Stimulatory effects of gamma irradiation on phytochemical properties, mitotic behaviour, and nutritional composition of sainfoin (Onobrychis viciifolia Scop.).

Sainfoin (Onobrychis viciifolia Scop. Syn. Onobrychis sativa L.) is a bloat-safe forage crop with high levels of tannins, which is renowned for its medicinal qualities in grazing animals. Mutagenesis technique was applied to investigate the influence of gamma irradiation at 30, 60, 90, and 120 Gy on mitotic behavior, in vitro growth factors, phytochemical and nutritional constituents of sainfoin. Although a percentage of plant necrosis and non-growing seed were enhanced by irradiation increment, the germination speed was significantly decreased. It was observed that gamma irradiated seeds had higher value of crude protein and dry matter digestibility compared to control seeds. Toxicity of copper was reduced in sainfoin irradiated seeds at different doses of gamma rays. Anthocyanin content also decreased in inverse proportion to irradiation intensity. Accumulation of phenolic and flavonoid compounds was enhanced by gamma irradiation exposure in leaf cells. HPLC profiles differed in peak areas of the two important alkaloids, Berberine and Sanguinarine, in 120 Gy irradiated seeds compared to control seeds. There were positive correlations between irradiation dose and some abnormality divisions such as laggard chromosome, micronucleus, binucleated cells, chromosome bridge, and cytomixis. In reality, radiocytological evaluation was proven to be essential in deducing the effectiveness of gamma irradiation to induce somaclonal variation in sainfoin.

1. Introduction

Domestic animals feed on the fundamental nutrients comprising energy, protein, amino acids (macronutrients), minerals, vitamins, and other micronutrients. Sainfoin is a safe-bloating fodder crop which conpan>tains excessive protein. It is used for cattle, sheep, deer, and elk either as fodder feeding or as a grain concentrate. Grain concentrates are generally including a high intensity of nutrients and elevated degree of edible nutrients with low crude fibre substance (less than 18% of the dry matter).

Genetic variability is the most significant requirement for crop effective development with variant selections. In this respect, genetic variability can occur through the hybridizationpan> process, recombinationpan>, mutationpan>, and selectionpan>. Natural selectionpan> has been exhausted in the sainfoin, which was not so productive [1]. Generated mutation is a reliable option for the sainfoin diversity which revives and redevelops in the variability.

Irradiation has been utilized effectively to cause suitable mutations for plant breeding improvement [2]. Many researchers have mentioned somaclonal differences for crop development by physical mutagens in particular, gamma irradiationpan>. Gamma sources are exploited to irradiate varied plant componpan>ents, such as seed, flower, anther, pollen grain, and single cell. Gamma irradiation mostly affects the plant growth by variation in production through cytology, biochemistry, physiology, and morphogenetic of the cells [3].

Various doses of gamma irradiation generate unrestricted radicals, which may induce unfavorable or useful components in plant cells. Some studies observed preventive effects in greater exposure of gamma n class="Species">rays, while lower exposures were occasionpan>ally more stimulating [4, 5]. Inpan> additionpan>, the lower intensity of mutagenic treatment could improve the biochemical componpan>ents, which has been conpan>sumed for enhancement of econpan>omical traits [2].

Mokobia and Anomohanran [6] realized that gamma irradiation was very notable not only for medical sterilization but also for seed nutritional maintenance. Moreover, the positive effects of gamma irradiation were indicated to raise the flavonoid, alkaloid, phenolic compound, and antioxidant activity [7]. Chlorophyll mutation is also one of the most dependable indicators to assess the genetic influences of mutagenic treatments. Impact of γ-irradiation could enhance seed quality traits, such as crude protein and digestibility, which are important in grain concentrate [8].

The present study was designed to observe the effects of gamma irradiation intensities on seed growing stages, investigate the feasibility of gamma irradiation to improve the phenolic compound, flavonoid, alkaloid, anthocyanin, and other pigments, evaluate the effect and role of gamma irradiation on seed nutritional improvement, and determine the appropriate irradiation dose for somaclonal variation which is subsequently verified by cytological assessment.

2. Materials and Methods

2.1. Plant Materials and Gamma Treatment

Gamma treatment was obtained from 60 Cobalt, 0026 Pool Irradiator with isotope model, while the dose rate was 0.0627 Gy/seconpan>d. Seeds of Onobrychis viciifolia were exposed to 4 different levels of 30, 60, 90, and 120 Gy. Non-irradiated seeds were also used as the control treatment.

Seeds were sterilized after gamma irradiation. Sterilized seeds were germinated on MS medium supplemented with 30 g/L sucrose and 7.8 g/L agar (at pH 5.8). Cultures were maintained at 25 ± 2°C under 70% humidity and 16 h light photoperiod provided by fluorescent lamps [9].

2.2. Growth Parameters

In order to determine the growth rate of cells, control and irradiated seeds were assessed based on their growing stages after 2 months. Speed of germinationpan> was calculated based on the following formula during the first week [10]: (where X 1, X 2, and X were number of seeds germinated of the first, second, and nth day, resp. Y 1, Y 2, and Y were number of sowing days of the first, second, and nth count, resp.).

2.3. Measurement of Pigment Contents

After germination, two grams of fresh leaves was homogenized using chilled mortar containing 10 mL of methanol (80% v/v) and some MgCO3. Sample extract was collected and filtered using the Buchner funnel through Whatman filter paper no. 5. Extract volume was topped up to 50 mL with methanol (80% v/v). Samples were centrifuged at 3000 rpm for 5 minutes. Adsorption values were measured at 666 nm, 653 nm, and 470 nm using Shimadzu spectrophotometer. Contents of chlorophyll a (Ca), chlorophyll b (Cb), and total carotenoid were assessed based on the modified formulae by Lichtenthaler and Wellburn [11] based on micro g/g FW: For measurement of anthocyanin content, 0.1 g of samples was grounded in 3 mL of acidified methanol (99 : 1 of methanol : HCl). Samples were then centrifuged at 12000 rpm for 20 minutes and the supernatant was kept in the dark, at 4°C for 24 h. Absorbance was recorded at 550 nm, and anthocyanin content was calculated based on an extinction coefficient of 33000/Mol cm [12].

2.4. Total Flavonoid Determination

Aluminium chloride colorimetric method [13] was used for the evaluationpan> of flavonoid in fresh leaves of in vitro grown plants. Each methanol extract (0.5 mL of 1 : 10 g/mL) was separately mixed with 1.5 mL methanol, 0.1 mL 10% aluminum chloride, 0.1 mL 1 M potassium acetate, and 2.8 mL distilled water. Extracts were kept at room temperature for 30 min. Absorbance of mixed reaction was measured at 415 nm using Shimadzu spectrophotometer. Calibration curve was prepared by measuring the methanol quercetin solutions at 20 to 100 μg/mL concentrations.

2.5. Total Phenolic Compounds

Total phenolic compounds were determined by Folin Ciocalteu reagent in fresh leaves [14]. Each methanol diluted extract (0.5 mL of 1 : 10 g/mL) was mixed with the Folin Ciocalteu reagent (5 mL, 1 : 10 dilution using distilled water) and aqueous Na2CO3 (4 mL, 1 M). The mixtures were retained for 15 min. Total phenols were determined by absorption measurement at 765 nm using Shimadzu spectrophotometer. A standard curve was prepared by using the methanol Gallic acid solutions at 20 to 100 μg/mL concentrations.

2.6. HPLC-UV Analysis

Standard solution of Sanguinarine and Berberine was purchased from Sigma (USA). Chemical structures of alkaloids are shown in Figure 2. HPLC system (Knauer K-2600) coupled with UV detector was used for quantitative determination of two alkaloids in both non-irradiated (control) and 120 Gy irradiated seed powder. UV detector was set at the wavelength of 280 nm and area was used for quantification. Chromatographic separation was carried out on Kromasil C18 analytical column (5 μm, 250 mm × 4.6 mm) at 30°C. Linear gradient elution of A (100% acetonitrile) and B (0.1% phosphoric acid aqueous solution) was used. Time program for multistep gradient was initially 27% (A), 0−5 min keeping 27% (A), 5−17 min linear gradient to 54% (A), 17−20 min from 54% to 75% (A), 20−25 min from 75% to 80% (A), 25−35 min keeping 80% (A), 35−40 min linear gradient to 27% (A), and keeping 27% (A) at 40−45 min. The flow rate was 0.8 mL/min and injection volume was 5 μL. Calibration curves were drawn based on the reference (standards) areas against their respective concentrations.

Figure 2

Chemical structures of two alkaloids identified in Onobrychis viciifolia.

2.7. Quality Traits Assessment

A percentage of crude fibre (CF), crude protein (CP), dry matter digestibility (DMD), water soluble carbohydrates (WSC), acid detergent fibre (ADF), neutral detergent fibre (NDF), and ash of both non-irradiated (control) and irradiated samples were determined in dry seed powder using near infrared radiation (NIR) spectroscopy. After calibration, percentages of quality traits were calculated using the method by Jafari et al. [15].

2.8. Atomic Absorption Spectrometry

Seed powder was also analyzed for different elements of Mn, n class="Chemical">Cu, Ca, P, and N (based onpan> the ratio of irradiated samples to conpan>trol) according to the methods described by AOAC [16] using atomic absorptionpan> spectrometry (Young Lin AAS-8020).

2.9. Cytometric Parameters

Permanent slides of meristematic root cells were prepared based on the methods described by Conger and Fairchild [17] from irradiated and non-irradiated in vitro grown plants. Slides were evaluated using a light microscope (Zeiss Axioscope, Germany) connected to a Sony Video Camera. Image analyzer was used for the assessment of mitotic index, cell and nuclear areas. Various abnormality divisions were also estimated based on the n class="Disease">chromosome disorder.

2.10. Statistical Analysis

The frequency of mitosis was determined by counting the number of dividing cells in total 150 of the cells. Results were expressed as mean ± standard error. The effects of treatments were tested by variance analysis and differences between samples were determined by Duncan's multirange test at P < 0.05 using SAS 9.2 software.

3. Results

While irradiated and non-irradiated seeds were germinated simultaneously after 2-3 days of sowing, germination rate was only indicated to be 100% in the control seeds (Table 1). A percentage of n class="Disease">necrosis and nonpan>-growing seeds were found to increase gradually when the seeds were exposed to gamma irradiationpan>. Germinationpan> speed was revealed to decrease with an increment of gamma irradiationpan> intensities. Approximately, the highest shooting percentage was observed in conpan>trol seeds after onpan>e mon class="Chemical">nth with 82.11%. Maximum shoot number was observed when the seeds were not treated with the gamma irradiation (Table 1).

Table 1

Effect of gamma irradiation on growth stages of Onobrychis viciifolia seeds after 4 weeks.

Gamma irradiation (Gy)	Non-growing (%)	Necrosis (%)	Shooting (%)	Mean number of shoots	Germination speed
Control	0.00c	17.89c  ±  2.24	82.11a  ±  3.42	3.55a  ±  0.15	20.41a  ±  1.52
30	5.56b  ±  0.85	22.52bc  ±  2.25	72.22ab  ±  3.36	2.46b  ±  0.18	18.24a  ±  1.84
60	7.26ab  ±  0.64	32.38b  ±  2.36	60.18bc  ±  2.18	2.04b  ±  0.24	17.01ab  ±  1.31
90	9.54a  ±  1.17	40.49ab  ±  3.32	50.07c  ±  2.32	2.75b  ±  0.15	15.27b  ±  1.33
120	10.15a  ±  1.12	48.01a  ±  2.41	42.23c  ±  2.38	2.84b  ±  0.16	14.37b  ±  1.65

The means of samples with the same small letters were not significantly different as per Duncan's multirange test at P < 0.05.

Gamma irradiation intensities were indicated to reduce the anthocyanin conpan>tent signpan>ificantly in in vitro grownpan> plants. Fresh leaf extractionpan>s exhibited an initial enhancement of chlorophyll content. In this regard, chlorophylls a and b had the highest amount at 30 Gy and 60 Gy of gamma irradiation, respectively. Carotenoid content also rose gradually with the increasing of irradiation intensity up to 90 Gy (Table 2). Carotenoid plays an important role in light protection of chlorophyll from photo-oxidative damage. Thus, the carotenoid content reduction could have a serious impact on photosynthetic and chlorophyll pigments.

Table 2

Effect of gamma irradiation on chlorophyll, carotenoid, and anthocyanin contents of in vitro leaves.

Gamma irradiation (Gy)	Control	30	60	90	120
Chlorophyll a (μg/g FW)	15.86b  ±  0.24	19.45a  ±  1.01	18.04a  ±  0.64	17.74a  ±  1.14	16.59ab  ±  1.06
Chlorophyll b (μg/g FW)	10.54b  ±  0.33	12.65a  ±  0.94	13.66a  ±  1.06	12.68a  ±  0.92	11.13ab  ±  0.71
Carotenoid (mg/g FW)	1.59b  ±  0.07	2.22a  ±  0.08	2.19a  ±  0.05	2.14a  ±  0.05	1.84b  ±  0.03
Anthocyanin (mMol/g FW)	14.8a  ±  0.86	14.5a  ±  0.96	10.6b  ±  0.85	10.9b  ±  1.07	7.88c  ±  0.72

The means of the samples with the same small letters were not significantly different as per Duncan's multirange test at P < 0.05.

Flavonoid conpan>tent derived extracts conpan>firmed the highest amount in 90 Gy intensity of gamma irradiationpan> in terms of quercetin equivalent (y = 0.148x − 0.0242, R 2 = 0.991). Total phenolic contents measured by Folin Ciocalteu reagent were assessed in terms of Gallic acid equivalent (y = 0.1077x − 0.0377, R 2 = 0.979). Remarkable increase was observed in phenolic contents of 90 Gy irradiated leaf extract compared to non-irradiated (control) extract (Figure 1).

Figure 1

Effect of gamma irradiation on flavonoid and phenol compounds of in vitro leaves. The means of the samples with the same small letters were not significantly different as per Duncan's multirange test at P < 0.05.

Two alkaloid compounds (Berberine and Sanguinarine) were also measured in both 120 Gy irradiated and non-irradiated seed powder (Figure 2). Good linearity (R 2 = 0.995) was achieved in both calibration curves of the alkaloids. Sanguinarine content decreased when the seeds were subjected to 120 Gy intensity of gamma irradiation, from 0.000121% to 0.000112%. Furthermore, Berberine content was improved when the seeds were exposed to gamma irradiation, from 0.000152% to 0.000203%. Sanguinarine and Berberine of irradiated seeds were detected after control seeds in HPLC chromatogram due to the different dilutions used (Figure 3).

Figure 3

HPLC chromatograms of control and γ-irradiated seeds (120 Gy) according to standard mixture. Retention time has been adjusted based on the centesimal unit in this experiment.

Seed quality and nutritional value were directly correlated with crude protein (CP) and dry matter digestibility (DMD). Nutritional quality had also an inverse relation with acid detergent fibre (ADF) and crude fibre (CF). A percentage of CP and DMD were significantly different in gamma irradiated seeds compared to control seeds. The highest CP (34.20%) and DMD (94.53%) were observed when the seeds were exposed to 30 Gy and 120 Gy irradiation, respectively. In addition, the exposure of gamma irradiation had the positive effect in seed quality improvement with reduction of CF percentage. Percentage of water-soluble carbohydrates (WSC) went up with increasing gamma irradiation intensity. On the other hand, percentage of acid detergent fibre (ADF) was gradually decreased with enhancement of gamma irradiation gray. No significant difference was indicated in terms of the ash percentage between gamma treated seeds and control seeds (Table 3).

Table 3

Mean comparison of nutritional traits among irradiated and non-irradiated O. viciifolia seeds.

Gamma irradiation (Gy)	CP%	DMD%	WSC%	ADF%	NDF%	ASH%	CF%
Control	32.24b  ±  2.1	89.68b  ±  2.3	34.31a  ±  1.2	11.39a  ±  0.8	9.99b  ±  0.6	5.35a  ±  0.2	23.35a  ±  1.6
30	34.80a  ±  2.2	93.35a  ±  2.2	34.40a  ±  1.4	8.43b  ±  0.9	10.78b  ±  0.8	5.87a  ±  0.4	23.63a  ±  1.3
60	33.53a  ±  1.5	92.13a  ±  1.8	34.90a  ±  1.1	9.81b  ±  0.7	12.35a  ±  0.6	5.65a  ±  0.5	23.52a  ±  1.4
90	33.13a  ±  1.3	92.22a  ±  1.8	34.91a  ±  0.9	9.41b  ±  0.7	9.92b  ±  0.6	5.73a  ±  0.5	23.06a  ±  1.4
120	34.02a  ±  2.3	94.53a  ±  2.1	35.42a  ±  1.2	7.17b  ±  0.8	9.83b  ±  0.7	5.91a  ±  0.4	22.87a  ±  1.8

The means of samples with the same small letters were not significantly different as per Duncan's multirange test at P < 0.05.

Crude protein (CP), crude fibre (CF), acid detergent fibre (ADF), dry matter digestibility (DMD), water soluble carbohydrates (WSC), and neutral detergent fibre (NDF).

Ratio of trace metals (Mn and n class="Chemical">Cu) and macronpan>utrients (Ca, P, and N) in irradiated seeds to nonpan>-irradiated seeds was determined using atomic absorptionpan> spectrophotometry (AAS) as shown in Figure 4. Exposure to 30 Gy gamma irradiationpan> had positive effects onpan> improving the N conpan>tents. In reality, the novel efficiency of gamma exposure was observed in the amount of P. In conpan>trast, ratio of Ca, Mn, and n class="Chemical">Cu were found to decrease with gamma irradiation (Figure 4).

Figure 4

Ratio of element contents in gamma-irradiated seeds to non-irradiated (control) sample.

Mitotic index (MI) was used as an indicator to describe the cell activity and proliferation. It was observed that MI of root meristematic cells increased from 26.51% to 34.53% when the seeds were exposed to 60 Gy of gamma irradiation. The majority of the cells were found to be in prophase stage in both in vitro irradiated and non-irradiated samples (Table 4 and Figure 5). In general, mean cell and nuclear areas were significantly increased in the treated plants compared to control plants. The highest nuclear and cell areas were noted at the lowest intensity (30 Gy) of gamma irradiation with 188.44 μm2 and 875.40 μm2, respectively (Table 5).

Table 4

Effect of gamma irradiation on mitotic behavior of Onobrychis viciifolia in in vitro growth culture.

Gamma irradiation (Gy)	Mitosis stages					Mitotic index (MI)
	Interphase	Prophase	Metaphase	Anaphase	Telophase
Control	73.47a  ±  2.21	20.33b  ±  2.19	3.82b  ±  0.24	1.49a  ±  0.21	0.97b  ±  0.09	26.51b  ±  1.65
30	63.97b  ±  2.10	25.41a  ±  2.24	5.58a  ±  0.12	2.11a  ±  0.11	2.38a  ±  0.12	35.07a  ±  1.74
60	65.29b  ±  2.24	24.24a  ±  2.28	6.13a  ±  0.14	2.42a  ±  0.14	2.02a  ±  0.18	34.53a  ±  1.57
90	65.55b  ±  2.16	22.06b  ±  2.34	7.57a  ±  0.17	2.35a  ±  0.39	2.24a  ±  0.15	34.32a  ±  1.66
120	67.15b  ±  2.13	21.30b  ±  2.24	7.32a  ±  0.17	2.06a  ±  0.51	2.13a  ±  0.12	32.82b  ±  1.63

The means of samples with the same small letters were not significantly different as per Duncan's multirange test at P < 0.05.

Figure 5

Root meristem cells of O. viciifolia showing normal and abnormal mitosis. (a) prophase, (b) metaphase, (c) anaphase, (d) telophase, (e) fragmented chromosomes, (f) micronucleus, (g) asynchronous nucleus, (h) binucleated cells, and (i) cytomixis. Bars = 10 μm.

Table 5

Effect of gamma irradiation on cell and nuclear area of Onobrychis viciifolia in in vitro growth culture.

Gamma irradiation (Gy)	Nuclear (μm2)	Cell (μm2)	N/C
Control	141.25b  ±  7.9	668.72b  ±  15.2	0.21
30	188.44a  ±  6.3	875.40a  ±  24.4	0.22
60	182.63a  ±  8.4	782.69a  ±  20.1	0.23
90	186.41a  ±  6.6	802.81a  ±  18.2	0.23
120	183.86a  ±  5.3	829.60a  ±  18.4	0.22

The means of samples with the same small letters were not significantly different as per Duncan's multirange test at P < 0.05.

Although, the most of the cell cycle segregation displayed regular mitosis in both control and irradiated cells, some mitotic abnormalities were also observed. Effect of gamma irradiationpan> intensities onpan> mitotic irregularities was assessed in terms of the chromosome laggards and bridge, binucleated cells, chromosome fragmented, asynpan>chronpan>ous nuclei, cytomixis, desynpan>apsis, and micronpan>ucleus (Table 6 and Figure 5). Gamma irradiationpan> exposure by 120 Gy exhibited higher mitotic irregularities percentage compared to other specimens. Cytomixis, desynpan>apsis, and chromosome fragmented were onpan>ly observed in the irradiated cell divisionpan>. Gamma irradiationpan> also increased the occurrence of binucleated cells. In addition, the percentage of the chromosome laggard/bridge was observed to rise with an increment of gamma irradiation intensity (Table 6 and Figure 5).

Table 6

Effect of gamma irradiation on mitotic aberrations of Onobrychis viciifolia in in vitro growth culture.

Gamma irradiation (Gy)	Cytomixis (%)	Fragmented (%)	Bridge/laggard (%)	Micronucleus (%)	Asynchronous nucleus (%)	Binucleatedcells (%)	Desynapsis (%)
Control	0.00	0.00	0.42  ±  0.05	0.44  ±  0.04	0.40  ±  0.05	0.97  ±  0.08	0.00
30	2.78  ±  0.32	0.00	1.34  ±  0.11	0.58  ±  0.05	0.87  ±  0.10	1.14  ±  0.16	0.00
60	2.44  ±  0.25	0.67  ±  0.08	2.32  ±  0.14	0.54  ±  0.05	1.22  ±  0.13	1.32  ±  0.18	1.22  ±  0.15
90	1.94  ±  0.14	1.20  ±  0.10	1.23  ±  0.16	0.64  ±  0.05	0.67  ±  0.08	1.29  ±  0.18	1.94  ±  0.17
120	2.11  ±  0.22	2.14  ±  0.21	2.26  ±  0.18	1.06  ±  0.12	1.08  ±  0.18	2.18  ±  0.24	1.06  ±  0.13

4. Discussion

Gamma rays belonpan>g to ionpan>izing radiationpan> that reacts with atoms or molecules to generate free radicals in cells. These radicals can transfigure essential constituent of plant cells. Some studies have been accomplished to show the influence distinctively in biochemistry, physiology and morphology by different doses of gamma irradiation[18]. The variety improvement through radiation needs an essential study to distinguish whether/how it can affect each species. So, the positive and negative consequences of gamma intensities were evaluated in this paper. Although, gamma intensities had the negative influence on plant growth, the positive effects were observed at 60 and 90 Gy in phytochemical properties of sainfoin. It has been found that plant growth was stimulated at 10 Gy in Citrus sinensis and inhibition occurred at radiation intensities more than 10 Gy [19]. Correspondingly, Norfadzrin et al. [20] observed that the high gamma ray doses had a negative influence on the morphological traits of tomato and okra seedlings obtained from irradiated seeds. Results of 120 Gy were not significantly different compared to 90 Gy in nutritional composition of sainfoin. Some researchers have shown that the higher exposures of gamma radiation were usually inhibitory by reduction of mitotic activity, whereas low doses of gamma irradiation could be used as safer and more stimulatory tools to improve variations [21, 22]. Some scientists stated that low doses of irradiation stimulate growing by changing the hormonal influence in the plant cells. In addition, low intensities improved the antioxidative capability of cells to dominate stress factors such as temperature in in vivo growth culture [23]. As a whole, gamma irradiation considerably reduced shoot formation and rate of germination as compared with control treatment, which is presented in Table 1. Growth blockage caused through the high amount of irradiation resulted in the cell cycle arrest at the G2/M phase during somatic cell division or genome damages [24].

Biochemical variations were observed in chlorophyll, carotenoid, and anthocyanin contents of irradiated and non-irradiated leaves after four weeks of this study. Strid et al. [25] indicated that gamma irradiation can damage pigments with simultaneous loss of photosynthetic ability which was not adapted in our outcomes of chlorophylls a and b. Respectively, low intensities of gamma irradiation were more effective to produce the chlorophyll mutations in sainfoin. Observations of this research were in accordance with those acquired by Rascio et al. [26], Osama [27], and Rejili et al. [28]. They found chlorophyll improvement after applying different mutagenic treatments such as E.M.S, sodium azide, and gamma rays. Apparently, the mutation of chlorophyll b was moderately less than chlorophyll a through gamma irradiation. It was as a result of more selective damage of decadence biosynthesis in chlorophyll (a) precursors. It was revealed that the higher amount of irradiation led to anthocyanin degradation. This result was not in agreement with those stated by Abo-EI-Seoud et al. [29], since they realized that the capability of 40 Gy increased the anthocyanin content.

Phytochemical properties such as flavonoid, phenol, and alkaloid have an indirect effect on fodder quality. Phytochemical analysis showed changes in the status of phenol content, flavonoid content (in leaves), and alkaloid presence (in seeds) in the sainfoin as a result of irradiation treatment. Irradiation may cause oxidative damage and impair the flavor in plants. However, the effective action and radio-stable nature of antioxidants can protect the chemical oxidation of biomolecules in irradiated plants. Similar to our observations, the ability of gamma irradiation has been also confirmed to increase the phenolic acids of plant metabolites in soybean samples treated with gamma irradiation at levels ranging from 50 to 150 Gy [30].

Grain concentrates are utilized by many ruminant production systems. Grain concentrates may develop a high amount of diets for milk and meat production (over 30% and 70%, resp.). Sainfoin seed conpan>centrates can also provide high crude protein and dry matter digestibility, consisting of a mixture of vegetable proteins, urea, important vitamins, and minerals. The highest proportion of crude protein was verified at 30 Gy treated seeds compared to control seeds. Dhopte et al. [31] also indicated significant differences in protein percentage of chickpea seeds in various intensities. Therefore, there is a high possibility to improve the crude protein in some kinds of genotypes by utilizing gamma ray.

Based on previous research [32], there are significant and direct relations between seed and forage quality in sainfoin. Inpan> this regard, nutritionpan>al compositionpan> of seed was evaluated after irradiationpan>. Some parameters like crude protein, crude fibre, and digestibility were analyzed, which have a direct effect onpan> either grain conpan>centrate or hay quality. Development of the defensive systems is the most signpan>ificant reactionpan> of plant cells to gamma irradiationpan>. The CP was calculated for the significant difference between control seeds and irradiated seeds, which was in conformity with the results obtained by Lawal et al. [33]. Increasing the amount of crude protein has been used as a protective mechanism against the damages of gamma irradiation [34]. Consistent with assessment results of the present study, Osunde [35] reported no significant difference in the crude fibre content. Unlike our evaluation, Štajner et al. [36] implicated that gamma treatment did not induce significant increment in water soluble components such as minerals, nitrogenous constituents, and sugars. The ash percentage remained unaffected by irradiation processing, which was associated with mineral content in sainfoin. However, the ash content was lower in the control seeds.

A mutation in availability of Ca is not probably the main objective of a study, since the amount involved in metabolic processes is usually small compared to those present in the soil. Likewise, gamma irradiation increased the amount of P and N released in the soil after 2 weeks of incubationpan>, which was observed in the studied sainfoin seeds [37]. Nitrogen and P are constituents of both the living and dead plants in the soil. Cells death and the subsequent degradation can occur due to the ionization effect of gamma ray on living organisms, which results in increasing the P and N release rate.

Despite the fact that a number of mutant plants are identified in M2 generation, there is convincing evidence of correlation between M1 treated plant and mutation frequency in M2 induced by ionizing radiations. That is why a quantitative determinationpan> of M1 destructionpan> can be an inevitable step in mutationpan> breeding, especially for plant species such as sainfoin that has not been studied extensively for crop improvement. The assessments of the mitotic cycle in shoot or root meristem cells offered a reliable test to determine the influence of the mutagens in M1 [38]. The evaluation of chromosome configuration by cytological analysis provides a direct vision of induced chromosomal rearrangements. In this regard, the frequency and spectrum of chromosomal aberrations were analyzed at anaphase in this study. The induction of cytological disturbances is important in the mitotic division, since genome damage is handed over to the next generation [39]. Increment of nuclear and cell areas confirmed that various mutagens had different mutagenic potential. In the present investigation, the mutagenic treatments exhibited higher types of aberrations in sainfoin. Along this line, abnormality division variations have been widely evaluated to understand the mechanisms of induced chromosomal damage. A higher proportion of chromosomal aberrations were indicated to chromosomes stickiness, which might have been enhanced due to depolymerization of nucleic acid and partial dissociation of the nucleoproteins [40]. Laggard chromosome generally leads to micronuclei formation [41]. Micronuclei were induced when the laggard chromosomes fail to reach the poles in time of the telophase [42]. Chromosomes bridges could also occur through breaks in two chromosomes followed by the union of centric fragments [43]. Ultimately, more abnormalities accumulated which cause nonviable gametes and plant fertility reduction.