Antimicrobial and Antioxidant Properties of a Bacterial Endophyte, Methylobacterium radiotolerans MAMP 4754, Isolated from Combretum erythrophyllum Seeds

This study reports on the isolation and identification of Methylobacterium radiotolerans MAMP 4754 from the seeds of the medicinal plant, Combretum erythrophyllum, for the purposes of investigating antimicrobial and antioxidant activities from this endophyte. The strain identity was confirmed by 16S rRNA-based phylogeny and Scanning Electron Microscopy (SEM). Ethyl acetate and chloroform (1 : 1 v/v) extracts from the endophyte were tested for antimicrobial and antioxidant activity on a total of 7 bacterial species (3 Gram-positive and 4 Gram-negative) using the standard Minimum Inhibitory Concentration (MIC) protocol and Quantitative Radical Scavenging activity using the 2, 2-diphenyl-1-picrylhydrazyl (DPPH) assay, respectively. The MICs were recorded at 250 μg/mL for B. subtilis ATCC 19659, B. cereus ATCC 1076, E. coli ATCC1053, and 62.5 μg/mL for K. oxytoca ATCC 13182 and M. smegmatis ATCC 21293, while an IC50 of 5.65 μg/mL was recorded with the DPPH assay. Qualitative phytochemical analysis was positive for alkaloids, flavonoids, and steroids. Gas chromatography/mass spectrometry (GC/MS) analysis revealed the presence of 9-octadecene, 2,4-dinitrophenyl acetate, and 2(5H)-furanone, which have been previously reported for the targeted activities. M. radiotolerans MAMP 4754 tested positive for antimicrobial and antioxidant activity and this is linked to the production of plant-derived secondary metabolites by this strain.


Introduction
e exponential increase in the number of drug-resistant pathogens coupled with immune-suppressing diseases has rendered infectious disease control a major global challenge.
is challenge necessitates the search for new bioactive compounds with pharmaceutical potential [1][2][3]. Over the years, continued bioprospecting of medicinal plants has generated 47% of drugs currently approved by the United States of America's Food and Drug Administration (FDA), with only 3% of these being antimicrobial [4]. e pharmaceutical properties of medicinal plants have been linked to the production of a wide variety of structurally diverse phytochemicals which include alkaloids, flavonoids, terpenes, steroids, curcumins, saponins, and phenolics, all of which can potentially serve as drug lead candidates for the development of antimicrobials and resistance modifiers [5,6].
According to the International Union for Conservation of Nature and the World Wildlife, there are an estimated 80 000 recognized medicinal flowering plant species globally, 15 000 of which are being threatened with extinction due to habitat destruction and overharvesting caused by unregulated informal markets [7,8]. In order to conserve currently endangered medicinal plant species from permanent disappearance, there is an increased interest in systems which offer potentially bioactive and chemically diverse compounds like those found in plants but with negligible environmental effects.
Endophytes are endosymbiotic microorganisms (commonly bacteria or fungi) that systematically colonize and proliferate within plant tissues without causing any signs of disease or harm [9]. In colonizing plant tissue, endophytes are also capable of establishing a symbiotic relationship with the plant thus making them efficient biocontrol and medicinal agents. Several research reports have demonstrated the activity of bacterial endophytes against various pathogens [10,11]. As such, there is continued research interest in developing drugs from endophytic compounds which could serve as an alternative to synthetic pharmaceuticals and/or plant-derived medicines. Endophytes are known to promote plant growth, enhance defence, increase abiotic and biotic stress tolerance, and improve nutrient acquisition [12]. Endophytes may actively modulate the host's biosynthesis pathways and gene expression systems to increase the production of significant secondary metabolites. An interesting case being that of the medicinal plant Withania somnifera whereby some isolated endophytes could induce the production of withaferin A (abundantly produced in the leaves) in the roots and while some upregulate the expression of 1deoxy-D-xylulose-5-phosphate synthase (DXS) and 1-deoxy-D-xylulose-5-phosphate reductase; (DXR) genes [13].
A key advantage of endophytes is that they can be easily isolated and cultured and are amenable to genetic manipulations and can be scaled up for bioactive compound production [14]. Considering the importance of bacterial endophytes to both plant and human health, there is an increased focus on developing endophytes into herbal remedies. e current study is based on Methylobacterium radiotolerans MAMP 4754 [15], a bacterial endophyte isolated from the seeds of Combretum erythrophyllum. e Methylobacterium genus is composed of bacterial species that are Gram-negative, pink pigmented [16], rod-shaped, strictly aerobic, and facultative methylotrophs [17]. Members of this genus are commonly found in various environments due to their phenotypic plasticity [18,19]. Crude and partially purified extracts of the Methylobacterium genus have been shown to possess antimicrobial, anticancer, and antioxidant properties [20,21]. e purpose of this study was to, therefore, analyse the antimicrobial and antioxidant activity of Methylobacterium radiotolerans MAMP 4754.
us, results obtained from this study will further affirm the significance of the Methylobacterium genus as a source of pharmaceutically relevant bioactivity.  [22]. Briefly, surface sterilization of the fruits was done by firstly washing them with tap water to remove dust, followed by treatment with Tween 80 for 10 minutes with vigorous shaking, and then rinsing with sterile distilled water. e washing was continued with 70% ethanol and 1% sodium hypochlorite (NaOCl) for 1 and 10 min, respectively, followed by thorough rinsing with sterile distilled water three times. e final wash was spread on Luria-Bertani (LB) agar plates to determine the success of the surface sterilization process. e outer surface of sterile fruits was then trimmed off to access the delicate seeds which were then macerated in phosphate buffer saline (PBS) for bacterial endophyte isolation. Serial dilutions of up to 10 − 3 were prepared and 0.1 mL of the dilutions was spread on LB agar plates in triplicates. ese plates and the controls were incubated at 30°C for up to 3 days with daily monitoring for the occurrence of colonies. e colonies that emerged after the incubation period were subcultured several times on LB agar to obtain pure cultures that were then stored in 50% glycerol at − 80°C for long-term future use.

DNA Extraction and 16S rRNA Gene Amplification.
A frozen stock of one of the isolates (M. radiotolerans MAMP 4754) was revived by spreading inoculum on LB agar and incubating overnight at 30°C. A single colony was picked to inoculate LB broth which was incubated until an optical density measured at 600 nm (OD 600 ) was about 0.4-0.5. Genomic DNA was then extracted from the culture using DNeasy blood and tissue kit (Qiagen, Germany) following the manufacture's protocol. e extracted genomic DNA was then quantified using a NanoDrop ™ ND-2000 UV-vis spectrophotometer ( ermo Fisher Scientific, USA).

Polymerase Chain Reaction (PCR) Amplification and
Sequencing of the 16S rRNA Gene. e 16S rRNA gene of the bacterial endophyte was amplified according to a method described by Tsuchida et al. [23]. e 16S rRNA gene of the endophyte was then amplified using the universal primers BacID 1F (5′-AGAGTTTGATCTGGCTCAG-3′) and BacID 1500R (5′-AAGGAGGTGWTCCARCC-3′) which were bought from Inqaba Biotechnological Industries (Pretoria, South Africa). Polymerase chain reaction (PCR) was in 50 μL total volumes using the following conditions; 1X initiation cycle at 92°C for 2 min, 30X denaturation cycles at 92°C for 30 sec, 30X primer annealing cycles at 52°C for 30 sec, 30X extension cycles at 72°C for 2 min, and a 1X elongation cycle at 72°C for 2 min followed by termination at 4°C. e PCR products were analysed on a 1.5% agarose gel by electrophoresis at a constant 100 V and 200 mA. e positive products were then excised from the gel and purified using the GeneJet gel extraction kit ( ermo Fisher Scientific, USA). e purified PCR products sequenced at Inqaba Biotechnical Industries.

Phylogenetic Analysis.
e individual sequences were assembled within Geneious (Geneious 8.1.9) and a contig was formed. is was preceded by a BLAST search on the NCBI GenBank nucleotide sequence database (https://www. ncbi.nlm.nih.gov/genbank/). Sequences of species closely matching the BLAST query sample along with their closely related taxa were obtained for the phylogenetic analysis. A matrix was generated with the query samples and the closest matching sequences, which were then aligned using Geneious Alignment at a Cost Matrix of 70% similarity. Using a Heuristic search followed by a Bootstrap analysis, a parsimonious phylogenetic tree was constructed using Parsimony (PAUP * 4.0).

Morphological Characterization of M. radiotolerans MAMP 4754.
To establish the morphological characteristics such as shape and Gram stain reaction, pure colonies were analysed by methods described by Collins et al. [24]. e slides were viewed using a compound bright-field microscope (OLYMPUS CH20BIMF200) with 100x magnification [25]. Morphological characteristics such as shape and Gram stain reaction and purity of stock cultures were analysed using a previously reported method. e prepared slides were viewed using a compound bright-field microscope (OLYMPUS CH20BIMF200) at 100x magnification.

Scanning Electron Microscopy.
Scanning electron microscopy (SEM) was performed using methods described by Golding et al. [26]; and Schadler et al. [27]. In brief, M. radiotolerans MAMP 4754 was grown at 30°C, shaking at 150 rpm, in LB broth (NB) until an OD 600 was 0.4-0.8. e bacterial cultures were then centrifuged at 10 823 rpm for 10 min and the supernatant discarded. Cells were then washed with sterile distilled water and the pellet was fixed with (1 : 1v/v) of 1% formaldehyde and 2% glutaraldehyde for 1 h at room temperature (25°C). Following fixation, samples were centrifuged at 10 823 rpm for 10 min, followed by discarding of the supernatant and washing of the pellet with 1 mL of sterile distilled water. For dehydration, bacterial cells were treated with increasing concentrations of ethanol (30,50,70,90,95, and 100%) with 10 min intervals.
Samples were stored open at 4°C overnight and mounted on SEM stubs the following day. ese were then coated with gold using Emscope SC 500 and viewed using Tescan Vega 3 (Tescan-Orsay, Czech Republic), which was operated at 6 kV accelerating voltage.
e extraction of secondary metabolites from M. radiotolerans MAMP 4754 was carried out using the method previously described in Balachandran et al. [20] with minor modifications. Briefly, LB broth (1 L) was prepared in 2 L Erlenmeyer flasks and autoclaved at 121°C for 20 min. Each of the 2 L flasks was inoculated with the endophytic bacteria and incubated at 28°C for 7 days shaking at 200 rpm. After the 7 th day, the culture was centrifuged at 10 000 rpm for 15 minutes for biomass removal. Equal volumes of ethyl acetate and chloroform (1 : 1 v/v) were added to the supernatant followed by vigorous shaking. e organic solvent layer was collected in a conical flask and the organic layer was concentrated using a vacuum rotary evaporator at 40°C. e extract was transferred to a 5 mL sterile vial and left to dry at room temperature. e phytochemical screening of M. radiotolerans MAMP 4754 crude extract was adopted from [28,29] with minor modifications shown in Table 1.

Antimicrobial Activity of Crude Extract from M. radiotolerans MAMP 4754.
Evaluation of the antimicrobial activity of the secondary metabolite crude extract was carried out using the disc diffusion method as previously described by Hoelzer et al. [30] and Zhang et al. [31]. Seven pathogenic bacterial strains (Gram-positive strains: Bacillus cereus ATCC 1076, Bacillus subtilis ATCC 19659, Mycobacterium smegmatis ATCC 21293, Enterococcus faecalis, Gram-negative strains: Escherichia coli ATCC 10536, Pseudomonas aeruginosa ATCC 25922, Klebsiella oxytoca ATCC 13182) and a fungal strain Candida albicans were grown overnight at 37°C in Mueller-Hinton (MH) broth, which was adjusted to McFarland Standard No. 0.5 such that the concentration was 10 7 to 10 8 colony-forming units per millilitre (CFU/ mL). e pathogenic strains were further spread on MH agar plates and sterilized circular paper discs (4 mm), soaked with the bacterial endophyte crude extract were placed on the plates containing a lawn of bacterial culture of the test pathogenic strains. For the positive control, 10 μL of 1 mg/ mL Ampicillin, Kanamycin, and Ketoconazole was also impregnated on the paper discs as described above and for the negative control, respective solvents (chloroform and ethyl acetate) were utilized. All the plates were then incubated at 37°C for 48 to 72 hours and antimicrobial activity was assessed by observing and measuring the zone of inhibition in mm. e antimicrobial experiments were performed in triplicate (n � 3).

Determination of Minimum Inhibitory Concentration.
e Minimum Inhibitory Concentration (MIC) was used in the study to determine the antimicrobial activity of M. radiotolerans MAMP 4754 by serial microdilution in a 96well microplate [32,33]. e same pathogenic strains that were utilized in the disc diffusion assay were used for the MIC test. e bacterial strains were grown at 37°C for 12 to 24 hours (depending on the growth rate of each pathogenic strain) in MH broth. To the wells in column A of the microtiter plate, a 100 μL of MH broth and 100 μL of M. radiotolerans MAMP 4754 extract (1 mg/mL) was added and mixed. Columns B to H were also loaded with 100 μL of MH broth and serial dilutions were carried out from column A to a final concentration of 3.9 μg/mL in column H. is was International Journal of Microbiology done in triplicate. Following the dilution process, each well was loaded with 100 μL of bacterial culture to a 0.5 McFarland's standard. Similarly, this was done with the positive controls of Ampicillin, Kanamycin, and Ketoconazole and for the negative control, 0.1% DMSO was used. e microtiter plate was sealed with parafilm and incubated at 37°C for 24 hours. After incubation, 10 μL of 4 mg/mL iodonitrotetrazolium chloride was added to each well. MIC was recorded as the lowest concentration with clear wells, which indicated the absence of microbial growth.

Scavenging 2, 2-Diphenyl-1-picrylhydrazyl (DPPH) Free
Radical Assay. Antioxidant activity of the M. radiotolerans MAMP 4754 crude extract was studied using the 2, 2diphenyl-1-picrylhydrazyl (DPPH) free radical scavenging assay. is was carried out using a modified method previously described by Takao et al. [34], with minor modifications. e crude extract of M. radiotolerans MAMP 4754 was dissolved in ethanol and mixed with a 90 μM DPPH ethanol solution to give a final concentration of 0.78-100 μg/ mL. Ethanol was used as solvent control, while ascorbic acid was used as a positive control. e extract with DPPH was incubated in the dark at room temperature for 30 minutes. e absorbances were measured at 492 nm (Bio-TekSynergy HT Multi-Detection Microplate Reader; USA). All experiments were done in triplicate and the IC 50 was calculated graphically with percentage inhibition calculated as follows: %inhibition � 100 × ((absorbance of control − absorbance of the sample)/absorbance of control).

Gas Chromatography High-Resolution Time-of-Flight
Mass Spectrometry (GC-HRTOFMS). Secondary metabolites were identified using gas chromatography high-resolution time-of-flight mass spectrometry (GC-HRTOFMS (LECO Corporation St. Joseph, MI, USA)), operating in high-resolution, equipped with a Gerstel MPS multipurpose autosampler (Gerstel Inc. Germany). For the analysis, the samples were run in a 30 m × 0.25 mm capillary column with a film thickness of 0.25 μm. e carrier gas was helium and it was maintained at a column flow rate of 1 mL/min. A 1 μL sample of the extract was injected and the column temperature was maintained at 75°C followed by temperature programming at 10°C/min to 235°C for 2 mins, and finally to 300°C at a rate of 40°C/min for 3 min (Scan range: 45-500 m/z). e mass spectrometer and transfer line were held at 250°C. Peak picking, peak and retention time alignment, and detection and matching were done on ChromaTOF-HRT ® software (LECO Corporation, St Joseph, MI, USA). A signal to noise (S/N) ratio of 100 was used and similarity/probability match was ˃70% before a name was assigned to a compound using Mainlib, NIST and Feihn metabolomics database through comparison of the mass spectra data, molecular formula, and the retention time.

Statistical Analysis.
e resulting data were analysed using analysis of variance (ANOVA). e antimicrobial and DPPH data were described as mean ± standard deviations (SD). is analysis was done using Microsoft Excel Office 365 ANOVA. p values less than 0.05 were considered to be statistically different.

Molecular and Morphological
Identification of M. radiotolerans MAMP 4754. Prior to endophyte isolation, C. erythrophyllum seeds were surface sterilized and the sterilization method was adequate as none of the control plates showed any microbial growth. e 16S rRNA gene of the bacterial endophyte was amplified and the expected amplicon size of 1500 bp was obtained (data not shown). e sequencing of the amplicon and similarity/BLAST searches revealed that the bacterial isolate, M. radiotolerans MAMP 4754, shared 99% homology to bacterial species belonging to Methylobacterium genus as indicated in Figure 1(a). e genus has over fifty published species; however, based on the 16S rRNA gene, multilocus sequence analysis, and genomic and phenotypic data, fifty-two Methylobacterium species can no longer be regarded in this genus. A new genus, Methylorubrum gen. nov. has been proposed to accommodate 11 species, which were previously held in the Methylobacterium genus [35]. Additionally, this isolate is in a Methylobacterium clade that is sister to Methylorubrum gen nov clade, as demonstrated in Figure 1(a).
e Gram stain reaction indicated that M. radiotolerans MAMP 4754 is a rod-shaped, Gram-negative bacterium as it did not retain the crystal violet stain used in the Gram staining method (data not shown) [36,37]. e bacterial morphology (with uniform cells indicating that the bacterial cultures were pure) was further confirmed by the SEM electron micrograph (Figure 1(b)). e isolation of endophytic bacteria has been reported for several medicinal plants such as Catharanthus roseus, Ocimum sanctum and Mentha arvensis [38], Lonicera japonica [39], and Ferula songarica [40]. However, there are currently a few reports on the isolation and characterization of endophytic Methylobacterium and in the context of bioactivity, some of the reports confirmed the antimicrobial compounds [41,42] and production of defensin-like antimicrobial peptides [43].

Phytochemical Analysis.
e results of the phytochemical screening indicated that M. radiotolerans MAMP 4754 consists of alkaloids, flavonoids, and steroids and contained no tannins and saponins (Table 1). is observation indicates that the bacterium shares some common secondary metabolite biosynthetic pathways with the host plant since Combretum species are rich in intermediate polar compounds such as flavonoids, stilbenoids, and triterpenoids [44][45][46]. Flavonoids are polyphenolic compounds generally found in plants, vegetables, fruits, tea, and coffee [47] and they are known to show antimicrobial, anticancer, anti-inflammatory, antiallergic, antioxidant, and antiviral properties [48]. Alkaloids also have pharmacological, veterinary, and medical properties [49]. Various alkaloids used in anticancer drugs include Camptothecin and Vinblastine, while Morphine and Codeine are used as analgesics and ephedrine is used for relieving asthma [50].
Bioactive compound production by endophytes is related to the evolution of the host microorganisms, which may have incorporated genetic information from higher plants through horizontal gene transfer [51][52][53]. is enables host plant adaptation and the achievement of functions which are vital to the plant such as protection from pathogens, insects, and grazing animals [52,54]. erefore, the presence of flavonoids, alkaloids, and steroids in M. radiotolerans MAMP 4754 is indicative of the therapeutic potential that endophytes contract from their hosts.

Antimicrobial Activity and MIC.
Crude secondary metabolites from M. radiotolerans MAMP 4754 were extracted using ethyl acetate and chloroform and the MICs for each pathogen tested are shown in Table 1. e ethyl acetate and chloroform extract (1 mg/mL) showed antibacterial and antifungal activity against selected pathogenic strains (Table 2). e results obtained indicated a significant difference in the antimicrobial activity of M. radiotolerans MAMP 4754 crude extract against all pathogens compared to the antibiotic controls.
M. radiotolerans MAMP 4754 was extracted using ethyl acetate and chloroform solvents. e ethyl acetate and chloroform extract (1 mg/mL) showed antibacterial and antifungal activity against selected pathogenic strains (Table 2). Statistical analysis of the antimicrobial activities showed that thep value was less than 0.05, which indicates   (Table 2A; supplementary data). e extract resuspended in chloroform showed zones of inhibition ranging from 12 to 17 mm with the most significant inhibition observed on B. subtilis (Table 2A; supplementary data). ese results were in correlation to previous studies conducted by Pansanit and Pripdeevech [55] and Salehan et al. [56], where ethyl acetate extracts of endophytes from Zingiber cassumunar proved to be the most effective inhibitors of fungal growth, Gram-positive and negative bacteria [55,56]. is is also consistent with the various literature reports, showing that ethyl ether and ethyl acetate, are hydrogen bond acceptor molecules and can, therefore, extract electron donor solutes better than chloroform [57]. Furthermore, in their study Kavitha et al. [58] effectively extracted antimicrobial compounds from Streptomyces sp. TK-VL_333 using ethyl acetate [58]. is was further confirmed in a study by Mtunzi et al. [59] where ethyl acetate fractions were observed to have been the best extractant for antimicrobial compounds in an MIC assay. Taken together, the antimicrobial activity observed in the current study along with previous studies can be associated with the presence of phenolic and polyphenolic compounds [60,61]. is, therefore, suggests that bacterial endophytes can produce similar bioactive compounds as their host plant [62][63][64].
e MIC values of the secondary metabolites ranged from 62.5 μg/mL to 250 μg/mL. e highest value was observed with B. subtilis, B. cereus, and E. coli with an MIC value of 250 μg/mL (Table 2). A notable value of 62.5 μg/mL was observed on K. oxytoca and M. smegmatis, showing that M. radiotolerans MAMP 4754 has great potential for the development of compounds containing bioactivities against human pathogenic microorganisms as shown in Table 2. Crude extracts exhibiting activity at a concentration of 1000 μg/mL or lower are considered significantly active [65]. Interestingly, in a study of antimicrobial activity of C. erythrophyllum plant crude extracts, MIC values ranging from 80 μg/mL to 125 μg/mL were observed, which compares to the findings of the current study. Furthermore, the results that were obtained for the potential activity of the M. radiotolerans MAMP 4754 crude extract against the tested pathogens correlate with those of Martini and Eloff [66] on Combretum spp. with the lowest value of 50 μg/mL [66]. is activity can be related to the presence of the flavonoid and phenolic content (Table 3) [78,79]. is is an initial report on the antimicrobial activity of secondary metabolites from an endophyte isolated from C. erythrophyllum.

Antioxidant
Activity. DPPH free radical assay was used in this study to test the scavenging effects of the M. radiotolerans MAMP 4754 extract. DPPH assay is a commonly used tool for the evaluation of the scavenging effect of natural products based on the quenching of stable coloured radicals [80]. However, DPPH is a preliminary method for antioxidant activity and should, therefore, be verified by other more sensitive assays such as the ferric reducing antioxidant power (FRAP) test and β-carotene bleaching assay [81,82]. Ascorbic acid, which had an IC 50 of 6.69 μg/mL, was used as a standard control because of the characteristic antioxidant and radical scavenger activities ( Figure 2). e M. radiotolerans MAMP 4754 extract showed antioxidant property at IC 50, of 5.65 μg/mL. A low IC 50 value is indicative of greater radical scavenging activity [83]. erefore, the IC 50 of M. radiotolerans MAMP 4754 observed in this study suggests that the extract of M. radiotolerans MAMP 4754 is an effective radical scavenger and can be used as a potential antioxidant supplement. ese findings correspond to a previous study of a C. erythrophyllum ethyl acetate plant extract showing a free radical scavenging activity at IC 50 4.3 μg/mL [59]. In their study Mtunzi et al. [59] ranked the activity of the plant crude extracts in the following order: ethyl acetate > dichloromethane > water > acetone > hexane [59]. Interestingly, high antioxidant activity in DPPH assays is associated with phenolic compound quantity in crude extracts [80,84,85] and this can be seen in our GC/ MS findings (Table 3) where several phenolic compounds were detected and identified.
Phenolic compounds were previously said to possess ideal structural chemistry for free radical scavenging activity Kanamycin was used as a positive control for pathogens marked with ( * ), Ampicillin was used for those marked with ( ), and Ketoconazole was used for those marked with ( ⁂ ). [86]. Furthermore, this activity corresponds to the presence of flavonoid compounds, which were detected in the phytochemical analysis (Table 1). Flavonoids have also been reported to play an important role in the reduction of lipid peroxidation and thus act as primary and secondary antioxidants [87]. Total flavonoid content has also been attributed to free radical scavenging activity in fungal endophyte extracts of Fritillaria uni bracteate var. wabuensis [88]. e free radical scavenging effects of the crude extract showed significant antioxidant potentials in comparison to the ascorbic acid, with this being a great indication that the endophytes can indeed be a good source of bioactive compounds relevant in the development of novel therapeutic drugs.

Gas Chromatography High-Resolution Time-of-Flight
Mass Spectrometry Analysis. e use of endophytes as a source of bioactive compounds is an advantageous alternative as they are known to produce similar secondary metabolites as their host plant. C. erythrophyllum has several medicinal properties such as antibacterial [63,64], antifungal [62], anti-inflammatory/oxidizing [89,90] and antitumor [91], and it continues to be used as a traditional medicinal plant. In order to identify the compounds responsible for the observed antimicrobial and antioxidant activities (Table 3) Table 3). ese findings are similar to those of Yogeswari et al. [92] and Naragani et al. [93] who, from the fungus Monochaetia kansensis, also observed antimicrobial activity owing to the presence of 9-octadecene, 3-eicosene, and 11tricosene [92,93]. In addition, these fatty acids are found in abundance in several plants and have also been reported to have anticancer and antioxidant activity [67,68,94].
Antioxidant activity of phenolic compounds, identified herein, can be described in terms of their intrinsic bioactivity  . Ascorbic acid (vitamin C) was used as a positive control. IC 50 values were 6.69 μg/mL and 5.65 μg/ mL for the ascorbic acid and the crude extract, respectively. Statistical analysis was performed using ANOVA and the differences were considered significant at p < 0.05. as free radical scavengers or indirectly as modulators of intracellular pro-and antioxidant enzymes [95]. Phenolic compounds have been shown to exert antioxidant properties both in vitro and in vivo [96]. One of the phenolic compounds identified in this study was p-tert-butyl (Table 3). is observation corresponds to that of Balasundram et al. [97] who reported on the antifungal, anticancer, and antioxidant activity of p-tert-butyl isolated and purified from Lactococcus sp. [97].
Furan derivatives, which were also detected in the current study, are used in the cosmetics and pharmaceutical industry due to their medicinal properties [71][72][73]. In a previous study by Zekeya et al. [73] and Sharma et al. [72], 2furanmethanol 5-methyl was detected from a methanol : chloroform extract of Gunnera perpensa. In that study, 2furanmethanol 5-methyl was detected with a percentage area of 0.34% and was reported to possess bioactivities such as anticancer, anti-inflammatory, and antimicrobial activity [72,73]. Other important bioactive compounds detected in this study were siloxane derivatives which have been shown to possess antifungal and antibacterial activity [75]. Antioxidant capacity has also been reported in methanol extracts of Merremia aegyptia and Merremia dissecta [77]. In their study, Joshi et al. [77] detected the presence of siloxane derivatives such as 3-ethoxy-1,1,1,7,7,7-hexamethyl-3,5,5tris (trimethylsiloxy) tetrasiloxane in the methanol extracts using GC-MS analysis [77]. Results obtained from our study are similar and comparable to those from previous reports and therefore justify the possible development of M. radiotolerans MAMP 4754 for pharmacological action. e data presented herein further confirms the notion that endophytes are a great source of bioactive compounds that can be utilized in drug discovery and could be a great source of natural antioxidants. Further studies are required to provide a better understanding of endophytes and the secondary metabolites produced and possibly elucidating the mechanism of action.

Conclusion
To our knowledge, this is the first study to report on the antimicrobial and antioxidant bioactivities of M. radiotolerans MAMP 4754. e ethyl acetate extract of M. radiotolerans MAMP 4754 exhibited a higher degree of antibacterial and antifungal activity showing high zones of inhibition against seven human microbial pathogens compared to the chloroform extract. Furthermore, the M. radiotolerans MAMP 4754 crude extract showed low MIC values of 62.5 μg/mL against K. oxytoca and M. smegmatis.
is is indicative of a high antimicrobial potential of the endophyte. Additionally, M. radiotolerans MAMP 4754 extract showed high antioxidant activity. e phytochemical analysis of M. radiotolerans MAMP 4754 revealed the presence of flavonoids, steroids, and alkaloids. Moreover, the screening of bioactive compounds of the ethyl acetate extract of M. radiotolerans MAMP 4754, indicated the presence of different compounds that have been previously reported to show potential applications in pharmaceuticals and agriculture. As such, future studies of bacterial endophytes can lead to the development of novel therapeutic drugs from the analysis of the secondary metabolites they produce and could aid in understanding the biochemical pathways for synthesis of some of these biologically active compounds.
Data Availability e bacterial endophyte reported herein has been deposited in GenBank with the following accession number: MF133459.