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World Journal of Pharmaceutical Sciences
ISSN (Print): 2321-3310; ISSN (Online): 2321-3086
Published by Atom and Cell Publishers © All Rights Reserved
Available online at: http://www.wjpsonline.com/
Research Article

Chemical composition, Antioxidant and Antibacterial activity of Thuja orientalis
Wajaht A. Shah* and Mahpara Qadir
Department of Chemistry, University of Kashmir, Hazratbal, Srinagar 190006, Jammu and
Kashmir, India
Received: 12-12-2013 / Revised: 21-12-2013 / Accepted: 27-12-2013

ABSTRACT
Essential oils derived from many aromatic plants are well known to possess cytotoxic, antioxidant, antifungal,
insecticidal and antimicrobial activities. Thuja orientalis (family: Cupressaceae) is widely cultivated as a
common ornamental plant. It possesses anti-plasmodial, antioxidant and elastase inhibitory activities. Chemical
composition and pharmacological potential of hydro distillate from Thuja orientalis are reported in this study.
Fresh fruits were subjected to conventional hydrodistillation. Antioxidant activity was assessed as free radical
scavenging capacity (RSC) towards 2, 2-diphenyl-1-picrylhydrazil (DPPH) radicals and antibacterial activity
was evaluated against six test bacteria by agar well diffusion method. Qualitative and Quantitative analysis of
Thuja orientalis hydrodistillate by gas chromatography coupled with mass spectrometry revealed the presence
of nineteen constituents, representing 94.6% of the total oil. The major constituents of oil were alpha-pinene
(83%), sabinene (2.6%), delta-3-carene (2.5%). The oil showed appreciable antibacterial effect against all
Gram-positive and Gram negative bacteria tested with MIC values between 12.8-25.6 mg/ml. Therefore this oil
could be used in the formulation of antimicrobial and antioxidant agents.
Keywords: Thuja orientalis, essential oil, antimicrobial, antioxidant, chemical composition.

INTRODUCTION
Thuja orientalis (family: Cupressaceae) is an
evergreen species, which grows naturally in china,
korea, japan and iran. Also this species is widely
cultivated as a common ornamental plant [1].
Essential oils derived from many aromatic plants
are well known to possess cytotoxic, antioxidant
[2], antifungal, insecticidal [3] and antimicrobial
activities [4].
Previous phytochemical investigations of this plant
resulted in the isolation of many chemical
constituents such as flavoniods [5] [6], terpenes
[7],[ 9] and phenolics [10]. Its crude extracts have
exhibited anti-plasmodial activity [11]. Several
biflavonoids and flavonoid glycosides have been
isolated from the fruits of Thuja orientalis. Also
their estimation of antioxidant and elastase
inhibitory activities is reported [12]. Antifungal
potential of Thuja orientalis is reported [13].
Phytochemical studies of its essential oil showed
the nineteen and twenty-eight constituents from the
fruit and leaf oil respectively. Alpha-pinene
(52.4%),
delta-3-carene
(14.2%),
alpha-

cedrol(6.5%) and beta-phellandrene were major
components in fruit oil, while alpha-pinene
(21.9%),
alpha-cedrol
(20.3%),
delta-3carene(10.5%) and limonene(7.2%) were the main
constituents in the fruit oil [14]. Antifungal activity
of leaf essential oil isolated from Thuja orientalis
against Alternaria alterata is known [15]. Therefore
the aim of this study was phytochemical analysis,
antioxidant activity and antimicrobial activity of
this essential oil against different microorganisms.
MATERIALS AND METHODS
Plant material: The Thuja orientalis plant material
was collected from University of Kashmir,
Srinagar. The plant was properly identified and the
voucher specimen of Thuja orientalis bearing
specimen no.1910 was deposited at herbarium in
Centre of plant Taxonomy, University of Kashmir,
Srinagar, J & K, India.
Essential oil isolation: The essential oil of the
fresh fruits of Thuja orientalis was obtained by
hydrodistillation using a clevenger-type apparatus
for three hours. The oil sample was dried over

*Corresponding Author Address: Dr. Wajaht A. Shah, Department of Chemistry, University of Kashmir – 190006. J&K. (INDIA). Email:doctorwajaht@gmail.com, ajaz.malik@rocketmail.com
Wajaht et al., World J Pharm Sci 2014; 2(1): 56-61

anhydrous sodium sulphate and kept in glass vials
at – 4oc prior to analysis.

The oil was dissolved in dimethyl sulphoxide and
added to the medium, and then diluted in order to
obtain concentrations in the range of 0.25– 25.6
mg/ml. Inoculum suspension with a final
concentration of 106 cfu/ml was added to plate. The
MIC was defined as the lowest concentration of the
essential oil at which the microorganism does not
demonstrate any visible growth after incubation at
37 ⁰C for 24 h.

Chemical composition:
GC–MS analysis: GC–MS analysis was carried on
a Varian Gas Chromatograph series 3800 fitted
with a VF-5 ms fused silica capillary column (60 m
× 0.25 mm, film thickness 0.25 µm) coupled with a
4000 series mass detector under the following
conditions: injection volume 0.5 µl with split ratio
1:60, helium as carrier gas at 1.0 ml/min constant
flow mode, injector temperature 230 ⁰C, oven
temperature was programmed from 60 to 280 ⁰C at
3 ⁰C/min. Mass spectra: electron impact (EI+)
mode, 70 eV and ion source temperature 250 ⁰C.
Mass spectra were recorded over 50–500 a.m.u
range.

Antioxidant activity
DPPH free radical-scavenging activity: DPPH free
radical scavenging activity was evaluated by
measuring the scavenging activity of the essential
oil on stable 2,2-diphenyl- 1-picryl hydrazyl
radical. A 0.5 mM solution of DPPH in methanol
was prepared and a stock solution of oil sample (1
mg/ml) in methanol was prepared. Various
concentrations (20–100 µg/ml) were added to 1ml
(0.5 mM DPPH) and final volume was made to 3
ml with methanol. The mixture was shaken
thoroughly and kept standing at room temperature
for 10 min. Then, the absorbance of the mixture
was measured at 517 nm on a spectrophotometer. A
decrease in the absorbance indicates an increase in
DPPH-radical scavenging activity.

Antimicrobial assay
Microbial strains and culture media: The
antibacterial activity of the essential oil of Thuja
orientalis were tested against a panel of six
bacterial strains obtained from Microbial Type
Culture Collection (MTCC), Institute of Microbial
Technology, Chandigarh, India. The bacterial
strains used were Bacillus subtilis (MTCC-441), P.
aeruginosa (MTCC-1688), S. aureus (MTCC 96),
K. pneumonia (MTCC-19), E. coli (MTCC-443)
and P. vulgaris (MTCC-1771). Bacterial strains
were grown on nutrient agar plates at 37 ⁰C and
maintained on nutrient agar slants. Cell suspension
of microorganisms in 0.9% NaCl was adjusted at
0.5 McFarland to obtain approximately 106 cfu/ml.
Antimicrobial activity and determination of
minimum inhibitory concentration (MIC): The
antibacterial susceptibility tests were carried out
using the agar well diffusion assay/microdilution
assay with some modification. First Muller Hinton
medium was prepared and 0.5% of tween-20 was
dissolved per 100 ml of agar medium in order to
facilitate proper diffusion of agar in the oil. 20 ml
aliquot was transferred in to each boiling tube.
After this sterilization of boiling tubes was carried
out in autoclave. Temperature of tubes was
regulated upto 38⁰C and oil samples were added in
the concentration range of 0.2-25.6 mg/ml.

The percentage inhibition was calculated by the
following equation:
DPPH radical scavenging= [(Ac- As)/Ac)×100]
Where, Ac is the absorbance of the control and As
is the absorbance of the sample.
L-ascorbic acid served as positive control.
RESULTS AND DISCUSSIONS
The chemical composition of the essential oil
isolated from the fruits of thuja orientalis analysed
by gas chromatography-mass spectrometry are
presented in the table 1, given below. The analysis
revealed the presence of nineteen constituents
representing 96.4% of the total oil. The order of
elution of various constituents from RTx-5
cpolumn are shown in figure1. The major
constituents of the oil were alpha-pinene (83%),
sabinene (2.6%), delta-3-carene (2.5%). The
percentage yield of oil was found to be .13 %
(v/w), as per their fresh weight. The components of
oil were classified into monoterpenes, accounting
94.7% and sesquiterpene hydrocarbons accounting
0.8%. Monoterpenes are represented by oxygenated
monoterpenes 0.4% while as oxygenated
sesquiterpenes are weakly represented by 0.5%.

The contents of the tube were transferred into
plates which were kept under laminar flow and
allowed to dry for 30 minutes. Finally bacteria
were inoculated from fresh cultures into the broth
and its turbidity was adjusted in the range of .080.13 at 625nm. Later 3µl of inoculums of each
bacteria was added into the plates. Streptomycin
sulphate (1000mg/l) was used as positive control
for bacteria. The MIC of oil was determined by the
microdilution method, recommended by the
National Committee for Clinical Laboratory
Standards (NCCLS) as described previously [16]

The in vitro antimicrobial activity of essential oil
was qualitatively and quantitatively assessed by the
presence or absence of inhibition zones, zone
diameters and minimum inhibitory concentration
(MIC) values. Results from antimicrobial activity
57
Wajaht et al., World J Pharm Sci 2014; 2(1): 56-61

by agar well diffusion method are presented in
table 2. The essential oil of Thuja orientalis
showed significant antibacterial effect against the
entire test microorganisms used for screening. This
oil was mainly effective against P. vulgaris and
E.coli with highest inhibition zones of 24 and 22
mm respectively. Streptomycin sulphate was used
as a positive control which showed inhibition zones
between 20 -30 mm against different
microorganisms tested. Therefore the antibacterial
activity of Thuja orientalis essential oil seems
closer to reference antibiotic. The MIC value of all
tested bacteria was found between 12.8-25.6
mg/ml. As can be clearly seen from the
photographs (Figure 2) that growth of all the six
bacteria was observed on the plates between the
concentration range of 0.4-12.6 mg/ml. While as no
growth of bacteria was observed on the plate at a
concentration of 25.6 mg/ml of oil. The previous
reports on antimicrobial activity of Thuja orientalis
essential oil against different microorganisms
support our result [17]. The antimicrobial activity
of this oil against K. pneumonaie, P. Aeroginosa
and P. Vulgaris is reported first time.

act as donor for hydrogen atoms in the
transformation of DPPH radical into its reduced
form DPPH2 was investigated. The examined oil
was able to reduce the stable purple coloured
DPPH radical into yellow coloured DPPH2. The
aforementioned oil showed promising radical
scavenging activity at concentration of 100μl/ml.
The results are plotted in the form of graph
(Figure.3). This plant oil exhibited prominent
DPPH free radical scavenging activity of 49.8% in
comparison to ascorbic acid and α-tocopherol
standard which showed the activity of 67.95 and
71.2%, respectively. The DPPH radical scavenging
assay is commonly employed in evaluating the
ability of antioxidants to scavenge free radicals.
This method has been used extensively to predict
the antioxidant activity because of the relatively
short time required for analysis. The change in
absorbance at 517 nm is used as a measure of the
scavenging effect of a particular sample for DPPH
radicals. The more rapidly the absorbance
decreases, the more potent the antioxidant activity
of the sample in terms of its hydrogen atomdonating capacity. It should be noted that our study
showed major constituent α-Pinene 83.0% instead
of 52% reported in literature. Antioxidant potential
is also first time reports from the essential oil of
Thuja Orientalis.

DPPH(1,1-diphenyl-2-picryl hydrazyl free radical)
free radical scavenging capacity of the essential oil
was measured by DPPH assay under in-vitro
conditions. The ability of the examined extract to

Table1: Chemical composition of the essential oil of Thuja Orientalis
S. No
Compound
% Peak Area
Methods of identification
1
α-Pinene
83.0
MS, RI, Std
Camphene
0.5
MS, RI
2
MS, RI
3
β-Phellandrene
1.0
MS, RI, Std
4
Tricyclene
2.2
Sabinene
2.6
MsS, RI
5
α-Phellandrene
0.2
MS, RI
6
MS, RI, Std
7
δ-3-Carene
2.5
MS, RI
8
α-Terpinene
Tr
P-Cymene
Tr
MS, RI
9
Limonene
1.1
MS, RI
10
1,8-cineole
0.2
MS, RI
11
γ-Terpinene
0.1
MS, RI
12
α-Terpinolene
1.5
MS, RI
13
4-Terpineol
0.2
MS, RI
14
β-Fenchol
Tr
MS, RI
15
β-Caryophyllene
0.3
MS, RI
16
α-Caryophyllene
0.4
MS, RI
17
Germacrene D
0.1
MS, RI
18
Cedrol
0.5
19
Total (%)
96.4
Monoterpene hydrocarbons
94.7
Oxygenated monoterpenes
0.4
Sesquiterpene hydrocarbons
0.8
Oxygenated sesquiterpenes
0.5

58
Wajaht et al., World J Pharm Sci 2014; 2(1): 56-61

Table 2: In Vitro Anti Microbial Activity of Thuja Orientalis Essential Oil and reference antibiotic determined
with Agar well Diffusion Method
S.No. Test bacteria
Zones of
Zone
of MIC (in mg/ml)
inhibition
inhibition of
(in mm)
antibiotic (in
mm)
Gram-Positive Bacteria
1
S. Aureus MTCC 96
2
B.subtilis MTCC 441
3
K.pneumoniae MTCC 19
Gram-Negative Bacteria
4
E.coli MTCC 443
5
P.aeroginosa MTCC 1688
6
P.vulgaris MTCC 426
FIG: 1

20
15
16

18
30
17

12.8-25.6
12.8-25.6
12.8-25.6

22
19
24

20
30
20

12.8-25.6
12.8-25.6
12.8-25.6

Order of elution of various constituents of analysed essential oil

Major components:
1= α-Pinene
2= β-Phellandrene
3= Tricyclene
4= Sabinene

59
Wajaht et al., World J Pharm Sci 2014; 2(1): 56-61

Fig 2 Plates shows antimicrobial activity of Essential oil.

Fig 3 Antioxident potential of essential oil from Thuja Orientalis

MP2; Essential oil, AA; Ascorbic acid, conc; concentration (µg/ml).
60
Wajaht et al., World J Pharm Sci 2014; 2(1): 56-61

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Asaadi M. Pinaceae,Taxaceae, cuprassaceae and ephedraceae. Institute of forests and range lands, Tehran 1998; 11-12.
Dar MY et al. Chemical composition , in vitro cytotoxic and antioxidant activities of the essential oil and major constituents
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Konstantopoulou I et al. Insecticidal effects of essential oils. A Study of the effects of essential oils extracted from eleven
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Janssen AM et al. Antimicrobial activity of essential oils: a 1976-1986 literature review. Aspects of the test methods. Planta
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Pelter A et al. Biflavonyl pigments from Thuja orientalis (Cupressaceae). Phytochemistry 1970; 9, 1897-1898.
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Sung S H et al. Diterpenes of Biota orientalis leaves. Kor. J. Pharmacog 1998. 29, 347-352.
Inoue M et al. Terpenoids from the seed of Platycladus orientalis. Phytochemistry, 1985; 24, 1602- 1604.
Tomita B et al. XVI new constituents of Biota orientalis. Tetrahedron Lett 1968; 9, 843-848.
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Guleria S, Kumar A. Antifungal activity of some Himalayan medicinal plants using direct autography. J. cell Mol. Biol 2006
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61

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Chemical composition, Antioxidant and Antibacterial activity of Thuja orientalis

  • 1. World Journal of Pharmaceutical Sciences ISSN (Print): 2321-3310; ISSN (Online): 2321-3086 Published by Atom and Cell Publishers © All Rights Reserved Available online at: http://www.wjpsonline.com/ Research Article Chemical composition, Antioxidant and Antibacterial activity of Thuja orientalis Wajaht A. Shah* and Mahpara Qadir Department of Chemistry, University of Kashmir, Hazratbal, Srinagar 190006, Jammu and Kashmir, India Received: 12-12-2013 / Revised: 21-12-2013 / Accepted: 27-12-2013 ABSTRACT Essential oils derived from many aromatic plants are well known to possess cytotoxic, antioxidant, antifungal, insecticidal and antimicrobial activities. Thuja orientalis (family: Cupressaceae) is widely cultivated as a common ornamental plant. It possesses anti-plasmodial, antioxidant and elastase inhibitory activities. Chemical composition and pharmacological potential of hydro distillate from Thuja orientalis are reported in this study. Fresh fruits were subjected to conventional hydrodistillation. Antioxidant activity was assessed as free radical scavenging capacity (RSC) towards 2, 2-diphenyl-1-picrylhydrazil (DPPH) radicals and antibacterial activity was evaluated against six test bacteria by agar well diffusion method. Qualitative and Quantitative analysis of Thuja orientalis hydrodistillate by gas chromatography coupled with mass spectrometry revealed the presence of nineteen constituents, representing 94.6% of the total oil. The major constituents of oil were alpha-pinene (83%), sabinene (2.6%), delta-3-carene (2.5%). The oil showed appreciable antibacterial effect against all Gram-positive and Gram negative bacteria tested with MIC values between 12.8-25.6 mg/ml. Therefore this oil could be used in the formulation of antimicrobial and antioxidant agents. Keywords: Thuja orientalis, essential oil, antimicrobial, antioxidant, chemical composition. INTRODUCTION Thuja orientalis (family: Cupressaceae) is an evergreen species, which grows naturally in china, korea, japan and iran. Also this species is widely cultivated as a common ornamental plant [1]. Essential oils derived from many aromatic plants are well known to possess cytotoxic, antioxidant [2], antifungal, insecticidal [3] and antimicrobial activities [4]. Previous phytochemical investigations of this plant resulted in the isolation of many chemical constituents such as flavoniods [5] [6], terpenes [7],[ 9] and phenolics [10]. Its crude extracts have exhibited anti-plasmodial activity [11]. Several biflavonoids and flavonoid glycosides have been isolated from the fruits of Thuja orientalis. Also their estimation of antioxidant and elastase inhibitory activities is reported [12]. Antifungal potential of Thuja orientalis is reported [13]. Phytochemical studies of its essential oil showed the nineteen and twenty-eight constituents from the fruit and leaf oil respectively. Alpha-pinene (52.4%), delta-3-carene (14.2%), alpha- cedrol(6.5%) and beta-phellandrene were major components in fruit oil, while alpha-pinene (21.9%), alpha-cedrol (20.3%), delta-3carene(10.5%) and limonene(7.2%) were the main constituents in the fruit oil [14]. Antifungal activity of leaf essential oil isolated from Thuja orientalis against Alternaria alterata is known [15]. Therefore the aim of this study was phytochemical analysis, antioxidant activity and antimicrobial activity of this essential oil against different microorganisms. MATERIALS AND METHODS Plant material: The Thuja orientalis plant material was collected from University of Kashmir, Srinagar. The plant was properly identified and the voucher specimen of Thuja orientalis bearing specimen no.1910 was deposited at herbarium in Centre of plant Taxonomy, University of Kashmir, Srinagar, J & K, India. Essential oil isolation: The essential oil of the fresh fruits of Thuja orientalis was obtained by hydrodistillation using a clevenger-type apparatus for three hours. The oil sample was dried over *Corresponding Author Address: Dr. Wajaht A. Shah, Department of Chemistry, University of Kashmir – 190006. J&K. (INDIA). Email:doctorwajaht@gmail.com, ajaz.malik@rocketmail.com
  • 2. Wajaht et al., World J Pharm Sci 2014; 2(1): 56-61 anhydrous sodium sulphate and kept in glass vials at – 4oc prior to analysis. The oil was dissolved in dimethyl sulphoxide and added to the medium, and then diluted in order to obtain concentrations in the range of 0.25– 25.6 mg/ml. Inoculum suspension with a final concentration of 106 cfu/ml was added to plate. The MIC was defined as the lowest concentration of the essential oil at which the microorganism does not demonstrate any visible growth after incubation at 37 ⁰C for 24 h. Chemical composition: GC–MS analysis: GC–MS analysis was carried on a Varian Gas Chromatograph series 3800 fitted with a VF-5 ms fused silica capillary column (60 m × 0.25 mm, film thickness 0.25 µm) coupled with a 4000 series mass detector under the following conditions: injection volume 0.5 µl with split ratio 1:60, helium as carrier gas at 1.0 ml/min constant flow mode, injector temperature 230 ⁰C, oven temperature was programmed from 60 to 280 ⁰C at 3 ⁰C/min. Mass spectra: electron impact (EI+) mode, 70 eV and ion source temperature 250 ⁰C. Mass spectra were recorded over 50–500 a.m.u range. Antioxidant activity DPPH free radical-scavenging activity: DPPH free radical scavenging activity was evaluated by measuring the scavenging activity of the essential oil on stable 2,2-diphenyl- 1-picryl hydrazyl radical. A 0.5 mM solution of DPPH in methanol was prepared and a stock solution of oil sample (1 mg/ml) in methanol was prepared. Various concentrations (20–100 µg/ml) were added to 1ml (0.5 mM DPPH) and final volume was made to 3 ml with methanol. The mixture was shaken thoroughly and kept standing at room temperature for 10 min. Then, the absorbance of the mixture was measured at 517 nm on a spectrophotometer. A decrease in the absorbance indicates an increase in DPPH-radical scavenging activity. Antimicrobial assay Microbial strains and culture media: The antibacterial activity of the essential oil of Thuja orientalis were tested against a panel of six bacterial strains obtained from Microbial Type Culture Collection (MTCC), Institute of Microbial Technology, Chandigarh, India. The bacterial strains used were Bacillus subtilis (MTCC-441), P. aeruginosa (MTCC-1688), S. aureus (MTCC 96), K. pneumonia (MTCC-19), E. coli (MTCC-443) and P. vulgaris (MTCC-1771). Bacterial strains were grown on nutrient agar plates at 37 ⁰C and maintained on nutrient agar slants. Cell suspension of microorganisms in 0.9% NaCl was adjusted at 0.5 McFarland to obtain approximately 106 cfu/ml. Antimicrobial activity and determination of minimum inhibitory concentration (MIC): The antibacterial susceptibility tests were carried out using the agar well diffusion assay/microdilution assay with some modification. First Muller Hinton medium was prepared and 0.5% of tween-20 was dissolved per 100 ml of agar medium in order to facilitate proper diffusion of agar in the oil. 20 ml aliquot was transferred in to each boiling tube. After this sterilization of boiling tubes was carried out in autoclave. Temperature of tubes was regulated upto 38⁰C and oil samples were added in the concentration range of 0.2-25.6 mg/ml. The percentage inhibition was calculated by the following equation: DPPH radical scavenging= [(Ac- As)/Ac)×100] Where, Ac is the absorbance of the control and As is the absorbance of the sample. L-ascorbic acid served as positive control. RESULTS AND DISCUSSIONS The chemical composition of the essential oil isolated from the fruits of thuja orientalis analysed by gas chromatography-mass spectrometry are presented in the table 1, given below. The analysis revealed the presence of nineteen constituents representing 96.4% of the total oil. The order of elution of various constituents from RTx-5 cpolumn are shown in figure1. The major constituents of the oil were alpha-pinene (83%), sabinene (2.6%), delta-3-carene (2.5%). The percentage yield of oil was found to be .13 % (v/w), as per their fresh weight. The components of oil were classified into monoterpenes, accounting 94.7% and sesquiterpene hydrocarbons accounting 0.8%. Monoterpenes are represented by oxygenated monoterpenes 0.4% while as oxygenated sesquiterpenes are weakly represented by 0.5%. The contents of the tube were transferred into plates which were kept under laminar flow and allowed to dry for 30 minutes. Finally bacteria were inoculated from fresh cultures into the broth and its turbidity was adjusted in the range of .080.13 at 625nm. Later 3µl of inoculums of each bacteria was added into the plates. Streptomycin sulphate (1000mg/l) was used as positive control for bacteria. The MIC of oil was determined by the microdilution method, recommended by the National Committee for Clinical Laboratory Standards (NCCLS) as described previously [16] The in vitro antimicrobial activity of essential oil was qualitatively and quantitatively assessed by the presence or absence of inhibition zones, zone diameters and minimum inhibitory concentration (MIC) values. Results from antimicrobial activity 57
  • 3. Wajaht et al., World J Pharm Sci 2014; 2(1): 56-61 by agar well diffusion method are presented in table 2. The essential oil of Thuja orientalis showed significant antibacterial effect against the entire test microorganisms used for screening. This oil was mainly effective against P. vulgaris and E.coli with highest inhibition zones of 24 and 22 mm respectively. Streptomycin sulphate was used as a positive control which showed inhibition zones between 20 -30 mm against different microorganisms tested. Therefore the antibacterial activity of Thuja orientalis essential oil seems closer to reference antibiotic. The MIC value of all tested bacteria was found between 12.8-25.6 mg/ml. As can be clearly seen from the photographs (Figure 2) that growth of all the six bacteria was observed on the plates between the concentration range of 0.4-12.6 mg/ml. While as no growth of bacteria was observed on the plate at a concentration of 25.6 mg/ml of oil. The previous reports on antimicrobial activity of Thuja orientalis essential oil against different microorganisms support our result [17]. The antimicrobial activity of this oil against K. pneumonaie, P. Aeroginosa and P. Vulgaris is reported first time. act as donor for hydrogen atoms in the transformation of DPPH radical into its reduced form DPPH2 was investigated. The examined oil was able to reduce the stable purple coloured DPPH radical into yellow coloured DPPH2. The aforementioned oil showed promising radical scavenging activity at concentration of 100μl/ml. The results are plotted in the form of graph (Figure.3). This plant oil exhibited prominent DPPH free radical scavenging activity of 49.8% in comparison to ascorbic acid and α-tocopherol standard which showed the activity of 67.95 and 71.2%, respectively. The DPPH radical scavenging assay is commonly employed in evaluating the ability of antioxidants to scavenge free radicals. This method has been used extensively to predict the antioxidant activity because of the relatively short time required for analysis. The change in absorbance at 517 nm is used as a measure of the scavenging effect of a particular sample for DPPH radicals. The more rapidly the absorbance decreases, the more potent the antioxidant activity of the sample in terms of its hydrogen atomdonating capacity. It should be noted that our study showed major constituent α-Pinene 83.0% instead of 52% reported in literature. Antioxidant potential is also first time reports from the essential oil of Thuja Orientalis. DPPH(1,1-diphenyl-2-picryl hydrazyl free radical) free radical scavenging capacity of the essential oil was measured by DPPH assay under in-vitro conditions. The ability of the examined extract to Table1: Chemical composition of the essential oil of Thuja Orientalis S. No Compound % Peak Area Methods of identification 1 α-Pinene 83.0 MS, RI, Std Camphene 0.5 MS, RI 2 MS, RI 3 β-Phellandrene 1.0 MS, RI, Std 4 Tricyclene 2.2 Sabinene 2.6 MsS, RI 5 α-Phellandrene 0.2 MS, RI 6 MS, RI, Std 7 δ-3-Carene 2.5 MS, RI 8 α-Terpinene Tr P-Cymene Tr MS, RI 9 Limonene 1.1 MS, RI 10 1,8-cineole 0.2 MS, RI 11 γ-Terpinene 0.1 MS, RI 12 α-Terpinolene 1.5 MS, RI 13 4-Terpineol 0.2 MS, RI 14 β-Fenchol Tr MS, RI 15 β-Caryophyllene 0.3 MS, RI 16 α-Caryophyllene 0.4 MS, RI 17 Germacrene D 0.1 MS, RI 18 Cedrol 0.5 19 Total (%) 96.4 Monoterpene hydrocarbons 94.7 Oxygenated monoterpenes 0.4 Sesquiterpene hydrocarbons 0.8 Oxygenated sesquiterpenes 0.5 58
  • 4. Wajaht et al., World J Pharm Sci 2014; 2(1): 56-61 Table 2: In Vitro Anti Microbial Activity of Thuja Orientalis Essential Oil and reference antibiotic determined with Agar well Diffusion Method S.No. Test bacteria Zones of Zone of MIC (in mg/ml) inhibition inhibition of (in mm) antibiotic (in mm) Gram-Positive Bacteria 1 S. Aureus MTCC 96 2 B.subtilis MTCC 441 3 K.pneumoniae MTCC 19 Gram-Negative Bacteria 4 E.coli MTCC 443 5 P.aeroginosa MTCC 1688 6 P.vulgaris MTCC 426 FIG: 1 20 15 16 18 30 17 12.8-25.6 12.8-25.6 12.8-25.6 22 19 24 20 30 20 12.8-25.6 12.8-25.6 12.8-25.6 Order of elution of various constituents of analysed essential oil Major components: 1= α-Pinene 2= β-Phellandrene 3= Tricyclene 4= Sabinene 59
  • 5. Wajaht et al., World J Pharm Sci 2014; 2(1): 56-61 Fig 2 Plates shows antimicrobial activity of Essential oil. Fig 3 Antioxident potential of essential oil from Thuja Orientalis MP2; Essential oil, AA; Ascorbic acid, conc; concentration (µg/ml). 60
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