Abstract
Triterpenic saponins represented in Calendula officinalis L. by oleanolic acid (OA) glycosides are pentacyclic triterpene compounds with a wide range of biological and medicinal properties. This report demonstrates nitrogen source impact on growth, saponin accumulation, and secretion in hairy root and suspension cultures of marigold. Hairy roots preferred nitrate as a mineral source of nitrogen, but its impact on growth, OA glycosides accumulation, and secretion were line-dependent. The best productivity of OA glycosides was found in CC16 line (74.86 mg flask−1) in ½ MS medium modified by 2.5× KNO3 and ammonium elimination with 2.5 g l−1 peptone. Organic nitrogen source at 27.5-g l−1 impairs the growth rate of hairy roots. Its effect on saponin accumulation and secretion to the surrounding medium depended on line and media composition. Nitrate:ammonium ratio of 4:2 for CC16 resulted in 5.7-fold increment of saponin secretion comparing to the standard medium. Embryo roots, apical bud, and hypocotyls explants were crucial for induction of suspension culture synthesizing saponins; however, effect of mineral form of nitrogen in cultivating medium had to be considered. The highest OA glycosides level (171.97 μg g−1 of dry weight) was recorded in the root derived culture with nitrate as a sole mineral form of nitrogen. Peptone from lactalbumin decidedly inhibited the saponin formation; however, it was essential for culture initiation, proliferation, and organ differentiation.
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Introduction
Oleanolic acid (OA) naturally occurs in plants as the form of glycosidic derivatives is a pentacyclic triterpenoid which has been identified in more than 1620 of edible and medicinal species (Fai and Tao 2009; Fukushima et al. 2011). This compound is widely distributed among the olive family (Oleaceae) and its name originated form olives Olea europaea (Simonsen and Ross 1957). Oleanolic acid in free form is hydrophobic and has numerous pharmacological properties including anti-tumor, anti-HIV, hepatoprotective, immunostimulatory, or anti-inflammatory (Laszczyk 2009; Kashiwada et al. 1998; Wang et al. 2010; Rios 2010). Other specific biological activity of OA molecules is associated with sugar chain linked to the aglycone with glycosidic bond. These complex structures, called saponins, have a better solubility in water and exhibit hemolytic, allelopathic, fungistatic (Szakiel et al. 2005), antibacterial, and antiparasitic properties (Szakiel et al. 2008; Doligalska et al. 2011). Those significant bio-activities and relatively non-toxic nature have made oleanolic acid a highly valuable compound. Novel research opportunities for cancer therapy were opened by the synthetic derivatives of OA. This modification consists of introducing cyano-, methyl-, or imidazole substituent to harvest from biological sources triterpene backbone. Improved molecules effectively induced apoptosis in different cancer cell lines and suppressed tumor growth in vivo (Liby et al. 2007; Deeb et al. 2008; Sporn et al. 2011). Latest important discoveries were Himoxol (ethyl 3-hydroxyimino-11-oxoolean-12-en-28-oate), semisynthetic OA derivative reported to exert its cytotoxic action in breast cancer cells by activating apoptosis and autophagy pathways (Lisiak et al. 2014) and PFOA (3-O-[N-(p-fluorobenzenesulfonyl)-carbamoyl]-oleanolic acid) which, apart from antiproliferative action, shows the ability to inhibit invasive breast cancer by preventing the cell migration and metastasis (Elsayed et al. 2015).
The molecule of OA is obtained solely from biological sources by laborious extraction and purification. Despite the considerable difficulty, the mentioned procedure has been carried on with satisfactory performance. There is still a risk of obtaining the plant material with low level of desired products. Their concentration in intact plants is affected by plenty environmental factors (Szakiel et al. 2011). An alternative source of oleanolic acid glycosides can be in vitro culture of marigold, with possibility of obtaining the line with stable contents of desired compounds. In addition, strictly defined conditions of in vitro culture ease studying the impact of different factors separately. Other important advantage is liquid medium which allows to obtain a precise application of the most factors and to simplify gathering of exudates. Both types of cultures used in our study, hairy roots and suspension culture of marigold, are considered as a key to achieve production on commercial scale. They differ in genetic stability and efficiency of metabolite synthesis: hairy root cultures offer higher stability and productivity than suspension culture which is composed of undifferentiated culture.
The nitrogen plays an important role in homeostasis of plants and, therefore, determines the growth, development, and yielding. Plants can utilize mineral form of nitrogen as a nitrate (NO3−) and ammonium (NH4+). Natural growth conditions determined the relative proportion of both forms depending on oxygenation, acidity, and humidity of the soil. Their assimilation can be realized by active transport carried out by specialized transporters; also ammonium ions can passively migrate through ion channels, as well (Taylor and Bloom 1998). Nitrate after uptake by plant roots may be reduced to ammonium and subsequently to amino acids, or be transported to leafs, accumulate in vacuole or is removed to the apoplast. Consumption of reduced form of nitrogen (NH4+) requires less energy than oxygenated (NO3−) form, but the assimilation of ammonium generates additional energetic costs associated with the supply of ketoacids from aerial parts (Bloom et al. 1992). In addition, for most cultivated and growing wild plants, using ammonium is toxic when used as a sole source of nitrogen (Britto and Kronzucker 2002). This phenomenon still needs an unequivocal explanation: one undeniable seems to be the pH influence. Both mineral forms adsorption which is associated with changes in pH of the rhizosphere: ammonium uptake decreases, while nitrate increases pH. Nitrogen can be additionally uptaken in form of organic compound, mainly as a mixture of amino acids. The availability of amino acids in the soil depends on proteolysis and the buffer capacity of the rhizosphere: distribution of individual amino acids is affected by their charge. Second important requirement determines the relationship between amino acids concentration and mediating transporters in the root plasmalemma (Näsholm et al. 2009).
In plant cell cultures, the nitrogen source may significantly affect the plant cell proliferation, root growth, and metabolite production (Cui et al. 2010; Zhang et al. 2011). Nitrate had a clear influence on the alkaloid content and on the atropine/scopolamine ratio in hairy root culture of Atropa belladonna (Bensaddek et al. 2001; Chashmi et al. 2008). Reduced level of ammonium combined with increased level of nitrate favors the production of triterpenoids: gymnaemic acid in Gymnema sylvestre (Praveen 2011) and withanolide A in Withania somnifera (Praveen 2013), while the elimination of nitrate from the media of Chrysanthemum cinerariaefolium culture induced twofold increase in accumulation of pyrethrin (Rajashekaran et al. 1991). However, all the aforementioned effects of the culture medium modifications differ among the species, lines, and type of cultures (Aoki et al. 1997).
In our study, the nitrate and ammonium concentrations of ½ MS medium were modified. Their effects on the growth, production of oleanolic acid glycosides, as well as their secretion into the medium were investigated. The suspension cultures originated from different explants and three lines of hairy roots were compared to bring out general tendencies for marigold.
Materials and methods
Plant material
Mature embryos of the marigold Calendula officinalis cv. Persimmon Beauty were excised from seeds and sterilized for 20 min with a commercial hypochlorite agent “Domestos” (Unilever) diluted with water (1:3, v/v). Subsequently, the embryos were rinsed three times in sterile liquid ½ MS medium (Murashige and Skoog 1962). Sterilized embryos were germinated on solid ½ MS in Ø 10 cm Petri dish.
Suspension cultures (SC) of marigold were initiated from apical buds (B), cotyledons (C), hypocotyls (H), and embryo roots (R) dissected from sterile 7–8-day-old seedlings. Explants were introduced into modified liquid ½ MS medium (MS4) supplemented with 1 mg L−1 of 2.4-D: buds and roots immediately, cotyledons, and hypocotyls after cutting on thin slices.
Hairy roots cultures (HR) of marigold were initiated according to the procedure described earlier (Długosz et al. 2013). Lines selected for current topics were: CC16, derived from cotyledons, after 36 and 72 subcultures; MC3, derived from cotyledons, containing the β-glucuronidase (GUS) reporter gene under the control of promoter (1058 bp upstream region from the ATG codon) of tomato NIK (Nematode-Induced Kinase) gene (DFCI Tomato Gene Index TC218759) (Święcicka et al. 2009), after 36 subcultures; CH2, derived from hypocotyls, after 72 subcultures.
Maintenance of the cultures
Established SC were subcultured every 2 weeks by transfer of 3-mL packed cell volume (PCV) tissue to 100-mL Erlenmeyer flask containing 50 mL of liquid medium. Established lines of HR were subcultured every 3–4 weeks by transfer of one piece cut of from young root to 50-mL Erlenmeyer flask with 25 mL of fresh medium. All types of cultures were maintained in complete darkness at 24 °C and shaken at 120 rpm. For OA content determination, SC and HR were transferred to 250-mL Erlenmeyer flasks containing 100 mL of liquid ½ MS medium (Table 1): 6 mL of PCV for SC and 1–2 fragments of incremental young tissue for HR, respectively, and were cultured for 14 (SC) or 30 (HR) days. Growth of SC was calculated as a percent of relative growth during a 14-day period which was calculated according to formula: [(FWF − FWI)/FWI] × 100 (where: FWF—final fresh weight, FWI—initial fresh weight). Appropriate capacities of inoculum were weighted at the beginning of the culture, and the final fresh weight was measured after the liquid filtration.
Regenerative capacity of established culture was verified through the transfer of cell aggregates (inoculum size 1/4–1/8-mL PCV 100 mL−1 medium) from proliferation media (MS1–6) to medium without growth regulators (MS1RC) under fluorescent illumination (54 μmol m2 s−1), with 16/8-h photoperiod.
Nitrogen source modification
The effect of nitrogen source on tissue growth and saponin production in SC and HR was estimated by changes in the concentration of ammonium and potassium nitrate in basal ½ MS medium, which contained 825 and 950 mg L−1, respectively. Second step was evaluation of the effect of rising concentration of potassium nitrate with ammonium omission. Proposed concentrations were 1-, 2.5-, 3.5-, and 4.5-times higher than in standard ½ MS. The final issue was to determine the impact of altering the ammonium:nitrate ratio for HR culture. Media supplemented with appropriate KNO3 and NH4NO3 quantities of 5:1; 4:2; 3:3 of NO3−/NH4+ ratio were added (to keep nitrogen level constant—60 mM, which was the level equal with a full salt strength MS medium).
Extraction of oleanolic acid
Cells and roots after drying in room temperature were ground with methanol and boiled under reflux for 60 min, the culture medium was extracted three times with 20 mL of 1-butanol. The extracts were evaporated under reduced pressure and subsequently hydrolyzed with 10% HCl in methanol. The hydrolysate diluted with two parts of water were extracted three times with 20 mL of diethyl ether and separated by thin-layer chromatography (TLC). Purified OA was methylated with an ether solution of diazomethane (Janiszowska and Kasprzyk 1977). Detailed description of the extraction procedure was published previously by Wiktorowska et al. (2010) and Długosz et al. (2013).
Quantification of oleanolic acid
Quantitative measurement of OA was performed by gas–liquid chromatography (GLC) at 270 °C on a Shimadzu GC-2014 instrument equipped with a flame ionization detector (FID). Samples were applied by split injection 1:5 on a ZB-1 30 m × 0.25 mm × 0.25 μm column (Phenomenex). The temperature of the injector and detector was 290 °C. Nitrogen was used as the carrier gas at a flow rate of 1.2 mL min−1. Peak identification (Fig. 1) and quantification of oleanolic acid were carried out by referring to a calibration curve prepared with an authenticated sample of methylated oleanolic acid as the standard (Długosz et al. 2013). In addition, the methyl ester of OA was identified by GLC–MS on an Agilent Technologies 7890A gas chromatograph coupled with a 5975C mass spectrometric detector. Samples (dissolved in 1–4 μL of a 5:1 diethyl ether:methanol mixture, v:v) were applied by split injection 1:10 on an HP-5MS 30 m × 0.25 mm, 0.25-μm column (Agilent Technologies). Helium was used as the carrier gas at a flow rate of 1 mL min−1. The following parameters were employed: column temp. 280 °C, inlet and flame ionization detector (FID) temp. 290 °C, MS transfer line temp. 275 °C, quadrupole temp. 150 °C, ion source temp. 230 °C, EI 70 eV, m/z range 33–500; FID gas (H2 from a hydrogen generator) flow 30 mL min−1, air flow 400 mL min−1. Identification was made by comparing the mass spectra with library data from Wiley 9th Ed. and NIST 2008 Lib. SW (version 2010) and, where available, by comparison of retention times and corresponding mass spectra with those of authentic standards.
Results
Suspension culture: growth and saponin content
Suspension cultures of marigold were induced from all tested explants. First reaction was observed after 2 weeks. Embryo-like structures appeared the earliest on the surface of apical buds, then on the hypocotyls and finally on the roots. Sliced cotyledons responded at the latest. Established SC were achieved after 3 months. During the first 2–6 months, the culture consisted of globular structures resembles early stages of somatic embryos which were showing single or in cluster proliferation (Fig. 2a). Afterwards, this globular structures were replaced by organogenic callus without advancing embryo stages (Fig. 2b), which periodically changed their morphology to small-aggregated (Fig. 2c). Similar tendency was found in established culture regardless of the origin. Different nitrogen forms influenced the diameter of aggregates. When organic form (edamine) predominated or proportion of mineral nitrogen as for ½ MS was used, aggregates were smaller (< 1 mm) than in the media with standard level of edamine and with unbalanced mineral nitrogen ratio (nitrate or ammonium form predominated). This effect was not observed for SC derived from cotyledon: small aggregate size was obtained in the medium with standard edamine concentration (250 mg L−1) and nitrate as a sole mineral source of nitrogen (Fig. 2c).
Next step was to measure effect of five different nitrogen source modifications to the ½ MS medium (Table 1). After two subcultures with 4 week intervals, the third subculture provided the data for growth and glycosides concentration in the cells. The influence of the media composition on growth values GV (%) of the culture originated from the four types of seedling explants is depicted on Fig. 3a. Suspension culture of marigold proliferated quickly in the media, in which they were initiated (MS4). In that medium, variant ammonium nitrate was eliminated, the content of potassium nitrate was increased 2.5 times, and content of edamine-peptone from lactalbumin—tenfold. GV (%) of the fresh weight ranged from 393.50 ± 17.66% for culture B originating from apical bud to 540.19 ± 25.05% for culture H derived from hypocotyl. In general, all cultures were characterized by high growth rate if the nitrate was only source for mineral nitrogen. If both forms of mineral nitrogen were balanced as in the standard MS medium, fresh weight was decreased twice. Supplementation of the edamine at the tenfold concentration to the medium, in which nitrate was the only mineral form (MS3), improved cells proliferation by over 30% on average (MS4), but only for C and H culture, it was statistically significant. The same lactalbumin hydrolysate concentration with both mineral forms coexistence at almost 1:1 (MS5, MS6), resulted in statistically significant increase in the growth value over 94%.
Regenerative capacity of established suspension culture was observed in the liquid medium MS1SE (Table 1). After 4 weeks, expanding globular somatic embryos usually fused with clusters and chlorophyll appeared area was observed (Fig. 2d). Some of the aggregates were equipped with thin embryo roots. However, no properly developed cotyledons and typical bipolar structure were present. Tissue showed secondary proliferation after removing it to the regeneration medium. Such embryo-like structures placed on the surface of solid medium were enveloped with callus which hampered their growth and differentiation (data not presented).
Crucial for initiation cultures able for saponins accumulation was root, apical bud, and hypocotyl explants; however, the composition of the medium was not insignificant. The highest OA glycosides concentration in culture cells originated from the root was present when cultivated in MS3 media: 171.97 ± 27.62 μg g−1 DW (Fig. 3b). The SC originated from other two explants accumulated saponins at ca. 74% lower concentration. Media supplemented with modified ratio of both mineral forms of nitrogen (1:1)—MS5—reduced the growth rate and saponin content except the C culture, for which such conditions created the compromise between culture growth and metabolite production. The results demonstrated for the SC show that there was no correlation between saponin content and biomass (FW or DW). Organic nitrogen source, represented here by peptone from lactalbumin at tenfold higher concentration, decidedly inhibited the synthesis of oleanolic acid glycosides. For the B culture so efficiently, that these compounds were completely absent in their cells. Supplementation with peptone accelerated the SC induction, as in the initial medium (MS4) which contains tryptophan—the auxin precursor—which interacts with nitrate and 2.4-D to enhance embryogenic capacity of the explants.
Hairy roots: growth, saponin content in tissue, and release into the media
The hairy root lines chosen for nitrogen feeding optimization were selected due to stable and fast growth in liquid media and efficient saponins production. In the first experiment, our objective was the comparison of growth and saponins concentration in hairy roots with suspension culture. Media used for cultivation were composed similarly, with exception of presence of plant growth regulators, and additional variant: standard medium (½ MS) supplemented with high edamine content (MS2). Oleanolic acid glycosides, which were secreted to the medium, were determined after cultivation time. Lines selected to this task were two of control lines: CC16 (after 36 subcultures) and CH2 (after 72 subcultures) and one modified—MC3 (after 36 subcultures) maintained in standard ½ MS medium. The growth of hairy roots culture measured in form of a dry weight (Fig. 4) was genotype-dependent: control lines (C) achieved the higher DW than modified line (M) under any proposed culture medium. In general, hairy roots of marigold had a better growth in standard ½ MS media (MS1) or modified by elimination of ammonium and increased concentration of nitrate (MS3). Tissue after 30-day growth in such media was in good condition: they were free of necrosis and callus formation (Fig. 5a), while in MS3, they had slightly darker colour (Fig. 5b). Media supplemented with high content of organic source of nitrogen (MS2, MS4, and MS6)–peptone, lactalbumin hydrolysate—in contrast to the SC—decreased the growth rate. However, line CH2 showed that adding peptone over standard level improved the biomass accumulation in the media with balanced ammonium/nitrate ions ratio like in ½ MS (MS2), as well as in media with equimolar concentration of both mineral forms (MS6). Depending on the line, after growth in high edamine concentration, tissue was vitrified and embedded by callus (line CH2: Fig. 5c) or showed inhibited growth and necrosis (line CC16: Fig. 5d). Content of DW (%) in hairy roots was generally twofold higher than in suspension culture of marigold (Table 2). As we showed in our previous report (Długosz et al. 2013), the percent of DW in modified line (M) was higher than in control lines (C). In this work, the differences raised up to 66%; in addition, the 2.5 times increased strength of nitrate (MS3) generated the highest content of DW (19.4%).
Proposed set of ½ MS modifications demonstrated strong impact of mineral and organic nitrogen source on oleanolic acid glycosides accumulation in hairy root cultures of marigold. Lines selected for evaluation varied in the origin, morphology, growth rate, and the saponin content. Figure 6 presents the accumulation of glycosides, expressed as an aglycone—oleanolic acid mass, in designed media after 30-day growth in shaken flasks. Elimination of the ammonium form (MS3) increased OA amount in tissue from 2.5 times for CH2 to 5 times for MC3 (Fig. 6a). Supplementation of nitrate with peptone from lactalbumin (MS4) generated a slight increase (MC3), slight decrease (CC16) and ca. 60% reduction (CH2) of OA. Medium where both mineral forms were equimolar (MS5) obtained OA concentration 2.5–3 times lower than for control culture, respectively, for CH2 and CC16 lines. Modified line (MC3) exceptionally accumulated OA in such conditions at ca. 1 mg g−1 DW over control. This case was also interesting regarding secretion: saponins released to the medium had over sixfold concentration than in control medium (Fig. 6b). General tendency found in analysis of culture media was the strong relation between secretion of glycosides to the medium and their inside accumulation. However, in the case of certain lines, impact of media composition was evident. Lines CH2 and MC3 generally with low secretion efficiency improved releasing the glycosides twofold in the media supplemented with high concentration of edamine but without ammonium salt (MS4). On contrary, in line CC16, the secretion was inhibited by over standard level of lactalbumin hydrolysate. It was over tenfold and nearly sevenfold lower, respectively, for MS1–MS2 and for MS3–MS4 media.
Hairy roots: effect of nitrate increase
Positive correlation between mineral nitrogen form modification and OA derivatives suggested the further study of this issue. Media lacking the ammonium ions and containing potassium nitrate, as a sole inorganic nitrogen source, at 1× to 4.5× concentration of ½ MS medium (Murashige and Skoog 1962) were used. Figure 7 shows the growth of two lines of hairy roots expressed as a dry weight. Line CC16 grows efficiently in the media with elevated level of nitrate in relation to control (½ MS) medium; however, some specific fluctuations of growth were observed. Removing of ammonium ions from the standard medium composition lowered the DW for CH2 (see column 1NO3− and 2.5NO3− on diagram Fig. 7) to rise over the control for 3.5NO3− and finally drop down at the highest concentration of NO3−. Elevated level of nitrate modulates hydration level of tissue, what was manifested by gradual increase of DW (%): from 8.85% for ½ MS to 13.21% for 4.5NO3− (Table 2). In CC16 line, % of DW increased, but the highest content of DW (%) was noted for 1NO3−—14.36% what represented 1.85-fold of control culture. Morphological appearance of the first line supplemented with rising nitrate concentration was similar to control culture (Fig. 8a–c). Second line (CH2) maintained that tendency (Fig. 8d–h); however, the highest concentration of nitrate reduced the growth and changed tissue morphology as the lateral roots were brownish and their number was reduced (Fig. 8h).
Triterpenic saponins accumulation expressed as an OA concentration in tissue (Fig. 9a) exhibited strong correlation to DW for CC16 line. Only the ammonium nitrate elimination (1NO3−) improved saponins accumulation more than threefold, but without continuing in further concentrations. Different correlations for CH2 were found. This line demonstrated the linear increase of OA in tissue from 5.39 to 8.31 mg g−1 DW until nitrate concentration reached 4.5—higher value than in standard medium. Such nitrate concentration decreased metabolite concentration about 30% under the control culture productivity. Modification of nitrate content in culture media enabled us to find the conditions favorable for OA glycosides release from the tissue. In line CC16, saponin concentration increased in medium 2.5—and twice in relation to control, respectively, for 2.5NO3− and 3.5NO3− medium (Fig. 9b). Second line (CH2) despite containing over twofold, higher OA glycosides in tissue than CC16 (control conditions) released these compounds moderately. In optimal conditions (3.5NO3−), CH2 achieved 0.18 mg L−1, which was only 85% efficiency of control conditions.
Hairy roots: effect of NO3 −/NH4 + ratio
Standard MS medium (Murashige and Skoog 1962) contains 60 mM of nitrogen, which is represented by potassium nitrate (39.4 mM) and ammonium nitrate (20.6 mM). Established hairy root cultures of marigold were maintained at ½ MS, where macro-element concentrations were decreased by half and nitrate/ammonium ratio was almost 2 to 1. In this kind of medium composition, both tested lines (CC 16 and CH2) differed in the growth (0.78 ± 0.03 and 0.93 ± 0.07 g of DW, respectively) and saponin content (2.12 ± 0.23 and 4.39 ± 0.20 mg OA g−1 DW, respectively). The growth rate differences between those lines were stronger after the proposed nitrate/ammonium modification. Line CH2 decreased their growth in all used media modification: 44% (5:1), 40% (4:2) until 79% (3:3) (Fig. 10). In contrary, line CC16 increased the DW in the first two cases: 36 and 64% for 5:1 and 4:2, respectively; however, equimolar concentration of nitrate/ammonium weakened the growth of hairy roots by 58%. Morphological appearance of two lines showed some differences mainly related to the hue and root thickness presented after the growth period in shaken flasks (Fig. 11). Line CC16 changed from pale yellow appearance in standard medium to straw colour in 5:1 (Fig. 11b) and 3:3 (Fig. 11d), whereas tissue from 4:2 was tawny (Fig. 11c). Hairy roots from 3:3 variant were thinner. Tissue of the line CH2 seemed to pale at 5:1 (Fig. 11f) and was clearly brighter at 3:3 medium (Fig. 11h).
Similar dependences of saponin content in tissue for both lines were noted (Fig. 12a). Highest triterpenic saponin quantity was measured for the CH2 line in the control medium. Proposed NO3−/NH4+ modification resulted in average twofold lower accumulation of OA. Similar content levels were found for CC16 cultured in the media with nitrate:ammonium 5:1 ratio. Next two medium types showed gradual reduction of OA content below the control level for 3:3 ratio. More interesting effects were observed in the culture media. Two of the applied medium modifications resulted in 3.4- and 5.7-fold increase of saponin secretion to the medium, respectively, for 5:1 and 4:2 ratio (Fig. 12b). Second culture (CH2) reduced the already low content of saponin in the medium from 0.14 to 0.04 mg L−1.
Discussion
Marigold C. officinalis despite the richness and variety of biologically active substances produced in its tissues still is poorly exploited on the area of modern plant biotechnology. One of the first reports, published in 2002 by our group, was concerned the seeking of explants and plant growth regulators suitable for culture initiation (Grzelak and Janiszowska 2002). The most efficient for callus induction on cotyledon and young leaf explants was auxin and cytokinin compilation. Finally 2,4-D and 2iP obtained the optimal growth and saponins concentration at 0.09 mg per gram of FW. Marigold suspension culture used in the present research was initiated immediately (without an intervening callus phase) in liquid medium, where modified mineral nitrogen source (2.5× KNO3, NH4NO3 omission—relative to ½ MS), tenfold organic nitrogen source, and only auxin (2,4-D) obtained fast (2–6 months, depending on explant) culture initiation and stabilization from four seedlings explants.
Nitrogen source in both mineral forms: ammonium and nitrate, or other organic supplementation may act as factors important for initiation, growth, and metabolite accumulation in plant cultures. Results presented in this paper showed significantly that nitrate and organic source of nitrogen were essential for suspension culture initiation; nitrate strongly accelerates cell proliferation and generally saponins accumulation. However, tenfold higher concentration of organic nitrogen source, represented here by peptone from lactalbumin, decidedly inhibited synthesis of oleanolic acid glycosides. Supplementation with peptone accelerated the SC induction, mainly by the high of tryptophan—the auxin precursor—which interacts with nitrate and 2.4-D to enhance morphogenetic capacity of the explants. Peptone, which is a complex nitrogen source, contains wide range of proteins, peptides and free amino acids, likewise the mixture of sugars, fats, and vitamins. Many reports indicated the beneficial effect of some supplements to the medium on the content of secondary metabolites. Phenylalanine promoted taxol production in Taxus cuspidata cultures (Fett-Neto et al. 1994). The lactalbumin hydrolysate had no effect on alkaloid synthesis in Leonurus heterophylus Sw. suspension culture; however, the addition of l-proline increased alkaloid content significantly (Yang et al. 2008), definitely recognized as a stachydrine precursor (He and Wang 2005).
Established cultures expressed their morphogenetic capacity after removing aggregates to media lack of 2,4-D. Somatic embryos grown in clusters and then developed distorted cotyledons contained chlorophyll. However, typical bipolar structure has never observed. The reasons for such abnormalities may be disorders of polar auxin transport in the arranged embryo. It is essential for the formation of meristems and plant growth. Number of reviews and reports focused on this topic: Yeung and Stasolla (2000), Souter and Lindsey (2000), van Berkel et al. (2013), Chen et al. (2010), and Elhiti and Stasolla (2011). Strong embryogenesis initiator, 2.4-D, was accumulated in tissue, where it was slowly deactivated. Tissue showed secondary proliferation after removing it to the regeneration medium. Embryo-like structure placed on the surface of solid medium was enveloped with callus which hampered their growth and differentiation.
Hairy root cultures of marigold can be maintained in both, solid and liquid ½ MS media; however, liquid media obtain the fastest growth and possibility of analysis of triterpenic saponins released to the medium. The effect of nitrogen source on saponins accumulation and secretion in hairy roots of C. officinalis was reported for the first time. Lines selected for the evaluation of tenfold organic source of nitrogen (peptone from lactalbumin) showed different reactions depended additionally on mineral form of nitrogen used in media composition. Yu et al. (2000) reported that peptone, but in lower (300 mg L−1) concentration, gave a slight enhancement of ginsenosides synthesis for Panax ginseng hairy roots. This effect was confirmed for the bioreactor culture of P. ginseng reported by the same group (Sivakumar et al. 2005) without growth impairment.
Nitrogen, after the carbon and phosphorus, constitutes the basics components for plant growth and metabolism. Nitrate and ammonium salt being main sources of mineral nitrogen are known to have various influence on plant metabolite synthesis, transport, and distribution. Numerous reports indicate nitrate as a preferred form leading to increase rate of synthesis of important bioactive substances. Adventitious roots of P. ginseng in Yu et al. (2001) report and P. quinquefolium suspension culture (Zhong and Wang 1998) accumulated the highest amount of ginsenosides when nitrate ions were the sole source of nitrogen in cultivation medium. Similar conditions with low or complete absence of ammonium form intensified the synthesis of protopanaxadiol and protopanaxatriol (dammarane-type tetracyclic triterpenoids) derivatives in bioreactor hairy roots of P. quinquefolium (Kochan et al. 2016).
Nitrate/ammonium ratio seems to be fundamental factor, which is modified in numerous reports referring to plant micropropagation (Teixeira Da Silva 2013) or/and metabolite synthesis (Lee et al. 2011). As it was demonstrated in the current studies, the impact of this important macroelement should be determined individually for each genotype, type of in vitro culture and kind of metabolite. Nitrate as sole nitrogen source in the medium improved the growth rate of the Camptotheca acuminata cell culture; however, high ratio of ammonium:nitrate (5:1) was propitious for camptothecin (alkaloid, anticancer agent) accumulation (Pan et al. 2004). Shikonin, the first biotechnological product (dye, naphthoquinone derivative) obtained in industrial scale was promoted by reduced level of NH4+ and increased level of NO3− in Lithospermum erythrorhizon suspension culture (Fujita et al. 1981). Predominance of ammonium ions for nitrate had a positive impact on berberine—antibacterial agent (alkaloid)—production in cell suspension culture of Thalictrum minus (Nakagawa et al. 1984). Triterpenic saponins are metabolites without nitrogen in their structure, although their accumulation in plant tissue remains under the strong impact of nitrate/ammonium ratio in mineral form. Such situation was result of assimilation and growth processes, genome background, and evolutionary aspect connected with ammonium toxicity/tolerance syndrome. Some authors suggest the changes of pH inside the cell compartments in response to assimilation of ammonium or nitrate, and therefore, regulation of enzymes in the final steps of saponins pathway can be achieved (Kochan et al. 2016). Marigold was included to a NH4+-sensitive plant (Britto and Kronzucker 2002), what was confirmed for suspension and hairy root cultures. Roots which have high responsiveness to nitrate—activator of 10% of plant transcriptome (Wang et al. 2003)—make the most complex area, where multidimensional relationship in metabolism creation impede their control. From the biotechnological point of view, it can be described as finding the compromise between satisfactory growth and cost-effective content of desired metabolite.
Conclusions
In current report, we first evaluated the effect of different nitrogen sources on the growth and oleanolic acid glycosides production in C. officinalis hairy roots and suspension cultures. Both types of cultures preferred nitrate as a mineral nitrogen source or coexistence with ammonium at ½ MS ratio. Organic nitrogen source represented here by peptone from lactalbumin was crucial for suspension culture initiation; however, high concentration of this compound decreased saponins accumulation in suspension culture and growth rate in most of hairy root lines. Peptone effect on saponins accumulation and secretion in hairy root culture was depended on line, age of culture, and media composition. Elevated level of nitrate ions may increase rate of production of listed above metabolites in hairy roots, but the lines exhibited different toxicity levels of this macro element. Saponins secretion to the surrounding medium was generally harmonized with their accumulation inside the tissue; however, NO3−/NH4+ ratio manipulation generated almost sixfold intensification of this effect.
Author contribution statement
Conceived and designed the experiments: MD. Performed the experiments: MD. Analyzed the data: MD. Contributed reagents/materials/analysis tools: MD, MM, and CP. Wrote the paper: MD. All authors read and approved the final manuscript.
Abbreviations
- 2,4-D:
-
2,4-Dichlorophenoxyacetic acid
- SC:
-
Suspension culture
- HR:
-
Hairy root culture
- OA:
-
Oleanolic acid
- B:
-
Bud
- C:
-
Cotyledon
- H:
-
Hypocotyl
- R:
-
Root
- PCV:
-
Packed cell volume
- TLC:
-
Thin-layer chromatography
- GLC:
-
Gas–liquid chromatography
- FID:
-
Flame ionization detector
- MS:
-
Murashige and Skoog (1962) media
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Funding
This study was supported by the State Committee for Scientific Research (KBN) through the Faculty of Biology University of Warsaw Intramural Grants BW: 1755-13 and 501/86-100007.
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Communicated by A. Krolicka.
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Długosz, M., Markowski, M. & Pączkowski, C. Source of nitrogen as a factor limiting saponin production by hairy root and suspension cultures of Calendula officinalis L.. Acta Physiol Plant 40, 35 (2018). https://doi.org/10.1007/s11738-018-2610-2
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DOI: https://doi.org/10.1007/s11738-018-2610-2