found highly effective phytocompounds with anticancer potential that come from a fungus, A. flavus, which is found in medicinal plants.
Interestingly, in recent years, materials and products with considerable medicinal values have been found to be produced by the microorganisms associated with plants, rather than by the actual plants [51]. The endophytic bacteria and fungi that thrive in apparently healthy internal plant tissues are either facultative or obligate symbiotic microbes [52]. As mentioned earlier, the Aspergillus species are an important source of novel active phytochemicals with potential therapeutic values [53]. The biggest advantages of endophytic fungi are their fast renewal, relatively easy cultivation, cost-effectiveness, and environmental safety [54]. Numerous bioactive substances with a wide range of activities have been found in endophytic fungi over the last 20 years [55]. These bioactive compounds could be classified as flavonoids, alkaloids, terpenoids, diterpenes, sesquiterpenes, polyphenols, phenolic acids, indole derivatives, aliphatic compounds, pyridine, pyrazolidine, pyrimidine, thiazole derivatives, etc. In this study, the bioactive compounds present in the endophytic fungi A. flavus, isolated from the root of C. dactylon, have been determined to have anticancer properties against human breast cancer cells. C. dactylon (Family: Poaceae) was described as containing numerous bioactive compounds, such as vitexin, orientin, homoorientin, friedlein, beta-carotene, triterpenoids, ergonovine, luteolin, ergometrinine, phytosterols, 2"-O-glycosylisovitexin, arundoin, apigenin, tricin, beta-ionene, 2-coumarinate, triglochinin, ferulic acid, phenyl acetaldehyde, syringic acid, vanillic acid, l-ascorbic acid, phytol, palmitic acid, docosanoic acid, hexadecanal, tritriacontane, furfuryl alcohol, furfural, etc., which are shown to exhibit therapeutic benefits [56].
Lead compound extraction is one of the important steps in isolating the desired bioactive compounds from natural sources [57]. Unfortunately, the quantity of lead compounds produced by plants and microorganisms is very minimal [58]. Thus, we need an ideal extraction technique for separating these traces of lead compounds from the natural resources. The selection of the ideal solvent, solvent concentration, temperature, and time, as well as a suitable extraction technique, might increase the quantity as well as the quality of the bioactive compounds obtained from an endophytic fungus [12]. In this study, fungal secondary metabolites (bioactive compounds) were successfully extracted through an ultrasoundassisted extraction method using 80% ethyl acetate as the extraction solvent. This method has found extended applications in recent years, owing to its enormous benefits, including reduced energy consumption, a shorter extraction time, less active component degradation, and a higher extraction yield compared to traditional extraction methods [34].
The extract induced cytotoxicity in MCF-7 cells. The IC 50 value against MCF-7 cells was 16.25 µg mL −1 . This is similar to the observations made in the endophyte Terminalia catappa, wherein the IC 50 against human cervical cancer HeLa cells was estimated to be 33.35 µg/mL [59]. Further analysis showed that the A. flavus extract induces apoptosis in the breast cancer cell line. Apoptosis is a phenomenon of programmed cell death and is the preferred type of tumor cytotoxicity in the treatment of cancer [60]. Therefore, quantitative and qualitative apoptosis assays were performed, including AO/EtBr double staining, flow cytometric analysis with Annexin V, PI, and FITC staining, along with DAPI staining assay and finally assays for changes in the mitochondrial membrane potential and measurement of ROS generation to assess and analyze apoptosis in them.
Mitochondria play a significant role in cellular functions, including the production of energy (ATP), the maintenance of Ca 2+ ions, cell signaling, cell cycle progression, and finally cell death, as the loss of mitochondrial membrane potential and Ca 2+ release are among the intrinsic signals triggering apoptosis. The mitochondrial membrane potential is generated by protons pumped into the inner membrane space of the mitochondria, an essential process in generating ATP. Mitochondrial membrane depolarization can be caused by an excessive generation of ROS, high intracellular calcium concentrations, or oxidative stress of the endoplasmic reticulum [61]. In this study, the IC 50 concentration of the A. flavus extract triggered mitochondrial membrane potential break down. This may lead to respiratory chain uncoupling and excessive ROS production, followed by oxidative stress with oxidative damages to essential biomolecules leading to cell cycle arrest, and, finally, induced apoptotic cancer cell death [62]. It has been previously shown that Aspergillus extracts can lead to oxidative stress [63].
The observed cytotoxicity can be the result of the activity of the compounds present in the A. flavus extract. Thus, to determine precisely which components of the A. flavus extract are involved, a GC-MS analysis has been performed. The GC-MS spectral data demonstrated the presence of bioactive compounds that might be responsible for the anticancer activities. The obtained GC-MS spectra show the presence of nine phytochemicals, and seven of them were considered as bioactive compounds. The cytotoxic activity of one of these bioactive compounds, i.e., 1H-isoindol-1,3 (2H)-dione, against the HeLa, C6, and A549 cancer cell lines has already been established [64]. Heptadecanoic acid inhibited cell proliferation in PC9 non-small cell lung cancer cells [65]. Similarly, tritetracontane has also already been proven to have anticancer efficacies [66].
Computational drug discovery tools are helpful in identifying highly active molecules, narrowing down the biological and synthetic research needs [67]. Moreover, these tools assist in predicting the pharmacokinetic and pharmacodynamic properties of the molecules, which are subsequently confirmed by in vitro and in vivo studies [68]. In addition to that, they provide information about how these molecules bind with, interact with, donate electrons to/accept electrons from, and up or down regulate the protein/enzyme activity. This may aid researchers in developing treatment alternatives for specific diseases. Surprisingly, some of the compounds identified in the extract exhibited structural features that showed structural properties that predisposed them to possible interaction with the Bcl-2 receptor, which is overexpressed on cells of the breast cancer subtype called Bcl-2-enriched breast cancer [69]. Thus, we performed a molecular docking analysis of the bioactive compounds, and identified the one among them, i.e., 3α, 5α-cyclo-ergosta-7,9(11),22t-triene-6β-ol, which showed the highest binding affinity (−9.5 Kcal/mol) against the overexpressed anti-apoptotic protein receptor Bcl-2 of breast cancer. The binding affinity score was close to that of the standard drug Venetoclax (−10.90 Kcal/mol), which targets Bcl-2 and some other receptor kinases and is clinically used in breast cancer treatment for that purpose. Recent evidence suggests that Bcl-2 can directly influence apoptosis by translocating to the mitochondria to inhibit cytochrome c release [70]. Altogether, the compounds identified in the endophytic fungal extract have a vast range of possible anticancer mechanisms against breast tumors. Not only can they hit the universal cellular energy metabolism system by uncoupling the membranes of the mitochondria and subsequently generating ROS, but they are also potentially effective against the Bcl-2-enriched breast cancer subtype.

Conclusions
To sum up, A. flavus is an endophytic fungus isolated from the roots of C. dactylon, and its ethyl acetate extract showed a potent anticancer activity against breast cancer (MCF-7) cells. The profiling of bioactive compounds from the ethyl acetate extract of endophytic fungus was detected through GC-MS analysis, and nine compounds were identified. Among them, two phytocompounds, namely, 3α, 5α-cyclo-ergosta-7,9(11),22ttriene-6β-ol, and 2,4,7-trinitrofluorenone, exhibited the highest binding affinities, −9.50 and −9.20 Kcal/mol, respectively, to the anti-apoptotic protein (Bcl-2) receptor. Molecular dynamic simulation studies confirmed that the stability of the intermolecular interactions of the ligands−receptor binding complexes of the A. flavus extract exerted cytotoxic effects, significantly reducing the viability of MCF-7 cells, with an IC 50 of 16.25 µg/mL. The extract-induced apoptosis in the MCF-7 cells was associated with a high ROS generation, nuclear material damage, and the dissipation of mitochondrial transmembrane potential. To conclude, A. flavus, an endophytic fungus isolated from the roots of C. dactylon, has the potential to be a source of novel therapeutic drugs. Additional studies are required to purify the compounds, elucidate the mechanism of action, and study its safety, so that these compounds can be developed as future drugs for cancer therapies.