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. 2014 Dec 16;14:377. doi: 10.1186/s12870-014-0377-1

Monochromatic light increases anthocyanin content during fruit development in bilberry

Laura Zoratti 1,, Marian Sarala 1, Elisabete Carvalho 2,3, Katja Karppinen 1, Stefan Martens 3, Lara Giongo 3, Hely Häggman 1, Laura Jaakola 4,5
PMCID: PMC4274681  PMID: 25511869

Abstract

Background

Light is one of the most significant environmental factors affecting to the accumulation of flavonoids in fruits. The composition of the light spectrum has been shown to affect the production of phenolic compounds during fruit ripening. However, specific information on the biosynthesis of flavonoids in fruits in response to different wavelengths of light is still scarce. In the present study bilberry (Vaccinium myrtillus L.) fruits, which are known to be rich with anthocyanin compounds, were illuminated with blue, red, far-red or white light during the berry ripening process. Following the illumination, the composition of anthocyanins and other phenolic compounds was analysed at the mature ripening stage of fruits.

Results

All the three monochromatic light treatments had significant positive effect on the accumulation of total anthocyanins in ripe fruits compared to treatment with white light or plants kept in darkness. The elevated levels of anthocyanins were mainly due to a significant increase in the accumulation of delphinidin glycosides. A total of 33 anthocyanin compounds were detected in ripe bilberry fruits, of which six are novel in bilberry (cyanidin acetyl-3-O-galactose, malvidin acetyl-3-O-galactose, malvidin coumaroyl-3-O-galactose, malvidin coumaroyl-3-O-glucose, delphinidin coumaroyl-3-O-galactose, delphinidin coumaroyl-3-O-glucose).

Conclusions

Our results indicate that the spectral composition of light during berry development has significant effect on the flavonoid composition of ripe bilberry fruits.

Electronic supplementary material

The online version of this article (doi:10.1186/s12870-014-0377-1) contains supplementary material, which is available to authorized users.

Keywords: Light quality, Vaccinium myrtillus L, Flavonoids, Anthocyanins, Bilberry, Berries, UPLC-MS/MS

Background

Anthocyanins, a class of flavonoid compounds, are the main pigments found in many flowers and fruits, in which they act as insect and animal attractants and protect the plant from light oxidative stress [1]. Furthermore, these metabolites are powerful antioxidants and therefore shown to be beneficial for human health [2]. Several reports have focused on their effects in the prevention of neuronal and cardiovascular diseases, cancer and diabetes as well as in promoting human nutrition [2,3].

Bilberry (Vaccinium myrtillus L.) is among the most significant wild berry species in the Northern and Eastern Europe. Bilberry fruits are rich in phenolic acids, stilbenes and flavonoids, particularly in anthocyanins, which are estimated to represent nearly 90% of the total phenolics in these berries [4,5]. Anthocyanins are biosynthesized via the phenylpropanoid/flavonoid pathway consisting of a number of enzymatic steps that catalyze a sequential reaction leading to the production of different anthocyanidins including delphinidins (Dp), cyanidins (Cy), petunidins (Pt), peonidins (Pn) and malvidins (Mv) (Additional file 1). In bilberry fruits, the quantitative and qualitative composition of flavonoids is known to be strongly affected by the fruit developmental stage [6,7]. Bilberry fruits are known to accumulate high yields of various anthocyanins both in skin and flesh during the ripening period, although genetic and environmental factors are also reported to affect the final composition [8-10]. Two families of transcription factors, the bHLH and MYB proteins, are strongly associated in the regulation of the anthocyanin pathway [11,12]. The phenylpropanoid pathway responds to various environmental stimuli such as temperature, photoperiod, soil fertility [10,13,14] and light in particular [15,16].

Plants can sense multiple aspects of the light signals including light quantity (fluence), quality (wavelength), duration (photoperiod) and direction [17], which are perceived through at least four different families of photoreceptors, including phytochromes (red/far-red light receptors), cryptochromes and phototropins (blue light receptors) and UV-B photoreceptor (UVR8). These proteins perceive specific wavelengths of the visible light spectrum (380–740 nm) or the UV-light (280–315 nm) and transduce the signal to regulate photosynthesis, photomorphogenesis, phototropism, circadian rhythms as well as biosynthesis of secondary metabolites [18].

The induction of flavonoid and anthocyanin production by visible light has been extensively studied in several plant species, and it was found that the composition of light spectra regulated the biosynthesis of anthocyanins in Arabidopsis [19], cranberry (Vaccinium macrocarpon Ait.) [20], Gerbera [21], grape (Vitis vinifera L.) [22,23], lettuce (Lactuca sativa L.) [24], strawberry (Fragaria x ananassa -Weston- Duchesne ex Rozier) [25] and turnip (Brassica napus L.) [26]. A significant increase in the amount of phenolic compounds has been seen in bilberry plants grown under direct sunlight when compared to plants grown under forest canopy [9,15,27], but there is no information available on the effects of specific light wavelengths on their biosynthesis. Therefore, the aim of the present study was to analyze the influence of monochromatic wavelengths of the visible light spectrum on the production of phenolic compounds in bilberry fruit. Our particular interest was to study whether specific light wavelengths during berry development affect the biosynthesis and content of phenolic compounds. For this purpose, bilberry plants were illuminated with blue, red, far-red or white light during the berry ripening process and composition of the accumulated phenolic compounds was analyzed in ripe fruits. We also investigated the expression of key genes of bilberry flavonoid pathway in order to better understand the regulatory processes affecting biosynthesis of phenolic compounds during berry development.

Results

Characterization and quantification of phenolic compounds in ripe bilberry fruits

The phenolic compounds other than anthocyanins present in ripe bilberry fruits were analyzed by a UPLC-MS/MS method that has been earlier optimized for berry fruit species [28]. The phenolic compounds found in ripe bilberry fruits are listed in Table 1. The most abundant of those were hydroxycinnamic acids, namely chlorogenic acid and neochlorogenic acid. Naringenin (the precursor of flavonoid compounds) varied between 0.08 and 0.44 mg/100 g DW, and was present in much higher concentration in the glycosylated form (naringenin 7-O-glucoside) which, to our knowledge, is reported for the first time in bilberry in the present study. Also among stilbenes, (−)-astringin was detected in this study for the first time to our knowledge in bilberry fruits. The flavone luteolin 7-O-glucoside was found only in trace amounts.

Table 1.

Concentration of phenolic compounds (mg/100 g DW) detected in ripe bilberry fruits after monochromatic light treatment (n = 3)

Compound Blue Red Far-red White Dark
Av. SD St. Av. SD St. Av. SD St. Av. SD St. Av. SD St.
Neochlorogenic acid 80 35 129 29 105 27 8 27 96 21
Chlorogenic acid 113 59 207 67 162 58 117 50 135 36
Total hydroxycinnamic acids 193 94 96 24 168 55 133 40 100 24
Naringenin 0.3 0.2 0.4 0.2 0.2 0.1 0.2 0.06 0.2 0.1
Naringenin 7 glucoside** 82 26 70 9 69 7 50 17 68 29
Total flavanones 83 26 70 9 69 7 50 17 68 29
(−)-Astringin** 0.2 0.1 0.2 0.1 0.2 0.1 0.1 0.06 0.1 0.05
Total stilbenes 0.2 0.1 0.2 0.1 0.2 0.1 0.1 0.06 0.1 0.05
Kaempferol 3 rutinoside 4 1 4 2 5 1 4 2 4 3
Quercetin 3 glu 5 3 3 1 4 2 4 2 4 2
Quercetin 3 gal 9 3 b 17 2 a 15 10 a,b 17 4 a 21 12 a,b
Quercetin 3 glucuronide 35 1 46 9 28 9 42 5 36 3
Syringetin 3 gal + glu 4 2 6 6 4 2 4 0.5 3 0.9
Myricetin hexoses 7 2 b 12 1 a 12 1 a 5 1 b 8 3 b
Total flavonols 65 5 86 19 66 19 76 10 75 13
Catechin 1 0.8 0.6 0.3 2 1 1 0.4 0.7 0.3
Epicatechin 45 6 45 19 30 11 43 7 35 10
Epigallocatechin 11 1 10 4 9 5 13 6 11 3
Gallocatechin 15 1 14 5 12 6 17 7 14 4
Procyanidin A2 0.25 0.07 a 0.08 0.06 b 0.09 0.03 b 0.25 0.10 a 0.23 0.18 a
Procyanidin B1 0.08 0.10 b 0.15 0.12 b 0.13 0.12 b 0.24 0.02 a 0.11 0.08 b
Procyanidin B2/B4 0 0 1.32 1.32 0.41 0.36 0.23 0.23 0.32 0.32
Procyanidin B3 44 10 45 16 33 15 41 6 35 8
Total proanthocyanidins 116 16 117 43 86 37 116 19 96 21

glu = glucose, gal = galactose, Av. = average of three replicates, SD = standard deviation, St. = statistics.

The compounds marked with asterisk (**) are first time detected in bilberry fruits to present. Significant differences by Tukey HSD (P < 0.05) in response to the light treatments are marked by different letters for each compound and total amounts of compounds.

Ripe bilberries also contained flavonols, which included kaempferol 3-O-rutinoside, the quercetin derivatives (quercetin 3-O-glucose, quercetin 3-O-galactose, quercetin 3-O-glucuronide) and the myricetin derivatives (syringetin 3-O-glucose, syringetin 3-O-galactose and myricetin hexoses) in amounts comparable with earlier reports for bilberry [29].

The detected proanthocyanidins included monomers of catechin, epicatechin, epigallocatechin and gallocatechin. Among polymers, the most abundant was procyanidin B3 accompanied by lowers amounts of procyanidin A2, procyanidin B1, procyanidin B2 and/or B4 (which could not be separated using the present method [28]).

Characterization and quantification of anthocyanins in ripe bilberry fruits

Anthocyanins are the most abundant class of flavonoids present in ripe bilberry fruits. The anthocyanin content in ripe bilberry fruits was analyzed by a UPLC-MS/MS method which had been earlier optimized for grapevine [30]. The method was slightly modified to allow the detection of anthocyanidin galactosides and arabinosides that have earlier been described for bilberry (see Methods).

The total amount of anthocyanins in ripe berries varied between 1860 to 3397 mg/100 g DW, which is comparable with the amounts reported earlier for bilberry [6,8]. Altogether 33 anthocyanins were detected (Table 2), including the known 15 anthocyanins; Dp’s, Cy’s, Pt’s, Pn’s and Mv’s combined with the sugars glucose, galactose and arabinose [8,31]. In addition, acetylated and p-coumaroyl-binded forms of anthocyanins, Pg’s and Cy 3-O-sambubioside compounds were found. To our knowledge, some of the acetylated (Cy acetyl 3-O-galactose and Mv acetyl 3-O-galactose) and coumaroylated compounds (Dp coumaroyl 3-O-glucose, Dp coumaroyl 3-O-galactose, Mv coumaroyl 3-O-glucose, Mv coumaroyl 3-O-galactose) that were detected in this study have not been previously reported in bilberry fruits. Acetylated compounds were present in low amounts, with an average concentration between 0.05 to 0.72 mg/100 g DW for the single compound detected (Table 2). The amount of p-coumaroylated anthocyanins was generally higher than the acetylated forms, even though the presence of these forms was more variable between the replicate plants. The contents ranged from the lowest of Mv coumaroyl 3-O-galactose to the highest of Pn and Mv coumaroyl 3-O-glucoside. However, the concentration of Pn and Mv coumaroyl 3-O-glucoside was in the same range with the known anthocyanins including Pt 3-O-glucoside, Pt 3-O-galactose, Mv 3-O-glucoside, Mv 3-O-galactose, Mv 3-O-arabinose, Pn 3-O-glucoside, Pn 3-O-galactose and Pn 3-O-arabinose (Table 2). The amounts of Pg derivatives were low in bilberry fruits, 0.36 mg/100 g of Pg 3-O-glucoside and 0.11 mg/100 g DW of Pg 3-O-galactose, while Pg 3-O-arabinose was not detected. The presence of Cy 3-O-sambubioside has also previously been reported in bilberry by Du et al. [32] in similar amounts that were found in our study.

Table 2.

Concentration of anthocyanin compounds (mg/100 g DW) detected in ripe bilberry fruits after monochromatic light treatment (n = 3)

Compound Blue Red Far-red White Dark
Av. SD St. Av. SD St. Av. SD St. Av. SD St. Av. SD St.
Cy acetyl 3 glu 0.59 0.88 0.49 0.64 0.33 0.16 0.54 0.38 0.74 0.73
Pt acetyl 3 glu 0.10 0.09 0.12 0.10 0.08 0.01 0.07 0.06 0.26 0.45
Pn acetyl 3 glu 0.18 0.07 0.11 0.09 0.21 0.10 0.39 0.24 1.12 1.42
Mv acetyl 3 glu 0.35 0.30 0.43 0.50 1.04 0.53 0.75 0.24 4.54 4.54
Cy acetyl 3 gal** 0.10 0.18 0.13 0.12 0.17 0.16 0.32 0.19 0.59 0.56
Mv acetyl 3 gal** 0.17 0.11 0.17 0.05 0.34 0.16 0.26 0.12 0.52 0.52
Dp acetyl 3 glu 0.07 0.06 0.05 0.09 0.00 0.00 0.03 0.05 0.00 0.00
Cy coum 3 glu 10 3 8 7 11 4 9 5 24 27
Dp coum 3 glu** 1.8 0.3 2.4 1.4 1.6 1.6 0.72 0.10 2 2
Pn coum 3 glu 15 6 18 15 27 8 28 13 93 127
Mv coum 3 glu** 24 9 31 12 41 5 24 2 121 181
Cy coum 3 gal 3 1 4 0.6 4.5 0.7 5 2 7 6
Dp coum 3 gal** 0.88 0.37 0.87 0.34 1.21 0.25 0.64 0.15 0.57 0.38
Pn coum 3 gal 0.69 0.28 1.22 0.49 1.63 0.20 3.05 2.14 3.32 3.32
Mv coum 3 gal** 0.22 0.21 0.52 0.44 0.97 0.22 0.49 0.41 1.96 1.96
Cy sambubioside 2.4 0.48 2.3 1.9 1.46 0.49 1.91 1.21 2.36 1.99
Cy 3 glu 600 174 470 314 557 71 497 106 554 103
Dp 3 glu 1135 29 a 1306 310 a 1075 96 a 665 164 b 579 37 b
Pt 3 glu 24 5 a 28 1 a 25 6 a 15 2 b 18 2 b
Pl 3 glu 0.49 0.48 0.16 0.28 0.16 0.28 0.49 0.49 0.49 0.01
Mv 3 glu 47 1 59 16 69 21 41 14 57 16
Pn 3 glu 11 1 10 3 13 3 12 2 19 4
Cy 3 gal 214 44 250 48 248 44 212 44 197 17
Dp 3 gal 95 9 a 100 5 a 108 17 a 61 12 b 47 3 b
Pt 3 gal 31 5 b 42 4 a 43 5 a 25 6 b 22 1 b
Pl 3 gal 0.05 0.04 0.12 0.11 0.09 0.08 0.10 0.02 0.19 0.08
Mv 3 gal 14 2 b 31 10 a 33 16 a 16 4 b 20 5 a,b
Pn 3 gal 39 12 55 36 60 29 53 17 72 7
Cy 3 ara 159 42 193 35 152 39 162 16 145 27
Dp 3 ara 152 15 a 167 16 a 159 14 a 90 18 b 70 12 b
Pt 3 ara 43 7 a,b 64 10 a 57 10 a 35 6 b 32 11 b
Mv 3 ara 23 4 b 48 15 a 46 17 a 25 2 b 43 15 a
Pn 3 ara 11 3 16 8 18 12 13 5 17 8

glu = glucose, gal = galactose, ara = arabinose, coum = coumaroyl, Av. = average of three replicates, SD = standard deviation, St. = statistics.

The compounds marked with asterisk (**) are first time detected in bilberry fruits to present. Significant differences by Tukey HSD (P < 0.05) in response to the light treatments are marked by different letters for each compound.

Effect of monochromatic light on phenolic composition of ripe bilberry fruits

In order to investigate the effect of light quality on flavonoid accumulation in ripe berries, bilberry plants were treated with selected wavelengths of the visible light spectrum (blue, red, far-red or white light) during the fruit development process or left in the dark, as detailed in Figure 1. The effect of monochromatic light treatments during berry development on phenolic compounds in ripe berries is shown in Table 1. Significant variations (P < 0.05) were detected in flavonols and proanthocyanidin compounds for some of the light treatments. The level of quercetin 3-O-galactose was significantly (P < 0.05) lower in blue light treated plants compared with the other treatments. The levels of myricetin hexoses on the other hand were significantly higher under the red and far-red light treatments. On the contrary, the amounts of procyanidin A2 were lower under red and far-red light treatments, and procyanidin B1 level was higher under white light treatment compared with all the other light treatments.

Figure 1.

Figure 1

Design of light treatments and sample collections during the ripening process of bilberry fruits. Bilberry plants with unripe berries (developmental stage 2, about 2 weeks after pollination) were kept for 14 h in darkness (0 h sample) and then exposed to continuous blue, red, far-red or white light for 48 h. A set of plants left in continuous darkness (dark treatment) for 48 h represented negative control. After the light treatments, plants were grown in greenhouse under natural photoperiod and controlled temperature (21 ± 1°C) until ripening of fruits (developmental stage 6).

Monochromatic light affects anthocyanin composition of ripe bilberry fruits

The most prominent effect of monochromatic light treatments was seen on anthocyanin content. Figure 2 shows the effect of light treatments on the total amount of each class of anthocyanidins (Dp, Cy, Pn, Mv, Pt, Pg) calculated from the sum of the individual anthocyanin glycosides (Table 2). From the results it is evident that the content of Cy and Pn was not affected by the light treatments, whereas Dp, Mv and Pt showed a significant (P < 0.05) increase (33%, 46% and 38%, respectively) in berries of the plants treated with monochromatic light wavelengths when compared to the berries of the plants grown in white light conditions, suggesting that light quality affects the flavonoid pathway. The content of Mv showed a different behavior than Dp and Pt content; the concentration of Mv was significantly higher (P < 0.05) in berries left in dark than under any of the light treatments (Figure 2). Table 2 shows effect of each of the light treatments on the accumulation of specific anthocyanin compounds. Red and far-red light treatment increased Dp, Mv and Pt compounds conjugated with glucose, galactose and arabinose sugars, but had no effect on the acylated and coumaroylated compounds. The same increase was induced by blue light, with the exception of Pt 3-O-galactose, Pt 3-O-arabinose, Mv 3-O-galactose and Mv 3-O-arabinose.

Figure 2.

Figure 2

Concentration of anthocyanidin classes in ripe bilberry fruits treated with different light wavelengths (blue, red, far-red or white) or in dark conditions (n = 3). Pg’s are not reported here due to their low amounts compared to the other classes of anthocyanidins (Dp, Cy, Pt, Pn, Mv). For each class of anthocyanidin and the total amount of anthocyanins, significant differences by Tukey HSD (P < 0.05) in response to the light treatments are marked by different letters.

The expression of flavonoid pathway genes VmCHS, VmF3′5′H, VmDFR, VmANS and VmANR, and the transcription factor VmMYB2 were also measured during the monochromatic light treatments at the stage of immature berries. The most of the examined genes showed increase in their expression during the first 12 hours of the study in the plants treated with monochromatic light compared with plants kept in darkness or under white light, even though variation between samples and time points was high (Additional file 2). However, VmANS showed the evident increase in the expression after 24 and 48 hours under monochromatic light when compared to dark treated plants. On the contrary, under white light, the expression was not increased compared to dark treated plants. Monochromatic light continued to up-regulate the expression of VmANS over dark treated plants throughout the light treatment until 48 h, when the gene was increased up to 3-, 2- and 3.5-folds under blue, red and far-red light treatments, respectively, compared to dark treated plants. Under white light, the expression was only slightly increased (up to 1.3-fold) compared to dark treated plants (Additional file 2).

Discussion

Recent studies have shown that bilberry populations growing at northern latitudes contain higher amounts of flavonoids, in particular anthocyanins, in comparison to the southern populations [8,9]. The phenomenon is known to be under strong genetic control [9] even though environmental factors may also be involved in the regulation. Solar radiation is one of these factors, and it is known to increase the expression of the flavonoid biosynthesis genes and the content of flavonoids in bilberry leaves [15,31]. Moreover, higher amounts of anthocyanins were found in bilberry fruits grown in controlled conditions in a phytotrone in 24 h natural daylight, mimicking the light conditions of Arctic summers [10]. In the present study, the total anthocyanin content in ripe berries was significantly increased by monochromatic lights of blue, red and far-red, in comparison to fruits treated with white light or kept in darkness (Figure 2). Various effects of monochromatic light wavelengths on anthocyanin biosynthesis have also been reported in other species. For example, in turnip hypocotyls, far-red light had the most prominent effect on anthocyanin biosynthesis, comparable with the amount reached under sunlight [26]. In Gerbera, anthocyanin accumulation in flowers was particularly stimulated by blue light [21]. Blue light has been found to significantly increase the biosynthesis of anthocyanins also in fruit species, such as strawberries [25] and grape fruits [22,23], while in cranberry fruits, red and far-red light increased the anthocyanin accumulation over white light [20].

A possible explanation of the present results can be found from the gene expression analyses of flavonoid pathway genes. The expression of the genes VmCHS, VmF3′5′H, VmDFR and VmANR was less influenced by the light treatments (Additional file 2), which was consistent with the detected levels of flavanones, flavonols, stilbenes and proanthocyanidins in the berries kept under different light treatments (Table 1). Moreover, in earlier studies it has been shown that flavonoid pathway genes, for instance CHS, can have a diurnal rhythm [33,34]. This is one factor that can have affected the variation in the gene expression results between the different time points. On the contrary, the expression of VmANS, which is the key gene in the biosynthesis of anthocyanins, shows a clear increasing trend under monochromatic light treatments, while white light and dark treatment does not have influence. Blue, red and far-red light all up-regulated the expression of VmANS already within the first 6 h after the beginning of the light treatment and also throughout the 2-day treatment (Additional file 2). According to Jaakola et al. [7], VmANS is expressed only at a very low level in bilberry fruits at the early stage of fruit development. However, the early stages of berry development appeared to be reactive to the light treatments in the present study. Monochromatic light treatments affected the accumulation of anthocyanins by increasing the expression of VmANS already at this early stage of berry development.

The higher amount of total anthocyanins in bilberry fruits in response to monochromatic light wavelengths was due to the increased production of Dp’s and Pt’s over Cy’s and Pn’s (Table 2, Figure 2). In the present study, the bilberry plants originated at the 65°N latitude and the amounts of Cy’s and Dp’s produced in plants treated with monochromatic lights were similar to the studies in which berries were grown in natural environment at similar latitudes (64°N [9] and 66°N [10]). Plants kept under white light or in darkness, showed a significant decrease in the content of Dp’s, indicating that the spectral composition of light is involved in the accumulation of this class of anthocyanidins. Considering that in northern latitudes, summer nights are characterized by long twilight with high ratios of blue and far-red light [35], the present study emphasizes that northern light environment promote the accumulation of anthocyanins in bilberry already at the early stages of fruit ripening, by inducing qualitative and quantitative changes in anthocyanin content of ripe fruits.

Conclusions

We showed that the treatment of bilberry plants under monochromatic light wavelengths of the visible light spectrum, for even short times during the ripening period of the fruits, is enough to induce a significant increase in the anthocyanin content in ripe fruits. Moreover, the quality of light affected particularly the biosynthesis of delphinidin glycosides. Our results indicate that the spectral composition of light regulates the accumulation of anthocyanins in fruits, showing an interaction between the flavonoid biosynthetic pathway and the composition of the light spectrum received by the plant.

Methods

Plant material

Bilberry (Vaccinium myrtillus L.) plants were harvested from three different locations I-III (I: 65° 06′ N, 25° 5′ E; II: 65° 04′ N, 25° 31′ E; III: 65° 03′ N, 25° 28′ E) in forest stands in Finland. Plants were collected, in each location, within an area of 10 m x 10 m, assuming that the plants within this area belonged to the same genetic background [36] and thus represented specific ecotypes. Plants were collected at the stage when their fruits were small and green, presenting developmental stage 2 (Figure 1). Plants were harvested with their root system and were placed in boxes (50 cm × 70 cm) containing forest peat soil.

After pollination, berries take usually six to seven weeks to ripe in natural stands of Finland. Bilberry fruit ripening stages were identified according to Jaakola et al. [6] and are presented in Figure 1. Developmental stage 2 represented small green unripe berries of 3 to 4 mm in size, approximately two weeks after pollination (end of June). At ripeness (developmental stage 6), which occurs about six weeks after pollination (end of July), the berries were 6 to 8 mm in diameter and turned to dark blue.

Light sources

Selador led lamps by PALETTA™ (BMI supply, Queensbury, NY, USA) were used to irradiate plants with blue (400–500 nm), red (600–700 nm), far-red (700–800 nm) and white light (400–800 nm, Figure 3) wavelengths. The plants irradiated under blue light received a photon fluence rate of 8.10 μmol m−2 s−1, under red 7.8 μmol m−2 s−1, under far-red 7.6 μmol m−2 s−1 and under white 43.04 μmol m−2 s−1. Plants exposed to white light were considered as a positive control. A set of plants kept in total darkness was considered as negative control. Light measurements were conducted by using USB RAD+ spectroradiometer (Ocean Optics Inc., Dunedin, FL, USA).

Figure 3.

Figure 3

Light spectra used for the 48 h light treatment experiments in bilberry plant. White, 400–800 nm; blue, 400–500 nm; red, 600–700 nm; and far-red, 700–800 nm.

Light treatments and sample collection

Bilberry plants were treated with each specific light wavelength during the berry ripening period, as shown in Figure 1. Pools of bilberry plants from each location (I-III), were used for the treatments. Plants holding berries at stage 2, were initially kept in darkness for 14 h and then exposed to the continuous blue, red, far-red or white light induction or placed to darkness for 48 h (Figure 1). The berry developmental stage 2 was selected for the experiments based on preliminary analyses (data not shown) which indicated stage 2 to be the most reactive one, among all the bilberry fruit ripening stages, in the expression of flavonoid pathway genes in response to the light illumination. The light treatments were conducted in growth chambers with controlled temperature (21 ± 1°C) and humidity (60%) to erase the effect of temperature on flavonoid biosynthesis. After the light treatment, growth of plants was conducted in greenhouse under controlled temperature condition (21 ± 1°C) and natural photoperiod. When fully ripened (stage 6, Figure 1), the berries were harvested and stored at −80°C before freeze-dried within six months. The light treatments did not affect the process of ripening of the berries. Freeze-dried berries were stored in a desiccator at −20°C until analysed for metabolic compounds.

Metabolic analyses

The ground material (100 mg out of 3 g) of each sample was extracted with 1.5 mL of 80% methanol on shaking for 1 h. Samples were centrifuged at 12000 g for 2 min (Sigma 3-30 k, Osterode, Germany) and the supernatants were collected. The extraction was repeated and the supernatants were combined and brought to a volume of 5 mL. After filtering (0.22 μm PVDF filters) and transferring to glass vials, the samples were randomized and analyzed for anthocyanins, flavonols, proanthocyanidins, stilbenes and other phenolic compounds by UPLC-MS/MS.

Analysis of phenolic compounds

Flavonols, flavanones, hydroxycinnamic acids, proanthocyanidins and stilbenes were analysed as described in Vrhovsek et al. [28]. Chromatography, mass spectrometry conditions and multiple reaction monitoring (MRM) transitions can be found in the referred literature. Quantification was made by external calibration curves, injecting authentic standards of each of the detected compounds at different concentrations.

Analysis of anthocyanins

Anthocyanins were analysed by using UPLC-MS/MS as described by Arapitsas et al. [30]. Anthocyanins were detected by MRM, by screening the MS/MS transitions and using the parameters described in Additional file 3. For some of the compounds, there were no standards available, but they could be tentatively identified on the basis of their MRM transitions and the relative retention time, in respect to known compounds and considering previous results [37]. For example, standards of the galactoside derivatives of cyanidin and peonidin were available, and these compounds seem to elute before but closely to the respective glucoside derivatives (peaks 1, 2 and 22, 23 in Additional file 3). As such, the peak eluting 0.15 seconds before malvidin glucoside showing the same MRM transition is likely to be malvidin galactose (peak 15 in Additional file 3), and this reasoning can also be applied to the other galactoside and arabinoside derivatives.

For quantification, external calibration curves were prepared by injecting authentic standards of each compound at different concentrations. In case the authentic standard was not available, the anthocyanins were quantified relative to malvidin-3-O-glucose, using the malvidin-3-O-glucose calibration curve (Additional file 3).

Statistical analysis

The effect of the light treatment on every metabolite analyzed in the berries was tested with One-way ANOVA. Multiple comparisons were made by Tukey HSD’s post-hoc test. The tests were performed using STATISTICA version 12.

Supplementary analyses

A supplementary study was conducted in order to study if the increased amount of anthocyanins was related to the gene expression of flavonoid pathway genes in bilberries (Additional file 1). Bilberry plants from locations I and II, with berries at developmental stage 2, were initially kept in darkness for 14 h (0 h sample) and then exposed to the continuous blue, red, far-red or white light induction or placed to darkness for 48 h. During the light treatment, berry samples were collected for RNA isolation after 0, 6, 12, 24 and 48 h of treatment. Samples were immediately stored at −80°C until analysed for gene expression.

Isolation of RNA and cDNA preparation

Total RNA was isolated from bilberry fruits at stage 2 that were collected after 0, 6, 12, 24 and 48 h from the beginning of the light treatments. The RNA was isolated according to the method of Jaakola et al. [38] with the exception that the phenol-chloroform extraction was substituted with the RNA purification protocol in E.Z.N.A.® Total RNA Kit I (Omega Bio-Tek, Norcross, GA, USA). The quality of the isolated RNA was verified by measuring the absorbance spectrum with NanoDrop N-1000 spectrophotometer (NanoDrop Technologies, Thermo Scientific, Wilmington, DE, USA) and on a 1% (w/v) ethidium bromide-stained agarose gel. RNA was converted to cDNA with RevertAid Premium Reverse Transcriptase (Thermo Scientific) in accordance with the manufacturer’s instruction. RNA extraction (and further gene expression analyses) was repeated twice for each set of plants.

Gene expression analysis

Transcript accumulation of the genes VmCHS, VmF3′5′H, VmDFR, VmANS and VmANR, and the transcription factor VmMYB2 was detected using the LightCycler SYBR Green qPCR Kit (Roche Applied Sciences, Indianapolis, IN, USA). The primers used for the amplification are listed in Additional file 4.

Analyses with qPCR were performed with a LightCycler 2.0 instrument and software (Roche). The PCR conditions were 95°C for 10 min, followed by 45 cycles of 95°C for 10 s, 60°C for 20 s, and 72°C for 10 s. VmACT gene (Additional file 4) was used as a reference gene for relative quantification. Differential gene expression levels were calculated by comparing each of treatments to treatment 0 h.

Acknowledgements

Our special thanks to Matti Rauman, for his professionalism and for the great contribution to this project by setting up the light systems. Kone Foundation (to LJ), the Finnish Doctoral Program in Plant Biology and the STSM (Short Term Scientific Program) program within the COST action FA1006 (PlantEngine) (to LZ) are acknowledged for the financial support.

Abbreviations

UPLC-MS/MS

Ultra performance liquid chromatography – tandem mass spectrometer

Dp

Delphinidin

Cy

Cyanidin

Pt

Petunidin

Pn

Peonidin

Mv

Malvidin

Pg

Pelargonidin

Glu

Glucose

Gal

Galactose

Ara

Arabinose

Coum

Coumaroyl

DW

Dry weight

VmCHS

Vaccinium myrtillus chalcone synthase

VmF3′5′H

Vaccinium myrtillus flavonoid 3′5′-hydroxylase

VmDFR

Vaccinium myrtillus dihydroflavonol 4-reductase

VmANS

Vaccinium myrtillus anthocyanidin synthase

VmANR

Vaccinium myrtillus anthocyanidin reductase

VmMYB2

Vaccinium myrtillus MYB2 transcription factor

VmACT

Vaccinium myrtillus actin

MRM

Multiple reaction monitoring

Additional files

Additional file 1: (78.8KB, png)

The flavonoid biosynthetic pathway of bilberry with particular emphasis on anthocyanin classes. Enzymes for each step are shown in capitals. Enzymes required for flavonoid synthesis; PAL, phenylalanine ammonia-lyase; C4H, cinnamate 4-hydroxylase; 4CL, 4-coumaroyl:CoA ligase; CHS, chalcone synthase; CHI, chalcone isomerase; F3H, flavanone 3′-hydroxylase; F3′ H, flavonoid 3′-hydroxylase; F3′5′ H, flavonoid 3′,5′-hydroxylase; FLS, flavonol synthase; DFR, dihydroflavonol 4-reductase; ANS, anthocyanidin synthase; ANR, anthocyanidin reductase; UFGT, UDP glucose-flavonoid 3-O-glucosyl transferase; MT, methyltransferase. The transcript levels of the genes CHS, F3′5′ H, DFR, ANS and ANR (in the figure marked with a square) was analyzed in response to the exposure to different light wavelengths.

Additional file 2: (490.9KB, png)

Relative transcript abundance of the flavonoid pathway genes VmCHS, VmF3′ 5H, VmDFR, VmANS and VmANR, and the transcription factor VmMYB2 in bilberry fruits (at stage 2) after 6, 12, 24 and 48 h under different light conditions. Data represent average and SD values of samples collected from two locations (see Methods).

Additional file 3: (62KB, doc)

UPLC-MS/MS data for anthocyanin quantification. In case of two MRM transitions for a given compound, the first was used as quantifier and the second as qualifier. RT = retention time, CV = cone voltage, CE = collision energy, Std = standard curve.

Additional file 4: (30.5KB, doc)

Sequences of the primers used in qPCR to determine gene transcripts.

Footnotes

Competing interests

The authors declare that they have no competing interests.

Authors’ contributions

LZ performed most of the experimental work together with interpretation of data, was involved in the design of the work, and most of writing and editing; MS contributed in performing the experiment and gene expression analyses; EC gave support with the metabolic analyses and contribution to the interpretation of the data; KK, SM and LG gave contribution with the interpretation of the data; LJ and HH provided contribution to the conception and the design of the work. All authors attended to the writing of the manuscript and read and approved the final manuscript.

Contributor Information

Laura Zoratti, Email: laura.zoratti@oulu.fi.

Marian Sarala, Email: marian.sarala@posti.talonetti.fi.

Elisabete Carvalho, Email: elisabete.carvalho@rhul.ac.uk.

Katja Karppinen, Email: katja.karppinen@oulu.fi.

Stefan Martens, Email: stefan.martens@fmach.it.

Lara Giongo, Email: lara.giongo@fmach.it.

Hely Häggman, Email: hely.haggman@oulu.fi.

Laura Jaakola, Email: laura.jaakola@uit.no.

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