Changes in proximate composition and oil characteristics during flaxseed development

SUMMARY: Atmospheric Pressure Photoionization-Mass Spectrometry (APPI-MS) and High Performance Liquid Chromatography (HPLC) are the two analytical methods that were used to characterize Triacylglycerols (TAGs) during flaxseed development. The HPLC method of the oils showed the presence of 15 TAG species. In contrast to the HPLC chromatograms, the APPI-MS showed 17 peaks of TAG. APPI-MS is more rapid than the HPLC method (11 min). The iodine value of the oils showed a gradual increase, while the oil stability continuously decreased. Proximate composition during flaxseed development revealed that flaxseed is potentially a good source of dietary energy and protein. At full maturity, flaxseed contained 37% oil and 24% protein on a dry-weight basis; albumin was the major storage protein (53% of total storage proteins) followed by globulin (33%) and glutelin fractions (11%). Prolamins had the lowest percentage with 3%. α -amylase activity was higher in the mature seeds than the young ones.


SUMMARY: Atmospheric Pressure Photoionization-Mass Spectrometry (APPI-MS) and High Performance
Liquid Chromatography (HPLC) are the two analytical methods that were used to characterize Triacylglycerols (TAGs) during flaxseed development. The HPLC method of the oils showed the presence of 15 TAG species. In contrast to the HPLC chromatograms, the APPI-MS showed 17 peaks of TAG. APPI-MS is more rapid than the HPLC method (11 min). The iodine value of the oils showed a gradual increase, while the oil stability continuously decreased. Proximate composition during flaxseed development revealed that flaxseed is potentially a good source of dietary energy and protein. At full maturity, flaxseed contained 37% oil and 24% protein on a dry-weight basis; albumin was the major storage protein (53% of total storage proteins) followed by globulin (33%) and glutelin fractions (11%). Prolamins had the lowest percentage with 3%. α-amylase activity was higher in the mature seeds than the young ones.

INTRODUCTION
Flaxseed (Linum usitatissimum L.), a member of the family Linaceae, is an economically important oilseed crop containing usually about 40% oil in the seeds. Flaxseed, besides its traditional oleochemical uses, is now gaining recognition as a functional food ingredient for human nutrition (Lei et al., 2003). It constitutes one of the key sources of omega-3 fatty acids, lignans and mucilage. The protein content in flaxseed has been reported to range from 20 to 35% (Oomah, 2001). Productions of purified vegetable proteins are gaining increasing commercial importance due to consumers' preferences for vegetable sources as a food and cosmetic ingredient (Kaur et al., 2007). During the last decade, there has been an increasing interest in human consumption of flaxseed in the diet in order to improve nutritional and health status. The health benefits of flaxseed are mainly attributed to its biologically active components such as α-linolenic acid, lignans, proteins, phenolic acids and flavonoids (Hosseinian et al., 2006).
In the life cycle of higher plants, seed development is a key process connected to distinct generations (Olsen et al., 2001). The developing embryo accumulates lipids in the form of triacylglycerols (TAG), esters of glycerol and fatty acids once early morphogenesis is achieved. The pathway of fatty acid biosynthesis in developing seeds involves different subcellular compartments and is well established (Miquel and Browse, 1997). During the maturation stage, the most abundant mRNAs in embryos are those encoding seed storage proteins, which are thought to serve as a source of nitrogen for the young seedlings (Pang et al., 1988). The understanding of seed metabolism and especially the accumulation of storage products is of major economic importance and could be a key factor for sustainable agriculture. In view of functional foods and the nutraceutical attributes of flaxseed, there is gaining focus on studying the phytochemicals of these crop components.
Although the changes in seed constituents has been studied during flaxseed development (Herchi et al., 2009;Herchi et al., 2011;Herchi et al., 2012), no comparative study is available on triacylglycerol composition during flaxseed maturity using different methods, no data on proximate composition, protein fraction or alpha amylase activity during flaxseed development. The aim of this study was to compare the analysis of triglycerides using HPLC and APPI-MS and to determine the change in proximate analysis, oil characteristics, protein fraction and α-amylase activity at different stages of flaxseed maturity.

Chemicals and Reagents
HPLC-grade chloroform, acetone, acetonitrile, toluene and isopropanol were purchased from the Fisher Scientific Company (Ottawa, Ontario, Canada-Ottawa Admin. Center 112 Colonnade Road Nepean, Ontario K2E 7L6 Canada). Methanol and Ethanol were purchased from Panreac Quimica SA (Barcelona, Spain). Petroleum ether, ethyl ether and acetic acid were from Fisher Scientific SA (Barcelona, Spain). TLC silica plates (silica gel 60 G F254, 20×20 cm, 0.2 mm thickness) were obtained from Merck (Darmstadt, Germany). All standards were acquired from Sigma Aldrich (Madrid, Spain). Other employed chemicals and solvents used in the experiments were purchased from Aldrich (Milwaukee, WI, USA).

Plant Materials
The variety of flaxseed "O116" was obtained from "Institut National Recherche Agronomie Tunis" (INRAT), Tunisia. This variety of flaxseed (Linum usitatissimum L.) was grown in restricted zones (15 m×3 m) on the Agronomy farm of the INRAT from the middle of November 2006 until the end of June 2007. Each sample was collected at intervals after a number of days after flowering (DAF) ranging from 7 DAF to 56 DAF. Moisture and seed weight were determined by weighing 100 seeds before and after drying to constant weight in a vacuum oven at 80 °C for 72 h. Seeds lengths were measured using a micrometer.

Lipid Extraction
The total lipids were extracted by the method of Folch et al. (1957) modified by Bligh et al. (1959). Flaxseeds (2.5 g) were washed with boiling water for 5 min to denature the phospholipases (Douce, 1964) and then crushed in a mortar with a mixture of CHCl 3 -MeOH (2:1, v/v). Fixing water was added and the homogenate was centrifuged at 3000 rpm for 15 min. The lower chloroformic phase containing the total lipids was dried in a rotary evaporator at 40 °C.

Lipid Analyses
Lipid class separation was performed by TLC according to the method of Mangold (1964) using petroleum ether/ethyl ether/acetic acid (70:30:0.4, v/v/v) as developing solvent. The oil samples were placed on thin-layer chromatographic plates (G60; Merck, Darmstadt, Germany) (20 cm×20 cm×0.2 mm) covered with silica gel using a microsyringe. Spots were revealed by brief exposure to iodine vapor. Iodine was then removed under nitrogen flux and by heating the plates at 60 °C. The TAG spots were then collected.

APPI-MS
A 50 mg sample of the extracted lipid was fully dissolved in 5 mL of dichloromethane. LC/ MS experiments were performed using an Agilent LC system (Agilent Technologies; Palo Alto, CA-2660 Matheson Boulevard East, Mississauga ON, L4W 5M2) coupled to an Applied Biosystem /MDS Sciex QSTAR Elite Q-TOF MS with a photoionization ion source. The TAG extracts were separated using an Ascentis TM C18 LC column (15 cm×2.1 mm, 3 μm) with C18 guard cartridge (Supelco). The mobile phase consisted of A, acetonitrile and B, isopropanol. A solvent gradient program was run from 30 to 90% B for 25 min. Subsequently, the LC system was programmed to return its initial solvent composition over 0.1 min, followed by a 5 min re-equilibration prior to the following injection. The injection volume was 5 μL and the flow rate was 200 μL·min −1 . The entire effluent from the column was directly transferred to the MS through the photoionization interface. MS analysis of the analytes was performed using APPI in the positive ion mode. Toluene was used as dopant delivered at a flow rate of 20 μL·min −1 by an isocratic pump (Agilent Technologies; Palo Alto, CA-2660 Matheson Boulevard East, Mississauga ON, L4W 5M2). Analyst QS 2.0 software was used for data acquisition and analysis. Nitrogen was used as curtain gas, nebulizing gas, drying and lamp gas (4 L·min −1 ). The mass range recorded was from 50 to 1300 amu. The other optimal instrumental conditions were as follows: photoionization voltage 1300V; curtain gas setting 25; gas 1 setting 20 and gas 2 setting 70; de-clustering potential (DP), 35V; focusing potential (FP), 150; second de-clustering potential (DP2), 15V; and ion source temperature: 400 °C. Estimations of TAG concentrations were achieved using the relative peak areas of each TAG. Although this method is only semi-quantitative, likely overestimating highly unsaturated components relative to saturates, it does allow for the evaluation of the estimation of relative TAG concentrations and the evolution of individual TAG species over the course of seed ripening. As examples of the results, the total ion current (TIC) chromatogram of flaxseed oil is given in Figure 1

Analysis of triacylglycerols by HPLC
TAGs were analyzed by HPLC on a SCHIMADZU apparatus equipped with an RP-18 stainless steel column (250 mm length×4.6 mm internal diameter), a guard column and a refractive index detector (differential refractometer). The mobile phase was acetonitrile/acetone 1:1 v/v. The flow rate was isocratically controlled at 1.5 mL·min −1 . Ten microliters of sample were injected at each run. The identification of TAG peaks was made by comparison of their Quantification of the contents of the TAG species (expressed in % of total TAG) was done using the following formula: content (%)=PAi/TPA, where PAi is the peak area of an individual TAG and TPA is the peak area of the total TAG. A typical HPLC chromatogram of flaxseed oil is shown in Figure 2.

Iodine Value (IV) Analysis
The AOCS Official Method was employed for the determinations of iodine value (IV) in the oil samples (AOAC, 1993).

Oil Stability
Oxidative stability was evaluated by the Rancimat method (Gutiérrez, 1989). Stability was expressed as the oxidation induction time (hours), measured with the Rancimat 743 apparatus (Metrohm Co., Basel, Switzerland), using an oil sample of 2 g warmed to 100 °C and an air flow of 10 L·h −1 .

Oil Content
Oil was extracted from 20 g of seed powder in a Soxhlet extractor for 5 h using petroleum ether (40-60 ºC) as a solvent. The result was expressed as the percentage of lipids (on a wet weight basis) (AOAC, 2005).

Protein Content
Protein contents were determined according to the AOAC official method (1984) using a micro-Kjeldhal apparatus. Protein was calculated according to the following formula: Data were expressed as percentages on a dry weight basis.

Ash Content
About 0.5 g of powdered seed samples were ignited and incinerated in a muffle furnace (Amalgam, Sheffield, England) at 550 °C for about 12 h. The total ash was expressed as a percentage on a dry weight basis.

Carbohydrate Content
The carbohydrate content was estimated by the difference of the mean values, i.e. [100− (protein+lipids+ash+moisture)].

Energy
The calorific value was estimated (in Kcal·100 g −1 ) by multiplying the percentage of crude protein, crude lipid and carbohydrate by the recommended factor (4, 9 and 4.125 respectively) used in vegetable analysis (Hunt et al., 1987).

Protein Fractionation
Protein fractions were isolated by sequentially extracting flaxseed with different solvents (the seed to solvent ratio was 1:10, w/v, in each case) according to the modified Osborne scheme (Osborne, 1924), as described by Chavan et al. (2001): Samples (1 g) were dispersed in 10 ml of distilled water by stirring with a magnetic stirrer and extracted over 45 min periods at room temperature (25 °C). The suspension was then centrifuged at 5,000×g for 15 min, and the resultant supernatant was filtered. The residues were re-extracted twice more with the same solvent and the recovered filtrates were combined and designated the ''water-soluble fraction". The residue was then extracted successively with a 0.5 M NaCl solution (pH 7.0) of 70% (v/v) ethanol at 65 °C in a shaking water bath, and 0.1 M sodium hydroxide in order to separate the total seed proteins into albumin, globulin, prolamin and glutelin fractions, respectively. The filtrates containing the desired protein fractions were dialyzed against distilled water for 48 h at 4 °C and separately lyophilized. The protein content of each fraction was determined by the micro-Kjeldahl procedure (AOAC, 1984).

Assay of α-amylase activity
Weighed flaxseed (500 mg seeds for each assay) were homogenized with four volumes of extraction buffer containing 50 mmol·L −1 Tris-HCl (pH 7.0), 3 mmol·L −1 CaCl 2 , and 4 mmol·L −1 NaCl and centrifuged at 8000 g for 20 min. The supernatant was centrifuged at 20 000 g for 20 min. A 200-mL aliquot of the final supernatant was mixed with 50 mL of β-limited dextrin made from potato starch with β-amylase (Kohno and Nanmori, 1991). After incubation at 37 °C for 5 min, 0.5 mL of a 0.1% iodine-0.3% potassium iodide solution (I 2 -KI), and 2 mL distilled water were added to the reaction mixture. The change in color was recorded at 620 nm with the extraction buffer as the blank control. A unit of activity was defined as the amount of enzyme that caused a decrease in absorbance of 0.1 at 620 nm under the assay conditions (Chen et al., 1998).

Statistics
Statistical analysis was performed using the Proc ANOVA in SAS (software version 8). Results are presented as the means ± SD from three triplicates of each sample.

Seed size change during fl axseed development
The stages and seeds lengths are given in Table 1. Flaxseed development can be divided into 8 stages. This study used seed size and color to determine time of maturity. The plant growth and especially the flowering were followed daily to provide a precise determination of the maturation stage which proved to be a very important parameter (Attoumbré et al., 2011). Seed size increased to a peak value at S7-S8 stages ( Table 1). The average length of mature flaxseeds was 6.0-6.5 mm. At stage S8, seeds were considered as mature according to the characteristic brown color of mature seeds.

Changes in triacylglycerols composition during fl axseed development
The HPLC technique with an RP-18 column separates TAG according to both length and unsaturation degree of their carbon chains. Oil samples were dissolved in acetone and directly injected into an HPLC column without any preliminary chemical derivatization or purification. The identification of TAG peaks was made by comparison of their retention times with authentic standards. The TAG peaks appear between 7 and 34 min retention time (27 min) and this is due to the various TAG species in flaxseed oils. The TAG composition during flaxseed development, expressed as a percentage of total TAG peak area, is presented in Table 2. The results show the presence of 15 TAG which differ in their contents during flaxseed development. The major forms observed were LnLnLn, LnLLn and LnOLn. Contrary to the HPLC method, the APPI-MS presented 17 TAG peaks with more information about the mass value of TAG. The TAG peaks provided by LC-APPI-MS appear between 10 and 21 min retention times (11 min). The method (APPI-MS) described is more rapid than the HPLC method. One of the main characteristics of APPI-MS, in addition to high mass resolution, is its outstanding sensitivity. These advantages result in extremely low detection limits, leading to a new dimension in speciation analysis. It has been reported that TAG content changes during seed development (Herchi et al., 2012). The average of Triunsaturated triacylglycerols was found between 75% and 85% during flaxseed development. The highest percentage of diunsaturated triacylglycerosls (25%) was found at 35 DAF. Using the TLC method, and compared to given results by LC/MS (Herchi et al., 2012), the same pattern of total TAG accumulation in flaxseed during seed development was revealed. At 7 DAF, the TAG represented a small fraction of the total lipid population (8%) but their proportion increased gradually to reach 94% at complete maturity (56 DAF). Each value is the mean ± SD of three determinations. SFA: saturated fatty acids, MUFA: monounsaturated fatty acids, PUFA: polyunsaturated fatty acids, TU: total unsaturated fatty acids, TU/TS: total unsaturated/total saturated fatty acids.

Changes in the fatty acid composition of triacylglycerols
The comparative fatty acid composition of TAGs was analyzed during flaxseed development for the first time, using HPLC and LC-APPI-MS (Table 3). The different FA and their percentages provided by LC-APPI-MS are in agreement with those listed by HPLC. Saturated fatty acids (SFA) did not exceed 9% while Monounsaturated fatty acids (MUFA) ranged from 13 to 22%. The monounsaturated fatty acids such as oleic acid have great importance because of their nutritional implication and effect on the oxidative stability of oils (Aguilera et al., 2000). Polyunsaturated fatty acids (PUFA) are the major fatty acids, ranging from 73 to 80%. The unsaturated / saturated ratio (ratio of the sum of unsaturated FA to the sum of saturated FA) was generally high and this high value gives this oil a good prevention of oxidation. Table 4 illustrates the changes in iodine value (I.V) during flaxseed development. The relatively high iodine value (156 g I 2 ·100 g −1 oil) and (176 g I 2 100·g −1 oil) during flaxseed development may be indicative of the presence of many unsaturated bonds and can thus be grouped as drying oils. The continuous increase in the iodine value during flaxseed development means that the oil is becoming more and more unsaturated in character. Oxidative stability is an important parameter to evaluate the quality of oils, as it gives a good estimation of their susceptibility to oxidative degeneration which is the main cause of their alteration. Oil stability decreased during flaxseed development (Table 4). This decrease in stability is due to the loss of natural antioxidants. These results are in accordance with those of Baccouri et al. (2007). The resistance to oxidative deterioration is usually attributed to two main factors: (I) the fatty acid composition, which in the case of flaxseed oil is characterized by a large amount of polyunsaturated fatty acids and (II) the pool of minor compounds of powerful antioxidant activity which is constituted mainly by tocopherols and polyphenols but also by chlorophylls and carotenoids.

Changes in proximate composition during fl axseed development
The changes in proximate composition during flaxseed development are shown in Table 5. The moisture content (74% at 7 DAF) decreased continuously in weight as maturity progressed to obtain a maximum of 5% at ripe seed (56 DAF). The gradual decline in relative water content is likely due to the accumulation of dry matter as it is Each value is the mean ± SD of three determinations.
Changes in proximate composition and oil characteristics during flaxseed development • 9 in agricultural species (Lee et al., 2008). The protein levels increased gradually from 8% at 7 DAF to 24% at complete maturity, which was attributed to the rapid synthesis of oil and carbohydrates in early seed development (Saldivar et al., 2011). The results indicate that flaxseed is a good source of protein and lipids for human consumption. The ash content showed a continuous increase during flaxseed development in that the highest level of ash (3.20%) was observed at complete maturity. This observation finds great support in the literature (Mueller et al., 2010). The level of total carbohydrates (by difference) fluctuated and no definite trend was obvious, although the highest amount (31%) was detected at complete maturity. The total energy values for the seeds analyzed indicated that the mature seeds (49 DAF) which contained significantly the highest oil content had more total energy (2400 Kj·100 g −1 ) than the other stages. Flaxseed could therefore be a good supplement as a source of energy in feed formulation. The estimated digestible crude protein ranged from 3% (7 DAF) to 19% (49 DAF). From the foregoing discussion, it may be concluded that flaxseed is potentially a good source of dietary energy and protein. Osborne (1924) classified seed protein into four groups on the basis of their different solubilities: albumins (water soluble), globulins (soluble in dilute salt solutions), prolamins (soluble in aqueous alcohols) and glutelins (dilute acid). Flaxseed accumulates albumin as a major protein ( Table 6). The highest percentage in albumin (65%) was observed at 28 DAF. The level of globulins increased at the beginning of seed development and decreased before the end of seed maturation. Both albumins and globulins represented the most abundant soluble protein (from 62 to 87% of total soluble proteins) during flaxseed development. Since albumins are mostly enzyme proteins (Bewley and Black, 1978), the synthesis of enzymes during ripening might be responsible for the apparent increase in the content of the water-soluble fraction. Prolamins declined rapidly during the initial 2 to 4 weeks of flaxseed development and then remained in a relatively constant content. Glutelins followed a similar pattern but then increased throughout the final ripening stages. Our results show that at full maturity, protein was a mixture of albumins (53%), globulin (33%), prolamin (3%) and glutelin (11%). These findings are in agreement with the results of Wanasundara et al. (1999) who reported that the major classes of flaxseed proteins were albumins and globulins.

Changes in α-amylase Activity
A low α-amylase activity was observed at the beginning of seed maturation ( Figure 3). However, from 28 DAF, the α-amylase activity in flaxseed increased to be more than 0.3 units/10mg. α-amylase was involved in starch breakdown at later development stages (Monma et al., 1991). The highest α-amylase activity was recorded at 49 DAF. After that, the activity of α-amylase decreased again. This decrease may be explained by the decrease in the break-down of starch at late developmental stages and with concomitant lower soluble sugar. Flaxseed has low starch content at complete maturity (1-2%) (Epaminondas et al., 2011). Relatively high α-amylase activity was concomitant with the lower starch content in flaxseed. It has an active role in the hydrolysis of the starch during seed development. It may also be responsible   Each value is the mean ± SD of three determinations.
for the maintenance of requisite water potential, by providing solute sugars during seed development (Murtaza and Asghar, 2012).

CONCLUSIONS
APPI-MS analyses give more information about the separation and molecular distribution of TAG molecules compared to HPLC. Oil characteristics change during flaxseed development. The proximate components are accumulated at different rates. It may be concluded that flaxseed is potentially a good source of dietary energy and protein. These results improve our knowledge about the effect of maturation on flaxseed quality and composition. The major classes of protein were albumins and globulins. The highest α-amylase activity was recorded at 49 DAF.