Effect of FFD-410 (HiOwna-Jr.), a Balanced Herbal Nutritional Supplement on Biochemical, Hematological, Immunological and Cognitive Parameters of Wistar Rats ()
1. Introduction
Dietary/Nutritional factors are well known to play a pivotal role in enhancement of health status and physical strength in human [1]. The portion of any nutrient that is immediately available for metabolic processes of the organism after absorption is called as available portion of the nutrition; nutritional value of a food is decided based on its chemical composition [2].
In US, majority of the adults are regularly using the products containing essential nutritional supplements in order to maintain wellness or treat an illness. In this context, natural products are very commonly used in the folk medicine to treat various nutrition related diseases/disorders, but the information supporting the efficacy of natural products was anecdotal [3].
However, high quality and hypothesis-driven studies in animals and humans as well as in vitro systems have greatly contributed to our knowledge of the safety and efficacy of these products and also have helped in understanding the underlying mechanisms [3]. As a consequence, an ever increasing number of phytochemicals are being recognized not only for their abilities to prevent disease states and support wellness (chemoprotective properties), but also to effectively treat various diseases [4].
In literature, several investigators have reported that, ingestion of some plant extracts and food supplements from fruits and vegetable origin are highly beneficial in combating the nutritional deficient states [5]. In addition to satisfying the daily nutritional demands, most of the daily consumed vegetables and fruits have been scientifically proved to possess medicinal properties such as immunomodulatory activity [6,7], anti-oxidant activity [8, 9], anticancer activity [10], anti-diabetic activity [11], antiulcer activity [12], anti-diarrheal activity [13], memory enhancing [14] and wound healing [15] activity. In this context, formulations/preparations containing herbal supplements are thought to be beneficial in fulfilling the daily nutritional demands and maintaining the normal gustatory functions.
FFD-410 (HiOwna-Jr.) is a herbal-based, nutritionally balanced pediatric health drink manufactured by the Himalaya Drug Company, Bangalore, India, as a supplement for childrens. Each five grams of FFD-410 contains extracts of plants Eleusine coracana—20 mg; Centella asiatica—15 mg and powders of Colostrum—7 mg; Emblica officinalis—50 mg and Piper nigrum—6 mg. FFD- 410 is nutritionally well balanced and rich in all the essential nutrients such as carbohydrates, proteins, fats, vitamins and minerals. Each 25 g of FFD-410 powders serves approximately 87.0 kcals of energy to meet the daily metabolic needs. With this background present study was undertaken to evaluate the effect of FFD-410 on biochemical, haematology, immunological and cognitive functions in rats; also in vitro antioxidant studies were carried out to evaluate its antioxidant/free radical capacity.
2. Materials and Methods
2.1. Drugs and Chemicals
Trolox (Sigma-aldrich, Bangalore), Fluoroscein (Sigmaaldrich, Bangalore), (1, 1-diphenyl-2-picrylhydrazyl (Sigma-aldrich, Bangalore), biochemical kits (Erba diagnostic) and all other chemicals and reagents used for the study were of Analytical grade and purchased from Himedia Laboratories Pvt Ltd.
2.2. Experimental Animals
Inbred wistar rats (Body weight of 120 - 140 grams, 6 weeks old) were used for the study. The animals were maintained in polypropylene cages at a temperature of 25˚C ± 1˚C and relative humidity of 45% to 55% in a clean environment under 12:12 h light-dark cycle. The animals had free access to food pellets (Pranav Agro Industry, Bangalore, India) and purified water.
All the experimental protocols were approved by Institutional Animal Ethics Committee (IAEC) of the Himalaya Drug Company and were conducted according to the guidelines of Committee for the Purpose of Control and Supervision of Experimentation on Animals (CPCSEA), India.
2.3. In Vivo Studies
Forty eight wistar rats (24 males and 24 females) were divided in to 3 groups of 16 each (G-I to G-III), each group consists of 8 males and 8 female animals. The male and female animals were housed separately in a false bottom cages. All the animals were provided with standard laboratory diet (Nutrilab). G-I served as Normal control (DM water, 20 ml/kg, p.o.), G-II received FFD- 410 (2.5 g/kg, p.o) and G-III received FFD-410 (5.0 g/kg, p.o.). The treatments were given for 90 days; feed intake and body weight were recorded every week till the end of the study. On 91st day, blood samples were collected from all the animals for the estimation of hematological and biochemical parameters. At the end of 10th week, the short-term cognition was evaluated for all the animals by modified elevated plus maze test.
2.3.1. Effect of FFD-410 on Cognitive Functions in Rats by Modified Elevated plus Maze Test
At the end of 10th week, one hour after the last administration, all the animals were tested on elevated plus maze for transfer latency. In brief, each animal was placed individually at the end of open arm facing away from centre of the maze and the time taken by animal to enter from open to closed arm is recorded (Transfer Latency). On day-1, all the animals were allowed to explore the plus maze for 90 sec, if the animal did not enter into one of the enclosed arm within 90 sec, it is gently pushed to one of the enclosed arms and TL was recorded as 90 sec (1st trial) and animal were allowed to explore the maze for another 10 sec and returned into the home cages after the 1st trial. Retention latency (RT) was assessed 24 hrs later, 1 hr after the drug administration.
2.3.2. Effect of FFD-410 on Serum Immunoglobulins
After scheduled treatment of FFD-410 for 10 weeks, blood samples were collected from all the animals and serum was separated used for estimation of immunoglobulin levels. A control tube containing 6 ml of distilled water was used as sample blank for each serum sample to be analyzed. To 6 ml of zinc sulphate solution 0.1 ml of serum was added, the test tube was inverted to enable complete mixing of the reagents with the serum and allowed to stand for 1 h at room temperature. The first tube served as blank and the second tube was taken as sample. The turbidity developed was measured. The turbidity obtained (sample-blank) was compared with that obtained with standard barium sulphate (BaSO4) solution. The turbidity obtained with this solution was expressed as zinc sulphate turbidity (ZST) units.Also, at the end of 10th week, all the animals were sensitized with a single intraperitoneal injection of 0.1 ml Sheep Red Blood Cells (SRBC 5 × 108 cells in PBS). On day 5 of sensitization, the blood samples were collected and subjected for estimation of hemagglutination antibody titre (HA Titre) with SRBC.
At the end of 90 days of treatment, blood samples were collected from all the animals for estimation of vital biochemical and haematological parameters, also the organs were collected, weighed and expressed as relative organ weight per body weight.
2.4. In Vitro Antioxidant Activity
Preparation of Test Drug Solution: All the drugs were prepared in DM water with a stock concentration of 10 mg/ml only water-soluble portion were used for the assay.
2.4.1. In Vitro DPPH Radical Scavenging Activity
DPPH Radical Scavenging Activity: To the 100 µl of test drug solution in water at different concentrations (The stock sample solutions was serially diluted with respective solvents to obtain lower dilutions) 100 µl of 0.1 mM solution of DPPH in ethanol was added. Thirty minutes later, the absorbance was measured at 517 nm. Lower absorbance of the reaction mixture indicates higher free radical scavenging activity. Vitamin C was used as standard. The capability to scavengse the DPPH radical was calculated using the following equation:
The antioxidant activity of the test drug was expressed as IC50 (mcg/ml). The IC50 (mcg/ml) value is defined as the concentration (in µg/ml) of test drug that inhibits the formation of DPPH radicals by 50%. The assays were run in quadruplicate and the average IC50 (mcg/ml) value was calculated and compared against the standard [16].
2.4.2. Reducing Power Assay
This method employs the Fe3+ - Fe2+ redox system and change absorbance with respect to concentration are recorded and plotted in the form of graph. Various concentrations of drug (The stock sample solutions were serially diluted to obtain lower dilutions) in 1.0 ml of deionized water was mixed with phosphate buffer (2.5 ml, 0.2 M, pH 6.6) and 1% potassium ferricyanide (2.5 ml). The mixture was incubated at 50˚C for 20 min’s. Aliquots of trichloroacetic acid (2.5 ml, 10%) were added to the mixture, which was then centrifuged at 1036 ×g for 10 min. The upper layer of solution (2.5 ml) was mixed with distilled water (2.5 ml) and a freshly prepared FeCl3 solution (0.5 ml, 0.1%). The absorbance measured at 700 nm. Increased absorbance of the reaction mixture indicates increased reducing power. Alternatively the assay was also miniaturized and was carried out in 96-well plate (Tarsons), where, volumes of reagents were proportionally reduced. The absorbance of each well was read using BIOTEK multimode (SYNERGY-HT) plate reader [16].
2.4.3. Oxygen Radical Absorbance Capacity (ORAC) Assay
The ORAC procedure used an automated plate reader (Synergy™ HT Multi-Detection Micro plate Reader KC4, Bio Tek, USA) with 96-well plates [16,17]. Analyses were conducted in phosphate buffer pH 7.4 at 37 1C. Peroxyl radical was generated using 2, 2’-azobis (2-amidino-propane) dihydrochloride which was prepared fresh for each run. Fluorescein was used as the substrate. Fluorescence conditions were as follows: excitation at 485 nm and emission at 520 nm. The standard curve was linear between 0 and 50 mM Trolox. Results are expressed as Total ORAC value as TE/g (Trolox Equivalent per gram) of fresh sample.
2.5. Statistical Analysis
The values were expressed as mean ± SEM. The results were analyzed statistically using one way ANOVA followed by dunnet’s test to find out the level of significance. The minimum level of significance is fixed at p < 0.05. All the in vitro antioxidant assays were carried out in triplicates, while the in vivo study was conducted at once.
3. Results and Discussion
From past few decades the use of phytochemicals, nutraceuticals and other herbal products have increased dramatically due to their low level of side effects and better therapeutic efficacy in providing health benefits [5]. Expanding research and anecdotal reports on nutraceuticals and related herbal products have convinced the healthcare community and the general population [5]. Numbers of nutritional supplements in the form of oral formulations have been developed from herbs are proved to be beneficial in treating the nutritional deficiency states. FFD-410 is one of such formulation developed by The Himalaya Drug Company, Bangalore, India and indicated as a heath supplement in pediatrics.
In present study, HiOwna-Jr. (FFD-410) was evaluated for its beneficial effect on parameters such as body weight, feed intake, biochemical and hematological paprameters, also evaluated for its beneficial effect on immunity, learning and memory in rats at 2.5 g/kg and 5.0 g/kg. p.o.
3.1. Effect of FFD-410 on Biochemical and Hematological Parameters
There was no statistically significant change clinical biochemistry (Tables 1 and 2), hematological parameters (Table 3) and relative organ weights (Table 4) were observed after 90 days of FFD-410 treatment at 2.5 and 5.0 g/kg dose levels. However there was statistically significant increase in hemoglobin and total RBC counts were observed in high dose of FFD-410 treated female rats. Further, there was a statistically significant decrease in SGPT and ALP levels were also observed at high dose treated male rats.
3.2. Effect of FFD-410 on Immune System
For evaluating the immunomodulatory property of FFD- 410, haemoagglutination test was conducted in rats to evaluate the effect of test formulations on humoral response. The findings of the study revealed that, pretreatment with FFD-410 (2.5 & 5.0 g/kg) could boost the immune system significantly and dose dependently by increasing the titer values and serum immunoglobulin levels compared to control group (Figures 1(a) and (b)). Based on these findings it can be concluded that, FFD- 410 has immunostimulant property in rats upon long term administration.
3.3. Effect of FFD-410 on Short Term Cognition and Memory
In present study, the short term cognition of memory was evaluated by means of modified elevated plus-maze test; the outcomes of the study showed that, pretreatment with FFD-410 at 2.5 and 5.0 g/kg for 90 days could appreciably decreased the transfer latency (TL) in a dose dependent manner, indicating beneficial effect of FFD-410 in improving the short-term cognition and memory (Figure 1(c)).
3.4. Antioxidant and Free Radical Scavenging Activity of FFD-410
Free radicals are atoms or groups of atoms with an odd (unpaired) number of electrons and can be formed when oxygen interacts with certain molecules. Once formed, these highly reactive radicals can start a chain reaction, like dominoes [18]. Their chief danger comes from the damage they can do when they react with important cellular components such as DNA, or the cell membrane and cells may function poorly or die if this occurs. Antioxidants are molecules which can safely interact with
(a)(b)(c)
Figure 1. Effect of FFD-410 on (a) Sheep Red Blood Cellinduced hemoagglutination titre, (b) Serum immuno-globulin levels by ZnS turbidity assay and (c) Short-term cognition by elevated plus-maze test.
free radicals and terminate the chain reaction before vital molecules are damaged [19]. Although there are several enzyme systems within the body that scavenge free radicals, the body cannot manufacture these micronutrients, so they must be supplied in the diet [18,19].
The food supplement rich in antioxidant constituents are thought to be much beneficial in treating oxidative stress-induced cell damage [20,21]. Especially the plant based constituents such as flavonoids and polyphenols are well proved to be highly beneficial in combating the oxidative stress-induced cellular damage by preventing the formation of free radicals and/or scavenging the formed oxidative radicals [18].
In present study, the in vitro antioxidant studies have showed that, FFD-410 a herbal based nutritionally balanced pediatric health drink has significantly and dose
Table 1. Effect of FFD-410 on serum clinical chemistry parameters in male rats.
Table 2. Effect of FFD-410 on serum clinical chemistry parameters in female rats.
Table 3. Effect of FFD-410 on hematological parameters.
Table 4. Effect of FFD-410 on relative organ weight (gm/100 gm body weight).
dependently scavenged the DPPH free radicals (IC50 value = 1162.6) and absorbed the peroxyl free radicals in the ORAC assay (ORAC value = 76.1 TE/g). In addition, FFD-410 has showed dose denependent antioxidant activity in reducing power assay by increasing the absorbanve of the reaction mixture dose dependently (Table 5). These findings proved that FFD-410 can prevent the formation of free radicals and also scavenge the free radicals formed.
Eleusine coracana, Centella asiatica, Emblica officenalis and Piper nigrum are the chief constituents of FFD- 410, In literature various plant parts and isolated actives from these plant parts have been scientifically proved to possess various pharmacological properties such as antioxidant activity [22-24], immunomodulatory activity [25- 28], cytoprotective activity [29-32], cognitive and memory enhancing activity [33-36] and so on.
In present study, the combination of all these beneficial constituents in FFD-410 showed potent antioxidant and immunostimulant activities associated with enhanced cognitive functions through one/more mechanisms. Also, it is worth to note that high dose of FFD-410 tested has increased the total RBC count and hemoglobin content in female rats.
Table 5. In vitro antioxidant activity of FFD-410.
4. Conclusion
Our findings suggest that FFD-410 possess very good antioxidant, cognition and memory enhancing properties apart from being a good immuno stimulant. The FFD-410 (500 mg/kg) treated female animals, also showed mild but statistically significant increase in haemoglobin levels. However, 90 days of treatment with FFD-410 doesn’t bring about any negative change in vital biochemical, haematological parameters and also relative organ weights, which could account for its wide safety of margin at tested dose levels (2.5 & 5.0 g/kg, p.o.).
5. Acknowledgements
The authors are thankful to Dr. Shyam Ramakrishnan, Chief Scientific Officer, R&D Center, The Himalaya Drug Company, Bangalore, India, for his constant support and encouragement.
NOTES
#Corresponding author.