Anum PHD Paper 2019
Anum PHD Paper 2019
Anum PHD Paper 2019
1*
Ishaq, A., 1Syed, Q. A., 1Khan, M. I. and 2Zia, M. A.
National Institute of Food Science and Technology, Faculty of Food Nutrition and Home Sciences,
1
Received: 18 September, 2018 Phenolic compounds present in clove extract have been reported to possess strong inhibitory
Received in revised form: effect against a vast range of microorganisms. The present work was aimed to optimise the
12 January, 2019 antioxidant and antimicrobial potentials of clove extract against major food-borne pathogenic
Accepted: 28 March, 2019
bacteria (Salmonella Typhimurium, Escherichia coli, Listeria monocytogenes). Results revealed
that clove extract obtained from n-hexane extraction had higher extraction yield (48.84%),
antioxidant potential (TPC = 54.05 mg/g of GAE, TFC = 15.54 mg/g, DPPH = 0.29 mg/mL,
FRAP = 0.69 mg/mL) and antimicrobial activity as compared to the extracts obtained from
Keywords ethanol, petroleum ether and steam distillation. Minimum inhibitory concentration of clove
extract (0.25%) was more effective against L. monocytogenes (ZI = 11.17 mm) in comparison
Clove extract
with S. Typhimurium (ZI = 8.8 mm) and E. coli (ZI = 9.27 mm). Additionally, clove extract was
Antioxidant potential
Antimicrobial activity also effective in disrupting cell membrane integrity and affecting membrane permeability of
Membrane permeability the assessed bacteria. It was also found that L. monocytogenes was more susceptible to clove
Cell membrane integrity phytochemicals as compared to the other bacteria. Hence, clove extract has strong potential to
be used as a natural antioxidant and antimicrobial agent in food industry.
© All Rights Reserved
*Corresponding author.
Email: [email protected]
1166 Ishaq, A., Syed, Q. A., Khan, M. I. and Zia, M. A./IFRJ 26(4) : 1165-1172
(BHT). In another study, Gülçin et al. (2004) (Germany) and Sigma-Aldrich (USA). The other
demonstrated 93.3% and 97.9% inhibition of linoleic materials were purchased from reputed scientific
acid oxidation at 20 and 60 µg/mL, respectively. store of Faisalabad, Pakistan. Bacterial strains
Additionally, studies have revealed that clove (S. Typhimurium, E. coli and L. monocytogenes)
extracts possess significant antibacterial potential were provided by Institute of Food Microbiology,
against several bacteria such as Enterococcus faecalis, University of Agriculture Faisalabad.
Staphylococcus aureus, Listeria monocytogenes,
Bacillus cereus, Escherichia coli, Salmonella Experimental design
typhi and Pseudomonas aeruginosa. The active The experiments for characterisation, extraction,
compounds in clove extract, particularly eugenol, antioxidant assay and antimicrobial analyses were
damage bacterial membranes and cause leakage of performed under Controlled Randomized Design
intracellular materials (Oyedemi et al., 2009). Clove (CRD) while experiments related to bacterial cell
extract also has inhibitory effect on the biofilms, integrity and membrane permeability were conducted
and it is evident from studies that clove extract can under CRD using factorial arrangement.
reduce the formation of biofilms up to 99% (Raja
et al., 2015). In another investigation, El-Maati Sample preparation and characterisation of clove
et al. (2016) studied phenolic extracts of clove for buds
their antioxidant and antimicrobial properties, and For the characterisation of clove, clove buds were
concluded that clove extract can be used in food and firstly ground and then clove powder was subjected
pharmaceutical products as natural antimicrobial or to proximate analysis.
antioxidant agent.
Above mentioned discussion strongly supports Moisture contents
the antioxidant and antimicrobial potential of clove The moisture contents of clove powder were
extracts. Studies have revealed the effect of clove oil/ measured by drying the samples in conventional
extract on bacterial reduction, but no studies have forced air laboratory oven (Model: DO-1-30/02,
been conducted on exploring the effect of applying PCSIR, Pakistan) at 105 ± 2°C until constant weight
clove extract on bacterial cell integrity and membrane was achieved (AACC, 2000).
permeability. So, the present work aimed to elucidate
the effect of clove extracts on cell membrane Crude protein
permeability and integrity against different food- The percentage of crude proteins was estimated
borne pathogenic bacteria; Salmonella Typhimurium, through Kjeltech Apparatus (AACC, 2000). Briefly,
Escherichia coli and Listeria monocytogenes. 1.5 g sample was taken and mixed with 5 g digestion
Additionally, the present work also evaluated the mixture (K2SO4, CuSO4 and FeSO4) and 30 mL H2SO4
antioxidant potential of clove extract obtained from in digestion flask. The mixture was then subjected to
different extraction techniques. mild heating (40°C) for 10 min and then temperature
was raised to 60°C until the completion of digestion
Materials and methods process i.e., turning of mixture to greenish colour.
After cooling, the volume was made up to 250 mL
The present work was conducted in Meat by adding distilled water. Then, the sample was
Science and Technology Laboratory (MSTL) and subjected to neutralisation process in distillation
Food Microbiology and Biotechnology Laboratory assembly by mixing 10 mL sample with 10 mL NaOH
(FMBL), National Institute of Food Science and solution (40%) in distillation tube against boric acid
Technology (NIFSAT), University of Agriculture solution (4%) with methyl red (indicator). Following
Faisalabad, Pakistan. In the present work, locally distillation, titration was performed against 0.1 N
cultivated variety of cloves was exposed to H2SO4 and the volume of acid was noted.
characterisation, antioxidant potential estimation and
antimicrobial assay. Crude fat
Crude fat was determined by using Soxhlet
Materials and chemicals Extraction System (AACC, 2000). Briefly, 2 g
Clove buds were purchased from the local market sample (oven dried) was taken in thimble and crude
in Faisalabad, Pakistan. All the other reagents for fat was extracted by using n-hexane after completing
extraction (ethanol, n-hexane, petroleum ether), five siphon cycles. Next, n-hexane was evaporated
compositional analysis, antioxidant assay and using rotary evaporator and crude fat contents were
microbial analysis were purchased from Merck estimated based on differences in the weights of
sample.
Ishaq, A., Syed, Q. A., Khan, M. I. and Zia, M. A./IFRJ 26(4) : 1165-1172 1167
added in the wells followed by dipping of sterilised on the release of cytoplasmic β-galactosidase activity
discs having diameter of 6 mm for 1 h. Commercial from bacterial cells by using ONPG (O-nitrophenyl-
antibiotics (10 μL) against S. Typhimurium (nalidixic β-D-galactoside) substrate. Briefly, bacterial cells
acid), E. coli (nalidixic acid) and L. monocytogenes were harvested, washed and resuspended in sterilised
(chloramphenicol) were also added in some wells and NaCl solution (0.9%). The optical densities (OD)
served as positive controls. Bacterial cultures were were adjusted to 1.2 by taking absorbances at 420
inoculated on their respective growth media (XLT4 nm using UV-Vis Spectro-photometer. Next, 1.6 mL
for S. Typhimurium, MacConkey Sorbitol medium bacterial suspension was mixed with 1.6 mL clove
for E. coli, MOX for L. monocytogenes) and discs extract and 150 μL ONPG (30 mM). Finally, the
were placed on the plates followed by incubation at absorbances were taken at 420 nm after every 10 min
37°C for 24 h. After prescribed incubation time, the up to 120 min (Liu et al., 2015).
zones of inhibition were measured for each pathogen.
Statistical analysis
Selection of best treatment The obtained data were statistically analysed
Based on antioxidant activity and antimicrobial using Statistics 8.1 software. Analysis of variance
susceptibility tests, clove extract obtained from (ANOVA) was performed to measure the level of
n-hexane was chosen for further analysis on significance. All pair-wise comparison was made
antimicrobial activity and its effect on cell membrane through Tukey’s Test (Montgomery, 2008).
integrity and membrane permeability against
pathogenic bacteria. Results and discussion
amongst all the solvents for many years. Hexane polyphenols which are effective in scavenging
has high ability to extract oil due to the presence of free radicals (Khalil et al., 2017). Clove extract
several isomers. It is preferred for solvent extraction principally contains eugenol and iso-eugenol which
due to its high volatility and low sensible heat (335 are majorly responsible for its antioxidant potential.
kJ/kg). Moreover, it can be easily removed from oil These phytochemicals form complexes with reduced
or extract with low use of energy. Additionally, the metals and impose inhibitory effect on lipid oxidation
azeotrope (95% hexane and 5% water) of hexane by eliminating free radicals and forming iron-oxygen
is quite efficient for the removal of contents from complexes (Ito et al., 2005).
solids at slightly lower boiling temperature (61.6°C) Ferrous (Fe2+) and ferric (Fe3+) ions are strong
by direct use of steam. Furthermore, hexane also pro-oxidants, and promote the generation of reactive
has good dissolving properties with oils which is oxygen species (ROS). Similarly, free radical chain
beneficial when washing off extracts from solids or reactions also promote lipid peroxidation. Minimising
fibrous materials (NFPA, 2009). the generation of ferrous ions and scavenging of
free radicals delay the process of lipid oxidation
Antioxidant activity of clove extracts in food and biological systems. Chelating agents
Different phenolic compounds present in plants disrupt the complex formation which results in the
possess strong therapeutic properties against several decrease in red colour. This discoloration is observed
life-style related ailments due to their antioxidant by spectrophotometer and chelating capacity of an
potential. The total phenolic and flavonoid contents, antioxidant is based on the extent of the discoloration.
FRAP and DPPH activities of clove extracts obtained Lower absorbance usually indicates high metal
from different extraction systems are shown in Table chelating activity of antioxidants. In the present work,
2. The TPCs of clove extracts ranged from 23.62 to the chelating ability of clove extract was described
54.05 mg/g GAE with HES exhibiting the highest by inhibiting the generation of ferrous and ferrozine
value and SES showing the least. The statistical complex by capturing ferrous ions before ferrozine. In
analyses revealed that extraction system had DPPH assay, antioxidants generally cause reduction
significant (p < 0.05) effect on TPCs of clove extract. of stable violet DPPH radicals followed by their
The differences in phenolic contents could be due to conversion to a yellowish compound i.e., diphenyl-
varied affinity of clove polyphenols towards different picrylhydrazine. The hydrogen-donating antioxidant
solvents. Similarly, the TFC of clove extracts were reduces alcoholic DPPH and converts it into non-
also significantly different. Maximum TFCs were radical form DPPH-H (Gülçin et al., 2012). Findings
recorded in HES (15.54 mg/g) followed by PES of the present work strongly support the power of
(14.63 mg/g), EES (12.46 mg/g) and SES (9.22 clove extract to reduce radical form of DPPH into
mg/g). non-radical form.
Table 2 also shows the results of FRAP and
DPPH analyses of clove extracts. It was revealed that Antimicrobial activity of clove extracts
clove extract of HES showed highest DPPH activity The antimicrobial activity of clove extracts
(0.29 mg/mL) followed by PES (0.24 mg/mL), EES obtained through different extraction systems (EES,
(0.21 mg/mL) and SES (0.15 mg/mL). Similar trend HES, PES, SES) against food-borne pathogenic
was also observed for FRAP. bacteria is demonstrated in Table 3. The highest
zones of inhibition were shown by HES; 24.27 mm
Table 2. Extraction yield and antioxidant activity of clove
extracts obtained from different extraction processes. for S. Typhimurium, 25.8 mm for E. coli and 29.67
TFC (mg FRAP DPPH
mm for L. monocytogenes. Results also suggested
Extraction TPC (mg that L. monocytogenes was more susceptible to
Treatments quercetin (mg/ (mg/
Yield (%) GAE/g)
/g) mL) mL) antimicrobial clove extract as compared to other
S1 41.47c 48.41c 12.46b 0.59b 0.21c pathogens. Other prepared extracts of clove also
S2 48.84 a
54.05 a
15.54 a
0.69 a
0.29a showed considerable antimicrobial potential, but
S3 43.86b 50.88b 14.63a 0.63b 0.24b their zones of inhibitions were smaller as compared
S4 11.72d 23.62d 9.22c 0.32c 0.15d to HES. Antimicrobial activity of clove extracts was
Different superscript letters in each column indicate significant compared with commercial antibiotics specific for
difference (p < 0.05). S1 = ethanol (95%); S2 = n-hexane (95%); S3 = each bacterial strain i.e., nalidixic acid was used
petroleum ether (95%); S4 = steam distillation.
for S. Typhimurium (31.57 mm) and E. coli (31.57
Several reports have demonstrated that plants mm) whereas chloramphenicol was used for L.
contain a variety of phytochemicals such as monocytogenes (38.8 mm).
1170 Ishaq, A., Syed, Q. A., Khan, M. I. and Zia, M. A./IFRJ 26(4) : 1165-1172
Figure 1: (a) Release of 260 nm absorbing materials and (b) Release of cytoplasmic β-galactosidase from cells of
Salmonella Typhimurium, Escherichia coli and Listeria monocytogenes with treatment of clove extract.
Chen, C. Z. and Cooper, S. L. 2002. Interactions between Khalil, A. A., Rahman, U., Khan, M. R., Sahar, A.,
dendrimer biocides and bacterial membranes. Mehmood, T. and Khan, M. 2017. Essential oil eugenol:
Biomaterials 23(16): 3359-3368. sources, extraction techniques and nutraceutical
Denyer, S. P. 1995. Mechanisms of actions of antibacterial perspectives. RSC Advances 7: 32669-32681.
biocides. International Biodeterioration and Liu, X., Xia, W., Jiang, Q., Xu, Y. and Yu, P. 2015. Effect
Biodegradation 36(3-4): 227-245. of kojic acid-grafted-chitosan oligosaccharides as
El-Maati, M. F. A., Mahgoub, S. A., Labib, S. M., Al- a novel antimicrobial agent on cell-membrane of
Gaby, A. M. A. and Ramadan, M. F. 2016. Phenolic Gram-positive and Gram-negative bacteria. Journal of
extracts of clove (Syzygium aromaticum) with novel Bioscience and Bioengineering 120(3): 335-339.
antioxidant and antibacterial activities. European Montgomery, D. C. 2008. Design and analysis of
Journal of Integrative Medicine 8(4): 494-504. experiments. 7th ed. India: Wiley India Pvt Ltd.
Franklin, T. J. and Snow, G. A. 1981. Biochemistry National Fire Protection Association (NFPA). 2009.
of antimicrobial action. 3rd ed. United Kingdom: NFPA 36: Standard for solvent extraction plants
Chapman and Hall. (adapted from table B-2, p. 19). Retrieved from NFPA
González-Rivera, J., Duce, C., Falconieri, D., Ferrari, C., website: https://www.nfpa.org/codes-and-standards/
Ghezzi, L., Piras, A. and Tine, M. R. 2016. Coaxial all-codes-and-standards/list-of-codes-and-standards/
microwave assisted hydrodistillation of essential oils detail?code=36
from five different herbs (lavender, rosemary, sage, Oyedemi, S. O., Okoh, A. I., Mabinya, L. V., Pirochenva,
fennel seeds and clove buds): chemical composition G. and Afolayan, A. J. 2009. The proposed mechanism
and thermal analysis. Innovative Food Science and of bactericidal action of eugenol, α-terpineol
Emerging Technologies 33: 308-318. and γ-terpinene against Listeria monocytogenes,
Guan, W., Li, S., Yan, R., Tang, S. and Quan, C. 2007. Streptococcus pyogenes, Proteus vulgaris and
Comparison of essential oils of clove buds extracted Escherichia coli. African Journal of Biotechnology
with supercritical carbon dioxide and other traditional 8(7): 1280-1286.
extraction methods. Food Chemistry 101(4): 1558- Quan, L., Li, S., Tian, S., Xu, H., Lin, A. and Gu, L. 2004.
1564. Determination of organochlorine pesticides residue
Gülçin, I. 2001. Antioxidant activity of eugenol: a structure- in ginseng root by orthogonal array design Soxhlet
activity relationship study. Journal of Medicinal Food Extraction and gas chromatography. Chromatographia
14(9): 975-985. 59(1-2): 89-93.
Gülçin, I., Elmastaş, M. and Aboul-Enein, H. Y. 2012. Rahman, U. U., Sahar, A., Pasha, I., Rahman, S. U.,
Antioxidant activity of clove oil-A powerful Sohaib, M., Ishaq, A., … and Zafar, H. 2017.
antioxidant source. Arabian Journal of Chemistry Augmenting quality and microbial safety of broiler
5(4): 489-499. meat at refrigeration storage by applying chemical
Gülçin, I., Şat, I. G., Beydemir, S., Elmastaş, M. and interventions. Journal of Food Processing and
Küfrevioǧlu, O. I. 2004. Comparison of antioxidant Preservation 41(4): article ID e13030.
activity of clove (Eugenia caryophylata Thunb) Raja, M. R. C., Srinivasan, V., Selvaraj, S. and Mahapatra,
buds and lavender (Lavandula stoechas L.). Food S. K. 2015. Versatile and synergistic potential of
Chemistry 87(3): 393-400. eugenol: a review. Pharmaceutica Analytica Acta 6(5):
Ito, M., Murakami, K. and Yoshino, M. 2005. Antioxidant article ID 1000367.
action of eugenol compounds: role of metal ion in the
inhibition of lipid peroxidation. Food and Chemical
Toxicology 43(3): 461-466.
Jang, A., Liu, X. D., Shin, M. H., Lee, B. D., Lee, S. K.,
Lee, J. H. and Jo, C. 2008. Antioxidative potential
of raw breast meat from broiler chicks fed a dietary
medicinal herb extract mix. Poultry Science 87(11):
2382-2389.
Jeyaratnam, N., Nour, A. H., Kanthasamy, R., Nour,
A. H., Yuvaraj, A. R. and Akindoyo, J. O. 2016.
Essential oil from Cinnamomum cassia bark through
hydrodistillation and advanced microwave assisted
hydrodistillation. Industrial Crops and Products 92:
57-66.
Jung, S., Choe, J. H., Kim, B., Yun, H., Kruk, Z. A. and Jo,
C. 2010. Effect of dietary mixture of garlic acid and
linoleic acid on antioxidative potential and quality of
breast meat from broilers. Meat Science 86(2): 520-
526.