Achievements in the Life Sciences 10 (2016) 5–10

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Achievements in the Life Sciences

journal homepage: www.elsevier.com/locate/als

Hepatoprotective effect of the Aqueous Extract and 5-Hydroxy, 7,8,2′

Trimethoxy Flavone of Andrographis alata Nees. in Carbon Tetrachloride
Treated Rats
Y.P. Nagaraja a,⁎, V. Krishna b
a
Department of Biotechnology, Nagarjuna College of Engineering and Technology, Venkatagiri kote Post, Mudugurki, Devanahalli, Bangalore 562164, Karnataka, India
b
Department of Biotechnology, Kuvempu University, Shankaraghatta, Karnataka, India

a r t i c l e i n f o a b s t r a c t

Article history: This study was designed to evaluate the hepatoprotective activity of aqueous extract and
Received 30 December 2015 isolated flavone (5-hydroxy, 7,8, 2’trimethoxy flavone) compound of Andrographis alata against
Accepted 10 May 2016 CCl4 induced hepatotoxicity. The hepatotoxicity was induced in albino rats CCl4 (i.p.). Analysis
Available online 8 June 2016
of serum ALT, AST and alkaline phosphatase activities with the concentrations of albumin, total
protein and bilirubin was carried out. The activities of all the marker enzymes reported a
Keywords: significant elevation in CCl4 treated rats, which were significantly recovered towards an almost
Andrographis alata Nees normal level in animals simultaneously administered with aqueous extract and flavone com-
Aqueous extract
pound. This work suggests that aqueous extract and isolated flavone compound of A. alata
Flavone compound
exert significant therapeutic effect on CCl4 induced hepatotoxicity in rats.
Hepatotoxicity
Carbon tetra chloride © 2016 Far Eastern Federal University. Hosting by Elsevier B.V. This is an open access article
Liver under the CC BY-NC-ND license (http://creativecommons.org/licenses/by-nc-nd/4.0/).

Introduction

Medicinal plants form the backbone of traditional system of medicine in India. Pharmacological studies have acknowledged the
value of medicinal plants as potential source of bioactive compounds (Prusti et al., 2008). The higher plant products have shown
to be effective sources of chemotherapeutic effects without having any side effects (Neetu and Meenakshi, 2003). All aerobic or-
ganisms including humans have antioxidant defense mechanisms that protect against oxidative damage. However, the natural an-
tioxidant defense mechanisms can be insufficient and hence dietary intake of antioxidant components is important and
recommended (Duh, 1998).
Andrographis alata Nees. (Acanthaceae) is a perennial branched erect herb is distributed abundantly in Southeast Asian coun-
tries namely India, Sri Lanka, Pakistan and Indonesia, but it is cultivated extensively in China and Thailand, the East and West In-
dies and Mauritius for medicinal purposes (Anonymous, 2001). The genus Andrographis posses immense medicinal value. More
than 20 diterpenoids and over 10 flavonoids have been reported from this species (Wenkui et al., 2007).
Since it has been demonstrated that flavonoids have potent antioxidant activities by scavenging hydroxyl radicals, superoxide
anions and lipid peroxyl radicals (Alan and Miller, 1996), it is reasonable to evaluate the antioxidant property of the aerial parts of
this plant. Thus this present investigation was undertaken to evaluate the hepatoprotective activities of aqueous extract and fla-
vone isolated compound of the leaves of A. alata against oxidative damage induced by CCl4 in rats.

⁎ Corresponding author. Fax: +80 227645900.

E-mail address: Drnagaraja_yp@rediffmail.com (Y.P. Nagaraja).
Peer review under responsibility of Far Eastern Federal University.

http://dx.doi.org/10.1016/j.als.2016.05.002
2078-1520/© 2016 Far Eastern Federal University. Hosting by Elsevier B.V. This is an open access article under the CC BY-NC-ND license
(http://creativecommons.org/licenses/by-nc-nd/4.0/).
6 Y.P. Nagaraja, V. Krishna / Achievements in the Life Sciences 10 (2016) 5–10

Materials and Methods

Animals

Male Swiss Wistar Albino Rats weighing about 150 to 200 g on the average were selected for clinical studies and were obtained
from National College of Pharmacy, Shimoga, Karnataka. The rats were fed with commercial diet (Pranav Agro Industries Ltd., Sangli)
and tap water ad-libitum during the experiments. The Institutional Animal Ethical Committee (Reg. No.144/1999/CPCSEA/SMG) per-
mitted this study. Acute toxicity studies were conducted according to ‘staircase’ method (Ghosh, 1984).

Chemicals

Chemicals used in this experiment are of analytical grade and purchased from various companies like Qualigens, Sisco research
laboratories Hi-media and Ranboxy. The reagents used were prepared in all glass-distilled water.

Plant Material and Extraction

The leaves of A. alata were obtained from forests of Malebennur Range, Davanagere and Joldhal range, Chitradurga, Karnataka,
India. The aerial parts of the plant were collected and shade dried for a week and powdered mechanically (Sieve no. 10/44).
Powdered materials were extracted using a Soxhlet apparatus with ethyl acetate for about 48 h. The extract was filtered and con-
centrated in a vacuum under reduced pressure using a rotary flash evaporator (Buchi, Flawil, Switzerland). The melting point was
determined using a melting point apparatus (Jindal, New Delhi). The characterization of the compound was done by IR, 1H NMR,
13
C NMR and mass spectroscopic studies.
100 g of leaf-powdered material of A. alata was extracted with 500 ml of distilled water. The aqueous extract was concentrated
in a vacuum using a rotavapour and the concentrated extract was dried over the water bath to get an anhydrous powdered ma-
terial. 500 mg of dried aqueous extract was taken in a conical flask and dissolved in 50 ml of distilled water (1 ml/10 mg). The
mouth of the flask was sealed with aluminum foil and the contents are autoclaved at 120 °C for 15 min. 500 mg of flavone com-
pound was taken in a conical flask into which 50 ml of distilled was added (1 ml/10 mg) and the contents are autoclaved at
120 °C for 15 min.

Experimental Design

The rats were randomly divided into four groups. The first group was administered with 0.2 ml/kg body weight of distilled
water, intraperitonially (i.p.). This was done biweekly for 4 weeks and was used as control. Liver damage was induced in the
groups of second, third and fourth groups by i.p. of CCl4. Each animal of these groups was administered with 0.2 ml kg body
weight of CCl4. This was done biweekly for a period of four weeks in a similar way. From the third day onwards the third
group was administered daily with 1 ml /kg body weight of aqueous extract. Similarly, the fourth group was administered
with 1 ml kg body weight of 5-hydroxy, 7,8,2′ trimethoxy flavone. Depending upon the administration of plant part and the
compound extract, each group of animals was fed separately.
After the experimental period of seven days, animals were sacrificed by light ether anesthesia and venous blood was collected
into sample bottles containing no anticoagulant (Adebayo et al., 2003). The blood samples were allowed to clot and the serum
was obtained by centrifuging at 3000 rpm for 5 min (Ogbu and Okechukwu, 2001). The clear serum was removed by pipetting,
which was used for the assay of biochemical parameters.

Biochemical Studies

The determination for the assay of aspartate aminotransferase (AST) and alanine aminotransferase (ALT) was done using the
method described by Reitman and Frankel, 1957 Further activities and the determination of concentrations of total serum protein,
albumin globulin ratio by Biuret method described by Kingsley, 1939, total bilirubin and estimation of serum alkaline phosphatase
activity by Bessay et al., 1964. The determination for the assay of aspartate aminotransferase (AST) was done using the method
described by Reitman and Frankel, 1957 and alanine aminotransferase (ALT) by Reitman and Frankel, 1957 activities and the de-
termination of concentrations of total serum protein, albumin globulin ratio by Biuret method (Kingsley, 1939), total biliburin. Es-
timation of serum alkaline phosphatase activity (Bessay et al., 1964).

Antihepatotoxic Studies

The liver samples were excised from the animals of each group washed with normal saline. Initially the materials were fixed in
10% buffered neutral formalin for 48 h. They are processed for paraffin embedding. The sections were taken at 5 μm thickness,
processed in alcohol-xylene series and were stained with alum hematoxylin and eosin. The sections were microscopically exam-
ined for the study of histological changes.
 Y.P. Nagaraja, V. Krishna / Achievements in the Life Sciences 10 (2016) 5–10 7

Fig. 1. 5-Hydroxy-7,8,2′ trimethoxy flavone.

Statistical Analysis

The statistical analysis was carried out by one way analysis of variance and Duncan multiple range test. p Values b 0.05 were
considered significant.

Results

Phytochemical investigations of different extracts of leaves of A. alata were studied. The petroleum ether extract contains ste-
roids, diterpenes. The chloroform extract contains alkaloids, lactones. Ethyl acetate extract contains flavonoids, lactones. Ethyl ac-
etate extract was collected and subjected to spectroscopic analysis and from the data the compound was identified as 5-hydroxy-
7,8,2′-trimethoxy flavone (Fig. 1).
In the present investigation, at the end of each week of treatment (4 weeks), the blood samples of CCl4 treated group showed
significant increase in the levels of serum total bilirubin, compared to normal group of animals. Simultaneous administration of
CCl4 aqueous extracts of A. alata leaves and the flavone compound to the animals significantly reduced (p b 0.05) the level of un-
conjugated bilirubin in serum to the range of control value (Table 1). The highest effect in reducing the toxic effect of CCl4 is no-
ticed in flavone administered group.
Albumin level in CCl4 treated groups was significantly decreased. The effect of aqueous extract and flavone compound was de-
termined individually and it has been noticed that, even with the toxic effect of CCl4 the A. alata is most effective in maintaining
the normal concentrations to a considerable extent and in decreasing the level of serum of total protein compared with the con-
trol group.
It was observed that in CCl4 treated groups due to chronic hepatotoxicity, the serum levels of AST and ALT were significantly
increased. Simultaneous administration of aqueous extract and flavone compound prevented the increase in the levels of AST and
ALT (Table 1). In all the treated groups, the level of these enzymes was invariably increased because secondary rise in the level of
enzymes noticed. Since, CCl4 was treated along with the plant extracts, there was a gradual increase in the levels of enzyme as
noticed from first to fourth week.
Serum alkaline phosphatase is a globulin enzyme of low molecular weight found in higher concentrations of bones,
hepatobiliary tract and kidney. In normal groups of animals, the concentration of this enzyme in the serum ranges from 8–9 in-
ternational units/mg of protein. In CCl4 treated group due to necrosis of hepatobiliary tract the level of the enzyme was signifi-
cantly increased when compared to that of the normal animals (Table 1).
Fig. 2 shows a magnification of the changes of liver histopathology from the normal control. Normal cellular architecture with
distinct hepatic cells, sinusoidal spaces and a central vein were observed in the normal control group (Fig. 2a). However, CCl4 in-
toxicated treatment exhibited severe histopathological changes, such as ascentrilobular hepatic necrosis, fatty change, Kupffer cell

Table 1
Effect of A. alata on the alteration of serum bilirubin, AST, ALT and alkaline phosphatase levels in albino rats against CCl4 induced hepatitis.

Biochemical tests I II III IV

Control 0.24 ± 0.03 9.39 ± 0.32 7.86 ± 0.32 09.01 ± 0.12

CCl4 treated 4.9 ± 0.12 42.2 ± 0.41 47.7 ± 1.08 33.40 ± 0.42
Aqueous extract of A. alata 1.96 ± 0.07 21.6 ± 0.27 16.7 ± 0.25 12.20 ± 0.12
Flavone compound of A. alata 1.87 ± 0.04 14.5 ± 0.4 15.4 ± 0.2 09.19 ± 0.13
F-value for material to material compensation 170.60 684.44 364.71 752.64
p Value at 5% level b0.05

The values are expressed as mg/dl and mean ± S.D. of four animals in each group.
I — serum bilirubin level.
II — serum AST level.
III — serum ALT level.
IV — serum alkaline phosphatase.
8 Y.P. Nagaraja, V. Krishna / Achievements in the Life Sciences 10 (2016) 5–10

Fig. 2. Photomicrograph of rat liver.

ballooning degeneration and infiltrating lymphocytes (Fig. 2c). Pretreatment with aqueous extract and flavone compound
prevented these histopathological changes associated with the hepatotoxicity from CCl4 intoxicated treatment (Fig. 2d).

Discussion

The hepatotoxicity induced by carbon tetrachloride induced liver enhances lipid peroxidation, which results in accumulation of
trigylcerides in the hepatic parenchymal cells (Schotz et al., 1964). The changes associated with CCl4 are biotransformed by the
cytochrome P-450 system to produce CCl3 a free radical, that binds to lipoprotein and leads to peroxidation of lipids of endoplas-
mic reticulum and finally result in cell death (Okuno et al., 1986; Recknagel et al., 1989).
In the present investigation, the effects of aqueous extracts and flavone compound of leaves of A. alata on CCl4 induced hep-
atotoxicity in experimental animals were evaluated. The animals of group II (received CCl4 alone) showed significant loss in their
body weight and they expressed hesitation for food consumption when compared to the normals (group-I). Animals of group III
received both CCl+ +
4 aqueous extracts of the leaves while, the group-IV received CCl4 flavone compound. These two treated groups
showed normal behaviors in food consumption when compared to CCl4 treated group. Similar type of behaviors in experimental
animals was reported by Farooq et al., (1997).
The histopathological studies are the evidence of efficacy of drug as protectant. Simultaneous treatment of aqueous extract and
flavone compound with CCl4 exhibits less damage to the hepatic cells as compared to the rats treated with CCl4 alone. Intralobular
 Y.P. Nagaraja, V. Krishna / Achievements in the Life Sciences 10 (2016) 5–10 9

veins are damaged but to a lesser extent, endothelium is disrupted at places. Hepatic cells adjoining to the intralobular vein show
damage. The sections of the liver treated with aqueous extract and flavone compound of A. alata and CCl4 reveal better hepato-
protective activity. Hepatocytes show normal appearance and only some cells show higher numbers of vacuoles in the cytoplasm.
The results of histopathological study also support the results of biochemical trials.
Bilirubin is the main bile pigment that is formed from the breakdown of heme in the red blood cells. It is transported to the
liver where it is secreted by the liver into the bile. Conjugation of bilirubin is a prerequisite for its excretion into the bile (Nelson
and Cox, 2000). Malfunctioning of the liver was evidenced by the significant increase (p b 0.005) in the level of unconjugated bil-
irubin in the serum of the group treated with only CCl4 when compared with control (Table 1). Increase in the level of unconju-
gated bilirubin in the blood may result from a defect in the function of the liver to conjugate the bilirubin being produced
(Tripathi et al., 1991; Venukumar and Latha, 2002). The ability of simultaneous administration of CCl4 with aqueous extract
and flavone to significantly reduce (p b 0.05) the level of serum total bilirubin when compared with that of the CCl4 treated
group suggests the potential of the A. alata in clearing bilirubin from the serum.
Albumin, a protein predominantly produced in the liver, decreased as the concentration of the CCl4 elevated. This suggests that
the CCl4 when present in toxic concentrations in the system impairs protein synthesis in the liver. They're in correlation between
the degree of serum hypoalbuminemia and hyperglobulinemia. In CCl4 administered animals, the serum albumin level was mildly
decreased with a moderate elevation of globulin in addition to the total protein level that also decreased because of the reversal of
albumin (A/G) ratio. Even with the toxic effect of CCl4 the aqueous extract of A. alata and flavone was most successful in altering
growth levels of total protein, albumin, globulin and A/G ratio. The results obtained in this experiment are concurrent with then
earlier workers of Visen et al., 1993. The site-specific oxidative damage of some of the susceptible amino acids of proteins is now
regarded as the major cause of metabolic dysfunction during pathogenesis (Bandyopadhyay et al., 1999). Hypoalibuminaemia is
most frequent in the presence of advanced chronic liver diseases. Hence, decline in total protein contests can be deemed as a use-
ful index of the severity of cellular dysfunction in chronic liver diseases, the lowered attainment of near normalcy in total protein
content of serum and a liver disease. The lowered level of total protein recorded in the serum of CCl4 revealed the severity of
hepatopathy. The attainment of near normalcy in total protein content of serum and a liver of CCl4 revealed the severity of
hepatopathy. The attainment of near normalcy in total protein content of serum and a liver of CCl+ +
4 aqueous extract and CCl4 fla-
vone treated rats further elucidated the hepatoprotective effect of A. alata.
Estimation of serum alanine transaminase, serum aspartate amino transaminase and alkaline amino transaminase individually
is helpful in the differential diagnosis of hepatic diseases. In acute hepatitis the rise of AST was greater than that of ALT
(Kontinnen, 1971). On the contrary elevation of ALT was more than AST in alcoholic cirrhosis of liver. Hepatotoxicity was also ev-
idenced by a significant increase (p b 0.05) in activities of serum AST and ALT in the group treated with only CCl4 when compared
with controls. This may be as a result of leakage from the cells through peroxidative damage of the membrane. This is evidenced
by the increase in liver malondialdehyde (MDA) content after the administration of CCl4 only (Pratibha et al., 2004). In the present
investigation also elevation in the ALT, AST and ALP and serum marker enzymes was observed in CCl4 treated group. Animals
administered with CCl+ +
4 aqueous extract and CCl4 flavone group significantly reduced the liver enzyme levels. However,
simultaneous administration of aqueous extract and flavone compound with CCl4 significantly reduced (p b 0.05) the activities
of these enzymes in the serum when compared to CCl4 treated group.
Alkaline phosphatase activity in the liver tissue was found to be increased due to CCl4 toxication but decreased in group-III and
IV. This suggests a protective effect of A. alata on the liver. In all the parameters studied, the hepatoprotective activity of aqueous
extract was significant as similar to that of flavone compound. However, the flavone compound is slightly effective than aqueous
extract.
This study has demonstrated the liver toxicity of A. alata in rats. Treatment with aqueous extract and flavone compound de-
creases the CCl4-induced elevation in biochemical parameters. These findings suggest that the flavone compound was more effec-
tive in bringing about functional improvement of hepatocytes.

Acknowledgments

The authors are grateful to National college of Pharmacy, Shimoga and Dept. of Biotechnology Kuvempu University for provid-
ing facilities to carry out the present research work.

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