Plant material was collected from various parts of Meghalaya, India, based on its ethno-medicinal usages by the ethnic tribals. Plants with no visible symptoms of disease were carefully selected, brought to the laboratory in sterile bags and processed within 24 hr after sampling.

Isolation of endophytic fungi was done according to the method described by Hallmann et al. [16] with minor modifications. The plant samples were rinsed gently in running water to remove adhered dust and debris. Samples were cut into 2 mm segments and were surface sterilized with 70% ethyl alcohol for 1 min, soaked in 4% sodium hypochlorite solution for 3 min, and then rinsed with 70% ethyl alcohol for 1 min. They were finally rinsed with sterile distilled water and blot dried on sterile filter paper. The excess water was dried under laminar airflow chamber. The surface sterilized explants were then inoculated into the Petri dishes containing potato dextrose agar (PDA) (Himedia, Mumbai, India) supplemented with 100 µg/mL of streptomycin and incubated at 25 ± 2℃ for 15 days. The plates were periodically observed for fungal growth. The fungus growing out from the plant explants was then subcultured in PDA plates.

The endophytic fungal isolates were tentatively identified microscopically on the basis of their critical morphological structure such as hyphal features, arrangement of spores and reproductive structures.

The amplified ITS products were purified from the gel slice using QIA Quick Gel Extraction Kit (Qiagen, Hilden, Germany) according to manufacturer's instruction.

For sequencing reaction, Big Dye Ready Reaction Dye Deoxy Terminator Cycle Sequencing kit (Applied Biosystems) was employed and sequencing was done in Applied Biosystems 3700 Genetic Analyser.

Sequence analysis was performed with sequences in the NCBI database using BLAST and sequences were aligned by using the Clustal W program and phylogenetic tree was constructed using MEGA 4.1 software. The sequences were deposited to the NCBI database and accession numbers obtained.

Each fungus was cultivated on potato dextrose broth by placing agar blocks of actively growing pure culture (3 mm in diameter) in 250 mL Erlenmeyer flask containing 100 mL of the medium. Each flask was incubated at 25 ± 2℃ for 3 wk with periodical shaking at 150 rpm. After incubation, the culture filtrate was extracted and filtered through three layers of muslin cloth to remove mycelia. Then the culture filtrate was filtered thrice with equal volumes of solvent ethanol. The organic phase was collected and the solvent was then removed by evaporation under reduced pressure at 45℃ using rotary vacuum evaporator. The dry solid residue was re-dissolved in ethanol (2 mg per mL) and evaluated for their antimicrobial and antioxidant activities.

Test microorganisms used in the study included Escherichia coli MTCC730, Enteroccocus faecalis MTCC2729, Salmonella enterica ser paratyphi MTCC735, Streptococcus pyogenes MTCC1925 and Candida albicans MTCC183 procured from Institute of Microbial technology (IMTECH, Chandigarh, India). Test bacteria were subcultured every two weeks on fresh nutrient agar slants and incubated at 37℃, whereas C. albicans was subcultured every four wk on fresh PDA slant and incubated at 37℃. All the cultures were kept at 4℃ until further use.

The antimicrobial assay using the crude extract was carried out on Mueller Hinton agar medium for test bacteria and PDA for test fungus. One mL of inoculum was swapped on molten agar plates. Using the sterile cork borer 7 mm wells were made in the plates in which 20 µL of crude ethanol fraction was loaded. After incubation for 24 hr at 37℃ for bacteria and at 25℃ for fungus, the plates were observed for zone of inhibition.

The reducing power of the fungal extracts was determined according to Chang et al. [19]. An aliquot of 0.5 mL sample extract were taken in a test tube and 0.1 mL of 1% potassium ferricyanide solution was added. The mixture was incubated at 50℃ for 30 min. After the incubation, 0.1 mL of 1% trichloroacetic acid and 0.1 mL of 1% ferric chloride solution was added to the mixture and left unattended for 20 min. The absorbance of the reaction mixture was read spectrophotometrically at 700 nm against water blank.

Different concentrations of the extracts were taken in separate test tubes and the volume was adjusted to 100 µL with ethanol. Five mL of 0.1 mM ethanolic solution of DPPH was added to these tubes. The mixture was shaken vigorously, left to stand for 30 min in the dark, and the absorbance was measured at 517 nm. The percentage inhibition of DPPH radical by the sample extract was expressed as the inhibition concentration (IC50) and was calculated using the following relation:

DPPH scavenging effect (%) = [(A0 - A1/A0) × 100],

where A0 is the absorbance of the control reaction and A1, the absorbance in presence of the extract.

The total polyphenolic content was determined calorimetrically following the Folin-Ciocalteau (FC) method according to Singleton et al. [20] with minor modifications. 0.5 mL of test sample was mixed with 0.2 mL of FC reagent and allowed to stand for 10 min to which 0.6 mL of 20% sodium carbonate was added and mixed. The reaction mixture was incubated at 40℃ for 30 min and absorbance of the reaction mixture was measured at 765 nm with gallic acid taken as standard.

All the tests were performed in triplicates. The results are expressed as mean ± SE values and data were tested by one-way analysis of variance. Differences were considered significant at p < 0.05.

A total of eleven isolates were isolated from roots, stem and leaves of the host plant (Table 1). Based on colony and microscopic features, four isolates exhibiting different morphological features were considered for molecular characterization. The rDNA-ITS region was amplified, the sequence data was then assembled and submitted to the NCBI GenBank with accession Nos. JQ322820, JQ322821, JQ322823, JQ322824. Based on BLAST search of ribosomal RNA gene sequence, the endophytic fungi were found to be closest homolog of Phomopsis sp., Epacris sp., Xylaria sp. and Diaporthe sp. (Fig. 1).

The crude metabolite of the fungi displayed considerable antimicrobial activity against some clinically significant pathogens (Table 2). The crude extracts of two endophytic fungi, Xylaria sp. and Diaporthe sp. showed effective inhibition of three test strains. However, the endophyte Epacris sp. had no effect on all the five test strains. None of the fungal extracts showed inhibition of E. coli MTCC730. C. albicans MTCC183 was inhibited by the crude extracts of Xylaria sp. and Phomopsis sp. but the other fungal isolates had no effect on the test fungus.

The reducing power of ethanolic extract of the endophytic fungi showed significant activity but was lower as compared to ascorbic acid (Fig. 2). The reducing powers for the metabolites of different endophytes were in the order of Phomopsis sp.>Xylaria sp.> Diaporthe sp.>Epacris sp.

The highest scavenging activity was shown by Phomopsis sp., and minimum was by Epacris sp. The free radical scavenging activities of the ethanolic extracts were found to be in the order of Phomopsis sp.>Diaporthe sp.>Xylaria sp.> Epacris sp. Variation was observed in IC50 values (concentration of sample required to scavenge 50% of free radicals) of ethanolic extract of different endophytic fungi and ascorbic acid (Table 3).

The TPC of endophytic fungal ethanolic extracts have been expressed as gallic acid equivalent i.e., mg gallic acid/g dry wt. A high phenolic content (12.5 ± 0.16) was found in Xylaria sp. and decreased in the order of Xylaria sp.>Phomopsis sp.>Diaporthe sp.>Epacris sp. (Table 4). Results showed that the levels of phenolic compounds in different endophytic fungi were significantly (p < 0.05) different from each other.