Antimicrobial Activity and Biochemical Profiling of Selected Medicinal Plants against Blood Cancer Clinical Isolates

1Department of Biochemistry, Faculty of Science, King Abdulaziz University, Jeddah, Saudi Arabia. 2Department of Biological Sciences, Faculty of Science, King Abdulaziz University, Jeddah, Saudi Arabia. 3Department of Botany, Faculty of Science, Govt: College University (Women) Faisalabad, Pakistan. 4Department of Bioinformatics & Biotechnology, Government College University Faisalabad, 38000, Pakistan.

susceptible to almost any type of infection, especially bacterial and fungal infections. As well as the infections complications remain an important cause of mortality and morbidity between these highly risk and infectious cancer cases.
The heavy antibiotics usage especially in high risk cancer patients cause a selection pressures that result in the emergence of resistant microorganisms. Currently, many cancer centers have highlighted the fact that an increase in quinolone resistant bacteria (primarily Escherichia coli and Pseudomonas aeruginosa) in patients receiving quinolone prophylaxis. The common use of broad spectrum agents like carbapenems has been linked with the development of multidrug resistant (MDR) in Stenotrophomonas maltophilia and Pseudomonas aeruginosa. Thus, the increase in antibiotic resistance activity is posing an everincreasing therapeutic problem in cancer patients and the ways by which bacteria overcome drug action are various and multiple, ranging from intrinsic impermeability to acquired resistance 3,4 .
Rapid spread of resistant clinical isolates in cancer cases indicates the high need to find new antimicrobial agents is of supreme importance for the treatment of infectious diseases. Due to rising of the resistant microorganisms to antibiotics and the price of contemporary allopathic medicines, the scientists are studying various medicinal plants, because of their safety, cost effectiveness and successful therapeutic measure against a wide range of antibiotic resistant microorganisms 5,6,7 .
A huge section of the world population depends on the traditional systems of medicine to treat a range of diseases. Researchers are increasingly turning their concentration to the medicinal plants. Medicinal plants occupy important position in conventional and modern system of medicines due to their low toxicity for both human and animals. The key benefits of using plant derived medicines are that they are relatively safer than synthetic alternatives, offering valuable therapeutic measures and more affordable treatments 8,9 . The scarcity of infective diseases in wild plants is in itself a sign of the successful defense mechanism developed by them.
Plants develop defense mechanisms against diseases due to the presence of a large number of alkaloids, phenols, terpenes derivatives compounds and other antimicrobial compounds makes the essential oils from plants more précised in their mode of action against the wide variety of pathogenic microorganisms. Hence, the essential oils could be used as better supplements or alternatives against the pathogenic microorganisms 10 . Keeping in view, the present study was designed to assess and compare the in vitro antimicrobial activity of medicinal plants used in Saudi Arabia against clinical bacterial isolates of human blood cancer cases and biochemical profiling through qualitative and quantitative analysis of phenolic acids from these medicinal plants by High performance liquid chromatography (HPLC).

Selection of medicinal plants for this study
Five medicinal plants were collected from different regions of Saudi Arabia for this study ( Table 1). The collected plants were identified in the laboratory by comparison of flora which made according to different references concerning with the medicinal plants (Royal Botanic Gardens Victoria, Indiana Native Plant and Wildflower Society).

Microorganisms
Fourty Clinical slants samples obtained from patients with infection were received from the radiotherapy unit of King Abdul Aziz Medical city, Jeddah, Saudi Arabia. These bacterial cultures were isolated from different blood cancer patients undergoing radiotherapy treatment. All the microorganisms were identified using Analytical profile index (API) system with biomerieux vitek 2. Bacterial strains Salmonella group B, Corynebacterium, Staphylococcus aureus, Klebsiall pneumonia and Streptococcus viridian were chosen for further study on the basis of preliminary analysis.

Preparation of Plants Crude Extract
Dried plants powder (25mg) was taken in 100 ml of 99.8% methanol in a conical flask, plugged with sterile cotton. The samples were placed for 24 hours in shaker with 37 o C and for another 24 hours in room temperature 11 . The extracts were then filtered using Whatman No. 1 filter paper. The extracts were evaporated using rotary vacuum evaporator to dryness under reduced pressure at 60 o C by a rotary evaporator.
After vacuum evaporation, the plant extracts were dissolve in 0.25% Dimethyl Sulphoxide (DMSO), which is maximum volume of DMSO that could be used to dissolve solid extracts, and stored at 4 o C for further use 12 . The solvent DMSO (2.5%) that would not inhibit growth of the microorganisms was used as the negative control for all the experiments 13 .

Standard Antibiotic Activity Assay
Standard antibiotic discs (Ciprofloxacin) were placed on the surface of a Mueller-Hinton agar that has been inoculated with test microorganisms. During incubation, the antibiotics diffuse outward from the discs creating a concentration gradient which appeared as inhibition zone around these disks. Inhibition zone diameters (mm) were read after 18 h of incubation at 35 o C.

Antimicrobial Activity of Plant Extracts by Paper Disk Diffusion Assay
A suspension of testing microorganisms was spread on Muller Hinton Agar (MHA) medium. The sterile filter paper discs (5mm in diameter) was placed on the agar plates which was inoculated with the tested microorganisms and then impregnating with 800-1000¼l of plant extract were made in the agar plate with forceps then plates were incubated at 37 o C for 18-24 hours. The antibacterial activity of the plant extract was determined by measuring the radius from the middle (center) of the disc to the edge of the zone. The antibacterial assay for each of the extracts against all microorganisms tested was performed in triplicates. The experimental details described earlier were follows to perform antimicrobial activity tests 14 .

Biochemical profiling of phenolic acids by High Performance Liquid Chromatography (HPLC) Plant Extraction
The extraction of the phenolic acids from the seeds of Fenugreek, leaves of basil, leaves of olive, leaves of mint and seeds of Frankincense were determined according to earlier described method 15,16 with some modification. The fresh leaves (200 g) of plant materials were shade dried and crushed to coarse powder. The powder (20 g) was macerated with 25 ml distilled water of 2 N-HCl and heated in water bath for 1 h at 100 o C using air condenser and filtered. The filtrate was extracted with diethyl ether using separating funnel. The diethyl ether layer was washed with distilled water, dried over anhydrous sodium sulphate and evaporated using rotary vacuum evaporator at 25 o C to obtain extract. The collected extract was re-dissolved in known amount of (5 ml) HPLC grade methanol. Prior to the injection into HPLC column the sample was filtered through 0.22µm organic filter (Millipore).   Gallic acid, Parahydroxy benzoic acid, Vanillic acid, Syringic acid and Ferulic acid were analyzed in this study and the detector response for individual phenolic compound was calibrated with authentic standard phenolic acids. All the standard phenolics were procured from Sigma-Aldrich Chemical Company, USA.
The statistical significance of the antibacterial tests was determined. All experiments were conducted in triplicate and the statistical test that generate mean values was used. The resulting data is presented in tabular form. For statistical analysis, OriginLab Origin Pro (version 9.0) was used and the P value < 0 .05 was considered as significant.

Evaluation of Antimicrobial Potential of selected Medicinal Plants
Antimicrobial activity of all five medicinal plant extracts in methanol and ethanol are presented in Table 2. The value represent zone of inhibition (mm) Mean ± Standard Error. 800µg of extract for all discs. (E) Ethanol, (M) Methanol, ND: No inhibition zone, Ciprofloxacin was used as positive control.
The methanol extracts of Boswellia sacra, Trigonella foenum-graecum and Ocimum basilicum presented higher activities than ethanol extracts i. e., Boswellia sacra showed the maximum antibacterial activity against Streptococcus viridian with 12.4 mm inhibition zone. Trigonella foenumgraecum showed the maximum antibacterial activity against Salmonella Group B 11.8 mm with crude extracts in methanol. The highest effect of ethanol extract was found against Staphylococcus aureus with 7.75 mm inhibition zone. The largest inhibition zones of Trigonella foenum-graecum were observed for methanol extract against Corynibacteria 11.5 mm ( Figure 1) and Salmonella Group B 11.8 mm (Figure 2).
The largest inhibition zones (3mm) of Ocimum basilicum were observed for methanol extract against Corynibacteria. On the other hand, the ethanolic extract of Mentha longifolia and Olea europaea showed higher activities than methanolic extract. The largest inhibition zones of Mentha longifolia were observed for ethanol extract against Staphylococcus aureus 7mm and Corynibacteria 4mm. The highest effect of Methanol extract against Streptococcus viridian 3.6mm. While, the largest inhibition zones of Olea europaea were observed for ethanol extract against Corynibacteria 4 mm and Staphylococcus aureus 9mm. The highest effect of methanol extract against Streptococcus viridian 4mm and Corynibacteria 3 mm.
The antimicrobial effect of the medicinal plants is well documented. The results of different studies provide evidence that some medicinal plants might indeed be potential sources of new antibacterial agents even against some antibioticresistant strains 17,18 . The antimicrobial effect of three species of Boswellia against eleven different bacterial strains including Corynibacterium, Staphylococcus aureus, Salmonella typhi and Klebsiella pneumoniae were studied previously and they found that the antibacterial activity mainly against the Gram-positive bacteria 19 . They observed the same interesting fact that the multiresistant staphylococcus strains showed great sensitivity to investigated plant extract supporting the results of this study. Highest antimicrobial activity against Salmonella, Klebsiall pneumonia and Staphylococcus aureus with essential oil of Mentha longifoli was recorded supporting the data of this study as described earlier 20 . Trigonella foenum-graecum was giving inhibition zone in the range of 2.3 -6.4 mm for ethanol and 1.0 -11.8 mm for methanol crude extracts. Trigonella foenum-graecum crude extract of methanol was found very effective compared to the antimicrobial effect of Ciprofloxacin (6 mm) against Gram negative (Salmonella B) and Gram positive (Corynibacterium and Streptococcus viridian) studied the antibacterial effect of Olea europaea with number of solvent include water, ethanol, methanol, Ethyl acetate, n-Hexane, n-Hexane and Diethyl ether and it recorded antibacterial effect of Olea europaea leaves against Klebsiella pneumonia, Salmonella and Staphylococcus aureus while, no effect on Salmonella was recorded 21 . All plants in this study (Boswellia sacra, Ocimum basilicum L, Mentha longifolia L., Trigonella foenum-graecum L and Olea europaea L) showed antimicrobial activity against different types of bacteria but the differences may be probably due to different environmental and genetic factors, different chemotypes and the nutritional status of the plants as well as other factors that can influence the oil composition 22 .

Qualitative and Quantitative Analysis of Phenolic Acids by HPLC
Qualitative and quantitative analysis of phenolic acids from five medicinal plants by HPLC are presented in Table 3 accordingly. Gallic acid and Ferulic acid were detected in all tested plants with different concentration. The highest concentration of gallic acid and ferulic acid were found in Ocimum basilicum 547.02 ng/g and 236.75 ng/g, respectively. Parahydroxy benzoic acid was found in all tested plant except Boswellia sacra and the highest concentration was detected in Olea europaea 797.8 ng/g. While, the highest concentration of vanillic acid and syringic acid were found in Mentha longifolia174.02 ng/g and 21.76 ng/g, respectively.
Phenolic acids have important biological and pharmacological properties and may be benefit for human health. From ages, these biochemical compounds are important components of the human food, due to their antioxidant activity, their potential to reduce oxidative stress, preventing tissue damage and resultant chronic diseases particularly for anticancer activities 23,24 . Gallic acid and Ferulic acid were also identified and quantified in ethanol extract previously 25 . The crude extracts of Mentha longifolia and Mentha spicata contained gallic acid compounds while those extracts differed in their content of other studied phenolic compounds 26 . In the ethanol extract of Mentha longifolia, Ferulic acids were identified in the aerial parts extract, but they were in very low concentration to be quantified 27,28 . Analysis of data by HPLC recorded that pararhydroxy benzoic acid was the phenolic acid with concentration 797.8 ng/g followed by gallic acid 397.91 ng/g in Olea europaea crude extract. The presence of phenolic compounds in olive leaves including phenols (tyrosol, hydroxytyrosol, vanillin, vanillic acid, and caffeic acid) and oleuropein were reported 29 . In olive fruit, Vanillic acid, Syringic acid, Gallic acid and Ferulic acid were reported earlier 30,31 . Phenolic acids are quite susceptible to degradation under environmental stress (pH, temperature, light and oxygen) that explain the differences between the studies 32,33,34 .

CONCLUSION
The antibacterial activity showed that Streptococcus viridian and Corynebacterium were more inhibited bacteria but Klebsiall pneumonia was found more resistant. Boswellia sacra and Trigonella foenum-graecum showed great antimicrobial potential against clinical bacterial isolates from cancer patients. Total phenolic analysis by HPLC revealed that Gallic acid and Parahydroxy benzoic acid were the major phenolic acid found among all the tested medicinal plants and may serve as antimicrobial agent against clinical bacterial isolates from cancer patients successfully. Based on the findings of this study it could be recommended that the extracts of these plants should be further analyzed to isolate the specific antibacterial compounds and defense mechanisms in them and speedy clinical trials should be carried out to explore the pharmaceutical potential of medicinal plants in the treatment of bacterial and fungal infectious diseases.