A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 207 Changes in content of major phenolic compounds during leaf development of sea buckthorn (Hippophaë rhamnoides L.) Anne Morgenstern1,2 , Anders Ekholm1, Petra Scheewe2 and Kimmo Rumpunen2,* 1Swedish University of Agricultural Sciences, Department of Plant Breeding, Balsgård, Fjälkestadsvägen 459, 291 94 Kristianstad, Sweden 2 Hochschule für Technik und Wirtschaft Dresden (University of Applied Sciences), Faculty of Agriculture and Landscape Management, Pillnitzer Platz 2, 01326 Dresden, Germany * e-mail: kimmo.rumpunen@slu.se Content of total phenolic compounds and antioxidant capacity (FRAP) were investigated in the leaves of three sea buckthorn (Hippophaë rhamnoides L.) cultivars: ‘Otradnaja’, ‘Gibrid Pertjika’ and ‘Ljubitelskaja’, at different dates. In addition, major phenolic compounds (catechin, kaempferol, quercetin, epigallocatechin, kaempferol-3-O-glu- coside, quercetin-3-O-galactoside, isorhamnetin-3-O-glucoside, rutin, gallic acid, procyanidin monomer glycoside, procyanidin dimer aglycone and hydrolyzable tannins I–III) were determined in ‘Ljubitelskaja’. Antioxidant capacity and the content of total phenolic compounds fluctuated during April, May and June, and then increased until the end of July, when the highest values were observed. Total phenolic compounds were strongly correlated with FRAP. Levels were generally higher in ‘Ljubitelskaja’ than in ‘Otradnaja’ and ‘Gibrid Pertjika’. In ‘Ljubitelskaja’, hydrolyzable tannins I–III occurred in higher amounts than did any of the other studied phenolic compounds. The developmen- tal stage of the leaves (harvesting date) had a strong influence on content of phenolic compounds and should be carefully considered when harvesting sea buckthorn leaves for different purposes. Key words: antioxidant capacity, flavonoids, FRAP, polyphenols, tannins Introduction Sea buckthorn (Hippophaë L.) belongs to the family Elaeagnaceae. The most widely distributed species, H. rham- noides, occurs in Central and Northern regions of Europe and Asia, and is divided into eight subspecies (Swenson and Bartish 2003). The plant is a thorny shrub, which can reach approx. six meters in height. About 90% of the genetic resources are located in China, but northern India, Russia and Mongolia are also rich in sea buckthorn (Singh 2003, Erkkola and Yang 2003, Ruan et al. 2013). The sun-loving plant grows in mountainous and coastal ar- eas on well-drained soils, and it is well adapted to dry conditions. Sea buckthorn is often used as a pioneer plant to counteract soil erosion and to improve soil fertility through its N 2 fixation capacity (Singh 2003, Qinxiao and Hongyan 2003). These features, together with the valuable fruits, make sea buckthorn an interesting multipur- pose crop for sustainable agriculture. Sea buckthorn fruits are important sources of vitamins, natural antioxidants, oils, triterpenes and other bioac- tive substances (Singh 2006, Geetha et al. 2002, Tsybikova et al. 2006). Both fruits (Rösch et al. 2003) and leaves (Yoshida et al. 1991, Heinäaho et al. 2006, Zu et al. 2006, Moilanen et al. 2013) are rich in polyphenols, and are part of Asian traditional medicine for treatment of, e.g., skin disorders (Upadhyay et al. 2011, Erkkola and Yang, 2003). Beneficial effects of sea buckthorn fruits have been documented through in vitro studies, animal trials and clinical intervention studies. Thus sea buckthorn pulp oil can inhibit platelet aggregation (Johansson et al. 2000), improve atopic dermatitis (Yang et al. 1999) and alleviate symptoms connected with dry eyes (Larmo et al. 2010) in humans. Sea buckthorn puree can lower the plasma high-sensitivity c-reactive protein level (Larmo et al. 2008), which is a marker for inflammation and a risk factor for cardiovascular disease. Furthermore, ethanol-soluble com- ponents of sea buckthorn fruits have been shown to affect postprandial hyperglycemia and insulin response (Le- htonen et al. 2010a) and the beneficial flavonols of sea buckthorn berries have proven to be highly bioavailable (Larmo et al. 2009, Lehtonen et al. 2010b). Manuscript received January 2014 A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 208 In addition to fruits, also sea buckthorn leaves have potential beneficial effects. In animal models an aqueous ex- tract of sea buckthorn leaves has shown adaptogenic properties (Saggu et al. 2007, Saggu and Kumar 2008) and has proven especially efficient for wound healing (Upadhyay et al. 2011), an effect that in part may be attributed to extractable polyphenols (Upadhyay et al. 2010). In vitro studies have, in addition to anti-inflammatory (Jayashan- kar et al. 2012) and free radical scavenging effects (Padwad et al. 2006), revealed strong anti-viral (Tolkachev and Sheichenko 2006, Jain et al. 2008) and α-glucosidase inhibitory effects (Kim et al. 2011) of leaf extracts that also may be attributed to the content of polyphenols. Detailed knowledge about factors influencing the content of sea buckthorn leaf phytochemicals is therefore much needed. Effects of different organic farming methods on the content of phenolic compounds in sea buckthorn leaves have previously been investigated on cultivars of H. rhamnoides subsp. rhamnoides (Heinäaho et al. 2006). Arimboor et al. (2008) studied the content of phenolic acids in leaves of H. rhamnoides subsp. turkestanica and Rongfu et al. (2003) studied the seasonal changes in content of total flavones in leaves of H. rhamnoides subsp. sinensis. In this study we investigate the influence of development stage of sea buckthorn leaves of H. rhamnoides hybrid cultivars on the total antioxidant capacity, total phenolic compounds, and on the content of major single pheno- lic compounds. Material and methods Plant material Leaf samples were collected from three sea buckthorn (H. rhamnoides) cultivars (‘Gibrid Pertjika’, ‘Otradnaja’ and ‘Ljubitelskaja’) of Russian origin grown at Balsgård, Kristianstad, in the south of Sweden. The plants were grown in a randomized field trial in three blocks, surrounded by H. rhamnoides seedlings as border plants. Each block contained nine plants per cultivar, and the trial was planted in 1997. The plants were not pruned, irrigated or fer- tilized during the sampling period. Grass was used as mulch. The leaves were sampled on eight occasions at an interval of two weeks from the end of April to the end of July in 2007: April 23, May 7, May 21, June 4, June 18, July 2, July 16 and July 30. On each sampling date, 12 leaves from each of two plants per cultivar and block were sampled to obtain a repre- sentative sample. Leaves were picked from the middle part of the branches. All samples of a cultivar were then pooled before subsampling for biochemical analyses. Measurements and preparation of leaves Leaf length was measured, and the fresh and dry weight was determined (in triplicates) before and after freeze-dry- ing. Dry matter of leaves was calculated, and the freeze-dried leaves were then milled to a fine powder with an IKA® type A10 mill, the powder was stored frozen at −20 °C until used for analyses of total antioxidant capacity and total phenolic compounds. For ‘Ljubitelskaja’ major single phenolic compounds were also analyzed. FRAP analysis of antioxidant capacity Analysis of antioxidant capacity was undertaken with the FRAP (Ferric Reducing Ability of Plasma) method accord- ing to Benzie and Strain (1996) with minor modifications. Leaf powder (25 mg) was extracted in duplicate with 1 ml of 90% MeOH. After a 15 min extraction in ultrasonic bath the samples were centrifuged for 10 min. The super- natant was then diluted 50 times by mixing an aliquot of 20 µl with 980 µl of 90% MeOH. A reagent solution was prepared as follows: 100 ml of acetate buffer solution (pH 3.61) was mixed with 10 ml of 2, 4, 6-Tris(2-pyridyl)-s- triazine (TPTZ) solution and 10 ml of iron(III) chloride hexahydrate (Fe3+) solution. The TPTZ solution consisted of 312 mg of TPTZ powder (Fluka) mixed with 100 ml of 40 mM HCl (30%, Suprapur®, Merck) in an ultrasonic bath for 3 min. A 20 mM Fe³+ solution was made from iron(III) chloride hexahydrate (Fluka) and a stock solution of 2 mM Fe2+ was made from iron(II) sulfate heptahydrate (Fluka) using distilled water. Then standards of 800, 400 and 200 µM Fe2+ solutions were prepared. Absorbance was recorded at 593 nm following a 240 s reaction period. The re- agent solution was kept in a water bath at 37 °C during the whole time. For analysis, 1 ml of the reagent solution was put into a 10 × 4 × 45 mm cuvette set in a Shimadzu (UV-2101PC) spectrophotometer, 10 µl of the standard solution or the sample were then added and mixed with the reagent solution in the cuvette. Each diluted sample was analyzed in triplicate against a blank that contained only the reagent. A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 209 Total phenolic compounds analysis Total phenolic compounds analysis (TP) was conducted with Folin–Ciocalteu’s reagent (BDH) according to Single- ton and Rosst (1965) with minor modifications. Leaf powder (25 mg) was extracted in duplicates with 1 ml of 50% EtOH (containing 0.338% of orthophosphoric acid), ultrasonicated for 15 min and centrifuged for 10 min. Then the extracts were diluted four times by mixing an aliquot of 250 µl with 750 µl of 50% EtOH solution. Next, 10 µl of each diluted extract was mixed with 100 µl of 5% aqueous EtOH, 2 ml of 15% sodium carbonate monohy- drate (175.05 g l-1 of Na 2 CO 3 •H 2 O), 200 µl of Folin–Ciocalteu’s phenol reagent and 1 ml of distilled water in a 10 x 10 x 45 mm cuvette. The samples were kept at room temperature for 2 h before spectrophotometric analysis. A standard stock solution of 705 µM gallic acid in 5% EtOH was prepared and diluted to make a 5 point standard curve for quantification. Absorbance was recorded at 765 nm using a Shimadzu (UV-2101PC) spectrophotometer. Standards and samples were analyzed in triplicates. The total content of phenolic compounds was quantified as gallic acid equivalents (GAE). HPLC-MS analysis of major single phenolic compounds For the HPLC-MS analysis of major single phenolic compounds samples were extracted in triplicates using the same procedure as for total phenolic compounds analysis and samples were kept at −20 °C until use. All extracts were diluted 20 times before analysis. Standards (Extrasynthèse, France) were prepared as follows. First, a standard mix A (StM A) was prepared: catechin, epicatechin, rutin and gallic acid were dissolved in 100% EtOH to obtain con- centrations of 82.5, 70.6, 47.4 and 65.1 µg/ml, respectively. Single standards of epigallocatechin, isorhamnetin, isorhamnetin-3-O-glucoside, kaempferol and kaempferol-3-O-glucoside, were also dissolved in 100% EtOH to ob- tain concentrations of 6.6, 5.6, 10.0, 9.6, 4.0, 6.44 and 9.78 µg/ml, respectively. After that, 0.1 ml of each single standard was mixed with 0.3 ml of StM A to obtain standard mix B (StM B). StM B was then diluted ten times with 50% EtOH and used for analysis. HPLC-MS analyses of major single phenolic compounds were undertaken with an API 150 EX Turbo Ionspray mass spectrometer according to a slightly modified method of Salminen et al. (1999). The HPLC system consisted of a Perkin Elmer 200 autosampler, two Perkin Elmer LC-200 Micro pumps, a guard column LiChroCART 4-4 100 RP-18 (5 µm) and a column LiChroCART 75-4 Superspher 100 RP-18. Injection volume was 8 µl. Elution was carried out at a flow rate of 1 ml min-1. The binary mobile phase consisted of (A) 0.4% for- mic acid and (B) MeCN (acetonitrile). The gradient elution profile was 0% B for 3 min, then from 3 to 30 min it was gradually increased to 30%, from 30 to 35 min gradually increased to 40%, and was then kept steady until 38 min when it was gradually decreased to 0% until 42.5 min. The mass spectrometer was operated in a negative mode. Mass spectra were obtained between 125 and 2250 amu. The nebulizer gas and the curtain gas were 9 and 12 ml min-1, respectively. Temperature was 300 °C and ion spray voltage (IS) was -4000. In the scan mode the orifice plate potential, the focusing ring potential and the entrance potential were -35 V, -220 V and -8.5 V, respective- ly. Based on initial tests in total 23 [M–H]- ions (m/z 169.1, 285.1, 289.1, 301.2, 305.2, 315.2, 435.2, 441.2, 447.3, 451.2, 457.4, 463.4, 477.4, 577.2, 593.4, 609.5, 623.5, 739.3, 901.2, 935.5, 937.2, 953.5, 1109.5) were selected for the HPLC-MS analysis. Of these reliable results could be obtained for 14 ions. The hydrolyzable tannins were quantified as gallic acid equivalents (GAE) since no other standards were available. For the same reason the pro- cyanidin monomer glycoside and procyanidin dimer aglycone were quantified as catechin equivalents. Querce- tin-3-O-galactoside and quercetin were quantified as rutin. Statistical analyses For chemical analyses a coefficient of variation (CV) of maximum 5% was allowed among replicates of a sample. In case of higher variation a new analysis was made. For statistical analysis a one-way ANOVA (analysis of variance) with a post-hoc LSD (least significant difference)- test was carried out using the program STATISTICA. Correlation analyses were performed by the software Microsoft Excel between antioxidant capacity (FRAP analysis) and total phenolic compounds (TP analysis) results, using average values of the three cultivars at each sampling date. The p-value used for reported statistical significance is 0.05. A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 210 Results Leaf length and dry matter Leaf length of the three studied cultivars increased 2–3 cm in every two weeks from the end of April until the be- ginning of June (Fig. 1). After this, leaf growth slowed down and almost stopped in the middle of July, reaching an average final leaf length of approximately 10 cm. Leaves were initially longer in ‘Otradnaja’ but ‘Ljubitelskaja’ had the longest leaves from the beginning of June to the end of the sampling period. Leaf dry matter content varied during the sampling period for all three cultivars, with comparatively low values between the end of May and the beginning of July (lowest average dry matter content for the three cultivars was less than 28% of fresh weight). After that, values increased until the end of July when the highest average dry mat- ter content reached almost 32%. The studied cultivars showed only minor differences in leaf dry matter develop- ment. Thus, leaves of ‘Otradnaja’ and ‘Gibrid Pertjika’ developed approximately in the same way, except for the last two sampling dates when dry matter of ‘Gibrid Pertjika’ increased more and reached almost 35%. Dry matter content of ‘Ljubitelskaja’ decreased from the end of April to the middle of June and then increased again in July to a final dry matter content of about 31%. Total phenolic compounds (TP) analysis The total content of phenolic compounds (average of single results for all cultivars) varied significantly during the sampling period (Fig. 2). Steady values on April 23 and May 7 (155 and 157 mg GAE/g dw, respectively) were fol- lowed by the lowest value on May 21 (122 mg GAE/g dw). After this, a small increase on June 4 (142 mg GAE/g dw) was followed by a larger increase on July 16 and July 30 (to 176 and 185 mg GAE/g dw, respectively). Pair- wise comparisons showed a significant decrease and increase before and after May 21, respectively. A significant increase was also found between July 2 and July 16. Total phenolic compounds results of the last two sampling dates differed significantly from results at all other dates but not from each other. The content of total phenolic compounds varied only slightly between the cultivars (Table 1). Cultivar ‘Ljubitelska- ja’ had the highest content of total phenolic compounds at five out of eight sampling occasions. Fig. 1. Length of sea buckthorn leaves at different sampling dates for cvs. ‘Otradnaja’, ‘Gibrid Pertjika’and ‘Ljubitelskaja’. Error bars represent standard deviation (n=12). A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 211 !" #!" $!!" $#!" %!!" %#!" &!!" '()*+"%&" ,-."/" ,-."%$" 0123"4" 0123"$5" 01+."%" 01+."$6" 01+."&!" 78'9":;;<+"73%=>$!!"?"@AB" 9C32<+*D"D<;(<12@E":;?"F'G>?"@AB" Table 1. Antioxidant capacity (FRAP analysis, n=2) and content of total phenols (Folin-Ciocalteu analysis, n=2) in sea buckthorn leaves for each sampling date and cultivar. For each analysis the average and standard deviation is presented (dw = dry weight, GAE = gallic acid equivalent). Analysis Cultivar April 23 May 7 May 21 June 4 June 18 July 2 July 16 July 30 Antioxidant capacity ‘Otradnaja’ 176 ± 3 189 ± 7 147 ± 4 174 ± 3 203 ± 2 200 ± 3 216 ± 1 234 ± 1 (mmol Fe2+/100g dw) ‘Gibrid Pertjika’ 167 ± 7 189 ± 5 152 ± 3 195 ± 5 197 ± 1 208 ± 2 221 ± 5 226 ± 2 ‘Ljubitelskaja’ 181 ± 4 223 ± 5 145 ± 2 211 ± 2 194 ± 2 219 ± 4 239 ± 1 276 ± 4 Phenols ‘Otradnaja’ 154 ± 8 151 ± 4 125 ± 4 135 ± 3 148 ± 4 140 ± 2 172 ± 5 183 ± 1 (mg GAE g-1 dw) ‘Gibrid Pertjika’ 154 ± 0 153 ± 5 125 ± 1 146 ± 1 143 ± 2 143 ± 4 176 ± 8 171 ± 7 ‘Ljubitelskaja’ 158 ± 2 168 ± 3 118 ± 2 147 ± 6 140 ± 1 151 ± 1 183 ± 6 203 ± 4 FRAP analysis of antioxidant capacity Average content of total antioxidants for the three cultivars varied significantly between the sampling dates when determined by FRAP analysis (Fig. 2). Thus, the content increased from about 175 to 200 mmol/100 g dw from April 23 to May 7, followed by a large decrease on May 21 when values reached a minimum (148 mmol/100 g dw). From June 4 to July 30, values increased steadily from 193 to 246 mmol/100 g dw. The average FRAP value on the last sampling date (July 30) was significantly higher compared to all other dates, except for July 16. There were only minor differences in antioxidant capacity between the cultivars, ‘Otradnaja’ and ‘Gibrid Pertjika’ being more similar compared to ‘Ljubitelskaja’. Cultivar ‘Ljubitelskaja’ had the highest FRAP values six out of eight sampling occasions. Antioxidant capacity and the content of total phenolic compounds of the sea buckthorn leaves developed simi- larly during the sampling period. The correlation coefficient (r) for antioxidant capacity and total phenolic com- pounds was 0.864. Fig. 2. Antioxidant capacity (FRAP analysis) and content of total phenolic compounds (Folin-Ciocalteu analysis) of sea buckthorn leaves (averages for separate samples of cvs ‘Otradnaja’, ‘Gibrid Pertjika’ and ‘Ljubitelskaja’). GAE = gallic acid equivalents. Error bars represent standard deviation. A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 212 HPLC-MS analysis of major single phenolic compounds HPLC-MS chromatograms of all standards used and a representative chromatogram of a sample based on all ions selected are presented in Figure 3. Chromatograms for each ion that was extracted and quantified are shown in Figure 4. A B Fig. 3. MS traces based on 23 [M–H]- ions shown for A) a representative leaf sample of cv. ‘Ljubitelskaja’ (July 2) and B) for the standards that were used for identification and quantification. For the standards the retention times are also presented. A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 213 Fig. 4. MS traces of a leaf sample of cv ‘Ljubitelskaja’ for A) catechin (m/z 289.1, rt 13.0), B) kaempferol (m/z 285.1, rt 31.7), C) quercetin (m/z 301.2, rt 20.7), D) epigallocatechin (m/z 305.2, rt 12.7), E) kaempferol-3-O-glucoside (m/z 447.3, rt 22.7), F) quercetin-3-O- galactoside (m/z 463.4, rt 20.9), G) isorhamnetin-3-O-glucoside (m/z 477.4, rt 23.0), H) rutin (m/z 609.5, rt 20.4), I) gallic acid (m/z 169.1, rt 4.9), J) procyanidin monomer glycoside (m/z 451.2, rt 12.2), K) procyanidin dimer aglycone (m/z 577.2, rt 12.4), L) hydrolyzable tannin I (m/z 935.5, rt 14.2, double peak), M) hydrolyzable tannin II (m/z 953.5, rt 14.6) and N) hydrolyzable tannin III (m/z 935.5, rt 17.8). A B C D E F G H I J K L M N A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 214 The content of each of the major single phenolic compounds quantified in leaves of `Ljubitelskaja` varied among sampling dates (except for kaempferol) but in different directions (Table 2). The content of catechin (m/z 289.1, rt 13.0) did not change from April 23 to May 7, but decreased on May 21 followed by a continuous increase for the rest of the sampling period. A higher content than on any other date was obtained on July 30 (958 µg g-1 dw). The content of kaempferol (m/z 285.1, rt 31.7) was lower than the content of most of the other studied phenolic compounds, fluctuating between 2.8 and 4.3 µg g-1 dw throughout the sampling period. In contrast, the content of quercetin (m/z 301.2, rt 20.7) was high, with a steady increase from April to July, and the highest content was obtained on July 30 (1381 µg g-1 dw). The highest content of epigallocatechin (m/z 305.2, rt 12.7) with 48 µg g-1 dw was already reached on April 23. Levels decreased in May and then slightly increased to the end of July reaching 26 µg g-1 dw. The highest content of kaempferol-3-O-glucoside (m/z 447.3, rt 22.7) was also reached at the two earliest sam- pling dates (101 and 104 µg g-1 dw, respectively). Subsequently, kaempferol-3-O-glucoside decreased until the end of the sampling period reaching 56 µg g-1 dw at July 30. The content of quercetin-3-O-galactoside (m/z 463.4, rt 20.9) decreased similar as the content of kaemp- ferol-3-O-glucoside. The highest content was noted for April 23 (458 µg g-1 dw) and the lowest on July 16 (199 µg g-1 dw). The content of isorhamnetin-3-O-glucoside (m/z 477.4, rt 23.0) was more or less the same during the sampling period. The highest content was reached at the last sampling dates (342 and 339 µg g-1 dw on July 16 and 30, re- spectively). In contrast, the content of rutin (m/z 609.5, rt 20.4) decreased considerably during the sampling period. The high- est content was reached on April 23 (1310 µg g-1 dw). Then the content decreased, and the lowest content was obtained in the middle of July (387 µg g-1 dw). Also the content of gallic acid (m/z 169.1, rt 4.9) decreased almost 10 times during the sampling period with the lowest content being reached at the last sampling date (39 µg g-1 dw). The content of procyanidin monomer glycoside (m/z 451.2, rt 12.2) instead increased largely from April 23 (5 µg g-1 dw) to July 30 (383 µg g-1 dw). Also the content of procyanidin dimer aglycone (m/z 577.2, rt 12.4) increased during the sampling period and reached a maximum on July 30 (205 µg g-1 dw). Hydrolyzable tannins I-III occurred in higher amounts than any other of the studied phenolic compounds. From a minimum on April 23 (1321 µg g-1 dw), hydrolyzable tannin I (m/z 935.5, rt 14.2, double peak) increased especial- ly at the beginning and middle parts of the sampling period, reaching its highest level on July 2 (9809 µg g-1 dw), and remaining approximately at the same level afterwards. The content of hydrolyzable tannin II (m/z 953.5, rt 14.6) fluctuated during the entire sampling period, with sig- nificant increases and decreases. The highest content was found on June 4 (10643 µg g-1 dw) and the lowest on April 23 (4304 µg g-1 dw). Following an initial increase from April 23 to May 7 (5882 and 8944 µg g-1 dw, respectively), hydrolyzable tannin III (m/z 935.5, rt 17.8) mainly decreased towards the end of the sampling period. The lowest content (1789 µg g-1 dw) was noticed for July 16. A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 215 Table 2. Catechin, kaempferol, quercetin (quantified as rutin), epigallocatechin, kaempferol-3-O-glucoside, quercetin-3-O-galactoside (quantified as rutin), isorhamnetin-3-O-glucoside, rutin, gallic acid, procyanidin monomer glycoside and procyanidin dimer aglycone (quantified as catechin) as well as hydrolyzable tannins I-III (quantified as gallic acid) (HPLC-MS analysis) in sea buckthorn leaves of ‘Ljubitelskaja’ for each sampling date, respectively. For each compound the average (in µg/g dry weight) and standard deviation (n=3) is presented. Compound April 23 May 7 May 21 June 4 June 18 July 2 July 16 July 30 Catechin 521 ± 30 548 ± 20 191 ± 7 282 ± 34 449 ± 38 595 ± 38 698 ± 103 958 ± 344 Kaempferol 2.8 ± 0.5 4.2 ± 1.0 3.5 ± 0.4 3.3 ± 0.7 2.8 ± 0.3 4.3 ± 0.8 4.2 ± 0.4 4.1 ± 0.2 Quercetin 332 ± 22 809 ± 42 939 ± 27 1145 ± 99 1138 ± 97 1358 ± 228 1243 ± 41 1381 ± 107 Epigallocatechin 48 ± 6 41 ± 3 13 ± 4 17 ± 3 14 ± 1 22 ± 1 23 ± 2 26 ± 2 Kaempferol-3- O-glucoside 101 ± 10 104 ± 13 85 ± 5 75 ± 4 69 ± 6 70 ± 8 54 ± 3 56 ± 4 Quercetin-3- O-galactoside 458 ± 5 440 ± 46 373 ± 14 217 ± 11 230 ± 13 221 ± 18 199 ± 16 205 ± 21 Isorhamnetin-3- O-glucoside 254 ± 12 293 ± 32 282 ± 13 227 ± 11 271 ± 14 308 ± 56 342 ± 23 339 ± 9 Rutin 1310 ± 144 1270 ± 182 993 ± 74 711 ± 28 543 ± 38 545 ± 72 387 ± 18 471 ± 20 Gallic acid 304 ± 5 267 ± 13 381 ± 2 293 ± 8 170 ± 10 72 ± 1 47 ± 2 39 ± 1 Procyanidin monomer glycoside 5 ± 1 9 ± 3 17 ± 4 57 ± 2 157 ± 15 250 ± 6 346 ± 8 383 ± 26 Procyanidin dimer aglycone 38 ± 5 51 ± 6 16 ± 4 35 ± 14 62 ± 11 95 ± 8 137 ± 24 205 ± 109 Hydrolyzable tannin I 1321 ± 145 3693 ± 526 2249 ± 112 7635 ± 1062 7842 ± 731 9809 ± 832 9737 ± 929 9753 ± 790 Hydrolyzable tannin II 4304 ± 601 9273 ± 1189 4772 ± 297 10643 ± 925 6153 ± 666 7770 ± 595 6143 ± 686 7495 ± 793 Hydrolyzable tannin III 5882 ± 709 8944 ± 1415 5108 ± 533 5061 ± 790 2595 ± 459 2854 ± 259 1789 ± 230 2640 ± 306 Discussion Changing content during leaf development Dry matter content of the sea buckthorn leaves fluctuated during the entire sampling period. Beside genetic ef- fects, precipitation and rate of leaf assimilation have probably contributed to these findings. In general, rainy weather is expected to result in lower dry matter content but in our study, dry matter increased to the highest values in July despite heavy rainfalls. The precipitation in April, May, June and July was 18, 45, 129 and 232 mm respectively (official data for Kristianstad, obtained from the Swedish Meteorological and Hydrological Institute). Furthermore, during July leaf growth (cell elongation) almost stopped. Since mature foliage leaves usually have higher assimilation rates compared to younger leaves, increased leaf maturation is the likely explanation to the increased content of dry matter towards the end of the sampling period. Contents of total phenolic compounds and the antioxidant capacity values were highest in July, and thus accom- panied the simultaneous increase in dry matter content. The highly significant correlations between antioxidant capacity and content of phenolic compounds are in agreement with previously published results (Singh 2006). A few studies have previously reported about the content of total flavonoids and total flavones in sea buckthorn leaves, which the present study did not investigate. Sea buckthorn leaves contain about 3.8–4% of total flavonoids (Singh 2006, Tsybikova et al. 2006), and plants growing in the west Pamirs had flavonoid contents ranging from 310 to 1238 mg/100g dry weight in the leaves (Singh 2006). Since these studies do not mention harvesting dates, a comparison with the results in the present study is difficult. Rongfu et al. (2003) however studied the influence of leaf developmental stage on total flavones in sea buckthorn leaves. Total flavones in H. rhamnoides of ssp. sin- ensis was reported to reach maximum levels during May–July, and then decreased from September onwards, to reach a minimum in the autumn. A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 216 Growing conditions and plant defense Environmental factors such as different field management practices have previously been reported to influence the content of antioxidant and phenolic substances in sea buckthorn leaves. Heinäaho et al. (2006) found that the content of phenolic compounds was significantly lower when plants were mulched with plastic compared to organic mulch treatments, e.g., conifer chips. In general, more phenolic compounds were produced when plants were grown on a flat surface compared to plants grown on low hills formed by an excavator. The flat ground was less aerated, and less solar heat was present, so that growing conditions were worse compared to the low hills. More phenolic substances, especially tannins, were produced, and it was suggested that this increase in phenol synthesis was caused by environmental stress to the plants. In the present study, plants were grown on a flat sur- face and no fertilizer or irrigation was used which may have favored production of a wider variety of plant phe- nolic compounds. The single phenolic compounds analyzed in our study showed much variation in contents from April to July, probably due to differences in synthesis, metabolism and functions in the plant. This may indicate that single phenolic compounds are produced by the plant when there is a need. The antioxidant capacity and the content of phenolic substances may also have been influenced by pollutants or pests, since plants can form antioxidants and phenolic substances as a defense under stressful conditions. Mayr et al. (1997) investigated the phenolic compounds of apples and their relationship to resistance against the fun- gal disease apple scab, and found that leaves and fruits of resistant genotypes contained higher flavanol contents than leaves and fruits of non-resistant genotypes, with phenol biosynthesis obviously being important in the ex- pression of resistance. The major phenolic compounds investigated by HPLC-MS analysis in our study were dominated by the hydrolyz- able tannins, which occurred in much higher amounts in sea buckthorn leaves compared to the other major phe- nolic compounds studied. Plant tannins have complex structures and can therefore be difficult to characterize and quantify. Based on mass number and fragments, hydrolyzable tannin I (m/z 935.5, rt 14.2, which occurred as a double peak in our analyzes) according to literature tentatively could be a mixture of stachyurin and casuarinin previously reported to be present in sea buckthorn leaves (Moilanen et al. 2013, Yoshida et al. 1991). Hydrolyz- able tannin III (m/z 935.5, rt 17.8) could tentatively be casuarictin. For hydrolyzable tannin II (m/z 953.5, rt 14.6) we have found no matching information in the published literature. Tannins are mainly located in the green parts of the sea buckthorn plant (Sheichenko and Tolachev 2006). Heinäa- ho et al. (2006) found that hydrolyzable and condensed tannins were the dominant phenolic groups in sea buck- thorn leaves. Tsybikova et al. (2006) and Singh (2006) referred to studies that reported about 10–15% tannins in leaves, 20–35% tannins in green shoots and only 0.13% tannins in fruits. During early growth of leaves, strictinin and isostrictinin were the predecessors of more complex tannins such as casuarinin, casuarictin and hippophaenin B, being accumulated in the later phases of growth. Maximum tannin content was found in the middle of July (Sheichenko and Tolachev 2006), which coincides approximately with the maximum of hydrolyzable tannin I (m/z 935.5, rt 14.2) in the present study. However, Sheichenko and Tolachev (2006) reported about the total tannin contents, whereas only some selected major tannins were investigated in the present study (HPLC-MS analysis). Besides, in our study not all tannins had their maximum content in July. The content of hydrolyzable tannin II (m/z 953.5, rt 14.6) and III (m/z 935.5, rt17.8) was highest in the beginning of May. Tannins are produced by many plant species as a chemical weapon against herbivores that avoid plants or parts of plants with high tannin contents. Since sea buckthorn plants in general contain high amounts of different tannins, these may constitute an important defense system against attacks of herbivores, such as Cacopsylla hippophaës Foerster (a psyllid), Capitophorus hippophaës Walker (an aphid) or Eriophyes hippophaënus Nalepa (a mite) all of which were found in the field where plants were harvested for leaves in our study. A G R I C U LT U R A L A N D F O O D S C I E N C E A. Morgenstern et al. (2014) 23: 207–219 217 Genetic variation When single phenolic compounds in the leaves were analyzed we found that quercetin and hydrolyzable tannins were present in the highest amounts. This confirms the results of Rongfu et al. (2003) who found that quercetin was the main component of total flavones in H. rhamnoides leaves, while isorhamnetin constituted 64% of the total flavones in H. tibetana leaves. Kaempferol content was higher in the original Chinese material of H. rham- noides of ssp. sinensis, than in the introduced Russian forms (Rongfu et al. 2003). The content of phenolic com- pounds thus seems to vary among species and subspecies, but there is also variation in phenolic content among different cultivars of the same species as revealed in the present study. In most cases during the sampling period, ‘Ljubitelskaja’ had higher total antioxidant capacity and total phenol content than ‘Otradnaja’ and ‘Gibrid Pertjika’. Cultivar ‘Ljubitelskaja’ was therefore used for a detailed HPLC-MS analysis. All three cultivars investigated in this study, are Russian hybrids between subsp. mongolica and subsp. rhamnoides. When analyzed with DNA markers (RAPD) together with a set of 52 other cultivars and hybrids of sea buckthorn, these three occurred in the same main cluster together with other hybrids and a few representatives of the paren- tal subspecies (Bartish et al. 2001). However, while ‘Otradnaja’ and ‘Gibrid Pertjika’ were relatively close together also in a more narrowly defined subcluster, ‘Ljubitelskaja’ belonged to a different subcluster indicating that it is less closely related to the other two. Similarly, in our study ‘Ljubitelskaja’ was relatively more dissimilar in leaf size and chemical contents (higher antioxidant capacity at four out of eight dates, and higher total phenol content at two dates) compared to the other two cultivars that rarely differed. Conclusions Total antioxidant capacity and content of total phenolic compounds in sea buckthorn leaves increased during leaf development, and were highest at the end of July when the last sampling was undertaken. However if maximum levels of single major phenolic compounds are desired due to specific bioactive benefits, the content of each sin- gle phenolic compound must be considered since not every compound had its maximum in fully developed leaves. 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Simultaneous determination of catechin, rutin, quercetin kaempferol and isorhamnetin in the extract of sea buckthorn (Hippophae rhamnoides L.) leaves by RP-HPLC with DAD. Journal of Pharmaceutical and Biomedical Analysis 41: 714–719. Changes in content of major phenolic compounds during leafdevelopment of sea buckthorn (Hippophaë rhamnoides L.) Introduction Material and methods Plant material Measurements and preparation of leaves FRAP analysis of antioxidant capacity Total phenolic compounds analysis HPLC-MS analysis of major single phenolic compounds Statistical analyses Results Leaf length and dry matter Total phenolic compounds (TP) analysis FRAP analysis of antioxidant capacity HPLC-MS analysis of major single phenolic compounds Discussion Changing content during leaf development Growing conditions and plant defense Genetic variation Conclusions Acknowledgements References