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Article

Nutrient Composition, Forage Parameters, and Antioxidant Capacity of Alfalfa (Medicago sativa, L.) in Response to Saline Irrigation Water

US Salinity Laboratory, 450 W. Big Springs Rd., Riverside, CA 92507, USA
*
Author to whom correspondence should be addressed.
Currently at INTA- Estaci
These authors contributed equally to this work.
Submission received: 17 April 2015 / Revised: 16 July 2015 / Accepted: 20 July 2015 / Published: 28 July 2015
(This article belongs to the Special Issue Forage Plant Ecophysiology)

Abstract

:
Although alfalfa is moderately tolerant of salinity, the effects of salinity on nutrient composition and forage parameters are poorly understood. In addition, there are no data on the effect of salinity on the antioxidant capacity of alfalfa. We evaluated four non-dormant, salinity-tolerant commercial cultivars, irrigated with saline water with electrical conductivities of 3.1, 7.2, 12.7, 18.4, 24.0, and 30.0 dS·m−1, designed to simulate drainage waters from the California Central Valley. Alfalfa shoots were evaluated for nutrient composition, forage parameters, and antioxidant capacity. Salinity significantly increased shoot N, P, Mg, and S, but decreased Ca and K. Alfalfa micronutrients were also affected by salinity, but to a lesser extent. Na and Cl increased significantly with increasing salinity. Salinity slightly improved forage parameters by significantly increasing crude protein, the net energy of lactation, and the relative feed value. All cultivars maintained their antioxidant capacity regardless of salinity level. The results indicate that alfalfa can tolerate moderate to high salinity while maintaining nutrient composition, antioxidant capacity, and slightly improved forage parameters, thus meeting the standards required for dairy cattle feed.

Graphical Abstract

1. Introduction

Alfalfa (Medicago sativa, L.) is the most cultivated legume worldwide and the fourth most cultivated crop in the United States. Alfalfa is cultivated in most continents and in more than 80 countries occupying more than 35 million ha [1]. In the USA, it is among the top three field crops cultivated in 26 states, thus contributing more than US $10 billion a year to the farm economy, primarily as an animal feed [2]. Alfalfa is considered to be the most important forage crop for providing protein to dairy and beef cattle, sheep, horses, birds, and other livestock [1]. Feeding of alfalfa hay to lactating dairy cows has decreased sharply in the past 10 years, primarily as a result of economic issues associated with high water use, the costs of multiple harvests, and storage [3]. These authors also mentioned the increased use of corn and cereal silages in animal diets to replace alfalfa. However, dry matter intake is significantly higher for cows fed alfalfa and barley silages than for cows fed oat and triticale silages [4]. According to these authors, alfalfa silage contains higher concentrations of all minerals analyzed compared with cereal silages, except for Na. Moreover, the cows also absorbed K better from alfalfa silage (89%) than from cereal silages (74% to 83%). Alfalfa is highly important to livestock considering its fast canopy recovery after each harvest, its relative tolerance of salinity, its capacity to endure temperature extremes (e.g., hot days and cold nights), its nutritional value, and palatability to livestock.
In arid lands, irrigation is necessary for high forage mass production. However, this irrigation is often associated with salinization. Among the approximately 270 million hectares of irrigated land worldwide, about 40% is located in arid/semiarid zones [5] where soil salinization generally occurs. Some of the typical agronomic parameters used to evaluate the salinity tolerance of crops include yield, survival, plant height, and relative growth rate or reduction [6,7,8]. Few researchers have evaluated alfalfa forage mass production, nutrient composition, and forage parameters for livestock under high salinity stress [9,10,11,12]. Further, we found no published reports on the effects of salinity on the antioxidant capacity of alfalfa. It has been reported that salinity stress imposed on a model legume (Lotus japonicus) increased antioxidant enzyme levels in leaves [13], and that the expression of genes associated with antioxidant enzymes increased in response to excessive levels of reactive oxygen species (ROS) generated by salinity stress [14]. These authors postulated that these enzymes protect plant tissues from ROS damage triggered by salinity stress, but there are no reports on the biosynthesis of non-enzymatic antioxidants, such as flavonoids and phenolic compounds, by alfalfa in response to salinity. Alfalfa shoots are a rich source of antioxidant flavonoids, mainly apigenin, tricin, luteolin, and chrysoeriol glycosides [15], and of phenolic compounds reported to have anti-inflammatory [16], antioxidant, and neuroprotective activity in mice [17]. The ratio of alfalfa antioxidant flavones acylated with hydroxycinnamic acid to non-acylated (lower antioxidant capacity) flavones increases in summer when plants are exposed to a higher amount of UV-B radiation [15]. Antioxidant flavonoids in Ligustrum vulgare were reported to increase under both UV-B and NaCl salinity stress [18]. Thus, although alfalfa is fed to livestock for its high protein content, digestibility, and palatability, there is a scarcity of information on the effects of salinity on alfalfa mineral composition and forage quality, while there is no information on its antioxidant capacity under salinity stress.
In this work, we evaluated four commercial alfalfa cultivars, tolerant to salinity, for their response to salinity when cultivated in outdoor sand tanks and irrigated at six salinity levels with water high in sodium, chloride, and sulfate. The goal of our work was to evaluate the effects of increasing salinity on the mineral nutritional composition, forage quality, and antioxidant capacity of alfalfa shoots.

2. Experimental Section

2.1. Plant Material and Growth Conditions

Four commercial non-dormant, salinity-tolerant, Medicago sativa L. cultivars “Salado”, “SW8421S”, “SW9215”, and “SW9720” (S&W, Fresno, CA, USA, www.swseedco.com) were grown from seeds in 24 outdoor sand tanks from 23 June 2011 to 17 April 2012 at the Salinity Laboratory (USDA-ARS) in Riverside, California. Irrigation water at different levels of electrical conductivity (EC) was applied to four cultivars in a split-plot design. The irrigation water EC (measured in deciSiemens per meter) levels consisted of a control using Riverside tap water (EC = 0.6 dS·m−1) plus fertilizers (EC = 3.1 dS·m−1), and treatments of 7.2, 12.7, 18.4, 24.0 and 30.0 dS·m−1, with four tanks (replicates) per treatment. The tanks measured 82 cm wide by 202 cm long by 85 cm deep. Further details on sowing density per cultivar and irrigation frequency are described elsewhere [19]. Salinity treatments and the irrigation water control (EC of 3.1 dS·m−1) were designed to simulate the drainage water composition of the Central Valley, CA, with subsequent concentration of salts considering mineral precipitation (calcite and/or gypsum) using the UNSATCHEM model [20], which simulates typical soil water interactions. All reservoirs had modified Hoagland’s solution, and added Na+, SO 4 2 , and Cl (including control water) to reach the target EC; the detailed composition is described elsewhere [19]. The composition of Riverside tap water (EC = 0.6 dS·m−1) in mmolc·L−1 was: 3.4 Ca2+, 0.8 Mg 2+, 1.6 Na+, 0.1 K+, 1.3 SO 4 2 , 0.8 Cl, and 0.49 NO3. The water composition of all the treatment waters is shown in Table 1.

2.2. Plant Growth and Nutrient Composition

Growth and forage mass measurements were collected at seven harvest dates except for the plants that were irrigated with water with an EC = 24.0 dS·m−1, which were harvested three times (4th, 6th, and 7th harvests) during the 299 days of cultivation and are presented elsewhere [19]. For this work, we present data on ionic and nutrient composition at 84 days after seeding (DAS) (2nd harvest, on 15 September 2011) and at 299 DAS (7th harvest, on 17 April 2012). The second harvest was conducted when the control plants were at the early flowering stage, corresponding to morphological stage 5 [21]. The seventh harvest was conducted when the control plants were at a late vegetative stage (due to the absence of flowering). The shoot fresh and dry weights (dried at 60 °C for 48 h) were recorded at each harvest and all plants were cut back to 5–8 cm above the sand surface.
Table 1. Chemical composition of the water used in the six salinity treatments in this study. EC, electrical conductivity of irrigation water that defines each salinity level (in deciSiemen per meter); mmolc·L−1, millimole of charge of each cation or anion listed.
Table 1. Chemical composition of the water used in the six salinity treatments in this study. EC, electrical conductivity of irrigation water that defines each salinity level (in deciSiemen per meter); mmolc·L−1, millimole of charge of each cation or anion listed.
Treatment12345
EC (dS·m−1)3.17.212.718.424.0
Ion Concentration in mmolc·L−1
Ca2+6.419.225.029.428.4
Mg2+4.014.324.140.758.5
Na+15.554.2101169229
K+6.46.46.26.46.6
SO42−15.353.385.0132182
Cl8.031.862.9104133
PO43−0.30.30.30.40.5
NO35.55.65.56.06.0
All salinity levels had the following added nutrients, (in mmolc·L−1): 0.3 KH2PO4, 5.0 KNO3, 3.1 MgSO4.7H2O, 3.0 CaCl2, and 1.0 KCl. Table modified from [19]. Highest salinity level (30 dS·m−1) not shown as all plants died at this level.
The levels of the macronutrients N, P, K, Ca, Mg, and total S, and of the micronutrients Fe, Cu, Mn, Zn, and Mo were determined from nitric acid digestions of the dried and ground plant material using Inductively Coupled Plasma Optical Emission Spectrometry (ICP-OES, 3300DV, Perkin-Elmer Corp., Waltham, MA, USA). There was insufficient plant material to analyze samples from the EC = 24 dS·m−1 treatment at 84 DAS, and there are no data from the EC = 30 dS·m−1 treatment as all plants died at this salinity level.

2.3. Oxygen Radical Absorbance Capacity (ORAC) and Total Phenolics (TP) Analyses

Ground dried samples (0.5 g) of alfalfa tops were mixed with 5 g of sand. Each mixture was then extracted in a pressurized stainless steel cell (ASE 350, Thermo Scientific/Dionex, Sunnyvale, CA, USA) using hexane to extract the lipophilic fraction and acetone:water:acetic acid (70:29.5:0.5 by volume) for the hydrophilic fraction. The extraction time was 5 min, followed by a 100% flush, a 60-s purge with 2 cycles, at 80 °C and 1500 psi. The hexane extract was evaporated to dryness with nitrogen in an evaporator (N-EVAP, Organomation, Berlin, MA, USA) at 37 °C and then redissolved in 10 mL of pure acetone; a 50-μL aliquot was collected for dilution and lipophilic ORAC analysis. After extraction with aqueous acetone by the ASE 350, the samples were made up to a volume of 25 mL in the acetone-water-acetic acid solution. A 150-μL aliquot of the aqueous acetone extracts was diluted for hydrophilic ORAC analysis. The ORAC assay is based on the inhibition of the peroxyl-radical-induced oxidation initiated by thermal decomposition of azo-compounds such as [2,2′-azobis(2-amidino-propane) dihydrochloride (AAPH)] [22]. Samples were analyzed for their antioxidant capacity (ORAC) in triplicate. The same ASE 350 aqueous acetone extracts were used for quantification of TP according to the Folin-Ciocalteu method [23,24] using gallic acid (cat. No. 398225, Sigma-Aldrich, Saint Louis, MO, USA) as the standard. A 20-μL aliquot of the extracts or a gallic acid standard solution was pipetted into a cell of a 96-cell microplate, followed by the addition of 100 μL of 0.4 N Folin Ciocalteu phenol reagent (stock solution F9252, Sigma-Aldrich, Saint Louis, MO, USA) and the addition of 80 μL of 0.94 M Na2CO3. The plate was covered with a plastic plate cover and allowed to develop color for 5 min at 50 °C. The absorbance was read at 765 nm using a microplate spectrophotometer (xMark™, BIO-RAD, Hercules, CA, USA).

2.4. Forage Quality

Shoots were dried at 60 °C for 48 h. Samples were ground to a size of 1.0 mm and analyzed for acid detergent fiber (ADF), neutral detergent fiber (NDF), and moisture by an independent laboratory (Analytical Feed & Food Laboratory, Visalia, CA, USA), according to AOAC International Methodology [25]. The parameters and analytical methods used were AOAC 973.18 for ADF, AOAC 2002.04 for NDF, and AOAC 930.15 for moisture. The parameters calculated according to ADF, NDF, and/or moisture include the net energy for lactation (NEL), calculated as NEL = 0.8611 – (0.00835 × ADF); relative feed value (RFV), calculated as RFV = (DMD × DMI)/1.29; dry matter intake (DMI), calculated as DMI = 120/NDF; and dry matter digestibility (DMD), calculated as DMD = 88.9 – (0.779 × ADF), according to National Forage Testing Association [26]. Crude protein (CP) was estimated as N% × 6.25 [27]. Nitrogen was determined by sample combustion in pure oxygen and measured by thermal conductivity detection (AOAC, 2000; ID 990.03) using a Vario Pyro Cube® (Elementar Americas, Inc., Mt. Laurel, NJ, USA).

2.5. Statistical Analysis

The nutrient composition data for each harvest were analyzed using a split-plot procedure, with the following statistical model:
Yijk = μ + Sj + Ri + Ck + (SC)jk + εijk
where R, S and C represent the replicates (i = 1,…4), salinity level (j = 1,…5), and cultivars (k = 1,…4) respectively. All effects were considered as fixed. Thus, Yijk is the response to replicate i in Sj and Ck, μ is the overall mean; and εijk represents the random error. The significance in the split-plot design was calculated by deriving the mean squares in the analysis of variance using the InfoStat program [28] with a completely randomized design (CRD). The significance of the main plot (salinity, S) was tested by S > R (salinity inside replicate) as an experimental error of the main plot, and the mean square error was used to test significance of the subplot (C) and the interaction S × C (salinity per cultivar). The mean differences were determined using the Fisher LSD test at p ≤ 0.05. Chemical analyses for forage parameters were performed on two samples per cultivar, which were combined to represent each salinity level (n = 8) per harvest. These data (Figure 1) were subjected to a one-way (salinity) ANOVA with means compared by the Fisher LSD test. For total phenolics (TP) and antioxidant capacity (ORAC) analyses, samples were analyzed in triplicate, where total phenolics were quantified from a gallic acid standard curve. The effects of salt as a main plot, cultivar as a subplot, and the interaction between salt and cultivar (salt × cultivar) for ORAC and TP concentrations were analyzed at p ≤ 0.05 using the GLM procedure with a standard split-plot test format in SAS (version 9.3; SAS Institute, Cary, NC, USA). The differences in ORAC and TP between the two harvests were analyzed at p ≤ 0.05 using the T-test procedure in SAS (version 9.3; SAS Institute, Cary, NC, USA).

3. Results

3.1. Forage Quality

The impact of salinity on forage quality, expressed as the mean of the four cultivars at each salinity level per harvest, is presented in Figure 1. The parameters used to evaluate forage quality include acid detergent fiber (ADF), neutral detergent fiber (NDF), net energy for lactation (NEL), crude protein (CP), and relative feed value (RFV).
Figure 1. Impact of salinity increase on acid detergent fiber (ADF), neutral detergent fiber (NFD), net energy of lactation (NEL), crude protein (CP), and relative feed value (RFV) of salt-tolerant alfalfa. Data points represent the means (±SD) of the salinity-tolerant cultivars (n = 8). Means with the same letter are not significantly different according to a Fisher LSD test (p ≤ 0.05). For the harvest at 84 DAS, the lack of data at 24 dS·m−1 was due to there being insufficient plant material for analysis because of growth limitations.
Figure 1. Impact of salinity increase on acid detergent fiber (ADF), neutral detergent fiber (NFD), net energy of lactation (NEL), crude protein (CP), and relative feed value (RFV) of salt-tolerant alfalfa. Data points represent the means (±SD) of the salinity-tolerant cultivars (n = 8). Means with the same letter are not significantly different according to a Fisher LSD test (p ≤ 0.05). For the harvest at 84 DAS, the lack of data at 24 dS·m−1 was due to there being insufficient plant material for analysis because of growth limitations.
Agriculture 05 00577 g001
Salinity had a significant effect on the forage quality for both harvests (p ≤ 0.001). At 84 DAS, there were no differences up to EC = 7.2 dS·m−1 for all parameters evaluated. Above that level, ADF and NDF decreased by approximately 8% and 9%, respectively, from 12.7 to 18.4 dS·m−1. Consequently, the RFV (related to the ADF and NDF contents) increased sharply between those levels. CP increased by 5.2% from 7.2 to 18.4 dS·m−1 (Figure 1). In addition, the mean NEL increased as salinity increased. At 299 DAS, salinity also affected all forage parameters (p ≤ 0.05). In contrast to 84 DAS, at 299 DAS significant differences between the control and salinity treatments generally were first observed at 12.7 dS·m−1 instead of at 7.2 dS·m−1 (Figure 1).

3.2. Nutrient Composition of Alfalfa

3.2.1. Macronutrients

The macronutrient (modified from [19]) data, including N and P, are expressed on a dry matter (DM) basis (Table 2). The main macronutrients found in alfalfa shoots (g·kg−1 DM) at both harvests were N, K, and Ca, while total S, Mg, and P were present at much lower levels (Table 2). Salinity had a significant effect on all macronutrients for both harvests, except for total S at 299 DAS. Nitrogen increased with salinity for both harvests, reaching levels that were significantly higher than those of the control at and above 12.7 dS·m−1 (84 DAS), and at and above 18.4 dS·m−1 (299 DAS). Shoot K decreased significantly (P ≤ 0.01) for all cultivars and harvests as salinity increased. The calcium content remained constant up to 7.2 dS·m−1 (84 DAS) or up to 12 dS·m−1 (299 DAS), but decreased significantly for both harvests (more drastically at 299 DAS) as salinity increased. The Mg levels significantly increased for both harvests, with salinity, from the control to the highest level of salinity (84% and 48% increases for 84 DAS and 299 DAS, respectively). Sulfur concentrations increased with salinity, being significant (p ≤ 0.01) at 84 DAS, but not at 299 DAS. Concentrations of P remained constant up to 12.7 dS·m−1, but increased significantly (p ≤ 0.01) above that salinity level for both harvests (Table 2). There was a significant (p ≤ 0.01) cultivar effect for all macronutrients (except for N) at 84 DAS, while at 299 DAS, there was a significant cultivar effect only for Ca and Mg (both at p ≤ 0.05). Both Na and Cl increased significantly (p ≤ 0.01) in shoots with increasing salinity, but these and detailed data by cultivar and salinity are presented in a companion paper [19].
Table 2. Average macronutrients (±SE) in alfalfa shoot dry matter (DM) according to salinity levels. EC, electrical conductivity of irrigation water in deciSiemens per meter. ND, not determined (insufficient biomass). Modified from [19].
Table 2. Average macronutrients (±SE) in alfalfa shoot dry matter (DM) according to salinity levels. EC, electrical conductivity of irrigation water in deciSiemens per meter. ND, not determined (insufficient biomass). Modified from [19].
NPKCaMgTotal S
DM (g·kg−1)
EC dS·m−1 Second Harvest (84 DAS)
3.140.8 c ± 1.432.6 b ± 0.0946.4 a ± 1.0514.1 a ± 0.42.6 c ± 0.143.5 d ± 0.08
7.242.1 c ± 1.042.7 b ± 0.0941.4 b ± 0.9413.5 a ± 0.52.7 c ± 0.163.9 c ± 0.10
12.746.0 b ± 0.562.9 b ± 0.0838.6 c ± 0.6213.0 c ± 0.693.4 b ± 0.224.8 b ± 0.20
18.450.5 a ± 0.803.8 a ± 0.1334.3 d ± 0.8812.1 b ± 0.244.8 a ± 0.077.4 a ± 0.17
24NDNDNDNDNDND
Seventh Harvest (299 DAS)
3.134.1 d ± 1.073.4 b ± 0.1740.3 a ± 1.1218.0 a ± 0.512.5 c ± 0.083.8 a ± 0.12
7.237.6 bc ±1.373.1 b ± 0.0630.4 bc ± 0.7418.3 a ± 0.612.8 bc ± 0.124.6 a ± 0.20
12.730.8 d ± 1.772.8 b ± 0.1431.0 b ± 0.6816.7 a ± 0.513.2 ab ± 0.124.8 a ± 0.15
18.445.3 a ± 2.114.1 a ± 0.1227.3 cd ± 0.5612.1 b ± 0.453.0 bc ± 0.104.8 a ± 0.15
2440.8 a ±1.924.3 a ±0.1626.7 d ± 0.6111.0 b ± 0.833.6 a ± 0.205.3 a ± 0.39
Different small letters within each column, and between EC levels, represent significantly different means according to Fisher’s LSD test (p ≤ 0.05), where n = 16 (except for N, n = 8) for EC levels.

3.2.2. Micronutrients

Shoot micronutrients analyzed for the four alfalfa cultivars were iron (Fe), copper (Cu), manganese (Mn), zinc (Zn), and molybdenum (Mo) (Table 3). At 84 DAS, there were no differences in mean Fe concentrations (ranging from 99.1 to 109.6 mg·kg−1 DM) or Cu (2.07–3.11 mg·kg−1 DM) as a function of increasing salinity (EC). Mean concentrations of Mn and Mo tended to increase with increasing salinity with significant (p ≤ 0.05 and p ≤ 0.01, respectively) differences between the control and the highest salinity level (18.4 dS·m−1) at 84 DAS. There was a significant (p ≤ 0.01) increase in Zn concentration at each level of salinity increase at 84 DAS. At 299 DAS, the Fe, Cu, Mn, and Zn levels remained mostly unchanged, but there was a small but significant (p ≤ 0.05) decline (16%–28%) in the Fe levels between the 3.1 dS·m−1 control (116 mg·kg−1 DM) and the other saline treatments. Mn showed a transient increase of 42% (17.3 to 24.6 mg·kg−1 DM) as salinity increased from 3.1 to 7.2 dS·m−1, and then declined to the salinity control levels. In general, the shoot Mo concentrations for all levels of salinity were significantly (p ≤ 0.05) higher than those of the control (Table 3).
Table 3. Average micronutrient concentrations (±SE) in alfalfa shoot dry matter (DM), according to salinity levels. EC, electrical conductivity of irrigation water in deciSiemens per meter. ND, not determined (insufficient biomass).
Table 3. Average micronutrient concentrations (±SE) in alfalfa shoot dry matter (DM), according to salinity levels. EC, electrical conductivity of irrigation water in deciSiemens per meter. ND, not determined (insufficient biomass).
FeCuMnZnMo
DM (mg·kg−1)
EC dS·m−1 Second Harvest (84 DAS)
3.1104.0 a ± 6.292.1 a ± 0.2725.5 b ± 3.3840.9 d ± 1.322.0 c ± 0.09
7.299.1 a ± 4.902.3 a ± 0.1031.7 ab ± 4.845.9 c ± 1.003.1 b ± 0.11
12.7106.5 a ± 5.893.1 a ± 0.1634.8 a ± 4.1054.9 b ± 1.113.2 b ± 0.14
18.4109.6 a ± 5.03.1 a ± 0.1934.8 a ± 1.1060.5 a ± 1.254.1 a ± 0.11
24NDNDNDNDND
Seventh Harvest (299 DAS)
3.1116.1 a ± 6.355.8 a ±0.8317.2 b ± 0.9197.6 a ± 3.362.7c ± 0.19
7.297.7 b ± 7.356.1 a ± 0.6424.6 a ± 1.4489.9 a ± 3.266.4 a ± 0.43
12.789.9 b ± 7.356.5 a ± 0.4118.9 b ± 0.99105.6 a ± 3.186.3 a ± 0.44
18.483.5 b ± 3.175.3 a ± 0.2617.4 b ± 1.05101.3 a ± 3.264.7 c ± 0.36
2492.3 b ± 7.695.7 a ± 0.4914.8 b ± 1.0498.3 a ± 3.854.2 c ± 0.21
Different lower case letters within each column, and between EC levels, represent significantly different means according to Fisher’s LSD test (p ≤ 0.05), where n = 16.

3.3. Antioxidant Capacity of Alfalfa

Salinity had no effect (p > 0.05) on either the oxygen radical absorbance capacity (ORAC) or the total phenolic levels of the four alfalfa cultivars. The hydrophilic fractions of shoots had most (68%–99%) of the shoot total antioxidant capacity (Table 4). At early plant development (84 DAS), alfalfa shoots had hydrophilic ORAC (ORACHydro) levels that ranged from 190–230 μmoles·TE·g−1 DM (Figure 2), while at 299 DAS, ORACHydro ranged from 229–274 μmoles·TE·g−1 DM, and the shoot total antioxidant capacity ranged from 244–287 μmoles·TE·g−1 DM (Figure 2, Table 4). Total phenolic (TP) concentrations ranged from 5.0–5.6 mg·GAE·g−1 DM for both harvests (Figure 2).
Table 4. Oxygen radical absorbance capacity of the lipophilic (ORACLipo) and hydrophilic (ORACHydro) fractions, and total antioxidant capacity (ORACHydro + ORACLipo), in micromoles of trolox equivalents per gram of dry matter (µmoles·TE·g−1 DM) of alfalfa irrigated with water of different electrical conductivities (EC). Plants were sampled on 17 April 2012 (299 DAS). Data are means ± SE combined for the four cultivars with two replicated analyses per sample (n = 8).
Table 4. Oxygen radical absorbance capacity of the lipophilic (ORACLipo) and hydrophilic (ORACHydro) fractions, and total antioxidant capacity (ORACHydro + ORACLipo), in micromoles of trolox equivalents per gram of dry matter (µmoles·TE·g−1 DM) of alfalfa irrigated with water of different electrical conductivities (EC). Plants were sampled on 17 April 2012 (299 DAS). Data are means ± SE combined for the four cultivars with two replicated analyses per sample (n = 8).
ECORACLipoORACHydroORACTotal
(dS·m−1)(μmoles·TE·g−1 DM)
3.115.0 ± 2.4239.5 ± 12.8254.5 ± 13.6
7.211.2 ± 1.5252.1 ± 11.6263.3 ± 11.0
12.713.4 ± 2.5273.6 ± 14.3286.9 ± 14.2
18.416.4 ± 1.7268.4 ± 14.0284.8 ± 15.5
24.015.3 ± 1.0228.8 ± 18.3244.1 ± 18.2
There was no effect of salinity (expressed as EC), cultivar, or the salt × cultivar interaction.
Figure 2. Total phenolics (TP) and hydrophilic shoot oxygen radical absorbance capacity (ORAC) of four salinity-tolerant alfalfa cultivars irrigated with saline water with different electrical conductivity levels. ORAC was measured in micromoles of trolox equivalents per gram of dry matter (μmoles·TE·g−1 DM). TP was measured as mg of gallic acid equivalents per gram of dry matter (mg·GAE·g−1 DM). Bars represent means (±SD), where n = 4. Plants were sampled at 84 and 299 days after sowing. For the harvest at 84 DAS, the lack of data at 24 dS·m−1 was due to growth limitations.
Figure 2. Total phenolics (TP) and hydrophilic shoot oxygen radical absorbance capacity (ORAC) of four salinity-tolerant alfalfa cultivars irrigated with saline water with different electrical conductivity levels. ORAC was measured in micromoles of trolox equivalents per gram of dry matter (μmoles·TE·g−1 DM). TP was measured as mg of gallic acid equivalents per gram of dry matter (mg·GAE·g−1 DM). Bars represent means (±SD), where n = 4. Plants were sampled at 84 and 299 days after sowing. For the harvest at 84 DAS, the lack of data at 24 dS·m−1 was due to growth limitations.
Agriculture 05 00577 g002

4. Discussion

4.1. Forage Quality

Forage quality was based on laboratory analyses of shoot biomass and evaluated in relation to recommended forage standards for livestock production output (e.g., milk, body weight gain) for animals consuming alfalfa of similar nutritional value and energy content [3,29]. Lower NDF translates into both increased DMI and milk yield within a forage family [3]. Regarding alfalfa protein, approximately 80% is degraded in the rumen of polygastric animals, but addition of tannins to alfalfa feed decreases rumen protein degradability and increases protein absorption [30].
Plant maturity is the main factor affecting forage quality [31], but the interaction between environmental and agronomic factors with maturity will influence the quality of alfalfa, even if harvested at the same stage of development [32]. Similarly, approaching harvest time, any stress that delays or accelerates alfalfa maturation affects the leaf-to-stem ratio and consequently, forage quality. The stems contain mostly structural components and are low in N, while the leaves contain mainly photosynthetic components and are richer in N than the stems. As a result, leaves have two to three times more CP than stems [33]. Increased leaf N leads to increased leaf area, thus increasing the leaf/stem ratio [34,35], but this could also be accounted for by the reduced stem height caused by salinity. The leaf-to-stem ratio increase leads to decreases in both ADF and NDF. Decreased ADF and NDF and increased shoot N lead to higher shoot CP levels in alfalfa irrigated with saline water. As reported in a previous study [19], plant height was significantly reduced by salinity only at 84 DAS, with the average difference in plant height between the control and EC = 18.4 dS·m−1 being 23 cm. Thus, we hypothesize that the decrease in height (shorter internodes) in salt-affected plants may have increased the leaf-to-stem ratio, shoot N, and CP by 61 g·kg−1 DM (6%). This decreased height of salt-affected plants also led to decreases in ADF and NDF of 107 and 122 g·kg−1 DM (10.7% and 12.2%) at 84 DAS and of 2.5% and 4% at 299 DAS, respectively, improving forage potential quality (Figure 1). This is in agreement with a previous report that salinity increased alfalfa leaf-to-stem ratio, slightly improving forage quality [36].
Al-Khatib and collaborators [7] reported that the leaf-to-stem ratio of alfalfa increased while forage mass decreased in response to increasing NaCl until 20 dS·m−1 (200 mM NaCl). At 299 DAS, there was also a significant increase in CP of 42.1 g·kg−1 DM (4.2%) between the control plants and those under 24 dS·m−1 (reflecting the increased accumulation of leaf N with increased salinity). This increase in CP was observed at both 84 and 299 DAS because N accumulation in shoots increased by 23% and 33%, respectively, in response to increased salinity (Table 2, Figure 1). Although plants had a fairly constant supply of N from NO 3 in all irrigation treatments (Table 1), shoots significantly accumulated NO 3 -N, leading to higher CP. This could be due to morphological changes (e.g., increased leaf-to-stem ratio) under salinity stress or because the roots in the sand tanks were found to be associated with rhizobia. Despite the differences in developmental stages between the second and seventh harvest, there was a tendency for CP to increase with salinity levels up to 18.4 dS·m−1. Although plants irrigated with salinity levels higher than the control had different stages of maturity, plant height has been used to predict forage parameters under field conditions [33,37].
Differences in forage parameters changed more sharply at 84 DAS (late summer) with salinity than at 299 DAS (early spring). These changes were likely caused by differences in climatic conditions combined with salinity [19]. Both climate and intervals between harvests (24 days before the second and 54 days before the seventh harvest) have a direct impact on maturity [33,38]. The RFV of alfalfa shoots in this experiment were similar to the values reported for alfalfa cultivars grown under field conditions with EC values ranging from 4–16 dS·m−1, although RFV did not change with salinity [39].
According to the classification of alfalfa hay [40], and judging from the parameters evaluated in this study, alfalfa herbage grown at the highest tolerated salinity fell within the “supreme” category. In comparison, forage grown at control salinity levels would be classified as “good” and “premium”. Hence, our results indicated that forage quality improved with increasing salinity (despite some variation), independently of the changes between harvest seasons. Similar increases in CP and decreases in ADF in the salinity-tolerant cultivars Salado and SW9720 under salinity stress have been reported [9,11]. An increase in CP of alfalfa cultivars less tolerant to salinity was also reported when salinity increased from 2.1 to 7.8 dS·m−1 [41] or when salinity ranged from 0.3–4.5 dS·m−1 in one out of three years of cultivation [42]. Both drought and salinity restrict the growth of alfalfa, and mild drought also improves the forage quality of alfalfa [43]. These authors explained that the increase in quality with drought was due to a delay in plant maturation and an increase in the leaf-to-stem ratio; the latter is related to a reduction in stem length. However, the results of a 90-day pot experiment indicated that there were no differences in CP or N concentrations in alfalfa shoots when an EC of 15 dS·m−1 was applied using only NaCl [44].
The NEL values of alfalfa irrigated with increasing salinity, and ranging from 1.38–1.58 Mcal·kg−1 for the second harvest (84 DAS) and from 1.3 to 1.37 Mcal·kg−1 for the seventh harvest (299 DAS), were within the average (1.47 Mcal·kg−1) required for lactating cows [29], although some supplementation may be required to maintain the required energy levels.

4.2. Mineral Nutrient Composition

When irrigated with non-saline water, the predominant macronutrients in alfalfa are N, K, Ca, Mg, P, and S [45]. In our plants, which were fertilized to achieve the desired macro and micronutrients concentrations for ideal crop growth, and irrigated with saline water, the three main shoot macronutrients were also N, K, and Ca, followed by Cl and Na (data presented in [19]) and S, as these were added to the irrigation water to achieve high salinity, then followed by Mg and P at similar concentrations (Table 2). This suggests that alfalfa plants were provided adequate nutrients for growth, and our results express mostly the effects of salinity in a properly fertilized crop. The discussion on macro- and micronutrient requirements is based on the specifications for lactating dairy cattle provided by the Nutrient Requirements of Dairy Cattle [29]. The NRC requirement level for animals producing 35 kg milk·day−1 (Holstein or Jersey) was used, based on the average milk production for 2012 in California [46].
Macronutrients and sodium—Although adequate mineral nutrition alone will not prevent animal diseases, susceptibility to infectious diseases in response to malnourishment has been recognized for several centuries [47]. Thus, it is important to know if crop stress induced by salinity alters the nutrient composition of alfalfa.
The lowest Ca concentration in shoots in response to salinity (11 g·kg−1) was still above the daily dietary requirement (6.1 g·kg−1) for dairy cattle [29], while the highest Ca concentrations (18 g·kg−1) were observed at ECs of 3.1 and 7.2 dS·m−1 at 299 DAS (Table 2). While dietary Ca concentrations above 10 g·kg−1 have been associated with reduced dry matter intake (Miller, 1983, in [29]), diets as high as 18 g·kg−1 have been fed to non-lactating dairy cows without problems (Beede et al., 1991, in [29]). Feeding Ca in excess of daily dietary requirements is suggested to improve performance, mainly when cows are fed corn silage diets [29]. Potassium is the third most abundant element in mammals and is important for cellular osmotic balance. The cellular homeostasis of Na and K is maintained by Na+/K+ pumps located inside the cell membrane. These two cations play an important role in electrical activity of nerve and muscle cells, in the acid-base balance, and in water retention. Potassium is a cofactor for the activation of enzymes, including those involved in protein synthesis and carbohydrate metabolism [48]. Because of increasing levels of Cl in irrigation water, shoot absorption of potassium decreased significantly (p ≤ 0.01) for both harvests (by 26%–33%). Sodium significantly increased (by 60%), both with salinity and harvest date (presented elsewhere [19]), which was expected due to its elevated concentration in the saline treatment water. The levels of K across harvests and salinity (2.6%–4.6%) were well above the required levels (1.04%) for average lactating cows [29]. However, diets supplemented with potassium carbonate increased K from 1.6% to 4.6% (w/w) and decreased milk yield and feed intake [49]. Thus, K levels in alfalfa shoots irrigated with saline water containing 6 to 6.5 mmolc·L−1 could be of concern, depending on forage intake.
A continuous supply of Mg from feed is desirable because a high K level in forage decreases Mg absorption from the rumen and can lead to tetany [50]. The frequency of tetany in cows, triggered by low Mg and/or Ca, and high K in forage, increases when the ratio of K: (Ca + Mg) exceeds 2.2 [51]. In our results, the ratio of K: (Ca + Mg) was higher than 2.2 at 84 DAS, but lower than 2.2 at 299 DAS, suggesting that Mg levels should be monitored in alfalfa irrigated with saline water. Thus, although our results indicate that salinity can lead to a small, but significant accumulation of Mg by alfalfa shoots, Mg supplementation is still a must due to its poor absorption (13% to 16% from ration) by cows [52].
Sulfur (S) is an important component of cysteine and methionine, of many enzymes, and of antioxidants such as glutathione and thioredoxin, but elevated concentrations of S in alfalfa shoots can be detrimental to animal feed intake and function. Although we discuss the concentrations of S in shoots of different ages, the saline water used here was sulfate-dominant to mimic the drainage waters of California’s Central Valley. Thus, levels of S might not be of concern where waters are Cl dominant. However, the S levels in our experiment remained similar at 299 DAS across salinity treatments. The lack of significant S uptake at 299 DAS may be explained by cooler temperatures and lower evapotranspiration before that harvest. The S concentration in shoots ranged from 0.38%, at the lowest EC, to 0.54% at the highest EC observed at 299 DAS. Regardless of season, a decrease in S in a later harvest (as seen here) was reported previously for alfalfa irrigated with sulfate-dominant water at both 15 and 25 dS·m−1 [53]. The authors reported an S range in alfalfa of 0.5%–0.9% at 25 dS·m−1. In the S range recorded at 299 DAS for this study, and considering that the average consumption of alfalfa is 4.26 kg·cow−1 [3], the S consumption would be 16.2 to 23.0 g·day−1, well below the 32 g S·day−1 upper limit recommended for a mature grazing beef cow [54], but 1.9 to 2.7 times above the 8.52 g S·day−1 (0.2% S/day) required for dairy cows [29]. Although no S toxicity has been reported [29], it is important to balance the diet in order to maintain S intake at a safe level (below 0.4% of DM daily), as levels of S of 0.4% in bailed alfalfa can lead to molybdenosis and reduced uptake of Cu and Se in beef cattle if alfalfa is the only source of feed [45].
The P requirement in the daily diet of average-producing dairy cows is 0.35% [29], but P levels regarded as adequate in alfalfa shoots are 0.08% to 0.15% [45]. P deficiency will lead to osteomalacia (softening of the bones) and fragile bones. The average levels of P in our alfalfa shoots at 299 DAS (0.28% to 0.44% DW) are considered to be high for shoot levels, relative to alfalfa grown in soils of the Mediterranean and desert zones [45]. In addition, according to nutrient tables presented by these authors, our Mg levels (0.25%–0.37%) were adequate, while shoot K and S were high.
Salinity significantly increased Na and Cl levels for both harvest dates by 40%–60%, as presented in a companion paper [19], resulting in shoot Na levels two to five times higher than the level required (0.23%) for average-producing lactating dairy cows [29]. Our data showed that alfalfa accumulates more Na and Cl over time, even at the same irrigation salinity level. As previously reported [19], shoot Na ranged from 3.5–10 g·kg−1, and Cl from 7–14 g·kg−1, across salinity levels and harvest times. We found no reference reporting Na toxicity to livestock, but increasing Na in the diet from 5.5–8.8 g·kg−1 caused no reduction of feed intake, milk yield, or toxicity (Schneider et al. 1986, in [29]). NaCl, often added to feed mixes, can be tolerated up to 3% (lactating cows) or 4.5% (growing animals) of dietary dry matter. Thus, Na and Cl levels in alfalfa irrigated with saline water present no safety concern.
Micronutrients—Micronutrients and some vitamins are essential for animals to achieve optimal immune function, growth, and reproduction. Cattle can have sufficient amounts of these minerals for growth and reproduction, but not have enough for optimal immune function [47]. Examples are Cu and Zn, which are required for the activity of the antioxidant enzymes Cu-Zn superoxide dismutase (SOD) [55].
The average iron concentration was not affected by salinity and ranged from 83.5–116 mg·kg−1 across harvests, regardless of salinity treatment. Concentrations of 50 to 100 mg·kg−1 of Fe in a basal ration are within the requirements for the growth of grazing cattle [47,56] and concentrations of 15 mg·kg−1 in daily feed are recommended for average lactating cows [29]. Iron is essential for the formation of new red blood cells and only levels ≥4000 mg·kg−1 affect weight gain and cause diarrhea in young calves [47].
Copper (Cu) and zinc (Zn) are important micronutrients for immune function, and levels of 20 mg·kg−1 Cu and 40–60 mg·kg−1 Zn were suggested as optimal for feeding in the total diet of dairy cattle [57], while levels of 11 mg·kg−1 Cu and 48 mg·kg−1 Zn are recommended for average lactating dairy cows [29]. The Cu levels found in shoots for both harvests were below 7.0 mg·kg−1, indicating the need for supplementation. In addition, the ratio of Cu to Mo in shoots was always approximately 1:1, well below the ratio of 10:1 that is considered a threshold for potential Cu toxicity [58].
Salinity significantly increased the Zn concentration in young plants (84 DAS) but not in established alfalfa plants (299 DAS), with concentrations ranging from 90–106 mg·kg−1. Considering that a minimum Zn concentration of 48 mg·kg−1 is required for average lactating cows [29], our plants contained levels more than adequate to support a healthy immune function in livestock [57]. Manganese levels in alfalfa shoots were the third highest, after Fe and Zn. Manganese is important for its role in enzymatic systems but it is poorly absorbed (14%–18%) and if deficient, can reduce fertility and delay estrous [56]. This author mentions that Mn deficiency can lead to abortion and deformed calves at birth, but elevated Mn in the diet is generally not toxic. Levels of Mn in our alfalfa cultivars were at least 14 mg·kg−1, as recommended for average lactating cows (NRC 2001). However, considering the poor absorption of Mn, mineral supplementation would be recommended.

4.3. Antioxidant Capacity of Alfalfa

Antioxidant flavonoids in the diet are believed to have health-promoting benefits to both humans and animals. In addition to protein, alfalfa is a rich source of flavonoid antioxidants and phytoestrogens including luteolin, coumestrol, and apigenin [59]. Phenolic compounds (including flavonoids) protect plants against the damaging effects of excessive reactive oxygen species (ROS) triggered by abiotic stresses, including salinity [60,61]. Although oxygen radical absorbance capacity (ORAC) has been widely accepted by industry to gauge the total antioxidant capacity of fruits, vegetables, spices, and other items consumed by humans, ORAC has only recently been used to estimate the antioxidant capacity of plants destined for livestock consumption [62,63,64]. The total antioxidant capacity is the sum of the lipophilic (ORACLipo) and hydrophilic (ORACHydro) fractions extracted from plants by hexane (lipophilic) and 70:30 acetone:aqueous buffer (hydrophilic). Our ORAC data (Table 4) confirmed those of others [63,64] who reported that the hydrophilic fractions of plant extracts contain most (68%–99%) of the total antioxidant capacity of shoots. Alfalfa shoots grown with saline water had 94%–96% of the total antioxidant capacity in the hydrophilic fraction with only 4%–6% in the lipophilic fraction, indicating that alfalfa shoots are low in lipophilic antioxidants such as tocopherols, carotenes, and fatty acids. The oven-dried alfalfa plants in our study had ORACHydro values that ranged from 229–274 μmoles·TE·g−1 DM (Table 4, Figure 2). Although these values may seem small compared with those of other leguminous forages, such as Lespedeza cuneata (ORACHydro = 530 μmoles·TE·g−1 DM), previously reported [63] alfalfa flavonoids and isoflavonoids present in hydrophilic (aqueous) extracts reduced oxidative stress and exerted hepatoprotective activity in rats treated with the liver-damaging compound carbon tetrachloride [65]. These results indicate that when animals consume alfalfa on a regular basis, it can provide benefits other than nutritional value.
The values for both ORAC and total phenolics (TP) remained unaltered by increased salinity, without differences for either ORAC or TP among cultivars (Figure 2). Our results agree with a previous report where there were no differences in antioxidant compounds among different cultivars of alfalfa in the absence of salt stress [15]. These authors also reported that the major antioxidants in alfalfa shoots, determined by HPLC, were tricin and apigenin glycosides (each approximately 40% of the total HPLC peaks), and luteolin and chrysoeriol glycosides (10% or less of the total HPLC peaks). Our results suggest that the salinity levels tested did not highly stress these salt-tolerant alfalfa cultivars. Previously, mostly the aglycons (flavonoids stripped of sugar moieties by acidic or enzymatic hydrolysis) have been determined, but the determination of full glycosidic forms (flavonoid plus sugar moieties) has also been conducted [59]. Flavonoids from alfalfa have the typical structure of several other flavonoids reported as beneficial to human diets and found in fruits and vegetables. Although sun drying (used to produce alfalfa hay) drastically decreased the antioxidant capacity of the antioxidant herb Artemisia annua, oven drying at 45 °C only slightly reduced the antioxidant capacity compared with freeze drying [66]. Thus, we consider that our oven-dried alfalfa shoots had an antioxidant capacity close to that of freeze-dried (or fresh) shoots. We could not find any published work on the antioxidant capacity of alfalfa shoots determined by ORAC or TP, except that the total ORAC (ORACHydro+Lipo) of alfalfa hay was 171 µmoles·TE·g−1, and the ORACLipo was only 3% of the total ORAC [63]. The antioxidant capacity of all cultivars used here was not affected by salinity, thus expanding the value of alfalfa beyond its contents of CP and minerals.
Although the value of antioxidants in animal and human nutrition is still debated by some, several benefits (e.g., anti-cancer, anti-inflammatory, etc.) of antioxidant-rich diets have been proposed. Dairy cows supplemented daily with 500 g of oregano (2082 μmoles·TE·g−1 DM) increased their milk fat concentration, feed and milk NEL efficiencies, and fat-corrected milk yield by 3.5% [67]. Although oregano has an ORAC value 8–9 fold higher than our oven-dried alfalfa shoots (225 to 256 μmoles·TE·g−1), the average consumption of alfalfa shoots by cows is 5.4 kg·day−1, which is 10-fold higher than the 500 g·day−1 oregano supplement from the above-mentioned study. Thus, daily alfalfa consumption can provide as much antioxidant flavonoid intake as oregano, thus adding to the forage value of alfalfa.

5. Conclusions

The effect of salinity in irrigation water on the suitability of alfalfa as a forage was based on shoot levels of macro- and micronutrients, and the forage quality estimated from ADF, NDF, and CP. Additional forage value was based on the antioxidant capacity and total phenolics in response to salinity. The nutrient composition of alfalfa can vary with salinity. Although our saline irrigation waters provided 27%–87% more SO4 than Cl and 60%–94% more Na than Cl, alfalfa shoots contained 20%–190% more Cl than total S and 20%–120% more Cl than Na. Although Na and Cl in shoots increased with salinity, reducing the K concentration by 26%–32% and Ca by 15%–32% in shoots, shoot K and Ca were considered high and adequate [1,45], respectively, at all salinity levels. Increased salinity also increased shoot N (23%–33%), P (21%–46%), Mg (20%–84%), and total S (100%–110%) for both harvests. In general, the levels of macro- and micronutrients were adequate or high for alfalfa forage [1,29,45] regardless of salinity. However, when irrigation water was sulfate-dominant, the S concentrations in alfalfa were close to the upper limits recommended for safe animal consumption and require monitoring for water EC higher than 12.7 dS·m−1. Regarding forage potential quality, shoots from plants irrigated with salinity levels higher than the control remained unaltered, or slightly improved compared with the salinity control levels, with NDF and CP at levels recommended for various classes of milking cows, but below the NDF values required for bulls and dry cows [39]. The antioxidant capacity was 15–23 fold higher for hydrophilic than for lipophilic fractions, but remained mostly unaltered by salinity, indicating that total antioxidant compounds, including phenolics and flavonoids (postulated to neutralize reactive oxygen species triggered by salinity stress), may remain fairly constant in alfalfa cultivars that are tolerant to salinity. These constant antioxidant levels, regardless of salinity stress, may play an extra beneficial role in helping to maintain animal health, as accepted for antioxidants in humans. Except for numeric values (such as reduced K and increased S), salinity levels up to 24 dS·m−1 did not alter the potential nutritional value and antioxidant capacity of alfalfa for livestock. The nutrient composition and antioxidant capacity of alfalfa are expected to play a dual role in the maintenance of health, body index, and milk production in dairy cows. This is the first report we are aware of, which has determined the total antioxidant capacity of alfalfa in response to salinity. Further studies involving animal performance are required to confirm the potential feed value of salt-stressed alfalfa under field conditions.

Acknowledgments

We acknowledge Nedda Saremi for help with the macro- and micronutrient analyses and Nahid Vishteh for determining the chemical composition of the saline water used in this study.

Author Contributions

Jorge Ferreira was responsible for the antioxidant method (ORAC), the data interpretation and discussion of forage nutritional value and antioxidant capacity, and the writing of the manuscript with Monica Cornacchione and Donald Suarez. Monica Cornacchione conducted the experiments, analyzed the data, and helped write the manuscript. Xuan Liu performed the tests for antioxidant activity (ORAC) and total phenolics (TP) and helped write the experimental section. Donald Suarez developed the experimental design, including the composition of the saline water, and assisted with the writing of the manuscript.

Conflicts of Interest

The authors declare no conflict of interest. The mention of proprietary brands and names is solely for the convenience of the reader and does not imply endorsement by the authors or the USDA versus similar products. The USDA is an equal-opportunity employer.

Abbreviations

ADF
acid detergent fiber
NDF
neutral detergent fiber
NEL
net energy for lactation
CP
crude protein
RFV
relative feed value
ORAC
oxygen radical absorbance capacity
TP
total phenolics

References

  1. Radović, J.; Sokolović, D.; Marković, J. Alfalfa—Most important perenial forage legume in animal husbandry. Biotechnol. Anim. Husb. 2009, 25, 465–475. [Google Scholar] [CrossRef]
  2. USDA-ARS. Roadmap for Alfalfa Research. Available online: http://ars.usda.gov/SP2UserFiles/Place/54281000/alfalfaroadmap2.pdf (accessed on 11 March 2014).
  3. DePeters, E. Forage Quality: Important Attributes & Changes on the Horizon. In the Proceedings of California Alfalfa and Grains Symposium, Sacramento, CA, USA, 10–12 December 2012; UC Cooperative Extension, Plant Sciences Department, University of California, Davis: Davis, CA, USA, 2012. [Google Scholar]
  4. Khorasani, G.R.; Janzen, R.A.; McGill, W.B.; Kennelly, J.J. Site and extent of mineral absorption in lactating cows fed whole-crop cereal grain silage of alfalfa silage. J. Anim.Sci. 1997, 75, 239–248. [Google Scholar] [PubMed]
  5. Smedema, L.K.; Shiati, K. Irrigation and salinity: A perspective review of the salinity hazards of irrigation development in the arid zone. Irrig. Drain. Syst. 2002, 16, 161–174. [Google Scholar] [CrossRef]
  6. Ashraf, M.; Harris, P.J.C. Potential biochemical indicators of salinity tolerance in plants. Plant Sci. 2004, 166, 3–16. [Google Scholar] [CrossRef]
  7. Al-Khatib, M.; McNeilly, T.; Collins, J.C. The potential of selection and breeding for improved salt tolerance in lucerne (Medicago sativa L.). Euphytica 1992, 65, 43–51. [Google Scholar] [CrossRef]
  8. Mass, E.V.; Grattan, S.R. Crop yields as affected by salinity. In Agricultural Drainage; Agron. Monograph 38; Skaggs, R.W., van Schilfgaarde, J., Eds.; ASA, CSSA, SSA: Madison, WI, USA, 1999; pp. 55–108. [Google Scholar]
  9. Robinson, P.H.; Grattan, S.R.; Getachew, G.; Grieve, C.M.; Poss, J.A.; Suarez, D.L.; Benes, S.E. Biomass accumulation and potential nutritive value of some forages irrigated with saline-sodic drainage water. Anim. Feed Sci. Technol. 2004, 111, 175–189. [Google Scholar] [CrossRef]
  10. Grattan, S.R.; Grieve, C.M.; Poss, J.A.; Robinson, P.H.; Suarez, D.L.; Benes, S.E. Evaluation of salt-tolerant forages for sequential water reuse systems: I. Biomass production. Agric. Water Manag. 2004, 70, 109–120. [Google Scholar] [CrossRef]
  11. Suyama, H.; Benes, S.E.; Robinson, P.H.; Grattan, S.R.; Grieve, C.M.; Getachew, G. Forage yield and quality under irrigation with saline-sodic drainage water: Greenhouse evaluation. Agric. Water Manage. 2007, 88, 159–172. [Google Scholar] [CrossRef]
  12. Steppuhn, H.; Acharya, S.N.; Iwaasa, A.D.; Gruber, M.; Miller, D.R. Inherent responses to root-zone salinity in nine alfalfa populations. Can. J. Plant Sci. 2012, 92, 235–248. [Google Scholar] [CrossRef]
  13. Rubio, M.C.; Bustos-Sanmamed, P.; Clemente, M.R.; Becana, M. Effects of salt stress on the expression of antioxidant genes and proteins in the model legume Lotus japonicus. New Phytol. 2009, 181, 851–859. [Google Scholar] [CrossRef] [PubMed]
  14. Mhadhbi, H.; Fotopoulos, V.; Mylona, P.V.; Jebara, M.; Elarbi Aouani, M.; Polidoros, A.N. Antioxidant gene–enzyme responses in Medicago truncatula genotypes with different degree of sensitivity to salinity. Physiol. Plant. 2011, 141, 201–214. [Google Scholar] [CrossRef] [PubMed]
  15. Stochmal, A.; Oleszek, W. Seasonal and structural changes in flavones in alfalfa (Medicago sativa) aerial parts. Int. J. Food Agric. Environ. 2007, 5, 170–174. [Google Scholar]
  16. Choi, K.C.; Hwang, J.M.; Bang, S.J.; Kim, B.T.; Kim, D.H.; Chae, M.; Lee, S.A.; Choi, G.J.; Kim, D.H.; Lee, J.C. Chloroform extract of alfalfa (Medicago sativa) inhibits lipopolysaccharide-induced inflammation by downregulating ERK/NF-κB signaling and cytokine production. J. Medic. Food 2013, 16, 410–420. [Google Scholar] [CrossRef] [PubMed]
  17. Bora, K.S.; Sharma, A. Phytochemical and pharmacological potential of Medicago sativa: A review. Pharm. Biol. 2011, 49, 211–220. [Google Scholar] [CrossRef] [PubMed]
  18. Agati, G.; Biricolti, S.; Guidi, L.; Ferrini, F.; Fini, A.; Tattini, M. The biosynthesis of flavonoids is enhanced similarly by UV radiation and root zone salinity in L. vulgare leaves. J. Plant Physiol. 2011, 168, 204–212. [Google Scholar] [CrossRef] [PubMed]
  19. Cornacchione, M.V.; Suarez, D.L. Emergence, forage production, and ion relations of alfalfa in response to saline waters. Crop Sci. 2015, 55, 444–457. [Google Scholar] [CrossRef]
  20. Suarez, D.L.; Simunek, J. Unsatchem: Unsaturated water and solute transport model with equilibrium and kinetic chemistry. Soil Sci. Soc. Am. J. 1997, 61, 1633–1646. [Google Scholar] [CrossRef]
  21. Kalu, B.A.; Fick, G. Quantifying morphological development of alfalfa for studies of herbage quality. Crop Sci. 1981, 21, 267–271. [Google Scholar] [CrossRef]
  22. Prior, R.L.; Hoang, H.; Gu, L.; Wu, X.; Bacchiocca, M.; Howard, L.; Hampsch-Woodill, M.; Huang, D.; Ou, B.; Jacob, R. Assays for hydrophilic and lipophilic antioxidant capacity [oxygen radical absorbance capacity (ORAC)] of plasma and other biological and food samples. J. Agric. Food Chem. 2003, 51, 3273–3279. [Google Scholar] [CrossRef] [PubMed]
  23. Singleton, V.L.; Rossi, J.A. Colorimetry of total phenolics with phosphomolybdic-phosphotungstic acid reagents. Am. J. Enol. Vitic. 1965, 16, 144–158. [Google Scholar]
  24. Slinkard, K.; Singleton, V.L. Total phenol analysis: Automation and comparison with manual methods. Am. J. Enol. Vitic. 1977, 28, 49–55. [Google Scholar]
  25. AOAC. Official Methods of Analysis of AOAC International, 17th ed.; Association of Official Analytical Chemists: Gaithersburg, MD, USA, 2000; p. 2000. [Google Scholar]
  26. National Forage Testing Association. Forage Analysis Procedures. Available online: http://www.foragetesting.org/files/LaboratoryProcedures.pdf (accessed on 27 May 2013).
  27. Atwater, W.O.; Bryant, A.P. The Chemical Composition of American Food Materials; USDA Office of Experiment Stations, Ed.; US Government Printing Office: Washington, DC, USA, 1906; p. 87.
  28. Di Rienzo, J.A.; Casanoves, F.; Balzarini, M.G.; González, L.; Tablada, M.; Robledo, C.W. Infostat. Grupo Infostat; FCA Universidad Nacional de Córdoba, Argentina. Available online: Http://www.Infostat.Com.Ar (accessed on 30 August 2013).
  29. NRC. Nutrient Requirements of Dairy Cattle, 7th ed.; National Academy Press: Washington, DC, USA, 2001. [Google Scholar]
  30. Getachew, G.; Pittroff, W.; DePeters, E.J.; Putnam, D.H.; Dandekar, A.; Goyal, S. Influence of tannic acid application on alfalfa hay: In vitro rumen fermentation, serum metabolites and nitrogen balance in sheep. Animal 2008, 2, 381–390. [Google Scholar] [CrossRef] [PubMed]
  31. Minson, D.J. Forage in Ruminant Nutrition; Academic Press: San Diego, CA, USA, 1990; p. 463. [Google Scholar]
  32. Buxton, D.R. Quality-related characteristics of forages as influenced by plant environment and agronomic factors. Anim. Feed Sci. Technol. 1996, 59, 37–49. [Google Scholar] [CrossRef]
  33. Putnam, D.H.; Robinson, P.; DePeters, E. Forage quality and testing. In Irrigated Alfalfa Management for Mediterranean and Desert Zones; Publication 3512; Summers, C.G., Putnam, D.H., Eds.; University of California/Agricultural and Natural Resources: Davis, CA, USA, 2008; pp. 241–264. [Google Scholar]
  34. Lemaire, G.; Avice, J.C.; Kim, T.H.; Ourry, A. Developmental changes in shoot N dynamics of lucerne (Medicago sativa L.) in relation to leaf growth dynamics as a function of plant density and hierarchical position within the canopy. J. Exp. Bot. 2005, 56, 935–943. [Google Scholar] [CrossRef] [PubMed]
  35. Lemaire, G.; Khaity, M.; Onillon, B.; Allirand, J.M.; Chartier, M.; Gosse, G. Dynamics of accumulation and partitioning of N in leaves, stems and roots of lucerne (Medicago sativa L.) in a dense canopy. Ann. Bot. 1992, 70, 429–435. [Google Scholar]
  36. Hoffman, G.J.; Maas, E.V.; Rawlins, S.L. Salinity-ozone interactive effects on alfalfa yield and water relations. J. Environ. Qual. 1975, 4, 326–331. [Google Scholar] [CrossRef]
  37. Mueller, S.C.; Teuber, L.R. Alfalfa growth and development. In Irrigated Alfalfa Management for Mediterranean and Desert Zones; Publication 3512; Summers, C.G., Putnam, D.H., Eds.; University of California/Agricultural and Natural Resources: Davis, CA, USA, 2008; pp. 31–38. [Google Scholar]
  38. Orloff, S.B.; Putnam, D.H. Harvest strategies for alfalfa. In Irrigated Alfalfa Management for Mediterranean and Desert Zones; Publication 3512; Summers, C.G., Putnam, D.H., Eds.; University of California/Agricultural and Natural Resources: Davis, CA, USA, 2008; pp. 197–207. [Google Scholar]
  39. Yurtseven, S. The nutrient and energy contents of medicago varieties growth in salt-affected soils of the harran plain. Hayvansal Üretim 2011, 52, 39–45. [Google Scholar]
  40. USDA-CO, D.O.A.M.N.S. California hay report. Available online: http://www.ams.usda.gov/mnreports/ml_gr311.txt (accessed on 9 May 2013).
  41. Hussain, G.; Al-Jaloud, A.A.; Ai-Shammary, S.F.; Karimulla, S. Effect of saline irrigation on the biomass yield, and the protein, nitrogen, phosphorus, and potassium composition of alfalfa in a pot experiment. J. Plant Nutr. 1995, 18, 2389–2408. [Google Scholar] [CrossRef]
  42. Isla, R.; Aragüés, R. Response of alfalfa (Medicago sativa L.) to diurnal and nocturnal saline sprinkler irrigations. I: Total dry matter and hay quality. Irrig. Sci. 2009, 27, 497–505. [Google Scholar] [CrossRef] [Green Version]
  43. Halim, R.A.; Buxton, D.R.; Hattendorf, M.J.; Carlson, R.E. Water-stress effects on alfalfa forage quality after adjustment for maturity differences. Agron. J. 1989, 81, 189–194. [Google Scholar] [CrossRef]
  44. Pessarakli, M.; Huber, J.T. Biomass production and protein synthesis by alfalfa under salt stress. J. Plant Nutr. 1991, 14, 283–293. [Google Scholar] [CrossRef]
  45. Meyer, R.D.; Marcum, D.B.; Orloff, S.B.; Schmierer, J.L. Alfalfa fertilization strategies. In Irrigated Alfalfa Management for Mediterranean and Desert Zones; Publication 3512; Summers, C.G., Putnam, D.H., Eds.; University of California/Agricultural and Natural Resources: Davis, CA, USA, 2008; pp. 73–87. [Google Scholar]
  46. te Velde, G. Milking Jersey’s vs. Holstein’s on a Commercial Dairy in California: Milk Production, Feed Efficiency, Intake, Costs, and Advantages; BS, California Politechnic State University: San Luis Obispo, CA, USA, 2013. [Google Scholar]
  47. Koong, L.-J.; Wise, M.B.; Barrick, E.R. Effect of elevated dietary levels of iron on the performance and blood constituents of calves. J. Anim. Sci. 1970, 31, 422–427. [Google Scholar] [PubMed]
  48. Ammerman, C.B.; Goodrich, R.D. Advances in mineral nutrition in ruminants. J. Anim. Sci. 1983, 57, 519–533. [Google Scholar] [PubMed]
  49. Fisher, L.J.; Dinn, N.; Tait, R.M.; Shelford, J.A. Effect of level of dietary potassium on the absorption and excretion of calcium and magnesium by lactating cows. Can. J. Anim. Sci. 1994, 74, 503–509. [Google Scholar] [CrossRef]
  50. Grattan, S.R.; Grieve, C.M.; Poss, J.A.; Robinson, P.H.; Suarez, D.L.; Benes, S.E. Evaluation of salt-tolerant forages for sequential water reuse systems: III. Potential implications for ruminant mineral nutrition. Agric. Water Manage. 2004, 70, 137–150. [Google Scholar] [CrossRef]
  51. Grunes, D.L.; Stout, P.R.; Brownell, J.R. Grass tetany of ruminants. In Advances in Agronomy; Brady, N.C., Ed.; Academic Press: London, UK, 1970; Volume 22, pp. 331–374. [Google Scholar]
  52. Jittakhot, S.; Schonewille, J.T.; Wouterse, H.; Focker, E.J.; Yuangklang, C.; Beynen, A.C. Effect of high magnesium intake on apparent magnesium absorption in lactating cows. Anim. Feed Sci. Technol. 2004, 113, 53–60. [Google Scholar] [CrossRef]
  53. Grieve, C.M.; Poss, J.A.; Grattan, S.R.; Suarez, D.L.; Benes, S.E.; Robinson, P.H. Evaluation of salt-tolerant forages for sequential water reuse systems: II. Plant–ion relations. Agric. Water Manage. 2004, 70, 121–135. [Google Scholar] [CrossRef]
  54. Arthington, J. Know the Sulfur Content of Your Forage—Test It. Available online: http://rcrec-ona.ifas.ufl.edu/pdf/publications/ona-reports/2013/5%202013/or5-13.html (accessed on 9 May 2013).
  55. Spears, J.W.; Weiss, W.P. Role of antioxidants and trace elements in health and immunity of transition dairy cows. Vet. J. 2008, 176, 70–76. [Google Scholar] [CrossRef] [PubMed]
  56. Corah, L. Trace mineral requirements of grazing cattle. Anim. Feed Sci. Technol. 1996, 59, 61–70. [Google Scholar] [CrossRef]
  57. Scaletti, R.W.; Amaral-Phillips, D.M.; Harmon, R.J. Using Nutrition to Improve Immunity Against Disease in Dairy Cattle: Copper, Zinc, Selenium, and Vitamin E; University of Kentucky: Lexington, KY, USA, 1999; pp. 1–4. [Google Scholar]
  58. Jones, M.; van der Merwe, D. Copper Toxicity in Sheep is on the Rise in Kansas and Nebraska; Kansas State University/Veterinary Medical Teaching Hospital: Manhattan, KS, USA, 2008; p. 5. [Google Scholar]
  59. Stochmal, A.; Piacente, S.; Pizza, C.; De Riccardis, F.; Leitz, R.; Oleszek, W. Alfalfa (Medicago sativa L.) flavonoids. 1. Apigenin and luteolin glycosides from aerial parts. J. Agric. Food Chem. 2001, 49, 753–758. [Google Scholar] [CrossRef] [PubMed]
  60. Petridis, A.; Therios, I.; Samouris, G.; Tananaki, C. Salinity-induced changes in phenolic compounds in leaves and roots of four olive cultivars (Olea europaea L.) and their relationship to antioxidant activity. Environ. Experim. Bot. 2012, 79, 37–43. [Google Scholar] [CrossRef]
  61. Tattini, M.; Remorini, D.; Pinelli, P.; Agati, G.; Saracini, E.; Traversi, M.L.; Massai, R. Morpho-anatomical, physiological and biochemical adjustments in response to root zone salinity stress and high solar radiation in two mediterranean evergreen shrubs, Myrtus communis and Pistacia lentiscus. New Phytol. 2006, 170, 779–794. [Google Scholar] [CrossRef] [PubMed]
  62. Brisibe, E.A.; Umoren, U.E.; Brisibe, F.; Magalhäes, P.M.; Ferreira, J.F.S.; Luthria, D.; Wu, X.; Prior, R.L. Nutritional characterisation and antioxidant capacity of different tissues of Artemisia annua L. Food Chem. 2009, 115, 1240–1246. [Google Scholar] [CrossRef]
  63. Ferreira, J.F.S. Artemisia Species in Small Ruminant Production: Their Potential Antioxidant and Anthelmintic Effects. In Appalachian Workshop and Research Update: Improving Small Ruminant Grazing Practices; Morales, M., Ed.; Mountain State University/USDA: Beaver, WV, USA, 2009; pp. 53–70. [Google Scholar]
  64. Katiki, L.M.; Ferreira, J.F.S.; Gonzalez, J.M.; Zajac, A.M.; Lindsay, D.S.; Chagas, A.C.S.; Amarante, A.F.T. Anthelmintic effect of plant extracts containing condensed and hydrolyzable tannins on Caenorhabditis elegans, and their antioxidant capacity. Vet. Parasitol. 2013, 192, 218–227. [Google Scholar] [CrossRef] [PubMed]
  65. Al-Dosari, M.S. In vitro and in vivo antioxidant activity of alfalfa (Medicago sativa L.) on carbon tetrachloride intoxicated rats. Am. J. Chin. Med. 2012, 40, 779. [Google Scholar] [CrossRef] [PubMed]
  66. Ferreira, J.F.S.; Luthria, D.L. Drying affects artemisinin, dihydroartemisinic acid, artemisinic acid, and the antioxidant capacity of Artemisia annua L. Leaves. J. Agric. Food Chem. 2010, 58, 1691–1698. [Google Scholar] [CrossRef] [PubMed]
  67. Tekippe, J.A.; Hristov, A.N.; Heyler, K.S.; Cassidy, T.W.; Zheljazkov, V.D.; Ferreira, J.F.S.; Karnati, S.K.; Varga, G.A. Rumen fermentation and production effects of Origanum vulgare L. Leaves in lactating dairy cows. J. Dairy Sci. 2011, 94, 5065–5079. [Google Scholar] [CrossRef] [PubMed]

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MDPI and ACS Style

Ferreira, J.F.S.; Cornacchione, M.V.; Liu, X.; Suarez, D.L. Nutrient Composition, Forage Parameters, and Antioxidant Capacity of Alfalfa (Medicago sativa, L.) in Response to Saline Irrigation Water. Agriculture 2015, 5, 577-597. https://0-doi-org.brum.beds.ac.uk/10.3390/agriculture5030577

AMA Style

Ferreira JFS, Cornacchione MV, Liu X, Suarez DL. Nutrient Composition, Forage Parameters, and Antioxidant Capacity of Alfalfa (Medicago sativa, L.) in Response to Saline Irrigation Water. Agriculture. 2015; 5(3):577-597. https://0-doi-org.brum.beds.ac.uk/10.3390/agriculture5030577

Chicago/Turabian Style

Ferreira, Jorge F. S., Monica V. Cornacchione, Xuan Liu, and Donald L. Suarez. 2015. "Nutrient Composition, Forage Parameters, and Antioxidant Capacity of Alfalfa (Medicago sativa, L.) in Response to Saline Irrigation Water" Agriculture 5, no. 3: 577-597. https://0-doi-org.brum.beds.ac.uk/10.3390/agriculture5030577

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