Physicochemical Contents , Antioxidant Activities , and Acute Toxicity Assessment of Selenium-Enriched Chinese Kale ( Brassica oleracea var . alboglabra L . ) Seedlings

Creative Chemistry and Innovation Research Unit, Department of Chemistry and Center of Excellence for Innovation in Chemistry (PERCH-CIC), Faculty of Science, Mahasarakham University, Maha Sarakham 44150, )ailand Faculty of Medicine, Mahasarakham University, Maha Sarakham 44000, )ailand Animal Feed Resources and Animal Nutrition Research Unit, Division of Animal Science, Faculty of Technology, Mahasarakham University, Maha Sarakham 44150, )ailand


Introduction
Selenium (Se) is an essential trace element which accomplishes important functions for animal and human health that are relevant to several pathophysiological conditions.Its deficit can cause many disorders, but an overdose can also lead to severe consequences [1].e functions of Se in the human body are mainly associated with essential roles in the function of important antioxidant enzymes, as well as being involved in major metabolic pathway and immune function [2].Se plays a crucial role in the component of glutathione peroxidases (GSH-Px), thioredoxin reductase (TRx), iodothyronine deiodinases, selenophosphate synthetase, selenoprotein P, and other selenoproteins [1][2][3].It helps to control the intracellular redox state via the family of Sedependent GSH-Px.Benefits of the redox function of Sedependent GSH-Px mean the protection of cell membranes against oxidation by reduction of the oxidative damage to biomolecules such as lipids, lipoproteins, and DNA [3]. is damage forms the basis of a wide variety of diseases, most notably cardiovascular disease and cancer [2,3].Consequently, in recent years, Se research has attracted tremendous interest because of its important role in antioxidative processes [3].Several plants and some types of yeast can produce organo Se by converting Se to selenomethionine (Se-Met) and incorporating it into protein and enzyme in place of methionine [4].Several forms of Se species have been widely studied as a potential antioxidant and anticarcinogenic compounds, such as selenocysteine (Se-Cys), Se-Met, and methylselenocysteine (MSeCys) [5].However, a narrow concentration range between therapeutic and toxic doses of Se has been reported [4].Human nutrition societies recommended amounts in a range of 0.025-0.065mg Se per day [6].An upper limit (UL) of 0.3 mg Se per day has been suggested [7].
Chinese kale (Brassica oleracea var.alboglabra L.) is a member of the family Brassicaceae, and it represents the most popular vegetable consumed in ailand.Chinese kale can reduce the toxicity of inorganic Se because it transforms inorganic Se to several organic species of Se.In a previous study, we cultivated Se-enriched Chinese kale seedlings with Se supplied at 0, 5, 10, 15, 30, and 45 mg/L Se from sodium selenite in a hydroponic nutrient solution based on Hoagland and Arnon [17] and harvested every 5 days (5, 10, and 15 days).Results indicated that the different Se concentrations and cultivation periods affect the growth rate of Se-enriched Chinese kale seedlings.e concentration 0−30 mg/L Se in solution did not affect the growth rate, and the highest total selenium accumulation was found in 15 days in 30 mg/L [18].Moreover, Se-Met and MSeCys were the major organic forms of Se-enriched Chinese kale seedlings [18].e bioavailability of Se from Se-enriched Chinese kale seedlings (Se-KS) is similar to that of Se-enriched yeast but higher than that of Se from sodium selenite in broilers [19] and laying hens [20].Furthermore, the toxicity of Se from Se-KS was studied in laying hens, and it showed less toxicity than Se from sodium selenite at 5 and 10 mg•Se/kg.e antioxidant property of Se-KS was evaluated by the GSH-Px activity in the red blood cell of laying hens (basal diet plus 5 and 10 mg•Se/kg from Se-KS) [21].Results showed that the GSH-Px activity markedly increased when compared to the hen receiving the basal diet.
Although the previous studies had reported antioxidant activity and toxicity of Se-KS in poultry, its toxicity has never been studied in mammal models.us, in the present study, the physicochemical contents of Se-KS, the Se bioaccesibility after in vitro-simulated gastrointestinal digestion, the antioxidant activity, and also the toxicity in a mammal model were evaluated.Data obtained from this study suggested that Se-KS could be beneficially established as a functional food.

Cultivation of Chinese Kale
Seedlings.Seeds of Chinese kale (Brassica oleracea var.alboglabra L.) were obtained from Chia Tai Company Limited ( ailand).e Chinese kale seedlings were cultivated according to the growth conditions described by Maneetong et al. [18].Briefly, the Chinese kale seeds were soaked in tap water for 15 h before planting.After that, the seeds were cultivated on a wet sponge (35 × 40 × 30 cm) at room temperature in the dark for 3 days until the seeds began to germinate.e covers of the plastic pots were released, and the germinated Chinese kale was subjected to light from a fluorescent lamp (36 W) with a12 h dark/light cycle and watered with tap water daily for 4 days.Afterwards, the germinated seedlings were cultivated in the adapted modified Hoagland's solution containing 0, 5, 10, 15, and 30 mg•Se/L in the form of sodium selenite.After 5, 10, and 15 days of cultivation, the Chinese kale seedlings were harvested, washed thoroughly with deionized water, dehydrated in a hot oven at 60 °C, gently ground, and stored in a freezer at −20 °C until analysis.

Antioxidant Activities of Chinese Kale Seedlings.
e extraction procedure was adapted from Xu and Hu [12].An accurate weight of one gram of the dried sample was extracted with 30 mL of 75% ethanol (ethanolic extract) or distilled water (aqueous extract).
e extractions were conducted in a water bath at 60 °C and shaker 200 rpm for 3 h.Each sample was extracted three times with the same volume of solvents.
e extracts were filtered and combined, and the combined filtrate evaporated to dryness in a vacuum and kept frozen at −20 °C until analysis of antioxidant activity (DPPH and ferric thiocyanate (FTC) methods).
e DPPH radical scavenging capacities of Se-KS extracts and the reference substance trolox and butylated hydroxyanisol (BHA) were evaluated with a method adapted from Xu et al. [22].
e radical scavenging capacities of samples and reference substances against the DPPH radical were evaluated.Briefly, 100 μL of the standard was extracted and mixed with 1000 μL of 0.1 mM ethanolic solution of DPPH radical, and absorbance was measured at 515 nm after 30 min of reaction in the dark.e percentage inhibition was calculated by the following equation: %inhibition � absorbance of blank − absorbance of sample absorbance of blank × 100. (1) e FTC method followed Xu and Hu [12]. 2 mL of 1000 µg/mL sample extracts or 2 mL of 200 µg/mL trolox and BHT served as standard solutions.2 mL of 2.51% w/v linoleic acid in ethanol, 4 mL of 0.05 M phosphate buffer (pH 7.0), and 2 mL of distilled water were mixed in a vial of 10 mL with a screw cap and then kept in a 40 °C water bath in the dark.A 100 µL amount of the above mixture was added to 9.7 mL of 75% v/v ethanol and 100 µL of 30% w/v ammonium thiocyanate.After 5 min, 100 µL of 0.02 M ferrous chloride in 3.5% v/v hydrochloric acid was added and then maintained at 40 °C in a water bath in the dark.e absorbance of the mixture was measured every 24 h at 500 nm until a steady absorbance value was achieved.All of the tests were performed in triplicate, and the results were averaged.
e DPPH and FTC methods were chosen to find out and confirm suitable germination time periods because they are simple, have low cost, and used stable free radicals.e percentage inhibition was calculated by the following equation: %inhibition � absorbance of blank − absorbance of sample absorbance of blank × 100. (2)

Physicochemical Contents.
e following physicochemical contents of the sample were determined: moisture, crude fat, crude fibre, ash, crude protein, and carbohydrate content using the standard Association of Official Analytical Chemists procedures [23].

Total Se Contents.
e dried samples were analyzed by using a hydride generation atomic absorption spectrophotometer (wavelength 196.0 nm, quartz cell temperature 890 °C, HG-AAS model VGA-77, Agilent Technologies, Inc., USA). e samples were digested with 1.5 mL of 65% nitric acid, and 1.5 mL deionized water was added and mixed in a glass vessel and then heated at 100 °C in a metal bath for 45 min.After cooling, 5 mL of concentrated HCl was added to reduce Se (VI) to Se (IV) for 30 min.e digested solution was transferred and stored in a freezer at 4 °C until analysis.
e digestion process was accurately validated with the percentage recovery test by spiking 20 µL (20 µg•Se/L) of Se standard solution into the sample.
e obtained recovery values were in the range of 90.65-102.49.

Se Bioaccessibility.
Gastrointestinal digestion was simulated using the method described previously [24].Briefly, accurate weight of one gram of the plant samples was mixed with 7.5 mL of gastric juice (6% w/v pepsin, 0.9% w/v sodium chloride at pH 1.8 (HCl)) and stored in a 37 °C incubator for 4 h in the dark.After that, gastric juice was adjusted to pH 6.8 with saturated sodium carbonate solution and then incubated with 5 mL of intestinal juice (1.5% w/v pancreatin, 0.5% w/v α-amylase in 0.9% w/v sodium chloride) at 37 °C approximately 4 h in the dark with gentle and continuous shaking.After centrifugation at 5000 g for 30 min, the supernatant was brought up to 100 mL with 0.9% w/v NaCl in a volumetric flask, filtered through filter paper, and used for antioxidant activity tests.As the blank of gastrointestinal digestion, 2.5 mL of deionized water was investigated in a gastrointestinal (GI) simulation test.Total Se of the samples after GI digestion was determined using previously described conditions.Total Se GI digestion and blank (without sample) were measured after the GI process.e percentage of the bioaccessibility was calculated by the following equation: %bioaccessibility � total Se GI digestion − total Se in blank total Se in sample × 100. (3)

Total Phenolic Compounds, Flavonoid Contents, and Antioxidant Activity after In Vitro Gastrointestinal Digestion.
Total phenolic contents were determined according to a modified procedure [25].Briefly, 100 µL of the digested samples was oxidized with 500 µL of 0.2 N Folin-Ciocalteu's reagent and added to 400 µL of 7.5% w/v sodium carbonate.e absorbance was measured at 765 nm after being mixed and incubated in room temperature for 60 min.e results were calculated as milligram per gram gallic equivalent (mg GE/gDW).
Total flavonoid contents were estimated using the aluminum chloride colorimetric method [26].Briefly, 100 µL of the digestion samples was mixed with 500 μL of 2.5% w/v sodium nitrite and 400 μL of 5% w/v aluminum chloride.e mixture was allowed to stand at room temperature for 30 min, and the absorbance was read at 415 nm. e results were expressed as milligram per gram quercetin equivalent (mg QE/gDW).
Antioxidant activities methods used DPPH, ABTS +• , and the ferric reducing antioxidant power (FRAP).e DPPH method was described in the previous section.For the ABTS +• assay [27], the ABTS +• solution was generated by mixing the two stock solutions of 7 mM ABTS and 2.45 mM potassium persulphate (1 : 1, v/v).e mixture was stored in dark at room temperature for 12 h before use.e ABTS +• solution was diluted to 0.7-0.8absorbance at 734 nm in deionized water.e 100 µL of different concentrations of the supernatant (0.1-1.0 mg/mL) was continually mixed with 900 μL of ABTS +• solution.e mixed solution was stored at room temperature for 15 min and followed by measuring the absorbance at 734 nm using deionized water as blank.Trolox and ascorbic acid were used as standard solutions.e percentage inhibition was calculated using the following equation: e FRAP method [28] of the extract was measured at low pH.Briefly, 100 µL of Se-KS extracts was mixed with 900 µL of FRAP reagent and incubated in a water bath at 37 °C for 15 min.e absorbance at 595 nm was measured.e results were calculated as milligram per gram trolox equivalent antioxidant capacity (mg TEAC/gDW).

Protocol of Acute Oral Toxicity and Determination of Body
Weight, Blood Analysis, and Histopathological Investigation of the Liver and Kidney in Experiment on Rat.
is experiment was performed to investigate the acute toxicity of R-KS and Se-KS in vivo and to confirm a toxicity for a new dietary supplement.e OECD guideline 423 was used to monitor the effect of oral toxicity test [29].
Healthy female Wistar albino rats, 8-12 weeks old, 180-220 g b.w. were purchased from the National Laboratory Animal Center, Mahidol.Two rats were housed in a stainless-steel cage in a room maintained under environmentally controlled conditions of 22 ± 3 °C and 50-60% relative humidity, with 12/12 light/dark cycle.Animals were fed conventional laboratory diets with an unlimited supply of drinking water.
e animals were acclimated to the laboratory conditions for 5 days prior to the start of the experiments.All animal procedures conformed to the Animals for Scientific Purpose Act, B.E.2558 (A.D. 2015), ailand, and approved by the Animal Ethics Committee of Mahasarakham University (Approval No. 005/2558).Animals were randomly divided into seven groups of 4 rats each.All animals were fasted overnight and the R-KS or Se-KS at different amounts was administered orally as a single dose.
e first group received corn oil (vehicle control).e 2 nd , 3 rd , and 4 th groups were treated with regular kale seedling (R-KS) in corn oil at doses of 1250, 2500, and 5000 mg/ kg•b.w. which consisted of 0.02, 0.04, and 0.08 mg Se/kg•b.w., respectively.Additionally, the 5 th , 6 th , and 7 th groups were treated with Se-enriched kale seedling (Se-KS) in corn oil at the same doses as R-KS and also consisted of 0.54, 1.08, and 2.16 mg Se/kg•b.w., respectively.
Animal behaviors were monitored at 0, 0.5, 1, 3, 6, 12, and 24 h during the first day and daily until 14 days after dosing.
e following signs of stress or distress such as labored breathing, discharge from nose or mouth, ruffled fur, hunched posture, minimal responsiveness, diarrhea, immobility, lethargy, labored breathing, minimal responsiveness, and uncontrolled bleeding or discharges were criteria prompting immediate euthanasia.e body weight of all rats was measured daily.e lethal dose of 50% (LD 50 ) was evaluated according to the method described by OECD guidelines 423.After 14 days, all animals were anesthetized with Nembutal 45 mg/kg•b.w.(i.p.), and blood samples were collected by cardiac puncture for hematological analysis into tubes with and without EDTA, respectively.All parameters of blood were analyzed by the Animal Hospital Faculty of Veterinary Medicine, Khon Kaen University, Khon Kaen, ailand.e organs including liver, kidney, heart, spleen, and lung were collected and weighed, and the relative organ weight was determined (based on terminal body weight).
Additionally, the heart, liver, and kidney were collected for histopathological examinations; tissues were processed into paraffin blocks, sectioned at a thickness of 5 μm, mounted on glass microscope slides, and stained with hematoxylin and eosin.
e histological assessments of the slides were examined with a light microscope.

Statistical Analysis.
e results were performed in triplicate and expressed as mean ± SD. e significance of difference was analyzed using one-way ANOVA.Independent t-tests were used to compare test results at p < 0.01 and 0.05 between R-KS and Se-KS.Correlations among variables were analyzed with Pearson's correlation test.

Antioxidant Activities of Se-KS (0-30 mg•Se/L Hydroponic Solution).
e H donation by the kale extracts and by trolox and BHA realizes a transfer of the DPP radical to DPPH with a decolourisation or absorbance decrease.In contrast, the FTC assay leads to an absorbance increase.It is a spectrophotometric method determining electron transfer by measuring the capacity of an antioxidant in its reduction with colour change.e corresponding increase or decrease of the absorbance at given wavelength is related to the concentration of antioxidant in the sample [30].e results showed that during the first 10 min, the reactions of DPPH radical with ethanolic extracts of the tested antioxidants Se-KS vs. R-KS vs. reference antioxidants (Figures 1(a)-1(c)) was more rapid than those with aqueous extracts (Figures 1(d)-1(f )) and reached a steady state within 15 min.e inhibition percentages of antioxidant activity on DPPH at 30 min were calculated.Se-KS at 30 mg Se/L for 15 days provided the highest inhibition percentage of 77% at 30 min when compared with other Se concentrations, but lower than trolox and BHA.
e antioxidant activity of Se-KS increased with increase of Se content, suggesting Se played a positive role in enhancing the antioxidant activity of Se-KS.Moreover, organic Se was more effective than inorganic Se on enhancing the hydroxyl radical scavenging ability [31].
In the FTC method, all the Se-KS extracts inhibited linoleic acid oxidation.High inhibition value exhibited higher activity than control (Figure 2).Also, lipid inhibitory activities of Se-KS ethanolic extracts (Figures 2(a)-2(c)) showed higher antioxidant activity than those of aqueous extracts (Figures 2(d)-2(f )).Se-KS extracts from 30 mg Se/L for 15 days of cultivation displayed significantly higher activity than the control and other Se-supplemented concentrations, but lower than those of trolox and BHA. e antioxidant activities from the FTC method showed almost the same patterns of activities as the DPPH method.From the antioxidant activity results, Se-KS at 30 mg•Se/L and 15 days after cultivation was selected for determination of   Journal of Chemistry physicochemical contents, Se bioaccessibility, and antioxidant activities (after passing through the in vitro gastrointestinal simulation).Also, in the acute toxicity assessment on rats, the variant R-KS at 0 mg Se/L and 15 days after cultivation as the control was tested in comparison with Se-KS at 30 mg•Se/L, 15 days after cultivation.

Physicochemical Contents, Total Se Contents, and Se Bioaccessibility and Antioxidant Activities of Se-KS and R-KS.
Table 1 shows the physicochemical contents and the total Se content of R-KS (untreated) and Se-KS (30 mg Se/L) each for 15 days after cultivation.In addition, the Se bioaccessibility in the in vitro simultaneous gastrointestinal simulation model is presented.e moisture and crude fat content of all Chinese kale seedlings was not significantly different (p < 0.05).e results indicated higher (p < 0.05) crude protein, total Se, and Se-bioaccessibility contents of the Se-KS when compared to the R-KS.
e content of crude protein increased in association with accumulation of Se in plants in line with an increase reported in [32].Various data revealed that the protein content of Se-enriched plants is higher than that of regular plants [33].e supplementation of Se increases the synthesis of selenoamino acid and protein content [32].Regarding the increase of crude fibre contents, a further report suggested that Se accumulation resulted in higher starch concentrations in upper leaves [34].e mechanism is maybe correlated to change in starch/glucose contents which are important substratess in cellulose synthesis.In this study, Se-KS exhibited 26-fold higher Se accumulations than did R-KS.
is finding is in good agreement with Chen et al. [35] who reported an accumulation of Se in rice after Se biofortification with selenate and selenite.Also, Xu et al. [22] reported that the Se accumulation in tea leaves increased by Se fertilization compared with plants not treated with Se.
Se bioaccessibility increased, following in vitro simulated gastrointestinal digestion.Fifty percentage of bioavailable capacity in Se-KS showed high absorbtion of Se contents in the gastrointestinal system simulation.ese results are in accordance with a previous investigation that reported higher Se bioavailability (64.5%) in Se-KS compared with sodium selenite (54.5%) in laying hens [21].Conversely, ash mainly consists of the oxide of calcium, zinc, magnesium, and potassium.e R-KS showed a significantly higher (p < 0.05) ash content than the Se-KS.Ash mainly consists of the oxide of calcium, magnesium, and potassium.Se biofortification in radish and maize plants can inhibit the absorption of calcium and potassium, copper, and zinc [36].However, ash contents are unknown in the cited studies, to explain satisfactorily the difference in the mineral content of R-KS and Se-KS.
Antioxidant activities (DPPH, ABTS, and FRAP) of R-KS and Se-KS supernatants after in vitro simulated GI digestion are presented in Table 2. e total phenolic content in Se-KS was significantly higher than that in R-KS (30.1 ± 0.1 mg GE/gDW vs. 18.5 ± 0.7 mg GE/gDW).However, there was no significant difference of total flavonoid content between R-KS and Se-KS.Antioxidant activities were determined by DPPH, ABTS, and FRAP assay.Se-KS showed the greatest potential for antioxidant activities on free-radical scavenging in different concentrations of DPPH (0.025-10.00 mg/mL) and ABTS (0.1-1.0 mg/mL) which were expressed as IC 50 values (the inhibitory concentration of a substance where the scavenging is reduced by half).In addition, free-radical scavenging of the R-KS was significantly less than that of Se-KS (p < 0.05).A high potential antioxidant effect of Se-KS was found in both DPPH (80.72%) and ABTS (75.52%) assays.Se-KS had higher total phenolic compound contents and also higher antioxidant activity than R-KS.
is underlines that the phenolic compounds are the main source of natural antioxidant in Brassica plants.Bachiega et al. [37] confirmed the broccoli biofortification with selenium showed significantly higher total phenolic contents and antioxidant capacity in different maturity stages (sprout and seedling).Se treatment increases phenolic compounds and antioxidant activity, but the mechanism is still not fully understood.It is hypothesized that the Se enhances accumulation of glucose which is an important substrate in many metabolic pathways [34,38].
e correlation coefficient between protein content, total Se content, Se bioaccessibility, and antioxidant activity has been reported.e relationship between total Se content (TSeC), protein content (PC), and Se bioaccessibility with antioxidant activity measured by DPPH, ABTS, and FRAP assays is shown in Table 3. e results demonstrated that Se Se bioaccessibility (%) ± 6 a 50 ± 0 b e data are expressed as mean ± SD (n � 3); identical superscripts in row denote no significant (p < 0.05) difference between mean values according to the independent t-test (SPSS 16.0).e data are expressed as mean ± SD (n � 3).e different lowercase letters indicate significant difference between rows at p < 0.05.DPPH � 2,2diphenyl-1-picrylhydrazyl; ABTS � 2,2-azino-bis (3-ethylbenzothiazoline-6-sulphonic acid), and FRAP � Ferric reducing antioxidant power.bioaccessibility and antioxidant activity were strongly correlated: DPPH, r � 0.96; ABTS, r � 0.92; and FRAP assay, r � 0.95.e PC of all Chinese kale seedlings showed a high correlation coefficient with antioxidant capacities of DPPH and ABTS of 0.91 and 0.94, respectively.Moreover, a positive correlation was found for TSeC/TPC (r � 0.99).ere were strong internal correlations between the results of the different antioxidant assay methods.Additionally, there was a significant positive correlation coefficient between TSeC, Se bioaccessibility, TPC, and antioxidant activity.In concordance with previous studies, our studies found that there is a positive correlation between TSeC and antioxidant activity in several Se-enriched plants such as brown rice [9], green tea [10], and Spirulina platenis T. [13].In conclusion, the accumulation and transformation of an inorganic Se form to a bioactive organic compound in Se-KS is responsible for higher Se bioaccessibility, total phenolic compounds, and antioxidant activities.

Acute Toxicity Study in Rats.
In the acute toxicity study, oral administration of varying doses of R-KS and Se-KS to rats exhibited no evidence of toxicity over a period of 14 days.No changes in rat behaviour were observed.No mortality or any morbidity was verified in all groups after administration.
ese results revealed that the LD 50 of Chinese kale seedlings in rats would be more than 5000 mg/ kg b.w.
Daily food and water consumption was found to be normal in both control and treatment groups.No significant changes in body weight of the rats which were given the Se-KS were observed when compared with the control group (data were not shown).Changing body weight is one of the indicators of toxicity effects of chemicals [39].erefore, it can be assumed that the ingestion and digestion of kale seedling (R-KS and Se-KS) did not affect the normal growth of rats.
e hematological analyses of blood parameters including hemoglobin content, packed cell volume (hematocrit), red blood cell count, total white blood cell count with neutrophils, and lymphocytes percentages and the derived red blood cell criteria MCV, MCH, and MCHC (for abbreviations, see footnote in Table 4) were exhibited within normal limits compared to the control group, as shown in Table 4. e hematological system is one of the most sensitive targets to toxic compounds [40].Consequently, the   results indicate that neither R-KS and Se-KS were toxic to blood cells nor interfered with blood cell production.Biochemical markers were also evaluated in the blood serum samples, and results are summarized in Table 4. e single oral administration of R-KS and Se-KS at doses of 1250, 2500, and 5000 mg/kg•b.w.did not have any significant adverse effects on liver enzyme activities of serum and further biochemical markers when compared with the control group.High serum activities of aspartate transaminase (AST) and alanine transaminase (ALT) are indicators of a predamaged or damaged liver function and biomarkers.In addition, alkaline phosphatase (ALP) is an enzyme that plays a major function in cell membrane transport in many tissues, including bone, intestine, kidney, liver, placenta, and white blood cells.Damage to these tissues causes the release of ALP into the bloodstream [41,42].Elevated ALP in plasma has been found in large bile duct obstruction, intrahepatic cholestasis, or infiltrative diseases of the liver [43].High TP levels indicate dehydration, inflammation, infections, and bone marrow disorders.A low TP level can suggest a liver disorder, a kidney disorder, or a disorder in which protein is not digested or absorbed properly.Low levels may be seen in severe malnutrition and with conditions that cause malabsorption [43].Uric acid (UA) is a product of the metabolic breakdown of purine nucleotides [44].
e presence of hyperuricemia should initiate an evaluation in conditions associated with increased purine metabolism or altered renal clearance of uric acid.
ese conditions have been linked to many disease states such as articular degenerative disorders, vascular inflammation, atherosclerosis, and cardiovascular as well as renal disease [45].High levels of BUN and creatinine indicate kidney failure or disease, dehydration, shock, high protein diet, certain toxin ingestions, poor circulation to the kidneys, and urinary obstruction [46].e administrations of all dosages of R-KS and Se-KS did not cause any organ atrophy, hypertrophy, or degenerative effect.e tissues did not show any changes in colour, volume, and texture when compared with the control group (data not shown).No significant difference was noticed in relative weight of primary body organs.Toxic substances induce abnormal metabolic reactions that may affect primary organs such as heart, liver, and kidney [41,47,48].
e histopathological examination of several tissues of heart muscle, liver, and kidney is shown in Figure 3; no changes were observed.erefore, our findings suggest that, in the Chinese kale seedlings, both R-KS and Se-KS at 1250, 2500, and 5000 mg/kg•b.w.did not affect the morphology of the organs.In former investigations, it has been reported that Se compounds such as selenite and MSeCys provided signs of toxicity at 3−5 mg•Se/kg•b.w. with almost no survival at 16 mg•Se/kg b.w.[49].Moreover, the LD 50 of Se-Met in rats which were given an intraperitoneal injection was evaluated as 4.25 mg•Se/kg b.w.[50].In our study, R-KS at doses of 1250, 2500, and 5000 mg/kg•b.w.consisted of 0.02, 0.04, and 0.08 mg•Se/kg•b.w., whereas Se-KS at doses of 1250, 2500, and 5000 mg/kg•b.w.consisted of 0.54, 1.08, and 2.16 mg•Se/kg•b.w., respectively.Moreover, our previous study found that the major organic forms of Se-KS were Se-Met and MSeCys [18].erefore, the amount of Se in Se-KS did not exceed the toxicity doses reported; for this reason, no signs of toxicity in animals were seen in the present experiment.Indeed, together with our previous research [18][19][20], good biological activity was proven for the Se-KS with low acute toxicity when compared with selenite.We suggest 0.05-0.15g of the air-dried Se-KS corresponded with 0.025-0.065mg Se per day [6] or a maximum dose of <0.7 g of the air-dried Se-KS corresponded with a tolerable dose 0.3 mg Se per adult and day [7].However, this hypothetical recommendation does not consider the Se ingestion via plant and animal source in food consumption.

Conclusions
Se-KS had a high Se concentration, a higher crude protein content, and a stronger antioxidant activity.In rat experimental, nontoxicity was shown.erefore, Se-KS has been proved to be a potential source of organic Se for use as a food supplement.

Figure 1 :
Figure 1: Kinetic behaviors of radical antioxidant activity of Se-enriched kale seedlings.e Se-enriched kale seedling ethanolic extracts (a-c) and aqueous extracts (d-f ) with 5 tested Se concentrations and the two reference antioxidants trolox and butylated hydroxyanisol (BHA) in 3 cultivation periods of 5 days (a, d), 10 days (b, e), and 15 days (c, f ).e standard represents the blank, the pure ethanol solution and the distilled water.

Figure 2 :
Figure 2: Kinetic behaviors of the ferric thiocyanate method of Se-enriched kale seedlings.e Se-enriched kale seedlings ethanolic extracts (a-c) and aqueous extracts (d-f ) with 5 tested Se concentrations and the two reference antioxidants trolox and butylated hydroxyanisol (BHA) in 3 cultivation periods of 5 days (a, d), 10 days (b, e) and 15 days (c, f ).e standard represents the blank, the pure ethanol solution and the distilled water.

Table 1 :
Physicochemical contents, total selenium, and Se bioaccessibility of air-dried substance of regular Chinese kale seedlings (R-KS) and Se-enriched Chinese kale seedlings (Se-KS).

Table 2 :
Antioxidant capacities after passing gastrointestinal system simulation of regular Chinese kale seedling (R-KS) and Seenriched Chinese kale seedling (Se-KS).

Table 4 :
Hematological and biochemical values of rats treated with Chinese kale seedlings for acute toxicity administration.