Fruit Extract Derived from a Mixture of Noni, Pineapple and Mango Capable of Coagulating Milk and Producing Curd with Antidiabetic Activities

Sample

Noni (Morinda citrifolia L.), pineapple (Ananas comosus L. cv. Sarawak) and mango (Mangifera indica L. cv. Apple) were obtained from various cultivators in the region of Kuantan, Malaysia, and their voucher specimens were deposited at the Institute of Biological Sciences, University of Malaya, Malaysia with voucher numbers HI1445, HI1446 and HI1447, respectively. The seeds (seed coat removed) of mango and the fruits of noni and pineapple were washed thoroughly to remove unwanted contaminants and then cut into pieces. The mango seeds were dried in an oven (Universal oven UN55; Memmert GmbH, Schwabach, Germany) with convection at 50 °C until dry and brittle enough to be pulverized into powder. Noni and pineapple fruits were used fresh to avoid spoilage by fungi under drying.

Preparation of extracts

A total of 10% (m/V) powdered mango seeds were mixed in water for aqueous extraction. The mixture was mixed at a constant speed in a magnetic stirrer (Nuova II Stir Plate; Thermolyne Corporation, Dubuque, IA, USA) for 5 h before removing large particles with a coarse muslin cloth filter followed by fine filtration with Whatman grade 1 filter paper (Sigma-Aldrich, Merck, St. Louis, MO, USA). The supernatant was freeze-dried (Labconco™ FreeZone™ Console freeze dryer; Thermo Fisher Scientific, Kansas City, MO, USA) and kept until further use. Each sample of noni and pineapple at 10% (m/V) in water was squeezed in a perforated stainless-steel filter and consequently fine filtered through Whatman grade 1 filter paper (Sigma-Aldrich, Merck) to obtain their sap before freeze-drying.

Supercoagulant formation

Noni, pineapple and mango extracts were combined at a ratio of 1:1:1, i.e. 10 g each was homogenized and dissolved completely in 500 mL of deionized distilled water. This mixture was then freeze-dried to obtain the supercoagulant powder, which was used throughout this study. Type II rennet, with chymosin as the main constituent, sourced from Rhizomucor miehei (Sigma-Aldrich, Merck) was used as the coagulant control for comparison.

Determining the milk coagulation time

The time was recorded after confirming three parameters: the change in viscosity and colour, and the appearance of white spots in a drop of milk supplemented with coagulant, which were verified under a light microscope (Eclipse E100 fitted with a digital imager DinoEye eyepiece camera software; Nikon, New York, NY, USA) at intervals of every 5 s. The tested milk mixture included 1 mL of 10% (m/V) skimmed milk (BD Difco, Franklin Lakes, NJ, USA) with 0.5 mL of either 5% (m/V) supercoagulant or 1% (m/V) rennet and 10 mM CaCl₂ (Sigma-Aldrich, Merck) at pH=6.5, 35 °C. Experiments were performed in quadruplicate. The pH=6.5 was used as it is the natural pH of milk, while CaCl₂ functions as a cofactor for milk coagulation by promoting the aggregation of casein micelles (9). The concentration of supercoagulant was 5% (m/V) and of rennet 1% (m/V) to achieve a standard coagulation initiation time of about 30 s for both coagulants as it is ideal for laboratory conditions for the purpose of analysis. A choice of too rapid coagulation initiation time was found to complicate the analysis and comparison between the coagulants.

Determining the visible changes and measuring the calcium content of the coagulated milk

The observations were performed on milk coagulated with the supercoagulant, milk coagulated with rennet and milk alone (control). In each test, 1 mL of 10% (m/V) skimmed milk (BD Difco) was treated with 0.5 mL of either 5% (m/V) supercoagulant or 1% (m/V) rennet or milk alone under conditions of pH=6.5, 35 °C and 10 mM CaCl₂ (Sigma-Aldrich, Merck). The samples were centrifuged at 10 062×g for 60 s using a microcentrifuge (Z 216 MK; Hermle, Wehingen, Germany) to separate the curd and whey for comparison with each other. Next, in separate tests, structural changes were observed using a standard light microscope (Eclipse E100 fitted with a digital imager DinoEye Eyepiece camera software; Nikon) at 100× magnification. Finally, the structural changes were also viewed at a higher resolution using a scanning electron microscope (Fei Quanta 50; Thermo Fisher Scientific).

For determining the amount of calcium, all parameters were similar to those for the evaluation of the visible changes except without the addition of CaCl_2, as this study investigated the contribution of the in situ calcium present in milk. After being left overnight for complete coagulation to take place, the curd together with whey and the milk alone were freeze-dried before measuring the calcium content by an inductively coupled plasma-optical emission spectroscopy (ICP-OES; Optima 7300 DV; Perkin Elmer Inc., Shelton, CT, USA).

Determination of antidiabetic activity of curd fortified with the supercoagulant

The supercoagulant-fortified curd (Fig. S1a) was prepared by allowing 5% (m/V) supercoagulant to react overnight with 10% (m/V) skimmed milk (BD Difco) at pH=6.5, 35 °C and 10 mM CaCl₂. The mixture was centrifuged (Z 216 MK; Hermle) at 10 062×g for 2 min to remove the whey; only the curd was freeze-dried and used for further study. Similarly, the prepared curd formed with 1% (m/V) rennet (Fig. S1b) was used as a control.

α-Glucosidase inhibitory assay

This assay was a modification of a previous method (10). Briefly, an equal volume of various sample aqueous solutions was mixed with 1 U/mL enzyme (α-glucosidase isolated from Saccharomyces cerevisiae, Sigma-Aldrich, Merck) in potassium phosphate buffer, pH=6.9, and incubated for 30 min at 37 °C. This was followed by an additional 15 min of incubation after adding 10 mM p-nitrophenol-α-glucopyranoside (Sigma-Aldrich, Merck). The reactions were stopped by adding 100 mM Na₂CO₃ (Merck, Darmstadt, Germany) to the mixture. The tested samples included supercoagulant-fortified curd, renneted curd and acarbose (100 mg of Glucobay tablet, Bayer Corp., Whippany, NJ, USA), and a control without any sample. All of the tests were conducted in multiples of five for the calculation of standard errors. The absorbance was measured at 405 nm using microplate reader (Infinite 200 PRO equipped with Magellan software; Tecan, Männedorf, Switzerland) and the inhibitory activity (in %) was calculated with the following equation:

where A is the absorbance at the specified wavelength.

A graph of enzyme inhibitory activity (in %) versus the concentration of the sample was used in estimating the IC₅₀ value.

α-Amylase inhibitory activity assay

The assay was a modification of a previous method (11). Briefly, 250 µL samples in increasing concentrations were mixed with 50 µL of 2 U/mL enzyme (α-amylase isolated from pig, Sigma-Aldrich, Merck) in potassium phosphate buffer (Sigma-Aldrich, Merck), pH=6.9, and incubated for 30 min at 25 °C. Next, the cells were incubated for an additional 10 min once starch (1% m/V) (Sigma-Aldrich, Merck) was added as a substrate for the reaction. The reaction was terminated by adding 50 µL 3,5-dinitrosalicyclic acid (DNS, Sigma-Aldrich, Merck) at 85 °C and immediately cooling for 5 min to room temperature. The tested samples included supercoagulant-enriched curd, renneted curd and acarbose (100 mg of Glucobay tablet, Bayer Corp.), and a control without any sample. All tests were conducted in multiples of five for the calculations of standard errors. The absorbance was measured at 540 nm using microplate reader (Infinite 200 PRO equipped with Magellan software; Tecan), the inhibitory activity (in %) was calculated with Eq. 1, plotted versus the concentration of the sample and used for estimating the IC₅₀ value.

Determining the effects of the supercoagulant curd in rats induced with diabetes

Approval to conduct an in vivo study was obtained from the Animal Ethics Committee of Universiti Malaysia Pahang (Approval No. UMPIACUC/2020/02) for the use of 12 Sprague-Dawley male rats. The rats, weighing between 200 and 300 g, were allowed to acclimatize for two weeks to laboratory conditions. The experiment involved three groups of four rats in each group: normal control (NC), diabetic control (DC) and supercoagulant-enriched curd (SC). Diabetes conditions were induced by streptozotocin (Sigma-Aldrich, Merck) using a previously described method (12). Briefly, the rats in the DC and SC groups were injected IP (intraperitoneally) with 60 mg/kg streptozotocin dissolved in 50 mM sodium citrate buffer (Sigma-Aldrich, Merck) at pH=4.5. Throughout the day, the rats were given 10% (m/V) sucrose (Sigma-Aldrich, Merck) in water and standard food pellets (Gold Coin Feed Mills Sdn. Bhd., Kuala Lumpur, Malaysia) for the initiation of the hypoglycaemic effect. The next day, they were given water and food ad libitum. Their initial mass and blood glucose concentrations were measured before (day 0) and after (day 5) inducing diabetes, with the blood glucose concentration of the latter being greater than 22 mmol/L.

The experiment commenced by giving the NC and DC groups 2 mL of water alone, while SC group was dosed with 300 mg/kg supercoagulant-enriched curd daily using oral gavage for a total of 20 days. Consequently, the mass and blood glucose after fasting were measured (Accu-Check Performa Glucometer, Roche Diabetes Care, Mannheim, Germany) for each rat at intervals of every 5 days. On day 20, the rats were sacrificed humanely by overdose with a ketamine and xylazine mixture (Laboratory Animal Science Association of Malaysia (LASAM), Universiti Kebangsaan Malaysia (UKM), Malaysia). A total of 1.0 mL blood was drawn directly from the heart once the midline of the abdomen was cut open to reveal the abdomen cavity. Next, the liver and right kidney were dissected and preserved in 10% formalin (Merck). The blood was sent in vacutainers for biochemical parameter diagnostics at Gribbles Pathology Laboratory, Malaysia. The organs were treated with xylene, embedded in paraffin wax, microtome sliced into 5-micron sections, then stained with haematoxylin and eosin, and the prepared slides were carefully graded under a light microscope (Eclipse TS100; Nikon) by an expert pathologist as described previously (13).

Statistical analysis

Data were analysed using IBM Statistical Product and Service Solutions (SPSS) Statistics v. 25 tools (14). All of the samples were assayed in multiples of five for the calculation of standard errors and data were expressed as mean value±standard error. The results were considered significant at p<0.05. An independent t-test was used to compare the data within the group, while one-way ANOVA was used to compare the data between groups, followed by Tukey’s post hoc test for multiple group comparison.

Milk coagulation and fortification of the curd

The supercoagulant contains extracts from noni (Morinda citrifolia L.), pineapple (Ananas comosus L. cv. Sarawak) and mango (Mangifera indica L. cv. Apple) mixed in a ratio of 1:1:1. The ratio was selected as the protein and phytochemical contents within the fruits vary from batch to batch and therefore, an equal mixing of the three fruits is required so that they can contribute equally to the milk coagulating ability and biological activity of the supercoagulant. These fruits have the ability to coagulate milk due to the presence of milk-coagulating proteases. It was found that 5% (m/V) supercoagulant had a coagulation time of (28.3±2.9) s, while 1% (m/V) rennet had a coagulation time of (31.7±2.9) s (data not shown). Rennet (a commercial milk coagulant) was chosen to be used at a random amount five times lower for testing than supercoagulant, as the former is a purified protease, while the supercoagulant crude plant extracts are known to contain mostly non-protein constituents. Earlier studies have proven that milk-coagulating proteases are present in each of the fruits that make up the supercoagulant. Studies have shown that noni contains proteases that are able to coagulate milk, while bromelain, a protein commonly found in pineapple, has also been found to have milk-coagulating ability (15,16). Previous studies have also shown that mango has milk-coagulating capability due to the proteases found in it (17).

Fig. 1 shows the visible changes in pure milk, milk coagulated with supercoagulant and milk coagulated with rennet after centrifugation, light microscope analysis and scanning electron microscopy (SEM) analysis. Separation was not observed in pure milk (Fig. 1a), while clear separation of solid curd and liquid whey was observed in the milk supplemented with supercoagulant (Fig. 1b) and rennet (Fig. 1c) after centrifugation (18). During the microscopic analysis, the pure milk (Fig. 1a) shows a confluent structure without dark spots or aggregation of casein, while the milk samples coagulated with supercoagulant (Fig. 1b) and rennet (Fig. 1c) show obvious dark spots and colloidal structures of casein micelles. Results of SEM analysis inFig. 1a show that the pure milk has a smooth surface with observable hair-like structures, which could be casein micelles with κ-casein (19). Spaced-out structures can be seen that show no aggregation of molecules and thus no coagulation. On the other hand, milk coagulated with supercoagulant (Fig. 1b) and rennet (Fig. 1c) display a rough surface without clear see-through spaces or translucent areas between the structures because the particles aggregated together due to coagulation. The dark aggregated spots shown during light microscopy and SEM analyses represent the aggregated casein micelle that would form the curd, while the clear spaces between them represent the whey (20). It can also be seen that rennet forms a denser curd than supercoagulant, as there are fewer spaces between the structures. This is because rennet is a purified protease and therefore it cleaves κ-casein at the Phe₁₀₅–Met₁₀₆ bond in the casein micelles more effectively than the supercoagulant, forming a more complex three-dimensional network of chains and clusters (21). A study also reported that low proteolytic activity forms a denser protein network, which is why the rennet-coagulated milk structure is denser (22).

Fig. 1 Observed changes in: a) pure milk, b) milk coagulated with supercoagulant, and c) milk coagulated with rennet. From left to right: after centrifugation at 10 062×g for 60 s, under a light microscope at 100× magnification, and SEM micrograph at 500× magnification, respectively

The casein micelles are made up of casein submicelles that contain colloidal calcium phosphate clusters and a ’hairy’ layer of protruding κ-casein, which gives the micelle steric and electrostatic stability (23). The function of calcium phosphate nanoclusters in milk is to prevent precipitation and calcification of the milk and to interlock the protein strands within the casein micelle (24). During cheese-making, a specific protease is added to the milk to cleave κ-casein on the surfaces of the casein micelles, which lowers the repulsive forces between them and causes aggregation (23). Theoretically, when κ-casein is cleaved, calcium phosphate nanoclusters are also disrupted and solubilize, which would lead to an increase in the total calcium content within the curd. Calcium is an essential element in the secondary stage of coagulation, where it helps with the aggregation of casein micelles (25).Fig. 2 shows the pure milk, the milk coagulated with supercoagulant and with rennet after the determination of calcium content using ICP-OES. The mass fraction of calcium in pure milk was 1654 mg/kg, and this value is similar to a previous study, which found that commercial skimmed milk in South Korea contains calcium 1184 mg/kg (26). Accordingly, a surge in calcium release was detected, and its mass fraction in the rennet-coagulated milk was almost twice as high as the calcium mass fraction of the supercoagulant-coagulated milk. This may be because rennet is a purified form of protease; therefore, the cleavage and coagulation it carries out is much more efficient and specific than that of the supercoagulant, which is in a crude form.

Fig. 2 Determination of calcium with inductively coupled plasma-optical emission spectroscopy (ICP-OES). The experiment was performed in quadruplicate, and the values are expressed as the mean±standard error, where p<0.05

In vitro antidiabetic activities of fortified curd

The inhibition of two important polysaccharide-degrading enzymes, α-glucosidase and α-amylase, by the supercoagulant curd is shown inFig. 3. It was compared with acarbose, a common drug used to treat type 2 diabetes mellitus. The IC₅₀ values of acarbose and the supercoagulant-enriched curd for α-glucosidase were (0.05±0.02) and (4.04±0.03) mg/mL, respectively. The IC₅₀ values for α-amylase were (0.03±0.02) and (3.42±0.02) mg/mL, respectively. The supercoagulant-enriched curd was found to have significant antidiabetic properties even though its IC₅₀ value was comparably higher than that of acarbose. The supercoagulant-enriched curd had an IC₅₀=4.04 mg/mL while the rennet curd shows no inhibitory activity. This is due to the presence of phytochemicals within the plant extracts that give the supercoagulant curd its antidiabetic properties. Mango seed extract and the noni fruit extract have been reported to possess excellent antidiabetic activity based on the studies conducted in tissue culture and animal models where they were found to inhibit the α-glucosidase and α-amylase enzymes, and reduce the blood sugar level (27).

Fig. 3 The inhibition of: a) α-glucosidase, and b) α-amylase with different log concentrations of the tested samples. The experiments were performed in quadruplicate, and the values are expressed as the mean±standard error, where p<0.05

For α-glucosidase inhibitory activity, mango seed extract and noni fruit extract have been found to have IC₅₀ values of 0.34 and 0.2 mg/mL, respectively (27,28). Similarly, for α-amylase inhibitory activity, mango seed extract and noni fruit extract have been found to have IC₅₀ values of 0.71 and 2.62 mg/mL, respectively (27-29). When compared with the literature, α-glucosidase and α-amylase inhibitory activities of the supercoagulant-enriched curd were not as strong as those of its individual fruits. The possible differences between the IC₅₀ values may be due to several factors, one being the leaching out of the antidiabetic components into the discarded whey during curd production (30). Other factors include differences in ripeness, varieties of fruits, and growth conditions (31). Nevertheless, the supercoagulant-enriched curd was still able to provide significant antidiabetic activity as opposed to rennet curd, which does not have inhibitory potency.

In vivo antidiabetic activities and safety evaluations of the fortified curd

The supercoagulant-enriched curd was then subjected to in vivo testing of its antidiabetic properties in rats.Fig. 4 shows the mean body mass and glucometer measurements of the fasting blood glucose level in normal control (NC), diabetic control (DC) and supercoagulant-enriched curd (SC) rats. The parameters showed no changes on day 0 for NC or for both DC and SC groups prior to the diabetes induction of the rats (p>0.05). The mass of NC rats progressively increased, being the highest on day 20 with a mean body mass of (355±24) g. Growth can be defined as a progressive increase in body mass of an animal during a specific time period due to the accumulation of proteins and fat and bone formation in the animals, which is why there is a constant increase in body mass in the NC group (32). On day 20, the DC group of rats had a mean body mass of (149±16) g, an unfavourable reduction of 34% compared to the initial mean body mass of (227±13) g. The SC group of rats also showed a reduction of mean body mass, but only by approx. 11%. The mean body mass of diabetic rats was found to decrease over time as the pancreatic β-cells were damaged, causing lower insulin production. This prevents the breakdown of glucose in body cells; therefore, the body cannot use glucose as a source of energy but instead uses proteins and fats in the body, which leads to a loss of body mass (33). However, oral treatment of the rats with supercoagulant-enriched curd reduced the drastic mass loss observed in the untreated animals.

Fig. 4 In vivo evaluations of: a) mean body mass of the rats, and b) mean fasting blood glucose concentration during 20 days. The experiments were performed in quadruplicate, and the values are expressed as the mean±standard error, where p<0.05

The fasting blood glucose concentrations increased in DC and SC groups on day 1 when diabetes was induced in the rats. The DC blood glucose concentration remained high and somewhat flat throughout the measurements until a final measurement of (26±2) mmol/L in comparison to SC, where it was reduced to (15±1) mmol/L; however, this value was still found to be almost twice higher than the value of NC, (8±1) mmol/L, on day 20. All of the differences in the measurements of DC and SC were found to be statistically significant compared to NC (p<0.05). The administration of streptozotocin destroys pancreatic β-cells and causes less insulin to be released into the body, which leads to the accumulation of glucose and the development of constant hyperglycaemia (34). The hydrolysis of carbohydrates to glucose and other monosaccharides in the body is caused by enzymes such as α-glucosidase and α-amylase. Due to the absence or ineffectiveness of insulin, the hydrolysis of carbohydrates causes an accumulation of glucose. Antidiabetic drugs such as acarbose are used to inhibit these enzymes so that the glucose level remains low in the body (5). Supercoagulant-enriched curd was found to have a similar effect to these drugs, as it was also found to lower the blood glucose concentration in the SC group rats. Studies have shown that certain plants have the ability to inhibit the α-glucosidase and α-amylase enzymes to lower blood glucose concentration, and similarly, the supercoagulant-enriched curd was found to have this ability during in vitro antidiabetic studies (35). The supercoagulant was able to reduce the increasing fasting blood glucose concentration, as evident in the diabetic rats after day 20.

Several biochemical diagnostic parameters were evaluated in the rat blood and are shown inTable 1. The measured amounts of aspartate aminotransferase, alanine transaminase, γ-glutamyl transferase and alkaline phosphatase were significantly the highest in the DC group (p<0.05). The amounts of aspartate aminotransferase, alanine transaminase and γ-glutamyl transferase were similar to those in SC rats, while alkaline phosphatase amounts were found to be low compared to those in untreated DC rats.

When liver tissues are damaged, additional enzymes are released into the bloodstream that increase the enzyme amount in the blood (36). The enzymes in the DC group were significantly higher than those in the other groups due to liver cell injury by streptozotocin in diabetic rats, which increased the release of liver enzymes into the blood (37). On the other hand, the SC group had enzyme amounts that were significantly lower than those of the DC group (p<0.05), which shows that even though the SC group was initially diabetic, treatment with the supercoagulant-enriched curd helped lower the diagnostic enzyme levels. The treatment was effective in lowering all of the enzyme amounts of the diabetic rats to almost normal levels except for alkaline phosphatase. The alkaline phosphatase amount of the SC group did not decrease as much as that of the other enzymes, but it still showed a significant reduction compared to the DC group.

The same trend was also observed for the tested protein concentrations, whereby the albumin, globulin and total protein concentrations were similar in NC and SC, but were significantly reduced in the DC group of rats (p<0.05). A total protein test was used to determine the amount of protein in the blood and to diagnose liver and kidney functions. If the total protein concentration is low, there may be a liver or kidney problem because the protein is not digested and absorbed properly by the body (38). The serum albumin concentration in the DC group was significantly lower than that in the NC group, possibly due to increased urinary excretion or low hepatic synthesis of albumin (39). However, this was not found in the SC group, as the albumin concentration was significantly higher (p<0.05) than that in the DC group and similar to that in the NC group. The DC group also showed lower concentrations of globulin than the NC and SC groups, but the difference was not significant (p>0.05). The total protein concentration is the measure of the total amount of albumin and globulin in the body, and the total protein concentration of the DC group was significantly lower than that of the NC and SC groups (p<0.05). This is because in diabetic rats, intense changes in protein metabolism and loss of nitrogen from organs take place, which causes a negative nitrogen balance (40). This was not seen in the SC group, as the protein concentration was found to be significantly higher due to the therapeutic effects of the supercoagulant-enriched curd.

For renal function diagnostics, urea and creatine were the highest in DC rats compared to NC and SC rats. A renal function test was used to determine the function and damage that occurred in the kidney due to diabetes in the rats. Urea and creatinine are waste products in the blood that are eliminated by the kidney. A high level of these waste products in the blood indicates damage to the kidney due to diabetes (41). The DC group had a significantly higher urea concentration than the NC group (p<0.05), which shows that the urea concentration in the blood was high due to significant renal damage. The rats in the SC group showed significantly lower urea concentrations (p<0.05) than those in the DC group. The DC group also showed the highest creatinine concentration compared to the other groups due to renal damage, which caused an accumulation of creatinine in blood. These concentrations of SC were comparable to those of the NC group, which shows that the treatment was effective in improving kidney function.

The liver of all rats from the NC, DC and SC groups, as shown inFigs. 5a, 5b and 5c, respectively, had normal morphology and no signs of damage. The central vein was prominent, and the hepatic sinusoids were well arranged amidst healthy parenchyma, which consisted of hepatocytes with prominent round nuclei and abundant cytoplasm. Untreated diabetes is usually associated with damage to the liver, as it increases oxidative stress and causes an aberrant inflammatory response that activates the transcription of proapoptotic genes and damages hepatocytes in the liver (42). It was found that the DC group had no visible overall structural changes as evaluated by the pathologist. These observations are common in an acute study. The duration of the current study was only 20 days and hence generalized as an acute rather than a chronic study, which is usually 8 to 10 weeks (43,44). Even though the liver function test revealed a preliminary elevation of biochemical markers in the blood, an acute study period of 20 days is insufficient to cause observable liver damage. According to a previous study, enlargement of the sinusoids and focal microvesicular fatty degeneration with vacuolization of liver cells could be seen only in the 6th week of diabetes (45).

Fig. 5 Photomicrographs of liver cross-sections of: a) normal control, b) diabetic control (b), c) rats treated with supercoagulant curd, and kidney cross-sections of: d) normal control, e) diabetic control and f) rats treated with supercoagulant curd at 10× magnification

Diabetes causes an accumulation of glucose in the body, and over time, a high level of glucose will damage the blood vessel clusters called glomeruli in the kidney, which filters waste from the blood (46). The kidneys of the rats in NC, DC and SC groups (Figs. 5d, 5e and 5f, respectively) showed adequate glomeruli that were well spaced with normal orientation of the tubules. The interstitium had no inflammation or oedema, and the tubules were empty without casts or haemorrhage. The glucose in the blood of the DC group did not cause observable damage to the kidneys 20 days after induction of diabetes; however, the renal function test revealed a preliminary elevation of biochemical markers of the urea and serum creatinine levels in the blood. The SC group showed similar normal kidney morphology without any observable damage. Such an outcome is attributed to the ability of the used plants to maintain low blood glucose level. Generally, most medicinal plants have been indicated to be protective towards vital organs such as liver (47), however, this should be evaluated over a longer period, i.e. in a chronic toxicological study. In histopathological evaluation of liver and kidney in this study, the curd obtained with noni, pineapple and mango as coagulants had no immediate toxic effect on liver and kidneys.