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Research Detail

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A. T. M. Nahid Hasan
Department of Microbiology, Stamford University Bangladesh, 51, Siddeswari Road, Dhaka-1217, Bangladesh

Trisha Saha
Department of Microbiology, Stamford University Bangladesh, 51, Siddeswari Road, Dhaka-1217, Bangladesh

Tasnia Ahmed*
Department of Microbiology, Stamford University Bangladesh, 51, Siddeswari Road, Dhaka-1217, Bangladesh

To combat the infections caused by antibiotic resistant bacteria, natural candidates are being studied to find out antibacterial activity against the drug-resistant microorganisms. Among the variety of natural candidates of plant origin, many fruits have been proved to have potent antibacterial activity. In the current study, we chose pineapple (Ananas comosus), and pomelo (Citrus maxima) to determine their efficacy against some clinical isolates. Fruit samples were subjected to prepare crude, ethanol, methanol and aqueous extract to determine their antibacterial potency. Clinical isolates were used to determine the antibacterial activity of the extracts against them. The isolates were found to be multidrug resistant. Out of twenty-eight antibiotics, Pseudomonas aeruginosa was resistant to ten antibiotics and Salmonella spp. was resistant to nine antibiotics. Rather than the crude extracts of the fruits, ethanol and methanol extracts showed antibacterial activity towards multi-drug resistant pathogenic bacteria. Aqueous extract did not show any significant antibacterial activity at all. Extracts of pomelo fruit exhibited the highest results whereas pomelo skin and pineapple peel crude extracts were the least effective compared to the other extracts. Ethanol extract of pineapple fruit (against all isolates but Staphylococcus aureus) and methanol extract of pomelo fruit (against all isolates) showed the lowest MIC (minimum inhibitory concentration) of 187.5 µg/ml. MBC (minimum bactericidal concentration) was found (within the range of 500 µg/ml to 1000 µg/ml) only with ethanol and methanol extracts of pomelo and pineapple. As the clinical isolates were found to be inhibited by the extracts, they can be used as an alternative for treating infections caused by these bacteria.

  Antibacterial activity, Antibiotic resistance, Extracts, Minimum Inhibitory Concentration, Minimum Bactericidal Concentration.
  Different markets of Dhaka city, Bangladesh
  00-09-2020
  00-12-2020
  Pest Management
  Bacteria, Pineapple

The aim of the study was to detect the antibacterial potency of pineapple (Ananas comosus), and pomelo (Citrus Maxima). Besides using the crude samples, ethanolic, methanolic, and aqueous extracts of both the fruits and their peel were used to determine their antibacterial activity. Minimal inhibitory concentration (MIC) and minimal bactericidal concentration (MBC) were also determined after confirming the antibacterial traits of these extracts against five different pathogenic multi-drug resistant bacteria collected from clinical samples. 

Study area and sampling. For detection of antibacterial activity of some natural products, five clinical bacterial isolates (Klebsiella pneumoniae, Escherichia coli, Pseudomonas aeruginosa, Staphylococcus aureus, and Salmonella spp.) were selected. Two local fruit samples pineapple (Ananas comosus), and pomelo. (Citrus maxima), were collected from different markets of Dhaka city, Bangladesh for detection of antibacterial activity against the selected clinical bacterial isolates. Both fruit and the peel of the fruit have been used for this study. The experiment was carried out during the time span of September 2020 to December 2020 in the microbiology laboratory of the Department of Microbiology, Stamford University Bangladesh.

Antibiotic susceptibility test of the pathogenic isolates. For the detection of antibiotic resistance traits of the clinical isolates, twenty-eight antibiotics commonly in use were selected. Meropenum (MME 10µg), Ceftazidime (CAZ 30µg), Cefuroxime (CMX 30 µg), Amoxyclav (AMC 30 µg), Amoxicillin (AX 25 µg), Azithromycin (AZM 15 µg)), Cefixime (CFM 30 µg), Ciprofloxin (CIP 5 µg), Colistin (CO 30 µg), Doripenum (DOR 10 µg), Doxycycline (DO 30 µg), Fusidic acid (10 µg), Gentamycin (GN 10 µg), Amikacin (AK 30 µg), Cephradine (CE 30 µg), Vancomycin (VA 30 µg), Teicoplanin (TEC 30 µg), Cotrimazole (COT 30 µg), Piperocillin/Tazobactam (PTZ, PIT 30 µg), Nitrofurantion (F 300 µg), Nalidixic acid (NAL 30 µg) Impenem (IPM 10 µg), Levofloxacin (LE 5 µg), Linezolid (LZD 30 µg), Clindamycin (CN 10 µg), Cefepime (CPM 30 µg), Tigecycline (TGC 15 µg) and Ceftriaxone (CRO 30 µg). Kirby Bauer disc diffusion method (22) was followed for the antibiotic drug resistance test. Using CLSI guidelines (23) the zone sizes were measured and determined the strains as sensitive or resistant. 

 Sample processing. The fruit samples were washed vigorously first with tap water and then with distilled water several times to wash out all kinds of impurities. Crude extracts were prepared by blending 10 g of the raw fruits and fruit peel separately with 90 ml saline. Before extraction, raw samples were shed dried for a week after cutting into small portions to make it all dry followed by blending to get a fine powder. The dried powder samples were then further processed for extract preparation.

Preparation of solvent extracts. About 20 g of each dried and powdered fruit and peel samples were mixed with 80 ml of 95% ethanol, methanol, and water separately in sterilized glass bottles followed by incubation at 37oC for 48 hours in shaking condition. After 48 hours, the ethanol, methanol, and aqueous extracts of all of these fruit and peel extract samples were filtered through sterilized cheesecloth and then through Whatman filter paper. Extracts were then concentrated by keeping them in evaporator and kept at 4oC until use as stock solution.

Determination of antibacterial activity of the extracts (crude, ethanolic, methanolic , and aqueous extracts). Bacterial suspensions were prepared until they reach McFarland turbidity standard (108 CFU/ml) and bacterial lawn was made using sterile cotton swab on the Muller Hinton agar media. Crude, ethanol, methanol, and aqueous extracts (100 µl each) of pineapple, pineapple peel, pomelo, and pomelo peel were placed into the well made in the media. Plates were then kept in the refrigerator in an upright position for better absorption for 20 to 30 minutes and then incubated at 37oC for 24 hours (25). Plates were observed for the presence of zone of inhibition after incubation and measured in mm.

Determination of MIC and MBC. Extracts of the samples were diluted in the concentrations of 500 µg/ml, 250 mg/ml, and 125 mg/ml with sterile nutrient broth followed by addition of 0.2 ml bacterial suspensions in each tube. After incubated at 37oC for 24 hours, tubes with no visible growth will be considered for determining MIC using the following equation, MIC=(lowest concentration of extract inhibiting growth+highest con. that allow growth)/2. To detect the concentration of extracts, loop fool samples from the visibly clear tubes were inoculated onto fresh nutrient agar plates where no bacterial growth occurs. The complete absence of visible growth on the agar plate after streaking onto the medium was determined as the MBC.

  Stamford Journal of Microbiology, 2021. Vol. 11, Issue 1, p. 1-6 ISSN: 2074-5346 (Print); 2408-8846 (Online)
  
Funding Source:
1.   Budget:  
  

Natural candidates are potent alternate sources for searching antibacterial activity which can be used against antibiotic-resistant bacteria. Many plants, fruits, leaves, barks have been proved to be effective in this way to treat infections. Pineapple fruit, pineapple peel, pomelo fruit, and pomelo peel also possess such antibacterial activity which was found against some multidrug resistant clinical isolates. Identification of the specific phytochemical would be the next step in determining the way to use these chemicals as therapeutic agents.

  Journal
  


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