Saponin synthesis and cotton growth is antagonistically regulated by solar UV-B radiation
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Earlier we have reported that the exclusion of solar UV-B increased the growth and yield of cotton plants as compared with ambient UV-B. The UV-B radiation effects on the saponins and the impact of ambient and reduced UV-B on the accumulation of saponins has not been investigated yet. Thus a field experiment was conducted to study the influence of solar UV-B on the growth response and saponin synthesis in cotton (Gossypium hirsutum) var. Vikram plants by the exclusion of UV-B. The cotton plants were grown in specially designed iron chambers, wrapped with filters that excluded UV-B (<315 nm), or transmitted ambient UV-B.
Exclusion of ambient UV-B enhanced the growth of cotton plants in terms of plant height and leaf area. Greater plant height in UV-B excluded plants was due to elongated internode and more number of nodes. Enhancement in growth was accompanied by a decrease in the accumulation of saponins, which was quantified by the spectrophotometric, TLC and HPLC methods. Solvent extraction of saponins from the internodes and leaves were used for the bioassay of Amaranthus hypocotyl growth and expansion of cucumber cotyledons. Extracts obtained from the UV-B excluded plants (leaves and internodes) promoted the growth to a larger extent as compared with the extracts obtained from ambient grown plants.
The result indicates that solar UV-B may possibly suppress the plant growth by regulating the synthesis of natural growth inhibitor’s like saponin.
KeywordsBioassay Cotton Growth Inhibitor Saponin UV radiation
Ultraviolet (UV)-B radiation (280–315 nm) is a natural component of sunlight. The amount of UV-B radiation reaching the Earth’s surface has increased over the last decade due to ozone depletion (Caldwell et al. 2003; McKenzie et al. 2011). Enhanced UV-B radiation can alter plant photosynthesis (Reddy et al. 2004), water metabolism (Fuhrer and Booker 2003) and the carbon partitioning from growth pools to secondary metabolic pathways (Bassman 2004).
The level of ambient UV-B radiation in sunlight varies with reference to latitude. Crop plants grown under tropical conditions receive approximately 50% higher dose of UV-B in the natural solar radiation compared with temperate regions due to small solar zenith angle and thin stratospheric ozone layer in tropics (Madronich et al. 1995; McKenzie et al. 2011). The impact of UV-B on plants is studied either by supplementation of UV-B with artificial light screen or by excluding the UV-B component from the solar spectrum using appropriate filters. Exclusion studies provide exact data on the impact of ambient UV-B on the plants. Enhancement of growth after the exclusion of UV-B component from the solar spectrum has been observed in plants like Amaranthus (Kataria and Guruprasad 2014), wheat (Kataria and Guruprasad 2012a, b), Cyamopsis and Vigna (Amudha et al. 2005), cucumber (Krizek and Mirecki 2004), cotton (Dehariya et al. 2012; Kataria et al. 2013) and soybean (Guruprasad et al. 2007; Baroniya et al. 2014; Zhang et al. 2014). Thus solar UV-B exclusion studies confirmed that ambient UV-B caused reduction in the plant height, internodal length and leaf area.
Saponin-triterpenoid glycosides are one of the most interesting groups of secondary metabolites. The saponins are a group of plant glycosides in which hydrophilic sugars are attached to alipophilic steroid or triterpenoid moiety. The growth inhibitory effects of triterpenoids saponins have been shown earlier using alfalfa seeds (Ohara and Ohira 2003). Three triterpenoids (betulin, betulinic acid and oleanolic acid) inhibited radical and hypocotyl growth in alfalfa seeds (Ohara and Ohira 2003). The inhibitory effects of triterpenoid saponins are thought to be attributed not to the property of their aglycons but to that of the whole of their molecules (Saha et al. 2010). Saponins are widely distributed in plants and involved in various biological activities such as antimicrobial, antitermitic, molluscicidol and anti-human immunodeficiency virus-1 (HIV-1) protease (Crombie et al. 1987; Marston and Hostettman 1987; Ohmura et al. 1997; Yang et al. 1999).
Furthermore, a few studies indicated a promoting effect of higher light intensities on saponin concentrations in plants (Mathur et al. 2000; Maulidiani et al. 2012). Besides flavonoids, the accumulation of other secondary compounds in response to UV-B exposure, probably act as UV-protectants (Zhang et al. 2009; Inostroza-Blancheteau et al. 2014). It was proposed that the saponins were increased by UV-B radiation (Afreen et al. 2005). Ambient UV-B also caused 70% increase in the saponins content of leaf extract of Coleus aromaticus as compared with the control (Kumari and Prasad 2014). However, findings are limited and even contradictory (Szakiel et al. 2011). Moreover, the impact of ambient and reduced UV-B on the accumulation of saponins has not yet been investigated. The objective of the present study was to extract the saponin and to analyze by bioassays as well as by TLC and HPLC from the cotton plants grown in the presence or in the absence of UV-B component of the solar spectrum. Cotton (Gossypium hirsutum), an important cash crop of India, is sensitive to UV-B radiation (Kakani et al. 2003). We present the results of the experiments in this paper that indicate the involvement of saponins as growth inhibitors and that UV-B components of the solar spectrum alter the saponin content in the plants.
Material and Methods
Plant material and growth conditions
Solar irradiance with and without UV-B was measured using a radiometer (Solar light Co. Inc. (PMA 2 100), Glenside, PA, USA) between 11:30 am and 12:00 pm during experimental period. The photosynthetic active radiation (PAR) during experimental period at midday was 1 450 μmol·m−2·s−1; the loss in light intensity at midday by −UV-B filters was 12.5% (1 270 μmol· m−2·s−1) and 4.2% (1 390 μmol·m−2·s−1) under polythene filter transmissible to UV (Filter Control).
Plant height, number of nodes, average internodal length and area of leaf (9th) were taken at 70 days after emergence (DAE) of seedlings. Area of leaf was taken by pressing the blotted dry leaf on the graph paper and tracing the exact outline. The mean of five leaves was taken as the average value. The calibration curve was prepared by weighing 0-1 000 mm2 area of graph paper.
Successive extraction method
Ethyl acetate layer in the final step was evaporated to dryness and dissolved in distilled water and used for the bioassays of longitudinal growth of Amaranthus hypocotyl and of expansion growth bioassay of cucumber cotyledons in darkness as well as in light.
Quantitative estimation of triterpenoids
The quantification of triterpenoids was determined by the modified method of Kolawole et al. (2006). Ethyl acetate fraction (2 mL) obtained from cotton leaf and an internodal segment (Control and –UV-B) was treated with 0.5 g of 2, 4-dinitrophenyl hydrazine dissolve in 100 mL of 2 mol·L-1 HCl. The orange coloration obtained due to the presence triterpenoids (saponin) and the absorbance was measured at 452 nm by a spectrophotometer (Shimadzu UV/Vis 1601). The amount of saponin was calculated as saponin equivalent from the calibration curve of standard saponin (100 to 1 000 μg·mL-1).
TLC analysis of the ethyl acetate fraction
Thin-layer chromatography of ethyl acetate fraction obtained by successive extraction from filter control and UV-B excluded leaves was carried out on a 10×10 cm (0.20 mm thick) silica gel plate (Merck Kieselgel 60 F254), using chloroform: ethanol: acetic acid (60:40:5 in volume of CHCl3, EtOH and AcOH) as a developing solvent. Plate was developed up to 7 cm from the starting line. Plate was sprayed with anisaldehyde- H2SO4 as a color reagent then heated (100 °C). Spots were observed under visible light (Cristian et al. 2005). After drying the plate, spots of all treatments (saponin Std, Control, -UV-B) at Rf 0.285 and these spots were scratched and dissolved in 50% methanol and UV spectra was taken at wavelength 200-700 nm in a UV/Vis spectrophotometer (Shimadzu 1601).
HPLC analysis of the ethyl acetate fraction
HPLC analysis of the ethyl acetate fraction of cotton leaves were performed with a Shimadzu HPLC system equipped with Phenomenex ‘Luna® 5 μm C18 100 Å, LC Column 250 × 4.6 mm’ column, LC10AT VP pumps, SCL-10AVP system controller, SIL-10AD VP auto injector, SPD-M10 AVP photodiode array detector and the data was processed using VP software.
For this method, the used mobile phase was a mixture of 0.05 mol·L-1 sodium sulphate buffer (pH 2.3) and acetonitrile (68.5: 31.5, in volume of sodium sulphate buffer and acetonitrile) at a flow rate of 1 mL·min-1 and the column temperature was maintained at 30 °C. The detection wavelength was set at 205 nm. The injection volume was 20 μL and the chromatography system was equilibrated by the mobile phase. The separation and quantification of the samples were conducted when the same retention time and peak areas of the repetitive injection of the standard solutions were obtained. The total run time was 75 min.
All the data are presented in triplicates (n=3) and the data are expressed as means ±S.E.M. and were analyzed by the analysis of variance followed by post hoc Newman-Keulis multiple comparison test by using Prism 4 software for Windows, Graf Pad Software, Inc., LaJolla, CA, USA.
UV exclusion and growth
Effect of exclusion of UV-B on number of nodes and internodal length of cotton seedlings var. Vikram
No. of nodes
17.6 ± 1.0
5.52± 0.6*** (137)
HPLC peak area and retention time of saponin in cotton leaves extracts
Peak area/arbitrary units
Comparison with control/%
27 728 515
18 664 129
Bioassays with standard saponin
The internodal extract inhibit Amaranthus hypocotyl growth
Leaf extract and cotyledon expansion
In light the cotyledon expansion was highly pronounced in the extracts obtained from the leaves of UV-B excluded plants (Fig. 9b), while the expansion growth was much lower in the extracts obtained from leaves of plant grown under ambient UV-B (FC). At higher concentrations, 20% (V/V) of the extracts obtained from UV-B excluded plants caused 59% increase in the expansion growth as compared with filter control (Fig. 9b).
Enhancement of growth in terms of plant height and leaf area after the exclusion of UV-B component of solar spectrum has been observed in several crop plants (Guruprasad et al. 2007; Dehariya et al. 2012; Baroniya et al. 2014; Zhang et al. 2014), which indicates that the small dose of UV-B in the natural solar radiation can make a significant photomorphogenic effect. In the present study, solar UV-B exclusion enhances both the longitudinal growth of stem as well as the expansion growth of the leaves in cotton plants as observed in other UV exclusion studies on soybean and cotton (Dehariya et al. 2012; Baroniya et al. 2014; Zhang et al. 2014).
Solar UV-B thus seems to primarily affect the photomorphogenic regulatory system of growth of roots, stem and leaves (Guruprasad et al. 2007; Kataria et al. 2013; Baroniya et al. 2014; Zhang et al. 2014). The inhibition of growth that can be induced with supplemental UV-B radiation was related to oxidation of auxin (Ballare et al. 1991; Jansen et al. 2001). UV-B could reduce cell expansion by changing turgor pressure or cell wall extensibility (Tevini and Iwanzik 1986) which suggested that direct oxidation of auxin and indole acetic acid (IAA) by UV-B resulted in reduction of cell wall expansion. IAA usually affects plant height by increasing cell numbers (through cell division). But it has been suggested that the elongation process was not through cell division, but rather through cell elongation, which is affected more by GA (Luo et al. 2006; Zhu et al. 2006). Similarly, the involvement of light induced synthesis of inhibitors of growth was reported in the regulation of elongation growth by white light in dicotyledonous seedlings (Hasegawa et al. 1989; Noguchi and Hashimoto 1990; Noguchi and Hashimoto 1997). There was no report relating any growth inhibitor specifically with UV-B induced inhibition of growth in plants.
UV-B stimulation of secondary metabolites has been reported in several studies, for example, phenolic compounds, surface flavonols (Cuadra et al. 1997), anthocyanins (Dubey and Guruprasad 1999), and terpenoids (Filella and Penuelas 1999; Zavala and Ravetta 2002). These compounds have been implicated both in plant’s defense (Chappell and Hahlbrock 1984) and protection against UV-light (Ziska et al.1992). Furthermore, Muller et al. (2013) found that ambient dose of UV-B and high PAR intensity distinctly affect the accumulation of flavonoids and saponins. Saponin content was found 70% higher in ambient grown plants than plants grown in growth chamber under UV-B excluded condition (Kumari and Prasad 2014).
Saponin content was higher in the leaves of cotton plants grown under ambient UV-B but lower in the UV-B excluded plants grown in the field conditions. It was also apparent by the results of the bioassays (hypocotyl and cotyledon expansion) performed in light as well as in dark; since kinetin induces the expansion growth of cucumber cotyledons in darkness and light grown plants responds to gibberellic acid (Narain and Laloraya 1974; Ray and Laloraya 1984). Our results indicated that growth of the hypocotyl and the cotyledon expansion were more in the extracts (leaves and internodes) obtained from the UV-B excluded cotton plants compared with the filter control plants. Phytochemical analysis of the leaf, stem and seed extracts of Cajanus cajan showed the higher amount of saponin content in leaves but not in stems (Sahu et al. 2014).
The results of the bioassay of the extracts, spectrophotometric analysis of saponin, overlay of UV spectra and the HPLC fractionation provide enough evidences to relate the biosynthesis of saponins to the UV-B induced inhibition of elongation as well as expansion growth in cotton plants. Results of the present study indicate that ambient UV-B may alter the metabolism to produce higher levels of secondary compounds which may act as inhibitors of growth. In general, exclusion of UV-B results in the reduction of several secondary metabolic products and UV absorbing substances (Kataria and Guruprasad 2014). In the present study, exclusion of UV enhances the expansion growth of leaves and elongation growth of plants by causing a reduction in the level of these natural growth inhibitors which is evident by performance of bioassay test like Amaranthus hypocotyl bioassay and cucumber cotyledons expansion. The quantification of saponins in the present study indicated a difference in the ethyl acetate fraction of the extract from plants grown under ambient UV-B and in the absence of UV-B. The ethyl acetate fraction obtained from UV-B excluded conditions caused significant promotion in both the hypocotyl length of Amarathus seedling as well as the expansion growth of cucumber cotyledons as compared with the fractions obtained from the filter control plants. Thus UV-B induced inhibition of growth in cotton is related to the level of saponin content in the tissues – at least partially.
In the absence of ambient UV, the reduced synthesis of secondary product, i.e. saponins, is probably associated with the enhancement of cotton plants growth. The solar UV-B inhibits growth of the plants by modulating the natural growth inhibitors and saponins are involved in this inhibition of growth as endogenous growth inhibitors. Saponins however may not be the only natural compounds responsible for inhibition of growth by UV-B, since UV-B modulates the biosynthesis of several secondary metabolic products.
Financial support by UGC Research Fellowship (F.4-1/2006 (BSR) to Dehariya P.) and Department of Science Technology Women Scientists-A Scheme (SR/WOS-A/LS-674/2013-2016) to Kataria S. are thankfully acknowledged.
Availability of data and materials
Data sharing not applicable to this article as no datasets were generated or analysed during the current study.
Dehariya P and Kataria S performed the experiments and analyzed the data; Guruprasad KN conceive and designed the experiments; Kataria S and Guruprasad KN wrote the paper and finalized the draft of MS. All authors read and approved the final manuscript.
Ethics approval and consent to participate
Consent for publication
The authors declare that they have no competing interests.
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