Chemopreventive Properties and Toxicity of Kelulut Honey in Sprague Dawley Rats Induced with Azoxymethane

Ethnopharmacological Relevance. Colon cancer has been a major problem worldwide. Kelulut honey (KH) is produced by the stingless bees from Trigona species and has strong antioxidant activities that could be one of the potential chemopreventive agents from natural resources. Aim of This Study. This study investigated the chemopreventive properties and toxicity of KH in Sprague Dawley rats induced with azoxymethane (AOM). Material and Method. Twenty-four male Sprague Dawley rats aged 5 weeks were divided into 4 groups: (G1) untreated group not induced with AOM, (G2) untreated group induced with AOM, (G3) treated group induced with AOM, and (G4) treated group not induced with AOM. Injection of AOM (15 mg/kg) was via intraperitoneal route once a week for two subsequent weeks. The treatment groups were given oral administration of KH (1183 mg/kg body weight) twice daily for 8 weeks. Results. Treatment with KH significantly reduced the total number of aberrant crypt foci (ACF) and aberrant crypts (AC) and crypt multiplicity. KH was not toxic to the animals since the level of blood profile parameters, liver enzymes, and kidney functions was in normal range. Conclusions. The current finding shows that KH has chemopreventive properties in rats induced with colorectal cancer and also was found not toxic towards the animals.


Introduction
Cancer has been a major problem worldwide. Although colon cancer has been ranked the fourth, the incidence is rising dramatically. Colon cancer ranks the first among males and third among females [1]. There are several treatment modalities for colon cancer such as chemotherapy, surgery, and radiotherapy. Nevertheless, chemotherapy has a few adverse effects such as neutropenia (reduction of leucocytes), diarrhea, and thromboembolic events (blockage of blood vessel) [2]. Hence, numerous researches have been carried out in finding new alternatives for management of colon cancer.
One of the alternative managements is via chemoprevention. Chemoprevention is defined as the use of natural or synthetic substances to reduce the risk of developing cancer or to reduce the chance of cancer to recur. Thus, it is important to inhibit the development of epigenetic and genetic alterations that are part of the process by which clonal proliferation of cells with abnormal genetic content cascades into dysplastic and later malignant cells [3]. In colon cancer, it is an alternative approach to reduce the mortality which involves long-term use of a variety of chemopreventive agents that can inhibit development of neoplasms in the large bowel [4].
Kelulut honey (KH) is produced by the stingless bees from Trigona species. The honey produced by this stingless bee is stored in clusters of small resin pots near their nest. Meanwhile, honey that is produced by normally found bee is stored in hexagonal-shaped combs [5]. KH is more diluted compared to other types of honey and it has distinct taste (sour like taste) as well as aroma [6]. Traditionally, KH is used for antiageing, enhancing libido and immune system, killing bacteria, treatment of bronchial phlegm, and relieving sore throat, cough, and cold [7]. KH has been proven to possess various pharmacological properties such as anti-inflammatory [8], antioxidant [5], antiageing [9], and antibacterial properties [10]. Since KH has strong antioxidant activities, it could be one of the potential chemopreventive agents from natural resources.

Experimental Animals.
A total of 24 male Sprague Dawley rats with body weight of 180 to 220 g at the age of 5 weeks were used. Prior to the experiment, the rats were acclimatized a week with free access to food and water ad libitum. The animals were housed in cages ( = 3) under standard laboratory conditions with 12-hour dark/light cycle, at 20-24 ∘ C with 40-50% relative humidity. Ethic approval was obtained from the Institutional Animal Care and Use Committee (IACUC) of Universiti Putra Malaysia prior to the study (UPM/IACUC/FYP.2015/FPSK.003).

Experimental Procedures.
The rats were divided into 4 groups ( = 6), which were (G1) negative control group (not induced with AOM, without treatment), (G2) positive control group (induced with AOM, without treatment), (G3) treatment group (induced with AOM, treated with KH (1183 mg/kg)), and (G4) toxicity group (not induced with AOM, treated with KH). After acclimatization, AOM (15 mg/kg) was injected intraperitoneally into the rats for two subsequent weeks, once per week, on the first day of each week. Next, KH was administered orally twice daily, in the morning and at night, for eight weeks. The body weight of the rats was recorded every three days. The dosage of KH was calculated based on human intake. Upon termination, the rats were fasted for 8 hours before blood collection. Prior to blood sampling, the rats were anesthetized with ketaminexylazine (75 mg/kg : 5 mg/kg) by intraperitoneal injection. The blood sample (7 mL) was collected by cardiac puncture using a 26 G, 1/2 needle (Terumo5, Belgium, Europe) into nonheparinized (5 mL) and EDTA-containing tube (2 mL) for biochemical (Roche Cobas, USA) and haematological (ABX Pentra 60, Japan) analyses, respectively. The blood collected in nonheparinized tube was then centrifuged at 10,000 rpm for 10 minutes to separate the serum. The organs (colon, liver, and kidney) were removed and weighed before being fixed in 10% formalin.

Determination of Incidence of Aberrant Crypt Foci and
Crypt Multiplicity. The colon was processed by first dividing it into three parts, which are proximal colon (near the caecum), middle colon, and distal colon (towards the rectum). Each part was cut into strip and placed in a cassette. For liver, it was grossed from a lobe of the liver and placed into a cassette. For kidney, the organ was cut into half and placed in a cassette. Next, the organs that had been grossed were processed using an automated tissue processor (LEICA TP 1020, USA) where the machine runs dehydration, clearing, and impregnating process. The organs were being embedded in molten paraffin with appropriate molds to support the tissue during sectioning process. The blocks were trimmed at 16 m thickness and sectioned at thickness of 0.4 m using a microtome. The thin sections of the tissue samples were placed in a water bath and fished onto glass slides. The slides prepared will be dewaxed first before being stained with hematoxylin and eosin (H&E) followed by mounting with Pxylene-bis-pyridinium bromide (DPX) and observed under a light microscope. The total number of ACF per colon, total number of aberrant crypts (AC), and crypt multiplicity of each rat in all groups were calculated.

Statistical
Analysis. The data were analysed by Statistical Package for Social Sciences (SPSS) version 21. One-way ANOVA analysis was performed followed by Duncan's test. The data was presented as mean ± SEM. Value of < 0.05 was considered as significant. Figure 1 shows the body weight of all groups throughout the experiment. There was a gradual increase in the body weight throughout the 8 weeks of study. The highest body weight was noted in G2 followed by G1, G3, and G4. However, there was no significant difference in the body weight among all groups ( > 0.05).  Table 1. Data show no significant difference in the blood profile among all groups ( > 0.05). Table 2 shows the liver enzymes and kidney function tests of rats in 4 different groups show no significant difference in all the parameters tested among all groups ( > 0.05). Table 3 shows the effects of KH on the length of the colon in all groups throughout the experiment. The highest colon length was noted in G1 followed by G3, G4, and G2. However, there was no Table 1: Effects of KH on the blood profile of rats after 8 weeks of study. The data were analysed by using one-way ANOVA and the values are expressed as mean ± SEM. Value of < 0.05 was considered significant.    Table 4 shows the total ACF and total aberrant crypts (AC). The total number of ACF and AC and crypt multiplicity were significantly lower in G3 compared to G2 ( < 0.05).

Histological Classification of Aberrant Crypt
Foci. ACF can be classified according to the number of crypts per foci, for example, 1 crypt, 2 crypts, 3 crypts, and ≥4 crypts per focus as being shown in Figure 2.

Discussion
This study was carried out to investigate the chemopreventive properties of KH towards Sprague Dawley rats induced with AOM. In this study, AOM was proven to induce ACF formation as reported by Bird [11]. In this model, ACF formation is used as biomarker to identify the progression of development of colon cancer. KH has chemopreventive properties against Body weight (g) Figure 1: Effects of KH on the body weight of rats after 8 weeks of study. The data were analysed using one-way ANOVA and the values were expressed as mean ± SEM. Value of < 0.05 was considered significant.
azoxymethane-induced colon cancer based on the reduction of total number of ACF, total number of AC, and crypt multiplicity. Gribel and Pashinskiȋ [12] reported that honey possesses moderate anticolon cancer activity. Even though they used normal honey, Souza et al. [13] stated that there is only a slight difference in properties between honey produced by Apis bees and honey produced by stingless bees. It is believed Table 4: Effects of KH on the incidence of azoxymethane-induced aberrant crypt foci of rats after 8 weeks of study. The data were analysed by using one-way ANOVA and the values are expressed as mean ± SEM. Value of < 0.05 was considered significant.  that one of the components of KH that is responsible for its anticolon cancer properties is caffeic acid ester [14]. According to Xiang et al. [15], caffeic acid esters suppressed the transcriptional activity of -catenin and hence can become an agent against colon cancer. Caffeic acid phenethyl ester (CAPE) is a phenolic antioxidant, which has biological and pharmacological functions that include immunoregulation, anti-inflammatory, antiviral, antibacterial, and antitumor activities [16]. CAPE has antiproliferative and apoptosisinducing effect in various tumor cells in vitro and in vivo [17,18]. According to Borrelli et al. [19], CAPE inhibited the development of AOM-induced ACF in the colon of rats.
In traditional usage, honey including KH is taken twice daily usually in the morning and at night. Based on the density, the daily intake of KH for human is 189.33 mg/kg. In this study, we were trying to mimic the way KH is being consumed by human. The dose of KH for rat consumption is calculated according to FDA dose translation formula. Thus, a rat received 1183 mg/kg bodyweight of KH.
Surprisingly, in this study, ACF were also found in the normal group. This could be due to the fact that normal body mutation also occurs. Mutation can occur in body because of several factors such as food, surroundings, and exposure to carcinogenesis agents [20].
KH was proven to be not toxic to the animals. There was no reduction in body weight. According to Peterson et al. [21], when there is a presence of toxicity, the body weight of the studied organism should be decreased. In addition, the levels of parameters for blood profile, liver enzymes, and kidney functions were in normal range. According to Wang et al. [22], abnormal values of blood profile, liver enzymes, and kidney function are an indication of toxicity.
In summary, KH has chemopreventive properties in rats induced with colon cancer by reducing the development of ACF, AC, and crypt multiplicity. KH was also to be found not toxic towards the animals.