Introduction

The number of diabetic patients is rising along with increased prevalence of obesity and physical inactivity. The global prevalence of diabetes has risen from 4.7% in 1980 to 8.5% in 2014 [1]. In 2005, the prevalence of diabetes mellitus (DM) in Iran was 7.7% (about 2 million people) [2]. It is predicted that 5.2 million Iranian people will have DM in 2025 [3]. Diabetes mellitus patients are not allowed to consume sweets because of their adverse effects on blood glucose [4]. Proper dietary alternatives for diabetic patients can be used as one of the available therapeutic strategies that give the patient a sense of satisfaction in addition to controlling blood glucose [5, 6]. Honey is suggested as a safe alternative sweetener for diabetic patients [7].

Moreover, DM is associated with decreased levels of serum insulin, increased lipolysis in adipose tissue, increased fatty acid content in the liver, and increased synthesis of endogen triglycerides (TG) [810]. Recent studies have shown that honey may have beneficial effects on the lipid profile in DM patients [1114]. However, the results of some other studies have not confirmed the beneficial effects of honey [15, 16]. These differences in the results of studies may be due to differences in the nutritional and non-nutritional components of the different types of honey [17, 18]. For example, antioxidant activity and phenolic contents were reported to be higher among Yemeni honey, Acacia edgeworhi honey, Ziziphus spina-christi honey, tropical blossom honey, American-orange source honey, and Iranian-tropical honey [19]. Another study showed that natural origin of the honey determines its chemical components, such as trace elements including Co, Cu, F, Fe, I, Mn, Ni, Sr, and Zn as well as macro minerals, including Cl, Na, K, and Mg [20]. The level of effective factors of honey such as antioxidants, anti-tyrosinase, and anti-bacterial agents are also different among the different types of honey [21].

This study aimed to investigate the effect of three types of honey (acacia, astragalus, and artificial honey) on serum lipid profile in DM and healthy rats.

Material and methods

This experimental study conducted on 64 male Wistar rats to compare the effects of acacia, astragalus, and artificial honey on the level of serum low-density lipoprotein (LDL), high-density lipoprotein (HDL), TG, and total cholesterol (Tchol) levels in type 1 DM and healthy rats. The subjects were 64 male Wistar rats aged 12–14 weeks and weighing 180 to 200 g, which were purchased from the Pasteur Institute, Tehran, Iran. The inclusion criterion was weight between 180 and 200 g, and the exclusion criteria were animal illness or death during the study.

The research was carried out at the animal lab of Hamadan University of Medical Sciences, Hamedan, Iran. According to previous studies, eight rats were considered for each group. Therefore, the total number of required rats was 64 for eight groups. There was no significant difference between the average weight of the rats in the groups. Two main groups, defined as the diabetic group and the healthy group, and each main group included four subgroups. Three subgroups of each main group were given 1 mg/kg of three types of honey (acacia, astragalus, and artificial honey) by oral gavage for 10 weeks, and distilled water was given to the control groups. Rats from each group were placed in two separate cages containing four rats. The rats were kept in standard conditions for 1 week to comply with the new environmental conditions. These conditions included an environment temperature of 20°C, 12 h of light and 12 h of darkness, the body and floor of the cages were made of plastic, and the doors were made of metal. Enough bangs were poured under the cages for having cleanliness and absorbing the moisture of urine and stools of animals, and the bangs were replaced every day for all groups. Dishes of water and food were placed on a metal shelf (cage door) in a specific place and were freely available for the animals.

Diabetes mellitus induction

Streptozotocin (STZ) was used to induce type 1 DM in rats. 60 mg/kg STZ was dissolved in 1 ml normal saline and injected intraperitoneally. Before the injection of STZ, the rats were weighed to determine the required amount of STZ. The blood glucose was monitored by glucometer three days after STZ injection, to confirm DM. A blood drop was obtained from the veins of the tail zone and placed on a glucometer strip to measure the amount of blood glucose. Only animals that had a plasma glucose level over 200 mg/dl were considered as DM. Four other groups were included the study as non-diabetic controls.

Intervention

Two types of honey (acacia and astragalus) were purchased from Hanita company, and artificial honey was obtained from a local producer in Yazd, Iran. The different types of honey or distilled water were given for 75 days to the eight groups by a special tube and a precision syringe gavage as follows: A – DM control group receiving 0.5 ml water per day, B – DM group receiving 1 g/kg astragalus honey, C – DM group receiving 1 g/kg acacia honey, D – DM group receiving 1 g/kg artificial honey, E – healthy control group receiving 0.5 ml water per day, F – healthy control group receiving 1 g/kg astragalus honey, G – healthy control group receiving 1 g/kg acacia honey, and H – healthy control group receiving 1 g/kg artificial honey.

Seventy-five days after the intervention, the rats were kept fasting for 16 h. The FBG was detected through direct puncture of the heart. Then the rats were then killed with ether. The final weight of the rats was measured using a validated scale. All the primary outcomes were measured by Enzyme-linked immunosorbent assay (ELISA), based on the instruction provided by the manufacturer of each kit.

Ethical considerations

This study was approved by the Ethics Committee of Shahid Sadoughi University of Medical Sciences in Yazd, Iran.

Statistical analysis

One-way analysis of variance was used to compare the mean serum levels of lipid profile between the eight groups. Statistical analysis of the data was performed using SPSS software version 16 (Chicago, IL, USA), and p < 0.05 was considered significant.

Results

Table I shows the LDL, HDL, TG, and Tchol levels of the three intervention groups and the control group in DM rats.

Table I

Comparison of mean LDL, HDL, TG, and Tchol levels of honey recipient groups in DM rats (mg/dl)

ParameterAcacia groupMean ± SDAstragalus groupMean ± SDArtificial honey groupMean ± SDControl groupMean ± SDF valueP-value
LDL22.00 ±13.5311.42 ±4.7048.28 ±10.814.94 ±10.8017.6930.001
HDL23.00 ±8.8033 .00 ±7.1016. 8 ±2.2031.90 ±6.708.1330.001
TG70.25 ±32.9050.00 ±27.10115.00 ±31.3062.40 ±16.606.0450.004
Tchol56.12 ±16.3050.00 ±26.60115.00 ±9.2062.40 ±10.207.0770.002

The mean LDL levels in DM rats were significantly different between the groups (p = 0.001). The mean level of LDL in DM rats treated with artificial honey was significantly higher than that seen in the other groups. Post hoc analysis indicated a significant difference in the mean level of LDL in rats treated with artificial honey compared to all other study groups (p = 0.001). The mean LDL level in DM rats treated with astragalus honey was significantly lower compared to all other groups, which indicates a beneficial effect of astragalus honey on the LDL level of DM rats compared to the other types of honey (Table I).

Moreover, there was a significant difference between four groups according to the findings on HDL levels (p = 0.001). The mean level of HDL in DM rats treated with artificial honey was lower than for other types of honey and control groups. The post hoc analysis indicated a significant difference in the mean level of HDL in rats treated with artificial honey compared to astragalus honey and the control groups (p < 0.05). Finally, the post hoc test indicated that the mean HDL level in DM rats treated with astragalus honey was higher compared to all the other groups, which confirmed the higher quality of astragalus honey in this regard compared to other types of honey. The astragalus honey group showed the highest and the artificial honey group showed the lowest levels of HDL among all four groups. Indeed, in DM subgroups, artificial honey decreased (49%) and astragalus honey increased (3.5%) HDL-cholesterol levels compared to the DM control subgroup (Table I).

The mean of Tchol levels in DM rats was also significantly different between the groups (p = 0.002) (Table II). The mean level of Tchol in DM rats treated with artificial honey was higher than for the other types of honey and the control groups. Post hoc analysis indicated a difference in the mean level of Tchol in rats treated with Nodoosh honey in comparison to the astragalus and acacia honey groups (p < 0.05) (Table I).

Table II

Comparison of mean LDL, HDL, TG, and Tchol levels of the groups of healthy rats receiving honey (mg/dl)

ParameterAcacia groupMean ± SDAstragalus groupMean ± SDArtificial honey groupMean ± SDControl groupMean ± SDF valueP-value
LDL45.86 ±44.9036.65 ±22.1052.62 ±14.4048.48 ±19.100.4750.702
HDL19.65 ±9.9016.06 ±6.8014. 25 ±4.0015.60 ±4.600.9200.444
TG134.00 ±34.20124.75 ±53.00116.62 ±36.90104.75 ±31.300.7800.515
Tchol82.00 ±10.2084.00 ±15.3089. 75 ±12.8086.25 ±16.600.4510.718

Moreover, the mean TG levels among DM rats were significantly different between the groups (p = 0.004). The mean level of TG in DM rats treated with artificial honey was higher than for other types of honey and the control group. Post hoc analysis indicated a difference in the mean level of TG in rats treated with artificial honey compared to astragalus, acacia honey, and control groups (p < 0.05). Finally, the post hoc test indicated that the mean TG level in DM rats treated with astragalus honey was lower compared to all other groups (Table II).

Table II shows the LDL, HDL, TG, and Tchol levels of the three intervention groups and the control group in healthy rats. There was no significant difference between the mean level of LDL, HDL, Tchol, and TG in healthy rats treated with different types of honey and the control group.

Discussion

The results of this study showed that the type of honey consumed has an effect on the serum lipid profile of diabetic rats. Astragalus honey decreased LDL, TG, and Tchol levels and increased HDL levels, and artificial honey increased LDL, TG, and Tchol levels and decreased HDL levels in DM rats. In healthy subgroups, the effects of three types of honey were not significantly different. Some other studies have reported a positive effect of the astragalus plant on blood lipid profile [2226], which is consistent with our findings. For example, Liao et al. reported that astragalus extracts could increase HDL in streptozotocin-induced diabetic rats. They believed that this effect of astragalus was due to its polysaccharides [24, 25]. It is reasonable that the beneficial effects of astragalus honey consumption in increasing HDL levels in DM rats can be attributed to its components. The abilities of each honey to modify the serum lipid profile is suggested to be related to its specific components [27]. In general, fructose has been reported as a stimulant for insulin secretion from pancreatic cells [28]. However, the effect of other active ingredients in honey could enhance or decline the effects of fructose [27]. Najafian et al. reported that flavonoids are one of the most important components of honey [29]. Trans-chalcone in honey acts as a mediator in the biosynthesis of flavonoids. The beneficial effect of trans-chalcone on the lipid profile in streptozotocin-induced diabetic rats was previously reported [30]. Wang et al. conducted a study on flavonoids of astragalus extracts and concluded that these flavonoids reduced Tchol and LDL and increased HDL. They recognised the effective flavonoids of plant extracts, including: β-sitosterol, formononetin, calycosin, daucosterol, formononetin-7-O-β-D-glucopyranoside, and calycosin-7-O-β-D-glucopyranoside [31]. According to the results, there was a significant difference between the effects of different honeys on serum Tchol. Tchol in the artificial honey group was the highest and in the astragalus honey group it was the lowest, among the four intervention subgroups. There are few studies on the effect of different honeys on Tchol levels. Mushtaq et al. reported beneficial effects of natural honey on Tchol in a clinical study [32], in line with some other studies [3235]. In the DM honey subtypes, but not in the healthy groups, artificial honey increased the Tchol level by 14% and astragalus reduced it by 34%. It seems that honey exerts its effects only in subjects with diabetes.

The effect of different honey types on serum LDL levels was significantly different, as the artificial honey group led to the highest and the astragalus honey group led to the lowest levels of LDL among all four DM groups. In fact, in the DM subtypes groups, LDL cholesterol levels were decreased by 23% in the Astragalus honey group and increased by 23% in the artificial honey group. This difference was observed only in DM rats, and the effect of the three types of honey on LDL was not significant in healthy subgroups. Lu et al. also reported that the astragalus extract decreased Tchol, TG, and LDL [35].

Based on the results of this study, there was a significant difference in TG levels between the effects of these honeys in the DM group. The artificial honey group had the highest and the astragalus honey group had the lowest levels of TG among all four DM groups after intervention. This difference was seen only in DM rats, and the effect of the three honey types was not significant in the healthy subgroups. A similar study showed that administration of gelam honey at dose of 5000 mg/kg to male rats for 14 days decreased TG levels. This study suggested that the honey might have good effects on blood TG levels and that polyphenol contents of honey may be attributed to the reduction of the TG level [36]. Recent studies reported that artificial honey in patients with hypertriglyceridaemia and hyperlipidaemia increased TG and LDL, while natural honey decreased both of them [37, 38], which is in line with the present study.

However, our study had some limitations. We did not measure the level of lipid profile at baseline. So, we only compared the level of TG, Tchol, and LDL between different diabetic and healthy groups at the end of the study. Further studies with before and after measurements are needed to identify the role of active components of honey and provide proper dietary recommendations to diabetic patients.

In conclusion, the results of this study showed that the different types of honey could have different effects on serum lipid profile. Astragalus honey decreased LDL, TG, and Tchol levels and increased HDL level in DM rats. On the other hand, artificial honey increased LDL, TG, and Tchol levels and decreased HDL level in DM rats. Further studies are needed to identify active components in different honeys and to provide proper dietary recommendations in this area.