Total Phenolic Content and Antioxidant Activity of Standardized Extracts from Leaves and Cell Cultures of Three Callistemon Species

doi:10.4236/ajps.2011.26100

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American Journal of Plant Sciences, 2011, 2, 847-850

doi :1 0.4236/ aj ps.2011 .26100 Publ i s hed Online December 2011 (http://www.SciRP.org/journal/ajps)

847

Total Phenolic Content and Antioxidant Activity of

Standardized Extracts from Leaves and Cell

Cultures of Three Callistemon Species

Mohamed I. S. Abdelhady1,3*, Amira Abdel Motaal2, Ludger Beerhues3

1Pharmaco gnos y Dep artment, Facu lty o f Phar macy, Helwan Univer sity, Cairo , Egypt ; 2Pharma cogn osy Dep artmen t, F acult y of P harma cy,

Cairo University, Cairo, Egypt; 3Institut für Pharmazeutische Biologie, Technische Universität Braunschweig, Braunschweig, Ger-

many.

Email: *mohibrahem@yahoo.com

Received S eptember 26th, 2010; revised October 24th, 2011; accepted November 5th, 2011.

ABSTRACT

A comparative study was carried out with ethanolic (80%) extracts from leaves and cell cultures of three Callistemon

species, namely C. lanceolatus (CL), C. viridiflorous (CV), and C. comboynensis (CC). Cell suspensions of the three

species were grown in liquid Murashige and Skoog (MS) medium (100 ml) supplemented with 0.9 mg·g–1 kinetin in

combination with 1.1 mg·g–1 NAA. The CL leaf extract was standardized to contain the highest amount of phenolics

(104 ± 2.0 mg·g–1), followed b y CC (95.8 ± 1.2 mg·g–1) and CV (79.8 ± 4.6 mg·g–1). On the other hand, cell cultures of

CV contained more phenolics (14.9 ± 0.6 mg·g–1) than those of the other two species, CL an d CC, which contained 12.2

± 0.16 and 9.12 ± 0.16 mg·g–1, respectively. Nevertheless, CV leaf extract exhibited the highest antioxidant activity

(91.4% ± 0.4%) at a concentration of 1000 µg·ml–1, comparable to 100 µg·ml–1 gallic acid (90.8% ± 1.5%).

Keywords: Callistemon, Phenolic Content, Antioxidant Activity, Callus, Cell Cultures

1. Introduction

The genus Callis temon (Myrtaceae) contains 34 species

of beautiful evergreen shrubs and small trees. The majo-

rity of the Callistemon species is endemic to the more

temperate regions of Australia, four species are found in

New Caledonia and seven species have been introduced

to India as ornamental trees [1]. They are commonly kno-

wn as bottle brushes because of their cylindrical brush-

like flowers resembling the traditional bottle brush.

C. lanceolatus, also named C. citrinus, is a well-

known shrub. Leaves of this plant are used as a tea sub-

stitute and have a refreshing flavor. Many phenolic com-

pounds of this plant have been identified [2]. Due to the

over-exploitation for its volatile oil and secondary me-

tabolites, there is a great need to develop alternative stra-

tegies of conservation and industrial production of the

bioactive compounds from this plant [3]. No reports of

works were found concerning the other two species, C.

viridiflorou s and C. comboynensis.

In vitro cultures have the potential to form secondary

metabolites and to exhibit bioactivity comparable to the

original plant [4,5]. Cultured cells may serve industrial

purposes, e.g. by immobilization of cells in a matrix for

use in bioreactors. Besides the genetic potential of the

donor plant for callus induction and growth of this callus

in in vitro cultures, a medium containing sufficient nu-

trients, such as the preferred MS medium, is required [4].

Antioxidants play an important role in the prevention

of human diseases. Antioxidant compounds may function

as free radical scavengers, complexing agents for pro-

oxidant metals, as well as reducing agents and quenchers

of singlet oxygen formation [6-8]. Antioxidants are often

used in oils and fatty foods to retard their autoxidation.

Therefore, the importance of the search for natural anti-

oxidants has greatly increased in recent years [9]. A fo-

cus is on plant-derived polyphenols because of their po-

tential antioxidant and antimicrobial properties. Phenolic

compounds exhibit considerable free-radical scavenging

activity, which is determined by their reactivity as hy-

drogen- or electron- donating agents, their reactivity with

other antioxidants and their metal chelating properties, as

well as the stability of the resulting antioxidant-derived

radicals [10,11].

Our present work is a comparative study of leaves and

Total Phenolic Content and Antioxidant Activity of Standardized Extracts from Leaves and Cell Cultures of

848 Three Callistemon Species

cell cultures of three Callistemon species with respect to

their potential as antioxidant agents in relation to their

total content of phenolic compounds.

2. Materials and Methods

2.1. Plan t Ma teria l

Plants of three Callistemon species, C. lanceolatus (CL),

C. viridiflorus (CV), and C. comboynensis (CC), were

collected from a cultivated area in Cairo, Alexandria

Road, Egypt. They were kindly authenticated by Prof. Dr.

M. Gebali (Plant Taxonomy and Egyptian Flora De-

partment, National Research Center, Giza, Egypt). A

voucher specimen of each was deposited at the herbar-

ium of the Pharmacognosy Department, Faculty of Phar-

macy, Helwan University, Cairo, Egypt.

2.2. Calli and Cell Cultures

Callus of CL was induced by a combination of 0.9

mg·L–1 kinetin and 1.1 mg·L–1 NAA [12]. Calli of CV

and CC were similarly induced (the detailed methodo-

logy will be published later on). Calli material (0.3 g

each) were collected in the active growth phase (after the

15th day of subculture) and placed in 250 ml flasks con-

taining 100 ml liquid MS medium supplemented with 0.9

mg·L–1 kinetin in combination with 1.1 mg·L–1 NAA.

The resulting cell cultures of the three Callistemon spe-

cies were incubated in a horizontal shaker at 100 rpm

and 25˚C for 21 days.

2.3. Preparation of the Extracts

The three cell suspension cultures were aseptically fil-

tered and the cells dried in a vacuum oven at 40˚C, to-

gether with the leaves of the three species. They were

then macerated in 80% ethanol for two days, filtered and

macerated for another two days. After filtration, they

were concentrated under vacuum at 50˚C.

2.4. Evaluation of the Antioxidant Activity

Determination of the free radical scavenging activity of

the different extracts was carried out using a modified

quantitative DPPH (1,1-diphenyl-2-picrylhydrazyl; Sigma-

Aldrich, St. Louis, MO, USA) assay [13]. Various con-

centrations of sample extracts in methanol were prepared

(1000, 500, 250, and 100 µg·ml–1). Gallic acid was used

as a positive control at concentrations of 100, 50, 25, and

10 µg·ml–1. Blan k sample s were r un using 1 ml metha nol

in place of the test extract. One ml of 0.2 mM DPPH in

methanol was added to 1 ml of the test solution, or stan-

dard, plus 1 ml of methanol for dilution and allowed to

stand at room temperature in a dark chamber for 30 min.

The change in colour from deep violet to light yellow

was then measured at 517 nm. Inhibition of free radical

in percent (I%) was calculated according to the following

equation:





I%A0A1 A0100 





, with A0 being

the absorbance of the control reaction (containing all re-

agents except for the extract) and A1 the absorbance of

the extract. Measurements were carried out in triplicates.

2.5. Determination of Total Phenolic Content

A spectrophotometric method after MacDonald [14] was

adopted for the determination of total polyphenols in the

prepared extracts. Folin-Ciocalteu reagent from Merck

(Darmstadt, Germany) was used and a standard calibra-

tion curve was prepared using different concentrations of

gallic acid in methanol (0.025 - 0.400 mg·ml–1). Cell cul-

ture and leaf extracts were prepared in methanol at a

concentration of 0.06 g/3 ml and 0.06 g/20 ml, respec-

tively. Absorbance was measured at 765 nm. For each

sample, three replicate assays were performed. The total

phenolic content was calculated as gallic acid equivalent

(GAE) by the following equation: TCVM . T is

the total phenolic content in mg·g–1 of the extracts as

GAE, C is the concentration of gallic acid established

from the calibration curve in mg·ml–1, V is the volume of

the extract solution in ml and M is the weight of the ex-

tract in g.

3. Results and Discussion

3.1. Phenolic Content of the Extracts

Ethanolic (80%) extracts from the leaves and cell cul-

tures of the three Callistemon species were standardized

for their contents of phenolic compounds. The calibra-

tion curve showed linearity for gallic acid in the range of

25 - 400 µg·ml–1, with a correlation coefficient (R2) of

0.999 (Figure 1). Leaves of CL contained the highest

content of phenolics (104 ± 2.0 mg·g–1), followed by CC

(95.8 ± 1.2 mg·g–1) and CV (79.8 ± 4.6 mg·g–1). On the

other hand, cell cultures of CV were standardized to

contain more phenolics (14.9 ± 0.6) than the cell suspen-

sions of the other two species, CL and CC, which con-

tained 12.2 ± 0.16 and 9.12 ± 0.16 mg·g–1, respectively

(Figure 2).

3.2. Antioxidant Activity of the Extracts

It is well known that there is a strong relationship be-

tween total phenol content and antioxidant activity, as

phenols possess strong scavenging ability for free radi-

cals due to their hydroxyl groups. Therefore, the pheno-

lic content of plants may directly contribute to their an-

tioxidant action [11,15,16].

The standardized Callistemon extracts were assessed

for their capacity to scavenge DDPH free radical along

with gallic acid as a positive control. The antioxidant

activity data are presented as percent of free radical inhi-

Total Phenolic Content and Antioxidant Activity of Standardized Extracts from Leaves and Cell Cultures of

Three Callistemon Species

849

Figure 2. Total phenolic content of leaf and cell culture ex-

tracts from three Callistemon species determined by the

Folin-Ciocalteu assay and calculated as GAE in mg·g–1 ex-

tract base d on dry we ight. Results are t he aver age of t ripl i-

cates ± SD.

Figure 1. Standard calibration curve of gallic acid at con-

centrations of 25, 50, 100, 200, 300 and 400 µg·ml–1. Spec-

trophotometric detection was at 765 nm.

Table 1. Antioxidant activity of Callistemon leaf and cell culture extracts assayed by the DPPH assay.

Conc. of ex tr a ct

µg/ml CL

leaves CV

leaves CC

leaves CL

cultures CV

cultures CC

cultures Conc . of s tandard

µg/ml Gallic acid

1000 73.5 ± 3.2 91.4 ± 0.4 74.4 ± 0.350.7 ± 0.2 71.1 ± 0.4 47.3 ± 1.9 100 90.8 ± 1.5

500 67.3 ± 0.2 78.4 ± 0.2 66.9 ± 0.941.7 ± 1.4 68.4 ± 0.2 44.4 ± 0.3 50 83.7 ± 0.6

250 60.3 ± 2.0 75.4 ± 0.4 57.8 ± 0.738.3 ± 0.4 53.5 ± 0.2 35.3 ± 0.2 25 76.3 ± 0.2

100 48.9 ± 3.7 57.4 ± 0.4 56.3 ± 0.335.9 ± 0.8 46.7 ± 0.2 34.1 ± 0.1 10 65.4 ± 0.1

Activity is expressed as inhibition of free radical in percent, I% ± SD (n = 3). Leaf and cell culture extracts were tested at 1000, 500 , 250 and 100 µg·ml–1 and

the positive control (gallic acid) at 100, 50, 25 and 10 µg·ml–1.

4. Acknowledgements

bition in Table 1. The ethanolic (80%) extracts of the

leaves of CV exhibited pronounced antioxidant activity

(91.4% ± 0.4%) at a concentration of 1000 µg·ml–1, com-

parable to 100 µg·ml–1 gallic acid (90.8% ± 1.5%), al-

though its phenolic content was less than that of CL and

CC (Figure 2). Furthermore, extracts of CV cell cultures

showed antioxidant activity (71.1% ± 0.4%) comparable

to that of leaf extracts of CL and CC at 1000 µg·ml–1,

even though their phenolic contents were approximately

7-fold that of CV cell cultures (Figure 2). It was previ-

ously reported that non-phenolic antioxidants might also

contribute to the antioxidant activity of plant extracts

[17,18]. Thus, compounds other than phenolics might be

responsible for the pronounced antioxidant activity ob-

served with CV extracts, which requires further investi-

gation. Polyphenolic compounds are also believed to

have chemopreventive and suppressive activities against

cancer cells by inhibition of metabo lic enzymes involved

in the activation of potential carcinogens or arresting the

cell cycle [19]. Nevertheless, a compound with strong

antioxidant potential can also contribute to DNA protec-

tion and prevent apoptosis [20]. Further studies are there-

fore required to detect potential anticancer activities of

the extracts reported here.

Part of this research work was funded by the DFG (De ut-

sche Forschungs G emeins chaft).

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