Antimicrobial Bioactivity and GC-MS Analysis of Different Extracts of Corchorus olitorius L Leaves

Results Crude extracts of Corchorus olitorius L leaves and their TLC-separated components demonstrated bioactivity against Staphylococcus aureus (14 mm), Streptococcus pneumoniae (16 mm), and Escherichia coli (11 mm) but neither against Candida albicans nor Mycobacteria tuberculosis. However, the overall zones of inhibition were smaller compared to the positive control (≥18 mm). GC-MS analysis of the active components revealed the presence of methyl esters. Conclusion Corchorus olitorius L is bioactive against both Gram-negative and Gram-positive bacteria but neither against fungi nor mycobacteria. The bioactivity is attributable to the presence of methyl esters. Since methyl esters already have proven bioactivity in some studies, they could be further studied and optimized for possible pharmaceutical use. Further, to provide a more comprehensive antimicrobial spectrum of Corchorus olitorius L in Uganda, purified active components could be investigated using a wider range of organisms.


Introduction
Plants offer an inexhaustible source of bioactive compounds and clinically useful drugs for infectious diseases, cancer as well as cardiovascular disorders [1,2]. Bioactive compounds play an immense role in drug discovery [3,4] beginning with bioactivity screening of crude extracts followed by fractionation to isolate the active compounds [5,6]. Regrettably, there has been limited pharmaceutical development of the plants with known bioactivity with a few pharmaceutical products for infectious diseases [7]. However, the increasing antimicrobial resistance to the currently available antimicrobial agents demands intense investigations into the antimicrobial properties of medicinal plants [8,9].
Corchorus olitorius L (C. olitorius), commonly known as jute mallow, belongs to the genus Corchorus and the family of Tiliceae [10]. It is a traditional medicinal vegetable worldwide [11]. e vegetable is propagated by seed as well as accepted as a wild plant in crop fields [10]. It has simple, finely indented leaves and small yellow flowers having five petals [10]. e vegetable is rich in vitamins A, B 1&2 , C, and E; fiber as well as minerals like calcium and iron [12,13]. e traditional medicinal uses of C. olitorius amongst various communities comprise the treatment of heart failure, gastric ulcers, typhoid fever, malaria, gonorrhea, common colds, tumors, and measles [10,14]. e vegetable also has antiviral [15], antioxidant [16], gastroprotective, and antidiabetic properties [14,17].
Although C. olitorius is used for infectious diseases, there are limited data regarding its antimicrobial spectrum in Uganda. To explore the antimicrobial spectra of C. olitorius, we investigated its bioactivity against Candida albicans (C. albicans), Staphylococcus aureus (S. aureus), Streptococcus pneumoniae (S. pneumoniae), Escherichia coli (E. coli), and Mycobacteria tuberculosis (MTB). C. olitorius was active against Gram-positive and Gram-negative bacteria.

Aim, Study Design, and Setting.
To investigate the bioactivity of C. olitorius, a laboratory-based experimental study was conducted at the Department of Medical Microbiology, Makerere University College of Health Sciences. e plant extraction process was done at the Department of Pharmacology and erapeutics, Makerere University College of Health Sciences.

Plant Collection and
Processing. C. olitorius (2 kg) leaves were harvested from Ayer village, Barapwo parish, Lira subcountry, Lira district (Northern Uganda) and taken to the Department of Pharmacology and erapeutics, Makerere University College of Health Sciences. A voucher specimen was deposited at a herbarium at the Department of Botany, Makerere University Kampala, Uganda (#50906). e leaves were washed clean and spread to dry at room temperature to a constant weight (900 g). After drying, the leaves were ground to powder and extracted using the serial solvent extraction method as described by Das et al. [18]. Diethyl ether, methanol, and distilled water were used as solvents according to their order of polarity. is was done to extract compounds with a wide range of polarity. Briefly, 500 g of ground dried leaves of C. olitorius were soaked in 3 L of diethyl ether (BDH AnalaR) and tightly closed in a flat bottomed conical flask while shaking every 6 hours for 48 hours. ereafter, the resultant solution was filtered using a Whatman filter paper (No. 1) using a funnel and the filtrate was concentrated using a rotary evaporator at 20-30°C. e residue was spread and allowed to dry at room temperature. After which, it was soaked in 3 L of methanol (UltraPure Solutions, Inc. 11485, Commercial Parkway, Castroville, CA 95012) and treated as mentioned above. e last residue was soaked in 3 L of distilled water while shaking every 6 hours for 48 hours and the resultant solution was also filtered using a Whatman filter paper (No. 1) and freeze-dried. After evaporation of the solvents, the extracts were accordingly labeled and stored in a refrigerator at −80°C.
For the bioactivity assay, 0.3 g each of the diethyl ether and methanol crude extracts were dissolved independently in 1 ml DMSO and made up to 10 ml using distilled water while 0.3 g of the aqueous crude extract was dissolved in 10 ml of distilled water to make stock solutions. 100 μl (3000 μg) of each crude extract (stock solution) was used to test for the bioactivity of C. olitorius against the organisms used in this study.

Culture Technique.
e agar well diffusion technique of culture and sensitivity testing was used [19,20].

Microbial Culture Procedure
(1) Bacterial culture. e culture media containing plates were briefly heated in an oven at 100°C (∼5 minutes) to remove any residual moisture. Colonies of S. aureus and E. coli were diluted to a turbidity of 0.5 McFarland standard [21] using normal saline and aseptically inoculated on welllabeled culture plates containing MHA. A sterile swab was then used to evenly spread the organisms on the culture plates. ereafter, wells were dug in the culture plates using a sterile cork (6 mm) and 100 μl (3000 μg) of each crude extract was accordingly pipetted into the wells. S. pneumoniae was likewise diluted to 0.5 McFarland standard [21] and aseptically inoculated on culture plates containing chocolate agar media and evenly spread using a sterile swab. ereafter, wells were dug in the culture plates using a sterile cork (6 mm) and 100 μl (3000 μg) of each extract was accordingly pipetted into the wells. 100 μl of distilled water served as the negative control while chloramphenicol (5 μg) served as a positive control for all tests. Finally, all the culture plates were placed up-right in a CO 2 incubator at 37°C for 24 hours. At the end of the incubation period, the culture plates were removed and examined for microbial growth inhibition by viewing under natural light. e inhibitory zones were measured in mm using a ruler. All the experiments were performed in duplicates. e crude extracts displayed bioactivity.

e Scientific World Journal
(2) Fungal culture. To examine the effects of C. olitorius extracts on fungal growth, 100 μl (3000 μg) of each extract was independently added to 15 ml of molten SDA; mixed, poured on a well-labeled culture plate, and allowed to solidify. To the negative control plate, neither extract nor C. albicans was added while the positive control plate had only agar. ereafter, the fungi (C. albicans) were aseptically and evenly inoculated on all the culture plates (except the negative control) which were thereafter placed in a CO 2 incubator at 37°C for 18-24 hours. At the end of the incubation period, the culture plates were removed from the incubator and inspected for fungal growth inhibition under natural light. ere was no fungal growth inhibition.
(3) Mycobacterial culture. To scrutinize the bioactivity of C. olitorius against MTB, the crude extracts mentioned above were sterilized using 0.22 μm syringe-driven filters. e 7H11 media plates were brought to room temperature having been stored at 2-8°C and inoculated with 0.5 ml of H37Rv 1.0 McFarland standard strain. ereafter, wells were dug in the media plates using a cork and 100 μl of each extract was loaded. To the negative control plate, neither H37Rv was inoculated nor extract added whereas for the positive control, the plates were inoculated with H37Rv but no extract was added. All the plates were incubated in a CO 2 incubator for 21 days and the growth of mycobacteria was inspected. No growth inhibition was exhibited.

TLC Separation of the Crude Extracts of C. olitorius Leaves.
To identify the components of C. olitorius responsible for its bioactivity, the methanolic and diethyl ether crude extracts of C. olitorius were subjected to thin layer chromatography (TLC). TLC plates (DC-Fertigfolien ALUGRAMR Xtra SIL G/UV254; MACHERY-NAGEL GmbH & CO. KG-Germany, 20 × 20 cm pre-coated (0.2 mm) with silica gel 60) were cut to a smaller size of 5 × 10 cm using a pair of scissors and used following a method described by Kagan and Flythe [22] with minor modifications. Specifically, instead of using a solvent ratio of 4 : 1 (ethyl acetate (Sigma Aldrich): methanol (BDH)), we used a ratio of 3 : 1 and in place of cutting the separated bands to use them as bio-discs, we scrapped off the bands from the TLC plates and dissolved them in 2 ml of DMSO. e TLC plates (5 × 10 cm) were first cleaned by placing them in a beaker containing the eluent (20 ml). e beaker was covered with an aluminum foil and the eluent was allowed to elute until the solvent front reached the top of the plate. ereafter, the plates were removed, allowed to dry, and checked for the presence of any bands. e absence of any bands indicated that the plate was clean and ready for use. en, 5 μl (150 μg) of each extract (stock solution) was independently spotted on the left and right-hand side of the TLC plates upon a line marked using a pencil and allowed to dry. A small volume (50 ml) of the eluent (ethyl acetate: methanol (3 : 1)) was poured into a 500 ml beaker, covered with filter papers, and allowed to saturate. en, the loaded (spotted) TLC plates were carefully placed into the beaker containing the eluent ensuring that the eluent was below the marked line and that the TLC plates did not touch each other. e beaker was then covered with filter papers and allowed to stand for 20-30 minutes while the elution was taking place. When the solvent front was almost reaching the top of the TLC plates, the plates were removed from the beaker and allowed to dry. e TLC plates were then checked for the presence of any bands visible under natural light. e bands were marked and labeled using a pencil starting with the first band from the spot. ereafter, these bands were carefully scrapped off the TLC plate and dissolved into 2 ml DMSO. A total of 8 bands (4 TLC plates) of each formed band were dissolved in the DMSO (2 ml).

Bioactivity Testing of the TLC Separated Components.
e resultant solutions (following TLC separation) were accordingly labeled and also assayed for bioactivity as described above (see bacterial culture). 100 μl (∼50 μg) of each solution (band) was pipetted into wells dug in the culture plates inoculated with the test bacteria as described above (see bacterial culture). e culture plates were also placed in a CO 2 incubator for 24 hours and observed for bacterial growth inhibition. e zones of inhibition were measured in mm using a ruler. e components portrayed bioactivity.

GC-MS Analysis of C. olitorius Components.
To establish the chemical composition of the bands obtained by the TLC that revealed bioactivity, GC-MS analysis was performed.
is was done at the Department of Chemistry, Government Analytical laboratories, Wandegeya, Kampala, Uganda, as follows: 100 μl (∼50 μg) of the solutions of the separated C. olitorius components were pipetted into separate vials. From each vial, 1 μl (0.5 μg) of the solution was injected into the GC-MS machine (Shimadzu QP2020 NX; Restek column dd5, 0.25 mm thickness) using hydrogen as a carrier gas (1.3 ml/min). e GC oven was held at 80°C and then increased by 4-6°C until 300°C and held for a minimum of 20 minutes. e identification of the compounds in each sample was based upon the mass spectral database in the MS library [23].

Ethical
Approval. Permission to conduct the study was secured from the Mbarara University of Science and Technology-Research and Ethics Committee (MUST-REC), e Uganda National Council for Science and Technology (UNCST), and the administrators of the respective departments.

Bioactivity of C. olitorius Crude Extracts and eir
Components. To assess the bioactivity of C. olitorius, the diethyl ether, methanolic, and aqueous crude leaves extracts of C. olitorius were tested against E. coli, S. aureus, S. pneumoniae, C. albicans, and MTB. C. olitorius inhibited bacterial growth but had neither effect on C. albicans or MTB (Table 1). C. olitorius leaves crude extracts were also separated into individual components using TLC plates and e Scientific World Journal each component was examined for bioactivity. All components displayed bioactivity. However, the overall growth inhibition was less compared to the positive control. Among the crude extracts, the diethyl ether extract exhibited the largest zone of inhibition against S. aureus (14.00 mm) and E. coli (11.00 mm) whereas the aqueous extract displayed the largest zone of inhibition against S. pneumoniae (19.00 mm). e methanolic crude extract showed moderate inhibitory zones against all the bacteria (11.00 mm, 11.50 mm, and 9.50 mm for S. aureus, S. pneumoniae, and E. coli, respectively). e positive control demonstrated the highest inhibition with 20.00 mm, 23.00 mm, and 18.00 mm zones of inhibition for S. aureus, S. pneumoniae, and E. coli, respectively. e negative control did not reveal any inhibition.
e results of this study were comparable to the findings of Ilhan and others who conducted a study in Turkey [24] during which different extracts of the C. olitorius showed bioactivity against E. coli, S. aureus, and Y. enterocolitica. In contrast to the findings of Ilhan et al. [24] however, where some fungal species were responsive to the extracts of C. olitorius (although most of the fungi were resistant), none of the extracts in the current study demonstrated bioactivity against C. albicans. In another study conducted by Sumengen Ozdenefe et al. [25], only the hexane extract demonstrated bioactivity against S. aureus and B. subtilis. ese findings indicate that C. olitorius is bioactive against bacteria but has limited activity against fungi. In the current study, the most responsive organism to the inhibitory effects of C. olitorius was S. pneumoniae with the aqueous extract demonstrating the highest degree of inhibition (19.00 mm) followed by the diethyl ether extract (16.00 mm) while the methanolic extract was the least bioactive (12.00 mm). is finding contradicts Ilhan et al. [24], where the petroleum ether extract of C. olitorius was the most bioactive against the organisms they tested. In the study conducted by Sumengen Ozdenefe et al. [25], only the hexane extract of C. olitorius demonstrated activity against B. subtilis. e other organisms (S. aureus and S. epidermidis) were resistant to the rest of the extracts (methanol, ethanol, hexane, and chloroform) tested.
Nevertheless, the methanolic extract of the current study showed activity against S. aureus. Zakaria et al. assayed C. olitorius to assess its in vitro activity against bacteria and found the methanolic extract active against C. diphtheriae and K. rhizophila while the chloroform extract demonstrated activity against S. aureus [26]. In the current study, all extracts tested showed activity against S. aureus including the methanolic extract unlike the findings of Zakaria et al. In related studies by Adegoke and Adebayo et al. [27] and Abir et al. [28] as well as Hayyawi [29], C. olitorius demonstrated antibacterial activity comparable to the present study. In the current study, C. olitorius demonstrated a broad spectrum nature of antibacterial activity comparable to the findings of Pal et al. [30].
To identify the bioactive components of C. olitorius responsible for its bioactivity demonstrated by the crude extracts, the diethyl ether and methanol crude extracts' components were separated using TLC. e diethyl ether extract was separated into 5 (five bands) although the 4th and 5th bands were poorly separated and were thus tested together while the methanol extract was also poorly separated into 2 (two) bands. e separated bands were assayed for bioactivity using the agar well diffusion method as described above (bacterial culture). All components showed antibacterial activity against E. coli and S. pneumoniae, while only ether bands 1 and 2 showed activity against S. aureus ( Table 2). Bands ether 1 and 2 demonstrated bioactivity against all the bacteria tested (S. aureus (10.00 mm), E. coli (12.00 mm), and S. pneumoniae (12.00 mm)). is suggested that the antibacterial activity of the diethyl ether extract against these organisms was due to the components of bands ether 1 and 2. Bands ether 3 to 5, did not show bioactivity against S. aureus but against E. coli (10.00 mm) and S. pneumoniae (12.00 mm). is indicated that these components were responsible for their bioactivity against these organisms. e methanol bands showed bioactivity against only E. coli (10.00 mm) and S. pneumoniae (12.00 mm). is suggested that bioactivity against S. aureus required all components of the methanol extract while bioactivity against E. coli and S. pneumoniae only required the   components present in the bands of the methanolic extract. e bioactive properties of C. olitorius can be attributed to the presence of phytochemicals such as alkaloids which have antibacterial activity [31]. e positive control revealed the highest level of growth inhibition while the negative control did not indicate any inhibition in all the bioassays.

Chemical Composition of the Bioactive Component of C. olitorius Leaves Extracts.
To identify the chemical composition of the components of C. olitorius that demonstrated bioactivity, GC-MS analysis of each bioactive component was performed. e results revealed the presence of methyl esters such as hexadecanoic acid, 9-octadecenoic acid (z), and methyl stearate (Figures 1 and 2 and Table 3). e methanol bands revealed the presence of hexadecanoic acid and 9-octadecenoic acid (Figure 1). e ether bands also revealed the presence of hexadecanoic acid and methyl stearate (Figures 2(a)-2(d)). Table 3, the composition of the major peaks revealed by the GC-MS analysis is shown. is was in contrast to the findings of Hassan and others who identified cedrane 5-one and c-terpinene as the major bioactive components of C. olitorius in a study conducted in Egypt [32]. In addition, a related study by Al-Yousuf et al. [33] showed the presence of hexadecanoic acid and 2,4-di tert butyl phenol in the leaves of C. olitorius. is partly concurs with the current study which also indicated the presence of hexadecanoic acid. Further, an additional study by Driss et al. in Tunisia [34] found benzaldehyde to be the major bioactive compound in C. olitorius leaves in contrast to the present finding. ese differences could be attributed to the locations and the harvest season of the plant. e findings of the current study were partly consistent with those of Hanan and others who found hexadecanoic acid in the leaves of C. olitorius [35]. Methyl esters such as hexadecanoic acid, 9-octadecenoic acid, and methyl stearate are reported to have antimicrobial activity [36][37][38]. In a study conducted by Johannes and Litaay [39], hexadecanoic acid was found to have antibacterial activity. All these findings support the antibacterial activity of C. olitorius in the current study.

Conclusion
C. olitorius is bioactive against both Gram-negative and Gram-positive bacteria but neither against fungi nor mycobacteria. It is more active against S. pneumoniae. e bioactivity is due to the presence of methyl esters. Since methyl esters have proven bioactivity in some studies, they could be further studied and optimized for possible pharmaceutical use. Further, to provide a more comprehensive antimicrobial spectrum of C. olitorius in Uganda, purified active components should be investigated using a wider range of organisms.

Abbreviations
Colitorius: Corchorus olitorius L DMSO: Dimethyl sulfoxide TLC: in layer chromatography REC: Research and ethics committee UNCST: Uganda National Council For Science And technology.

Data Availability
e data generated during the study are available from the corresponding author upon reasonable request.
Ethical Approval e study was approved by the REC of Mbarara University of Science and Technology and the Uganda National Council for Science and Technology (UNCST).

Conflicts of Interest
e authors declare that there are no conflicts of interest.

Authors' Contributions
RN conceived the idea and spearheaded the study design and data collection, analyzed the data, and made the first draft of the manuscript. SBA participated in data collection, analysis, and wrote the manuscript. FB had oversight over microbiology and manuscript writing. CDS monitored chemistry e Scientific World Journal 7 data collection and participated in writing of the manuscript. JO and PA provided general intellectual input and supervision right from the inception of the idea, data collection, and manuscript writing. All authors read and approved the final manuscript.