Protein, dietary fiber, minerals, antioxidant pigments and phytochemicals, and antioxidant activity in selected red morph Amaranthus leafy vegetable

Authors: Umakanta Sarker ^aff001; Shinya Oba ^aff002
Authors place of work: Department of Genetics and Plant Breeding, Faculty of Agriculture, Bangabandhu Sheikh Mujibur Rahman Agricultural University, Gazipur, Bangladesh ^aff001; Laboratory of Field Science, Faculty of Applied Biological Sciences, Gifu University, Yanagido, Gifu, Japan ^aff002
Published in the journal: PLoS ONE 14(12)
Category: Research Article
doi: https://doi.org/10.1371/journal.pone.0222517

Summary

Amaranth has two morphological types (morphs), one is red and another is green morph. Red morph amaranth is a marvelous source of nutrients, antioxidant pigments, minerals, and phytochemicals compared to green morph amaranth. For this purpose, we selected 25 red morph genotypes to evaluate in terms of proximate, minerals, antioxidant pigments and phytochemicals and antioxidant activity in RCBD design in three replicates. The leaves of red morph amaranth are an excellent source of dietary fiber, carbohydrates, moisture, and protein. We found remarkable potassium, calcium, magnesium (24.96, 10.13, 30.01 mg g^-1), iron, manganese, copper, zinc (1089.19, 243.59, 25.77, 986.61 μg g^-1), chlorophyll a, chlorophyll b (31.79, 16.05 mg 100 g^-1), β-cyanins, total flavonoids (102.10 RE μg g^-1 DW), β-xanthins, betalains (33.30, 33.09, 66.40 μg 100 g^-1), carotenoids, total phenolics (172.23 GAE μg g^-1 DW), β-carotene (1225.94, 1043.18 μg g^-1), vitamin C (955.19 μg g^-1), and antioxidant activity (DPPH and ABTS⁺) (19.97 and 39.09 TEAC μg g^-1 DW) in the red morph amaranth leaves. We can select the genotype RA5, RA8, RA18, RA22, and RA25 as antioxidant-enriched red morph amaranth. It revealed that amaranth β-cyanins, phenolics, betalains, flavonoids, β-xanthins, carotenoids, vitamin C, and β-carotene had strong antioxidant activity. These phytochemicals contributed significantly in the antioxidant potentials of red morphs amaranth. Red morph amaranth could be a potential source of nutrients, antioxidant pigments, minerals, and phytochemicals as these compounds scavenged ROS and served as potential antioxidants in our daily diet to attaining nutritional and antioxidant sufficiency.

Keywords:

Vitamin C – Leaves – Antioxidants – Pigments – Chlorophyll – Phenols – Carotenoids – Phytochemicals

Introduction

The acceptability of foods largely depends on the color of the food products. Recently, the demand for natural pigments such as carotenoids, β-xanthins, β-cyanins, anthocyanin, betalains, and chlorophylls have increased the interest in consumers in the safety, nutritional, and aesthetic aspects of food. A few families in the order Caryophyllales have water-soluble natural pigments like β-cyanins, β-xanthins, and betalains. Amaranthus (red amaranth) is a unique source of betalains, β-xanthins, β-cyanins that have potential free radical detoxifying ability [1]. Red to purple colored betalains are β-cyanins and yellow colored betalains are β-xanthins [2]. Similarly, α-carotene, xanthophyll, and beta-carotene are different carotenoids pigments. Among edible vegetables, red beet and amaranth have natural pigments, like betalains, β-cyanins, β-xanthins. Red morph Amaranthus is a marvelous source of color pigments like β-cyanins, β-xanthins, betalains, anthocyanin, amaranthine, carotenoids, and chlorophylls. These pigments detoxify free radicals in the human body and act as potent antioxidants [3] and have a significant contribution to human health. The anti-inflammatory property of the active ingredients of carotenoids, betalains, β-cyanins, and β-xanthins protect against lung and skin cancers and cardiovascular disease. For this reason, these natural pigments are widely used as an additive for cosmetic products, drugs, and food [4].

Vegetable amaranth is a C₄ leafy vegetable. It is a marvelous source of proximate, minerals, phytopigments, bioactive compounds that had pronounced significance as a food natural antioxidants and ROS scavenger [5–10]. It is inexpensive and abundant sources of protein, dietary fiber, pigments, minerals and antioxidant phytochemicals like flavonoids, β-carotene, phenolics, and vitamin C. Amaranth protein are enriched with nutritionally important amino acids such as lysine and methionine [11–14]. It is also tolerant to abiotic stresses like drought and salinity [15–20]. Amaranth has two morphological types (morph), one is red and another is green morph [21]. Red morph amaranth is an abundant source of pigments as well as minerals, proximate, bioactive phytochemicals, and antioxidants. There are a lot of red morph amaranth germplasms available in Bangladesh, Asia, Africa and South America with great variability and phenotypic plasticity [22] that have multipurpose uses. In Bangladesh including south-east Asia, Africa, and South America, red morph amaranth leaves are very popular as a vegetable. Its nutritional value, taste, and attractive leaf color make it popular in the rest of the continent and elsewhere. In Bangladesh, red morph amaranth is grown year-round and it can be grown in the hot summer, a gap period of foliage vegetables [11–12].

Recently, researchers and consumers have shown interest in natural antioxidants in red morph vegetables. Red morph amaranth has abundant flavonoids, pigments, β-carotene, phenolics, and vitamin C [13, 23]. These natural antioxidants protect cancer, emphysema, cardiovascular diseases, atherosclerosis, diabetes, retinopathy, osteoporesis, neurodegenerative diseases, arthritis, cataracts, inflammation, and prevent aging [23–25].

Although red morph amaranth is a cheap and abundant source of minerals, pigments, dietary fiber, phytochemicals, protein, and antioxidant activity. There is a scarce of information in red morph Amaranthus leafy vegetable. To our knowledge, there is a lack of information on proximate and mineral compositions, pigments, phytochemicals, and antioxidant activity in a huge number of diversified red morph amaranth germplasms available in Bangladesh and elsewhere. Therefore, to fill these gaps, the present investigation was undertaken to evaluate proximate and mineral compositions, antioxidant pigments, phytochemicals, and antioxidant activity and their variability in 25 red morph amaranth genotypes.

Materials and methods

Experiment materials, design, layout, and cultural practices

Twenty-five selected genotypes of red amaranth from our earlier collected 120 germplasm were grown in open field of Bangabandhu Sheikh Mujibur Rahman Agricultural University in a randomized complete block design (RCBD) with three replications. The unit plot size of each genotype was 1 square meter. The spacing of each red amaranth genotype was 20 cm distance from row to row and 5 cm distance from the plant to plant. Recommended fertilizer, compost doses, and appropriate cultural practices were maintained. Thinning was done to maintain appropriate spacing between plants of a row. As a necessity, weeding and hoeing were done to remove the weeds. To maintain the normal growth of the crop proper irrigations were provided. At 30 days after sowing of seed, leaf samples were collected.

Chemicals

Solvent: acetone and methanol. Reagents: H₂SO₄, HNO₃, HClO_3, NaOH, dithiothreitol (DTT), caesium chloride, ascorbic acid, standard compounds of pure Trolox (6-hydroxy-2, 5, 7, 8-tetramethyl-chroman-2-carboxylic acid), gallic acid, rutin, folin-ciocalteu reagent, DPPH (2, 2-diphenyl1-picrylhydrazyl), ABTS⁺, aluminium chloride hexahydrate, sodium carbonate, potassium acetate, and potassium persulfate. All solvents and reagents were bought from Merck (Germany) and Kanto Chemical Co. Inc. (Tokyo, Japan).

Estimation of proximate composition

AOAC method was followed [26] to estimate the ash, moisture, crude fat, fiber, crude protein contents, and gross energy. Micro-Kjeldahl method was followed to determine crude protein multiplying nitrogen by 6.25 (AOAC method 976.05). The sum of crude protein, moisture, crude fat, and ash percentage was subtracted from 100 to estimate carbohydrate (g kg^-1 FW).

Determination of mineral composition

Leaves of red amaranth were dried at 70°C in an oven for 24 hours. Dried leaves were grounded finely in a mill. Nitric-perchloric acid digestion method [26] was followed to determine calcium, potassium, magnesium, iron, manganese, copper, and zinc from powdered leaves. For this digestion, in the presence of carborundum beads 40 ml HClO₄ (70%), 400 ml HNO₃ (65%), and 10 ml H₂SO₄ (96%) were added to 0.5 g dried leaf sample. After digestion, the solution was appropriately diluted in triplicate for measuring phosphorus following ascorbic acid method. Addition of ascorbic acid and antimony to the yellow-colored complex solution converted to a blue-colored phosphomolybdenum complex. Sarker and Oba [26] method was followed to read the absorbance by atomic absorption spectrophotometry (AAS) (Hitachi, Tokyo, Japan) at a wavelength of 285.2 nm (magnesium), 76 6.5 nm (potassium), 248.3 nm (iron), 422.7 nm (calcium), 279.5 nm (manganese), 213.9 nm (zinc), 324.8 nm (copper).

Determination of chlorophylls and carotenoids

The leaves of red amaranth were extracted in 80% acetone to estimate chlorophyll ab, chlorophyll b, total carotenoids, and chlorophyll a according to the method of Sarker and Oba [26]. A spectrophotometer (Hitachi, U-1800, Tokyo, Japan) was used to read the absorbance at 663 nm for chlorophyll a, 646 nm for chlorophyll b, and 470 nm for total carotenoids, respectively. Data were calculated as mg chlorophyll per 100 g fresh weight (FW) and μg total carotenoids per g FW.

Determination of β-cyanins and β-xanthins content

The leaves of red amaranth were extracted in 80% methyl alcohol having 50 mM ascorbate to measure β-cyanins and β-xanthins according to the method of Sarker and Oba [26]. A spectrophotometer (Hitachi, U-1800, Tokyo, Japan) was used to measure the absorbance at 540 nm for β-cyanins and 475 nm for β-xanthins, respectively. The results were expressed as microgram betanin equivalent per 100 gram FW for β-cyanins and micrograms indicaxanthin equivalent per 100 gram FW for β-xanthins.

Estimation of β-carotene

Method of Sarker and Oba [26] was followed to extract and determine β-carotene content. In a mortar and pestle, 10 ml of 80% acetone was added in 500 mg of fresh leaf sample and ground thoroughly. The extract was centrifuged at 10,000 rpm for 3–4 min. The final volume was brought up to 20 ml after removing the supernatant in a volumetric flask. A spectrophotometer (Hitachi, U-1800, Tokyo, Japan) was used to take the absorbance at 510 nm and 480 nm. Data were expressed as μg β-carotene per g fresh weight (FW).

The following formula was used to measure the β-carotene content:

β-carotene = 7.6 (Abs. at 480) - 1.49 (Abs. at 510) × Final volume/ (1000 × fresh weight of leaf taken)

Estimation of Vitamin C

The fresh red amaranth leaves were used to measure ascorbate (AsA) and dehydroascorbic acid (DHA) acid through a spectrophotometer. For pre-incubation of the sample and reduction of DHA into AsA Dithiothreitol (DTT) was used. AsA reduced Fe₃⁺ to Fe₂⁺ and estimation of AsA was made by the spectrophotometric (Hitachi, U-1800, Tokyo, Japan) measuring Fe₂⁺ complexes with 2, 2-dipyridyl [26]. Finally, the absorbance of the sample solution was read. Data were recorded as μg vitamin C per g fresh weight (FW).

Sample extraction for TPC, TFC and TAC analysis

30 DAS red amaranth leaves were harvested. For chemical analysis, the leaves were dried in the air in a shade. 40 ml of 90% aqueous methanol was used to extract 1 g of grounded dried leaves from each cultivar in a bottle (100 ml) capped tightly. A shaking water bath (Thomastant T-N22S, Thomas Kagaku Co. Ltd., Japan) was used to the extract for 1 h. The extract was filtered for determination of polyphenols, flavonoids, total antioxidant capacity.

Determination of polyphenols

Method of Sarker and Oba [27] was followed to estimate the total phenolic content of red amaranth using the folin-ciocalteu reagent with gallic acid as a standard phenolic compound. Folin-ciocalteu reagent was previously diluted 1:4, reagent: distilled water. In a test tube, 1 ml of diluted folin-ciocalteu was added to 50 μl extract solution and then mixed thoroughly for 3 min. 1 ml of Na₂CO₃ (10%) was added to the tube and stand for 1 h in the dark. A Hitachi U1800 spectrophotometer (Hitachi, Tokyo, Japan) was used to read the absorbance at 760 nm. A standard gallic acid graph was made to determine the concentration of phenolics in the extracts. The results are expressed as μg gallic acid equivalent (GAE) g^-1 DW.

Determination of flavonoids

The AlCl₃ colorimetric method [28, 29] was used to estimate the total flavonoid content of red amaranth extract. In a test tube, 1.5 ml of methanol was added to 0.1 ml of 10% aluminum chloride, 0.1 ml of 1 M potassium acetate, 2.8 ml of distilled water and 500 μl of leaf extract for 30 min at room temperature. A Hitachi U1800 spectrophotometer (Hitachi, Tokyo, Japan) was used to take the absorbance of the reaction mixture at 415 nm. TFC is expressed as μg rutin equivalent (RE) g^-1 dry weight (DW) using rutin as the standard compound.

Antioxidant capacity (TAC)

Diphenyl-picrylhydrazyl (DPPH) radical degradation method [30] was used to estimate the antioxidant activity. In a test tube, 1 ml of 250 μM DPPH solution was added to 10 μl of leaf extract solution (in triplicate) and 4 ml of distilled water and allowed to stand for 30 min in the dark. A Hitachi U1800 spectrophotometer (Hitachi, Tokyo, Japan) was used to read the absorbance at 517 nm. Method of Sarker and Oba [31] was followed for ABTS⁺ assay. 7.4 mM ABTS⁺ solution and 2.6 mM potassium persulfate were used in the stock solutions. The two stock solutions were mixed in equal quantities and allowing them to react for 12 h at room temperature in the dark for preparation of the working solution. 2850 μl of ABTS⁺ solution (1 ml ABTS⁺ solution mixed with 60 ml methanol) was mixed with 150 μl sample of leaf extract and allowed to react for 2 h in the dark. A Hitachi U1800 spectrophotometer (Hitachi, Tokyo, Japan) was used to read the absorbance against methanol at 734 nm. The percent of inhibition of DPPH and ABTS⁺ relative to the control were used to determine antioxidant activity using the following equation:

Antioxidant activity (%) = (Abs. blank- Abs. sample/Abs. blank) × 100

Where, Abs. blank is the absorbance of the control reaction [10 μl methanol for TAC (DPPH), 150 μl methanol for TAC (ABTS⁺) instead of leaf extract] and Abs. sample is the absorbance of the test compound. Trolox was used as the reference standard, and the results were expressed as μg Trolox equivalent g^-1 DW.

Statistical analysis

At first, sample data of each trait were averaged replication-wise. The mean data of three replications for all traits were also statistically analyzed by ANOVA using Statistix 8 software, and the means were compared by the Tukey’s HSD test at 1% level of probability. The results were reported as the average of three replications ± SD.

Results

The analysis of variance demonstrated that all the traits significantly varied between the different studied genotypes (Tables 1, 2, 3 and 4). Proximate and mineral compositions, antioxidant leaf pigments, vitamins, TAC (DPPH), TFC, TPC, and TAC (ABTS⁺) of the 25 tested red morph amaranth genotypes are presented in Tables 1, 2, 3 and 4.

Proximate compositions (g kg<sup>-1</sup> fresh weight) and dietary fiber (μg g<sup>-1</sup> FW) of 25 red morph amaranth genotypes. — **Tab. 1. Proximate compositions (g kg^-1 fresh weight) and dietary fiber (μg g^-1 FW) of 25 red morph amaranth genotypes.**

Mineral compositions (Macroelements mg g<sup>-1</sup> DW and microelements μg g<sup>-1</sup> DW) of 25 red morph amaranth genotypes. — **Tab. 2. Mineral compositions (Macroelements mg g^-1 DW and microelements μg g^-1 DW) of 25 red morph amaranth genotypes.**

**Tab. 3. Mean performance for antioxidant leaf pigments in 25 vegetable amaranth genotypes.**

Mean performance for β-carotene, vitamin C, TPC, TFC, TAC (DPPH) and TAC (ABTS<sup>+</sup>) of 25 vegetable amaranth genotypes. — **Tab. 4. Mean performance for β-carotene, vitamin C, TPC, TFC, TAC (DPPH) and TAC (ABTS⁺) of 25 vegetable amaranth genotypes.**

Proximate compositions

Proximate compositions of red morph amaranth are presented in Table 1. The genotype RA11 exhibited the highest moisture content (884.73 g kg^-1 FW), while the genotype RA3 and RA18 had the lowest moisture content (814.64 and 814.83 g kg^-1 FW). The moisture content ranged from 814.64 to 884.73 g kg^-1 FW. Red morph amaranth leaves exhibited noticeable variations in protein content. The genotype RA3 had the highest protein content (62.26 g kg^-1) followed by RA11 and RA15, whereas the genotype RA6 exhibited the lowest protein content (11.38 g kg^-1). For protein content, ten genotypes performed better over their mean value. Among them, eight genotypes RA3, RA8, RA11, RA15, RA5, RA9, RA18, and RA19 showed higher protein content as leafy vegetables. The highest fat content was observed in the genotype RA7 (4.35 g kg^-1 FW) against the lowest content recorded for the genotype RA25 (1.42 g kg-1 FW) with an average of 2.93 g kg^-1 FW.

The highest carbohydrates content were noted in the genotype RA16 and RA6 (98.54 and 97.51 g kg^-1 FW) followed by RA1, RA25, and RA20, while the lowest carbohydrates content was observed in RA19 (15.48 g kg^-1 FW) with an average of 71.41 g kg^-1 FW. The genotype RA18 and RA3 had the highest energy (56.07 and 55.33 Kcal 100 g^-1 FW) followed by RA3, RA8, RA15, and RA25, while the lowest energy was obtained from the genotype RA19 (26.95 Kcal 100g^-1 FW) with an average of 43.40 Kcal 100 g^-1 FW. Ash content was the highest in the genotype RA3 (56.55 g kg^-1 FW) followed by RA8, RA5, RA19, RA15, and RA18, while the lowest ash content was noted in RA24 (20.57 g kg^-1 FW) with an average of 38.86 g kg^-1 FW. Dietary fiber content exhibited remarkable variations in 25 red morph amaranth studied. The dietary fiber content was the highest in RA25 and RA2 (91.94 and 91.66 μg g^-1 FW) followed by RA2, RA4, RA22, RA21, RA9, RA1, RA16, RA8, and RA20, while RA23 exhibited the lowest dietary fiber content (59.96 μg g^-1 FW) with an average of 78.27 μg g^-1 FW.

Mineral compositions

Mineral compositions of red morph amaranth are presented in Table 2. In the present investigation, K content ranged from 6.55 mg g^-1 to 16.28 mg g^-1 DW. The genotypes RA13, RA15, RA3, RA11, and exhibited high K content, while genotype RA17 and RA23 showed the lowest K content with an average of 10.13 mg g^-1 DW. Thirteen genotypes performed much better than their average performance of K content. Calcium content ranged from 16.02–34.82 mg g^-1 DW.

The genotypes RA21, RA6, RA19, RA8, RA12, and RA22 showed high Ca content, while the genotype RA9 and RA25 had the lowest Ca content with an average Ca content of 24.96 mg g^-1 DW. Twelve genotypes had better Ca content over their corresponding mean. Mg content was the highest in RA13 and the lowest in RA14, with an average of 30.01 mg g^-1 DW. The genotype RA13, RA15, RA7, RA6, RA9, RA18, RA19, RA21, RA5, RA8, and RA12 showed higher Mg content. In this study, the genotypes did not show considerable variations in terms of Mg content (24.51 to 35.43 mg g^-1 DW).

The significant and remarkable variations were detected for iron content (195.12 μg g^-1 DW in RA24 to 2057.02 μg g^-1 DW in RA18). The genotypes RA18, RA15, RA13, RA14, and RA23 exhibited the highest iron content. Conversely, the genotype RA24 showed the lowest iron content, with an average value of 1089.19 μg g^-1 DW. Nine genotypes had higher iron content over their average performance. In this study, the manganese content ranged between 132.65 μg g^-1 DW and 356.84 μg g^-1 DW, with an average of 243.59 μg g^-1 DW. The genotype RA13, RA14, RA15, RA13, RA1, RA8, RA4, and RA12 had high manganese content, however, the genotype RA18 showed the lowest manganese content (132.65 μg g^-1 DW). The copper content had significant and notable variations in the studied genotypes (12.09–45.12 μg g^-1 DW). The highest copper content was noted in RA5 (45.12 μg g^-1 DW), followed by RA11, and RA19. Twelve genotypes exhibited higher Cu content over their corresponding grand mean. The genotypes differed significantly and remarkably in zinc content (601.37 μg g^-1 DW (RA18) to 1525.92 μg g^-1 DW (RA15). Eight genotypes showed higher zinc content over their mean performance (986.61 μg g^-1 DW).

Antioxidants leaf pigments

Antioxidant leaf pigments of red morph amaranth are presented in Table 3. Chlorophyll a content (15.30 to 65.82 mg 100 g^-1) exhibited prominent variations among genotypes. The highest chlorophyll a content (65.82 mg 100 g^-1) was observed in the genotype RA25, while the genotype RA5 showed the lowest chlorophyll a content (15.30 mg 100 g^-1).

The genotypes RA3 and RA15 had high chlorophyll a content. Ten genotypes exhibited higher chlorophyll a content over their resultant grand mean. Like chlorophyll a, significant and marked differences were observed in chlorophyll b content (7.32 to 29.73 mg 100 g^-1) in 25 red morphs amaranth genotypes. The highest chlorophyll b content (29.73 mg 100 g^-1) was recorded in the genotype RA11 followed by RA25, RA3, RA8, RA15, and RA18. In contrast, the genotype RA19 exhibited the lowest chlorophyll b content (7.32 mg 100 g^-1). Chlorophyll ab showed significant and remarkable variation (24.17 to 95. 04 mg 100 g^-1). The genotype RA3, RA69, RA15, RA11, RA8, and RA18 exhibited high chlorophyll ab content, whereas, the lowest chlorophyll ab content was recorded in RA13 (24.17 mg 100 g^-1). Ten genotypes had higher chlorophyll ab content over their mean value. β-cyanins ranged from 13.96 to 56.78 μg 100 g^-1 with an average value of 33.30 μg 100 g^-1. The genotype RA8 exhibited the highest β-cyanins content (56.78 μg 100 g^-1) followed by RA3, RA15, RA18, and RA25. Conversely, the genotype RA19 showed the lowest β-cyanins content (13.96 μg 100 g^-1). Among genotypes, significant and remarkable variations were observed in β-xanthins content, with a range of 12.57 to 58.12 μg 100 g^-1. β-xanthins content was the highest in RA8 (58.12 μg g^-1) and higher in RA3, RA15, RA18, and RA25. On the other hand, the genotype RA19 showed the lowest β-xanthins content (12.57 μg 100 g^-1). Ten genotypes showed better performance over their grand mean. Betalains varied significantly and markedly and ranged from 26.52 to 114.89 μg 100 g^-1. The genotype RA8 had the highest betalains content (114.89 μg 100 g^-1), and genotype RA3, RA15, RA18, and RA25 had higher betalains content. Whereas, the genotype RA19 had the lowest betalains content (26.52 μg 100 g^-1). Nine genotypes showed better performance over the grand mean. Total carotenoids content ranged from 564.66 μg g^-1 in RA9 to 1677.26 μg g^-1 in RA17. The genotype RA18, RA20, RA5, RA2, RA1, RA3, RA49, RA10, RA58, RA14, and RA19 had high total carotenoids. Fourteen genotypes had better performance over their mean value.

Antioxidant phytochemicals and antioxidant activity

Vitamins, TAC, TFC, and TPC of red morph amaranth are presented in Table 4. β-Carotene content ranged from 559.29 μg g^-1 in RA4 to 1524.41 μg g^-1 in RA5. The genotype RA5 exhibited the highest β-carotene content (1524.41μg g^-1) and the genotype RA18, RA25, RA15, RA20, and RA2 demonstrated high β-carotene content. Sixteen genotypes performed better than their grand mean. Vitamin C content ranged from 103.53 μg g^-1 in RA22 to 1990.58 μg g^-1 in RA5 with an average of 955.19 μg g^-1. The genotype RA3, RA19, RA6, and RA18 exhibited high vitamin C content. Ten genotypes performed better over their respective grand mean. Total polyphenol content (TPC) ranged from 96.21 GAE μg g^-1 DW (RA13) to 260.84 GAE μg g^-1 DW (RA15) with an average TPC content of 172.53 GAE μg g^-1 DW. The genotype RA15 had the highest TPC. The genotype RA25, RA3, RA5, and RA18 had higher TPC values. Eleven genotypes had a higher performance of TPC over their respective grand mean. TFC exhibited much noticeable variation in terms of genotypes, which ranged from 35.19 RE μg g^-1 DW in the genotype RA1 to 171.26 RE μg g^-1 DW in the genotype RA15. The average mean of TFC was 102.10 RE μg g^-1 DW. The genotype RA15 exhibited the highest TFC showing the following order: RA15 ˃ RA25 ˃ RA5 ˃ RA18. Eleven genotypes exhibited better performance over their respective grand mean. TAC (DPPH) ranged from 11.17 TEAC μg g^-1 DW (RA1) to 31.70 TEAC μg g^-1 DW (RA25). The higher TAC (DPPH) was recorded in the genotype RA18, RA5, RA22, RA8, RA15, and RA3. In contrast, the genotype RA1, RA10, and RA20 had the lowest TAC (DPPH) with an average of 19.25 TEAC μg g^-1 DW. Nine genotypes had better performance over their respective grand mean. TAC (ABTS⁺) ranged from 21.86 TEAC μg g^-1 DW (RA1) to 62.03 TEAC μg g^-1 DW (RA25). The genotype RA25 had the highest TAC (ABTS⁺) which was statistically similar to the genotype RA18, RA5, and RA22. The higher TAC (ABTS⁺) was noticed in the genotypes, RA8, RA15, and RA3. In contrast, TAC (ABTS⁺) was the lowest in RA1 (21.86 μg g^-1 DW), RA12 (21.89 μg g^-1 DW), and RA10 (22.42 μg g^-1 DW) with an average of 39.09 TEAC μg g^-1 DW. Nine genotypes showed much better performance over their respective mean betalains.

Correlation coefficient analysis

Correlation of bioactive compounds of red morph amaranth is presented in Table 5. The analysis of correlation coefficients presented in Table 5 exhibited exciting results. The chlorophyll ab, chlorophyll b, and chlorophyll b exhibited positive and significant associations among each of them and with β-cyanins, β-xanthins, betalains, TAC (ABTS⁺), TFC, TPC, and TAC (DPPH). Carotenoids and β-carotene exhibited a significant negative association with all leaf pigments, whereas, these two traits had a significant positive relationship with TAC (ABTS⁺), TFC, TPC, and TAC (DPPH). Carotenoids and β-carotene were positively associated with each other. Conversely ascorbic acid exhibited insignificant interrelationships with all the traits. TAC (ABTS⁺), TFC, TPC, and TAC (DPPH) exhibited substantial positive association among each other, all leaf pigments, and vitamins.

**Tab. 5. Correlation coefficient for antioxidant leaf pigments, β-carotene, vitamin C, TPC, TFC, TAC (DPPH) and TAC (ABTS+) in 25 vegetable amaranth genotypes.**

Discussion

Color, flavor, and taste predominantly influenced the acceptability of foods products. Considering the safety, nutritional, and aesthetic aspects of food, the demand for natural pigments have been increased in consumers day by day. Red morph amaranth was a unique and inexpensive source of color pigments such as β-cyanins, β-xanthins, betalains, anthocyanin, amaranthine, carotenoids, and chlorophylls that have potential free radical detoxifying ability and act as potent antioxidants [1,3]. The active ingredients of these pigments have significant contributions to human health as they provide protection against lung and skin cancers, cardiovascular and inflammatory disease [4]. Red morph amaranth also had abundant natural antioxidant phytochemicals such as flavonoids, β-carotene, phenolics, and vitamin C along with protein, dietary fiber, and minerals. These natural antioxidants protect cancer, emphysema, cardiovascular diseases, atherosclerosis, diabetes, retinopathy, osteoporesis, neurodegenerative diseases, arthritis, cataracts, inflammation, and prevent aging [23–25]. It is a widely distributed leafy vegetable in Bangladesh, Asia, Africa and South America with great variability and phenotypic plasticity [22]. In Bangladesh, red morph amaranth was grown year-round and in the hot summer, a gap period of foliage vegetables [11–12]. Its attractive leaf color, nutritional value, and taste make it popular in the rest of the continent and elsewhere. Its production and consumption have been remarkably increased due to the presence of excellent nutritional and natural antioxidants such as antioxidant leaf pigments, vitamins, phenolics, and flavonoids. So, red morph amaranth could significantly contribute to local, regional and international nutritional and antioxidants security challenges by reducing the hidden hunger and attaining nutritional and antioxidant sufficiency in the world. In this study, we comprehensively evaluated 25 red morph amaranth genotypes in terms of proximate and mineral compositions, antioxidant pigments, phytochemicals, and antioxidant activity and their variability. Our results demonstrated that red morph amaranth had abundant natural pigments, phytochemicals with high antioxidant activity along with nutritional components. However, the components varied significantly in terms of genotypes.

One of the interesting findings of our study was that we obtained abundant antioxidant pigments and phytochemicals with high antioxidant activity along with nutritional components in the red morph amaranth genotypes which could contribute to local, regional, and international nutritional and antioxidant sufficiency by reducing the hidden hunger and attaining antioxidant sufficiency in the world. We found remarkable chlorophyll a (31.79 mg 100 g^-1), chlorophyll b (16.05 mg 100 g^-1) and chlorophyll ab (47.83 mg 100 g^-1) content in the red morphs amaranth, whereas, Khanam and Oba [32] observed comparatively lower chlorophyll content in red morphs amaranth. We observed remarkable β-cyanins (56.78 μg 100 g^-1), β-xanthins (58.12 μg 100 g^-1), betalains (114.89 μg 100 g^-1), and total carotenoids (1677.26 μg g^-1) in the red morphs amaranth, similarly, Khanam and Oba [32] observed more or less similar trend in β-cyanins, β-xanthins, betalains, and total carotenoids content of red morphs amaranth. Regarding phytochemicals, we found remarkable β-carotene (1524.41 μg g^-1), vitamin C (1990.58 μg g^-1) in the red morphs amaranth, which exhibited comparatively higher values in terms of our previous studies in A. tricolor [12]. TPC (260.84 GAE μg g^-1 DW) obtained in this study were also higher than the results of Khanam and Oba [32] in A. tricolor. TFC (171.26 RE μg g^-1 DW), TAC (DPPH) (31.70 TEAC μg g^-1 DW), and TAC (ABTS⁺) (62.03 TEAC μg g^-1 DW) obtained in this study were more or less similar to the results of Khanam et al. [33] in A. tricolor. The genotypes RA25 had the highest TAC (DPPH, ABTS+), chlorophylls, high betalains, total carotenoids, β-carotene, phenolics, and flavonoids. The genotype RA18 had high TAC (DPPH, ABTS+), chlorophylls, betalains, total carotenoids, β-carotene, phenolics, and flavonoids. The genotype RA15 exhibited high TAC (DPPH, ABTS+), chlorophylls, betalains, total carotenoids, β-carotene, and the highest phenolics and flavonoids. The genotype RA5 and RA3 had high TAC (DPPH, ABTS+), chlorophylls, betalains, total carotenoids, moderate β-carotene, phenolics, and flavonoids. These five genotypes could be used as antioxidant profile enriched high-yielding varieties. We can conclude that red amaranth has abundant phenolics, pigments, flavonoids, vitamins, and antioxidant that offered enormous prospects for nourishing the vitamin and antioxidant scarce people.

As lower moisture content was desirable to confirm the higher dry matter, six genotypes such as RA3, RA18, RA15, RA8, RA5, and RA25 showed 18–19% dry matter might be selected for dry matter. The moisture content of red morph amaranth leaves directly related to the maturity of the plant. Similar results were reported by Sun et al. on sweet potato leaves [34]. Eight genotypes RA3, RA8, RA11, RA15, RA5, RA9, RA18, and RA19 showed higher protein content as leafy vegetables. Vegetarian and poor people of the low-income countries mainly depend on red amaranth for their protein source. So, red morph amaranth might be an excellent source of protein for vegetarian and poor people. The protein content of red morph amaranth (33.99 g kg^-1) was much higher as compared to A. tricolor (1.26%) in our earlier study [2]. The fat content in the present study agreed to the results of Sun et al. [34] in sweet potato leaves. They mentioned that fat involved in the insulation of body organs and maintenance of body temperature and cell function. Fats have abundant omega-3 and omega-6 fatty acids. Fats play a significant role in absorption, digestion, and transport of fat-soluble vitamins A, D, E, and K. Dietary fiber has a significant role in palatability, digestibility, and remedy of constipation [14]. From the results, we observed that red morph amaranth leaves have abundant carbohydrates, protein, moisture, and dietary fiber. As red morph amaranth had low energy content, this may not impact significantly on energy contribution to the human body as low amounts of this vegetable consumed in a day. Like other leafy vegetables, the low carbohydrate content of red morph amaranth may not have a significant impact on carbohydrate contribution to the human body considering the low amount of vegetable uptake per day and a very high daily requirement for the human body.

Amaranth had higher mineral contents than commonly consumed leafy vegetables, such as spinach, lettuce, and kale [35]. In our present study, we found remarkable K (10.13 mg g^-1), Ca (24.96 mg g^-1), and Mg (30.01 mg g^-1) in the red morph amaranth, albeit we estimated in dry weight basis. Jimenez-Aguiar and Grusak [35] noted abundant K, Ca, and Mg in different amaranths including red amaranth. They also found amaranth K, Ca, and Mg was much higher than spinach, spider flower, kale, and black nightshade. Zinc and iron content of red morph amaranth is higher than the cassava leaves [36] and beach pea [37]. In this study, we found remarkable Fe (1089.19 μg g^-1), Mn (243.59 μg g^-1), Cu (25.77 μg g^-1), and Zn (996.61 μg g^-1) in red morph amaranth, although we estimated in dry weight basis. Similarly, Jimenez-Aguiar and Grusak [35] noted abundant Fe, Mn, Cu, and Zn in different amaranths including red amaranth. They also found amaranth Fe, Mn, Cu, and Zn were much higher than spinach, spider flower, kale, and black nightshade. The U.S. Department of Agriculture’s National Nutrient Database for Standard Reference [35] lists a serving size of spinach as 30 g fresh weight FW (1 cup). As red amaranth has higher mineral concentrations than spinach so, a serving size of leaves of 30 g FW is enough for nutritional sufficiency.

The chlorophyll ab, chlorophyll b, and chlorophyll b exhibited positive and significant associations among each of them and with β-cyanins, β-xanthins, betalains, TAC (ABTS⁺), TFC, TPC, and TAC (DPPH). It revealed that increment of one leaf pigment straightly associated with an increase of another leaf pigment. The significant positive correlation of all leaf pigments with TAC (ABTS⁺), TFC, TPC, and TAC (DPPH) signifies that all the leaf pigments had strong antioxidant activity. Significant positive association of carotenoids and β-carotene with TAC (ABTS⁺). TFC, TFC, TPC, and TAC (DPPH) suggested that carotenoids and β-carotene had strong antioxidant activity. Ascorbic acid exhibited insignificant interrelationships with all the traits indicating negligible contribution in the antioxidant potentiality of red morphs amaranth. Jimenez-Aguilar and Grusak [35] reported similar findings for ascorbic acid in amaranth. A similar trend of the insignificant association was also observed by Shukla et al. [38] in their earlier work in amaranth. TAC (ABTS⁺), TFC, TPC, and TAC (DPPH) exhibited substantial positive association among each other, all leaf pigments, and vitamins representing the involvement of these phytochemicals in antioxidant activity. In the present investigation, it revealed that phenolics, pigments, flavonoids, and vitamins contribute significantly in the antioxidant potentiality of red morphs amaranth.

Conclusions

Red morphs amaranth leaves have abundant antioxidant pigments and phytochemicals such as β-carotene, chlorophyll, vitamin C, β-cyanins, carotenoids, β-xanthins, TAC, betalains, TPC, and TFC. It also has abundant protein, dietary fiber, and minerals such as Ca, K, Mg, Fe, Cu, Zn, and Cu compared to leafy vegetables. Correlation study revealed that natural antioxidant pigments and phytochemicals had strong antioxidant capacity. It could be a potential leafy vegetable as a source of natural antioxidant pigments and phytochemicals having strong antioxidant activity along with nutritional components in our daily diet to combat with the hidden hunger and attaining nutritional and antioxidant sufficiency. Hence, red morphs amaranth with rice, wheat, and maize in our daily diet could contribute to attaining nutritional and antioxidant sufficiency.

Zdroje

1. Cai Y, Sun M, Corke H. Antioxidant activity of betalains from plants of the Amaranthaceae. Journal of Agricultural and. Food Chemistry, 2003, 51, 2288–2294. doi: 10.1021/jf030045u 12670172

2. Stintzing FC, Carle R. Betalains–emerging prospects for food scientists. Trends in Food Science and Technology, 2007, 18, 514–525.

3. Esatbeyoglu T, Wagner AE, Schini-Kerth VB, Rimbach G. Betanin- a food colorant with biological activity. Molecular Nutrition and Food Research, 2015, 59, 36–47. doi: 10.1002/mnfr.201400484 25178819

4. Isabelle M, Lee BL, Lim MT, Koh WP, Huang D, Ong CN. Antioxidant activity and profiles of common fruits in Singapore. Food Chemistry, 2010, 123, 77–84.

5. Sarker U, Islam MT, Rabbani MG, Oba S. Genotypic variability for nutrient, antioxidant, yield and yield contributing traits in vegetable amaranth. Journal of Food Agriculture and Environment, 2014, 12, 168–174.

6. Sarker U, Islam MT, Rabbani MG, Oba S. Genotypic diversity in vegetable amaranth for antioxidant, nutrient and agronomic traits. Indian Journal of Genetics and Plant Breeding, 2017, 77, 173–176.

7. Sarker U, Islam MT, Rabbani MG, Oba S. Variability in total antioxidant capacity, antioxidant leaf pigments and foliage yield of vegetable amaranth. Journal of Integrative Agriculture, 2018a, 17, 1145–1153.

8. Sarker U, Islam MT, Rabbani MG, Oba S. Phenotypic divergence in vegetable amaranth for total antioxidant capacity, antioxidant profile, dietary fiber, nutritional and agronomic traits. Acta Agriculturae Scandinavica Section B- Soil and Plant Science, 2018b, 68, 67–76.

9. Sarker U, Islam MT, Rabbani MG, Oba S. Antioxidant leaf pigments and variability in vegetable amaranth. Genetika. 2018c, 50, 209–220.

10. Chakrabarty T, Sarker U, Hasan M, Rahman MM. Variability in mineral compositions, yield and yield contributing traits of stem amaranth (Amaranthus lividus). Genetika, 2018, 50, 995–1010.

11. Sarker U, Islam MT, Rabbani MG, Oba S. Variability, heritability and genetic association in vegetable amaranth (Amaranthus tricolor). Spanish Journal of Agricultural Research, 2015a, 13, 1–8. http://dox.doi.org/10.5424/sjar/2015132-6843

12. Sarker U, Islam MT, Rabbani MG, Oba S. Genotype variability in composition of antioxidant vitamins and minerals in vegetable amaranth. Genetika, 2015b, 47, 85–96.

13. Venskutonis PR, Kraujalis P. Nutritional components of amaranth seeds and vegetables: a review on composition, properties, and uses. Comprehensive Review in Food Science and Food Safety, 2013, 12, 381–412.

14. Sarker U, Islam MT, Rabbani MG, Oba S. Genetic variation and interrelationship among antioxidant, quality and agronomic traits in vegetable amaranth. Turkish Journal of Agriculture and Forestry, 2016, 40, 526–535.

15. Sarker U, Oba S. Catalase, superoxide dismutase, and ascorbate-glutathione cycle enzymes confer drought tolerance of Amaranthus tricolor. Scientific Report, 2018d, 8, 16496. doi: 10.1038/s41598-018-34944-0 30405159

16. Sarker U, Oba S. Drought stress enhances nutritional and bioactive compounds, phenolic acids and antioxidant capacity of Amaranthus leafy vegetable. BMC Plant Biology, 2018e, 18, 258. https://doi.org/10.1186/s12870-018-1484-1

17. Sarker U, Islam MT, Oba S. Salinity stress accelerates nutrients, dietary fiber, minerals, phytochemicals and antioxidant activity in Amaranthus tricolor leaves. PLOS One, 2018f, 13, 1–18. https://doi.org/10.1371/journal.pone.0206388.

18. Sarker U, Oba S. Salinity stress enhances color parameters, bioactive leaf pigments, vitamins, polyphenols, flavonoids and antioxidant activity in selected Amaranthus leafy vegetables. Journal of the Science of Food and Agriculture, 2019a, 99, 2275–2284. doi: 10.1002/jsfa.9423 30324618

19. Sarker U, Oba S. Augmentation of leaf color parameters, pigments, vitamins, phenolic acids, flavonoids and antioxidant activity in selected Amaranthus tricolor under salinity stress. Scientific Report, 2018g, 8, 12349. doi: 10.1038/s41598-018-30897-6 30120319

20. Sarker U, Oba S. Drought stress effects on growth, ROS markers, compatible solutes, phenolics, flavonoids, and antioxidant activity in A. tricolor. Applied Biochemistry and Biotechnology, 2018h, 186, 999–1016. https://doi.org/10.1007/s12010-018-2784-5.

21. Shukla S, Bhargava A, Chatterjee A, Pandey AC, Mishra B. Diversity in phenotypic and nutritional traits in vegetable amaranth (A. tricolor), a nutritionally underutilized crop. Journal of the Science of Food and Agriculture, 2010, 90, 139–144. doi: 10.1002/jsfa.3797 20355024

22. Rajan S, Markose BL. Horticultural Science Series-6. In Peter KMV. (Ed.), Propagation of horticultural crops. New Delhi, India: New India Publishing Agency. 2007.

23. Repo-Carrasco-Valencia R, Hellstrom JK, Pihlava JM, Mattila PH. Flavonoids and other phenolic compounds in Andean indigenous grains: Quinoa (Chenopodium quinoa), kaniwa (Chenopodium pallidicaule) and kiwicha (Amaranthus caudatus). Food Chemistry, 2010, 120, 128–133.

24. Dusgupta N, De B. Antioxidant activity of some leafy vegetables of India: A comparative study. Food Chemistry, 2007, 101, 471–474.

25. Steffensen SK, Rinnan A, Mortensen AG, Laursen B, Troiani RM, Noellemeyer EJ, et al. Variations in the polyphenol content of seeds of field grown Amaranthus genotypes. Food Chemistry, 2011, 129, 131–138.

26. Sarker U, Oba S. Response of nutrients, minerals, antioxidant leaf pigments, vitamins, polyphenol, flavonoid and antioxidant activity in selected vegetable amaranth under four soil water content. Food Chemistry, 2018i, 252, 72–83. doi: 10.1016/j.foodchem.2018.01.097 29478565

27. Sarker U, Oba S. Antioxidant constituents of three selected red and green color Amaranthus leafy vegetable. Scientific Reports, (2019b), (Accepted). doi: 10.1038/s41598-019-52033-8 31796754

28. Sarker U, Oba S. Nutraceuticals, antioxidant pigments, and phytochemicals in the leaves of Amaranthus spinosus and Amaranthus viridis weedy species. Scientific Reports, (2019c), (Accepted). doi: 10.1038/s41598-019-50977-5

29. Sarker U, Oba S. Nutritional and antioxidant components and antioxidant capacity in green morph Amaranthus leafy vegetable. Scientific Reports, (2019d), (Accepted).

30. Sarker U, Oba S. Nutrients, minerals, antioxidant pigments and phytochemicals, and antioxidant capacity of the leaves of stem amaranth. Scientific Reports, 2019e, (accepted).

31. Sarker U, Oba S. Nutraceuticals, pigments, phytochemical, and radical scavenging capacity in selected Amaranthus leafy vegetables. PLOS One, (2019f), (accepted).

32. Khanam UKS, Oba S. Bioactive substances in leaves of two amaranth species, Amaranthus lividus, and A. hypochondriacus. Canadian Journal of Plant Science, 2013, 93, 47–58.

33. Khanam UKS, Oba S, Yanase E, Murakami Y. Phenolic acids, flavonoids and total antioxidant capacity of selected leafy vegetables. Journal of Functional Foods. 2012, 4, 979–987.

34. Sun H, Mu T, Xi L, Zhang M, Chen J. Sweet potato (Ipomoea batatas L.) leaves as nutritional and functional foods. Food Chemistry, 2014, 156, 380–389. doi: 10.1016/j.foodchem.2014.01.079 24629984

35. Jimenez-Aguilar DM, Grusak MA. Minerals, vitamin C, phenolics, flavonoids and antioxidant activity of Amaranthus leafy vegetables. Journal of. Food Composition and Analysis, 2017, 58, 33–39.

36. Madruga MS, Camara FS. The chemical composition of “Multimistura” as a food supplement. Food Chemistry, 2000, 68, 41–44.

37. Shahidi F, Chavan UD, Bal AK, McKenzie DB. Chemical composition of beach pea (Lathyrus maritimus L.) plant parts. Food Chemistry, 1999, 64, 39–44.

38. Shukla S, Bhargava A, Chatterjee A, Srivastava J, Singh N, Singh SP. Mineral profile and variability in vegetable amaranth (Amaranthus tricolor). Plant Foods for Human. Nutrition, 2006, 61, 23–28. doi: 10.1007/s11130-006-0004-x 16736385