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Improved stability of blueberry juice anthocyanins by acidification and refrigeration

Abstract

BACKGROUND: Blueberry anthocyanins are susceptible to degradation during juice processing and storage of juice at ambient temperature. Methods are needed to stabilize the health-promoting anthocyanins in blueberry and other anthocyanin-rich berry juices.

OBJECTIVE: In this study we determined the effect of acidification (pH 2.1, 2.5 and 2.9) of blueberry juice on changes in anthocyanins and percent polymeric color in response to juice processing and during eight months of storage at ambient and refrigerated temperatures.

METHODS: Three subsamples of non-pasteurized blueberry juice were adjusted to three pH levels: 2.9 (control, no pH adjustment), 2.5, and 2.1. After pH adjustment, juices were pasteurized and placed in storage at 4 and 25°C. Samples were analyzed before (non-pasteurized) and after pasteurization, and after 2, 4, 6, and 8 months of storage at each temperature (4 and 25°C) for anthocyanin composition by HPLC and percent polymeric color.

RESULTS: Blueberry juice acidified to pH 2.1 retained higher levels of total anthocyanins and had lower percent polymeric color values than juice acidified to pH 2.5 and control juice (pH 2.9) following pasteurization. Anthocyanin arabinosides were more susceptible to thermal degradation than glucosides, galactosides and acetylated derivatives. Levels of total anthocyanins declined markedly over 8 months of storage, but juices stored at 4°C had on average 56% higher levels of total anthocyanins than juices stored at 25°C. Juice acidified to pH 2.1 had on average 12% and 26% higher levels of total anthocyanins than pH 2.5 and control juices, respectively. After 8 months of storage, juice acidified to pH 2.1 had 11 and 22% higher levels of total anthocyanins than pH 2.5 and control juices stored at 4°C, and 26% and 59% higher levels of total anthocyanins than pH 2.5 and control juices stored at 25°C. Acetylated derivatives were more prone to losses during storage than glycosides, especially in acidified juices.

CONCLUSIONS: Acidification of blueberry juice coupled with refrigerated storage are effective treatments to retain health-promoting anthocyanins.

Abbreviations

Ace

acetyl

Ara

arabinoside

Cyd

cyanidin

Dpd

delphinidin

Gal

galactoside

Glu

glucoside

Pnd

peonidin

Ptd

petunidin

Mvd

malvidin

1Introduction

Blueberries are a popular functional food due to their abundant levels of health-promoting polyphenols. The berries are exceptionally rich in anthocyanins, procyanidins and hydroxycinnamic acids and they also contain moderate levels of flavonols [1–3]. The high polyphenol content of the berries is responsible for the high free radical scavenging capacity measured in various in vitro assays [4–6]. In addition to protection against oxidative stress [7], the polyphenols in blueberries are known to exhibit a variety of biological properties including anti-inflammation, anti-cancer, anti-heart disease and anti-aging protection [8, 9] and may play an important role in protection against a number of chronic diseases.

Fresh blueberries are susceptible to decay and have a limited shelf-life, hence they are commonly processed into various shelf-stable products including juices, jams, jellies, syrups, purees and berries canned in water or syrup. Unfortunately, processing has been shown to have a detrimental effect on blueberry polyphenols. Juice processing in particular has been shown to markedly reduce levels of blueberry anthocyanins [10–12] as a result of enzymatic degradation, physical removal of skins during pressing, and thermal treatments. In addition to losses during processing, anthocyanins readily decline during ambient temperature storage and are accompanied by increased polymeric color value values [12–14]. Several researchers have investigated ways to improve retention of anthocyanins during blueberry juice processing. Blanching blueberries prior to mashing has been shown to result in greater retention of anthocyanins due to inactivation of polyphenol oxidase [11, 15–17]. Other factors such as pasteurization time and temperature, oxygen, light and pH have also been shown to influence anthocyanin retention in blueberry juice [18, 19]. Although the mechanism(s) responsible for anthocyanin losses during storage of blueberry juice are unknown, refrigeration has been shown to ameliorate losses [20, 21].

The stability and color of anthocyanins is strongly impacted by pH. Under acidic conditions (pH of 2 or less) anthocyanins exist in the flavylium cation form and possess a red or orange color, but as the pH increases above 3 hydration of the flavylium cation occurs giving rise to a colorless carbinol pseudo-base, which following ring opening is converted to the unstable chalcone pseudo-base [22]. Consistent with the scheme proposed by Brouillard [22] standard solutions of petanin and cyanidin 3-glucoside in pH 1.0, 2.4 and 3.1 buffers exhibited 90% or greater color stability over 60 days storage at 10°C [23]. Acidification of blueberry juice may be a viable treatment to prevent anthocyanin losses during processing and storage.

The objective of this study was to determine how acidification of blueberry juice (natural pH of 2.9) to pH 2.5 and 2.1 impacts anthocyanin composition and percent polymeric color during processing and over eight months of storage at ambient and refrigerated temperatures.

2Materials and methods

2.1Materials and juice processing

Blueberries (cv. ‘Bluecrop’) harvested at the fully ripe stage were obtained from a commercial grower in Fayetteville, AR. The fruit were stored at –20°C for less than two weeks prior to juice processing. Formic acid, citric acid, HPLC grade methanol, and potassium metabisulfite were obtained from Sigma Chemical Company (St. Louis, MO). A mixture of anthocyanin delphinidin, cyanidin, petunidin, peonidin, pelargonidin and malvidin glucosides was obtained from Polyphenols Laboratories AS (Sandnes, Norway).

Blueberries were processed into non-clarified juice using protocol previously described [12]. After measuring the pH of blueberry juice (2.9), we decided to acidify the other two treatments to pH values of 2.5 and 2.1 to determine if a high acid environment could afford protection against degradation of anthocyanins during pasteurization and juice storage. Three subsamples of juice were adjusted to three pH levels 2.9 (control, no pH adjustment), and 2.5, and 2.1 by drop-wise addition of a saturated (73%) citric acid solution. After pH adjustment, the pH 2.5 and 2.9 juices were adjusted with water to the same volume as the pH 2.1 juice. Juices were filled into 170 mL glass bottles and pasteurized by heating in a steam box (American Sterilizer Co., Erie, Pa) until the juice temperature monitored using a thermocouple reached 90°C (∼90 sec). The bottle caps were then tightened and the juices were allowed to cool overnight. Samples of each juice treatment were stored in the dark at 4 and 25°C. Samples (3 bottles/treatment) were analyzed before (non-pasteurized) and after pasteurization, and after 2, 4, 6, and 8 months of storage at each temperature (4 and 25°C).

2.2HPLC-PDA and HPLC-MS analysis of anthocyanins

Juice samples were passed through 0.45×um PTFE syringe filters (Varian, Inc., Palo Alto, CA) prior to HPLC analysis. The anthocyanins were separated on a 250×4.6 mm Symmetry C18® column (Waters Corp., Milford, MA) using the conditions detailed in Cho et al. [2]. The mobile phase included a linear gradient of 5% formic acid in water (A) and methanol (B) from 2% B to 60% B for 60 min at a flow rate of 1 mL/min. The anthocyanin peaks were monitored at 510 nm using a Waters Model 996 photodiode array detector. Individual cyanidin, delphinidin, peonidin, petunidin, and malvidin glycosides were quantified as corresponding equivalents of the five anthocyanin glucosides using external calibration curves of authentic standards ranging from 5 to 125μg/mL. Total anthocyanins were calculated as the sum of individual anthocyanin glycosides with results expressed as mg per 100 mL juice.

Anthocyanins were identified by HPLC-MS using identical conditions described above with the HPLC interfaced to a Bruker Esquire LC/MS ion trap spectrometer (Billerica, MA). Mass spectral analysis was conducted in positive ion electrospray mode using conditions previously described [2].

2.3Percent polymeric color analysis

Percent polymeric color (PC) of juices was determined using the spectrophotometric assay of Giusti and Wrolstad [24]. Sample extracts were diluted with water in order to have an absorbance reading between 0.5 and 1.0 at 512 nm when evaluated by an 8452A Diode Array Spectrophotometer (Hewlett Packard, Palo Alto, CA). For analysis, 0.2 mL of 0.90 M potassium metabisulfite was added to 2.8 mL diluted sample (bisulfite bleached sample) and 0.2 mL of DI water was added to 2.8 mL diluted sample (non-bleached, control sample). After equilibrating for 15 min, but not more than 1 h, samples were evaluated at λ= 700 nm, 512 nm, and 420 nm. Color density was calculated using the control sample according to the following formula:

Color Density = [(A420nm – A700nm)+(A512nm – A700nm)] × Dilution Factor

Polymeric color was determined using the bisulfite-bleached sample using the following formula:

Polymeric Color = [(A420nm – A700nm)+(A512nm – A700nm)] × Dilution Factor

Percent polymeric color was calculated using the formula:

% Polymeric color = (polymeric color/color density) × 100

2.4Statistical analysis

All statistical analysis was performed in the fit model platform of JMP (JMP Pro version 12.1.0, SAS Institute, Cary, NC). The statistical model for all responses for the pasteurization data set involved 3 pH levels (2.1, 2.5 and 2.9), non-pasteurized and pasteurized in a 3 × 2 design with three replications for each of the six treatment combinations. The statistical model for all responses for the storage study involved a 3 × 4 × 2 factorial design with three pH levels, 4 storage times (2, 4, 6, and 8 months), and 2 storage temperatures (4 and 25°C) also with three replications for each of the 24 treatment combinations. Tukey’s HSD multiple comparisons were utilized to report mean differences among interactions simple and main effects were appropriate using α= 0.05 significance level in all cases.

3Results and discussion

3.1Anthocyanin composition of blueberry juice

A typical HPLC chromatogram of non-pasteurized juice produced from ‘Bluecrop’ blueberries is shown in Fig. 1. Seventeen peaks were identified by HPLC/MS: peak 1, delphinidin 3-O-galactoside (m/z 465/303); peak 2, delphinidin 3-O-glucoside (m/z 465/303); peak 3, cyanidin 3-O-galactoside (m/z 449/287); peak 4, delphinidin 3-O-arabinoside (m/z 435/303); peak 5, cyanidin 3-O-glucoside (m/z 449/287); peak 6, petunidin 3-O-galactoside (m/z 479/317); peak 7, cyanidin 3-O-arabinoside (m/z 419/287); peak 8, petunidin 3-O-glucoside (m/z 479/317); peak 9, peonidin 3-O-galactoside (m/z 463/301); peak 10, petunidin 3-O-arabinoside (m/z 449/317); peak 11, malvidin 3-O-galactoside (m/z 493/331); peak 12, malvidin 3-O-glucoside (m/z 493/331); peak 13, peonidin 3-O-arabinoside (m/z 433/301); peak 14, malvidin 3-O-arabinoside (m/z 463/331); peak 15, delphinidin 3-O-(6”-acetylglucoside) (m/z 507/303); peak 16, petunidin 3-O-(6”-acetylglucoside) (m/z 521/317); peak 17, malvidin 3-O-(6”-acetylglucoside) (m/z 535/331). Monomeric anthocyanins Mvd (41.2%), Dpd (27.1%), Ptd (18.3%), Cyd (3.4%) and Pnd (1.1%) accounted for 91.1% of the total anthocyanins present in the non-pasteurized juice, while acetylated anthocyanins accounted for 8.9%. These values are consistent with previous percentage distribution values reported for ‘Bluecrop’ blueberries, Dpd (26–41%), Cyd (6–11%), Ptd (17–21%), Pnd (1-2%) and Mvd (32–44%) [2, 10, 25]. The percentage distribution of glycosides followed the order of Gal (39%), Glu (33%) and Ara (28%), which agrees well with previous values Gal (39%), Glu (31%) and Ara (30%) reported for ‘Bluecrop’ blueberries [2].

3.2pH effect on anthocyanins and percent polymeric color of non-pasteurized and pasteurized blueberry juice

The effect of pH on total anthocyanin content and percent polymeric color of non-pasteurized and pasteurized blueberry juice is shown in Fig. 2, and the pH effect on individual anthocyanins is presented in Table 1. Acidifying the non-pasteurized juice from the natural blueberry pH of 2.9 to 2.5 and 2.1 had little to no effect on total anthocyanins and percent polymeric color. The pasteurization step resulted in 14, 21 and 20% losses of total anthocyanins in pH 2.1, 2.5, and 2.9 juices, respectively. The pH 2.1 juices had a lower % polymeric color value (11.7) than pH 2.5 (14.7) and pH 2.9 (14.3) juices following pasteurization, which is consistent with greater retention of monomeric anthocyanins in juices acidified to pH 2.1. Several studies have demonstrated that acidification improves anthocyanin and color stability in model solutions [23, 26, 27]. Additionally, acidification of blueberry juice to pH 1 was shown to improve anthocyanin stability and prevent the increase of percent polymeric color values observed in juices adjusted to pH 4 and 7 [19]. Improved stability of anthocyanins in blueberry juice at 2.1 following pasteurization as opposed to pH 2.5 and 2.9 juices is due to shift of the anthocyanin structure to the flavylium cationic form, which confers a red color, whereas at pH 2.5 and 2.9 the quinoidal blue species predominate [22].

All individual anthocyanins declined following pasteurization with the exception of Cyd 3-gal, Cyd 3-glu, and Pnd 3-gal, which were present in low amounts (Table 1). Following pasteurization, the pH 2.1 juices had higher levels of Dpd 3-glu, Cyd 3-gal, Ptd 3-glu, Mvd 3-gal and Mvd 3-glu than pH 2.9 juices, and pH 2.1 juices also contained higher levels of Ptd 3-gal, Ptd 3-glu, Mvd 3-gal, Mvd 3-glu, and Mvd 3-ara than pH 2.5 juices. However, pH 2.1 juices had lower levels of Mvd 3-ace-glu than pH 2.5 and 2.9 juices. Degradation of anthocyanins appeared to be minimally affected by anthocyanidin structure. Percent retention of anthocyanidins after pasteurization were Pnd (100%), Cyd (93%), Dpd (82%), Ptd (82%) and Mvd (80%), which agrees reasonably well with the retention order of Cyd>Pnd>Ptd>Dpd>Mvd for anthocyanidins in blueberry-Aronia nectar [28]. In contrast, Skrede et al. [10] reported that the order of anthocyanin stability in response to pasteurization of blueberry juice was Pnd = Mvd>Cyd = Ptd>Dpd. Excluding the two anthocyanins (Cyd and Pnd) which were present in minor amounts, retentions of the three major anthocyanidins, Dpd, Ptd and Mvd were similar (80–82%), suggesting that anthocyanidin structure does not play a major role in stability of anthocyanins in response to thermal degradation confirming results of West and Mauer [27].

In terms of sugar and acetyl compounds attached, Glu (85%), Gal (84%), and GluAce (83%) showed greater retention than Ara (74%). These results were consistent with previous studies reporting anthocyanin hexosides to be more stable than pentosides [14, 28–30]. Additionally, West and Mauer [27] reported that sugar structure, namely glucoside, and acylated derivatives of glucosides (acetyl, malonoyl, and coumaroyl) did not affect degradation of anthocyanins in purified and semi-purified extracts from grape pomace, purple corn, and black rice. Our results for glucosides, galactosides and acetylated derivatives of glucosides support their findings, but our results indicate that arabinosides, which were not measured in the study of Mauer and West [27], were more prone to degradation in response to pasteurization than other glycosides. However, in another study investigating anthocyanin losses during blueberry juice processing, anthocyanin losses were reported to be affected more by aglycone structure than by type of sugar moiety attached [10]. Discrepancies among studies may reflect differences in processing steps employed or variation in glycosidase activities of enzyme preparations used for juice processing [31–33].

3.3pH, storage temperature and storage time effects on anthocyanins and percent polymeric color of pasteurized blueberry juice

The concentrations of total anthocyanins and percent polymeric color values of pasteurized blueberry juice as affected by pH, storage temperature and storage time are shown in Fig. 3. Marked losses of total anthocyanins occurred from time 0 (pasteurized juice) to two months of storage in juices that were stored at 25°C. During this time, juices acidified to pH 2.1 retained higher levels of total anthocyanins (78%; 84.1 mg/100 mL) than both pH 2.5 (71%; 71.9 mg/100 mL) and control juices (62%; 62.3 mg/100 mL) (Std Err Diff = 2.36). The initial large loss of anthocyanins was unexpected, but may be the result of heat resistant forms of polyphenol oxidase or peroxidase that were not totally inactivated by the pasteurization step [34], or ascorbic acid catalyzed degradation of anthocyanins [35, 36]. Levels of total anthocyanins continued to decline over 2 to 8 months of storage regardless of storage temperature, but as expected juices stored at 4°C retained much higher levels of total anthocyanins than juices stored at 25°C. Juices stored at 4°C had on average 56% higher levels of total anthocyanins (98.7 mg/100 mL) than juices stored at 25°C (63.3 mg/100 mL) (Std Err Diff = 2.80). Retention of total anthocyanins was also influenced by juice pH, with juices acidified to pH 2.1 (90.5 mg/100 mL) having on average 12% and 26% higher levels of total anthocyanins than pH 2.5 (80.5 mg/100 mL) and pH 2.9 (72.1 mg/100 mL) juices, respectively (Std Err Diff = 5.86). After 8 months of storage, juices acidified to pH 2.1 (94.9 mg/100 mL) had 11 and 22% higher levels of total anthocyanin than pH 2.5 (85.7 mg/100 mL) and 2.9 juices (78.5 mg/100 mL) stored at 4°C (Std Err Diff = 2.29). After eight months of storage at ambient temperature, juices acidified to pH 2.1 (62.9 mg/100 mL) had 26% and 59% higher levels of total anthocyanins than pH 2.5 (49.7 mg/100 mL) and 2.9 juices (39.7 mg/100 mL) (Std Err Diff = 2.48). A reduced model fit for each temperature (with R2 = 0.94 respectively concludes that in each storage temperature environment there were only the significant main effects of storage duration and pH. The analysis for both room and refrigerated suggests statistically significant retention with each lower pH level and significant loss of the total anthocyanins with each storage treatment level beyond 4 months. A linear model could capture 98% of the variability of the total anthocyanins without any significant Lack of Fit. Furthermore, we could conclude from that reduced model that total anthocyanins tend to decline (beyond the first four months) linearly about 4.8 (mg/100 mL) per month on average independent of temperature and pH treatments.

The degradation of anthocyanins in juices subjected to long-term storage at ambient temperature in this study are consistent with other studies on berry juices. Control juices (pH 2.9) in this study lost 50% of total anthocyanins over six months of storage, while non-clarified juices of black raspberries, blueberries and blackberries lost 62%, 68% and 75% of total anthocyanins, respectively over the same storage period [12, 13, 37]. Extensive losses of total anthocyanins were also reported for blueberry-aronia juices stored for 207 days in glass (89% loss), and juice stored for 183 days in cartons (92% loss) [28].

Consistent with loss of total anthocyanins, percent polymeric color values increased over eight months of storage and refrigerated storage ameliorated the increase in percent polymeric color in juices stored at 25°C (Fig. 3). Juices stored at 4°C had on average 20% polymeric color, while juices stored at 25°C had 33% polymeric color (Std Err Diff = 1.41). Percent polymeric color was also impacted by pH with juices acidified to pH 2.1 and 2.5 having lower average polymeric color (24%) than non-acidified pH 2.9 juices (31%) (Std Err Diff = 2.46). After 8 months of storage at 4°C, pH 2.1 and 2.5 juices had lower polymeric color (20 and 22%) than non-acidified pH 2.9 juices (26%) (Std Err Diff = 0.78). A similar trend was observed after 8 months of storage at 25°C, with and pH 2.1 and 2.5 juices having 35 and 37% polymeric color compared to 49% for pH 2.9 juices (Std Err Diff = 2.58). Levels of total anthocyanins and percent polymeric color values over storage showed a significant inverse correlation (rxy = 0.91), indicating that the low amount of anthocyanins remaining after 8 months of storage were present to a large degree in polymeric form. All individual anthocyanins showed inverse correlations with polymeric color values with the exception of acetylated derivatives of Dpd, Mvd, and Ptd, which tended to have much lower correlations than all monoglycosides (data not shown). We believe the lower correlation for the acetylated derivatives is due to their instability, especially under acidic conditions. It is possible that anthocyanins react with proanthocyanidins via a direct condensation reaction during storage to form polymeric pigments. However, another possibility is that the concentration of anthocyanin-proanthocyanidin polymers do not change appreciably during storage, but the compounds are much more resistant to degradation than monomeric anthocyanins. This scenario would also result in increased percent polymeric color values over storage. More research is needed to isolate and quantify anthocyanin-proanthocyanidin polymers in order to determine their fate during storage.

Levels of all individual anthocyanins decreased over eight months of storage, but the losses were affected by storage temperature and pH. Over all storage times, juices stored at 4°C had on average 41, 56, 57, 62 and 32% higher levels of total Cyd, Mvd, Ptd, Dpd and Pnd derivatives than juices stored at 25°C. Over all storage times and temperatures, juices acidified to pH 2.1 had on average 8, 13, 12, 9, and 11% higher levels of total Cyd, Dpd, Mvd, Pnd and Ptd derivatives than juices acidified to pH 2.5, and 28, 25, 26, 19 and 25% higher levels of total Cyd, Dpd, Mvd, Pnd and Ptd derivatives than non-acidified juices (pH 2.9).

Changes in individual anthocyanins expressed as percentage of total anthocyanins are shown in Fig. 4 for refrigerated juices and Fig. 5 for juices stored at 25°C. In juices stored at 4°C (Fig. 4), Ptd 3-glu, Mvd 3-glu, Dpd 3-glu, and Cyd 3-glu accounted for a larger percentage of total anthocyanins over storage at each pH, while Ptd 3-gal, Pnd 3-gal, Mvd 3-gal, Dpd 3-gal, Cyd 3-gal, Ptd 3-gal and Cyd 3-ara changed little and Mvd 3-ara, Dpd 3-ara, Cyd 3-ace-glu, Ptd 3-ace-glu, Mvd 3-ace-glu and Dpd 3-ace-glu decreased. The effect of juice pH on anthocyanin composition was minimal with the exception of acetylated derivatives of anthocyanidins. Levels of Ptd 3-ace-glu, Mvd 3-ace-glu and Dpd 3-ace-glu accounted for a lower percentage of total anthocyanins in juices acidified to pH 2.1 than juices acidified to pH 2.5 or juices with natural pH of 2.9. The acetylated anthocyanins were much more stable over storage in juices with natural pH of 2.9 than both acidified juices.

Similar changes in anthocyanin composition over storage were observed in juices stored at 25°C (Fig. 5), with Ptd 3-glu, Mvd 3-glu, Dpd 3-glu, and Cyd 3-glu accounting for a larger percentage of total anthocyanins over storage at each pH, Ptd 3-gal, Pnd 3-gal, Mvd 3-gal, Dpd 3-gal, Cyd 3-gal, Ptd 3-gal, and Cyd 3-ara changing little and Mvd 3-ara, Dpd 3-ara, Cyd 3-ace-glu, Ptd 3-ace-glu, Mvd 3-ace-glu and Dpd 3-ace-glu decreasing. Similar to results obtained with refrigerated juices, the effect of pH on anthocyanin composition over storage was minimal, with the exception of acetylated derivatives, which accounted for a much lower percentage of total anthocyanins in pH 2.1 juices than both acidified juices.

The instability of acetylated derivatives over storage was surprising since acylated anthocyanins are reported to be much more stable than monomeric anthocyanins as a result of their intra- and intermolecular co-pigmentation properties [38, 39]. However, acylated anthocyanins from purple carrot, red potatoes, red radish, and red cabbage showing greater stability than monomeric anthocyanins typically have one or more aromatic acids such as p-coumaric, cinnamic, or ferulic esterified to the 6-OH of the sugar moieties attached at C3 on the pyrylium ring [39]. Our results indicate that the esterified acetyl moiety is labile to acidic conditions making the acetylated derivatives more prone to degradation during storage of blueberry juice than glycosides. The observed increases in Ptd 3glu, Mvd 3-glu, Dpd 3-glu and Cyd 3-glu as a percentage of total anthocyanins during storage may be due to cleavage of the acetyl moiety from their acetylated counterparts. Further work employing purified compounds is needed to confirm if acetylated derivatives can be converted to monomeric anthocyanins under acidic conditions.

4Conclusions

Acidification of blueberry juice to pH 2.1 ameliorated anthocyanin losses and increase in percent polymeric color observed in control (pH 2.9) and juices acidified to pH 2.5 following pasteurization. Anthocyanin arabinosides were more susceptible to degradation in response to pasteurization than glucosides, galactosides and acetylated derivatives. Levels of total anthocyanins declined markedly over 8 months of storage, but acidification of juices to 2.1 and refrigerated storage were both effective in mitigating anthocyanin losses. After 8 months of storage, juice acidified to pH 2.1 had 11 and 22% higher levels of total anthocyanins than pH 2.5 and control juices stored at 4°C, and 26% and 59% higher levels of total anthocyanins than pH 2.5 and control juices stored at 25°C. Acetylated derivatives were more prone to losses during storage than monoglycosides, especially in acidified juices.

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Figures and Tables

Fig.1

Typical HPLC chromatogram (Abs 520 nm) of blueberry juice anthocyanins. peak 1, delphinidin 3-O-galactoside (m/z 465/303); peak 2, delphinidin 3-O-glucoside (m/z 465/303); peak 3, cyanidin 3-O-galactoside (m/z 449/287); peak 4, delphinidin 3-O-arabinoside (m/z 435/303); peak 5, cyanidin 3-O-glucoside (m/z 449/287); peak 6, petunidin 3-O-galactoside (m/z 479/317); peak 7, cyanidin 3-O-arabinoside (m/z 419/287); peak 8, petunidin 3-O-glucoside (m/z 479/317); peak 9, peonidin 3-O-galactoside (m/z 463/301); peak 10, petunidin 3-O-arabinoside (m/z 449/317); peak 11, malvidin 3-O-galactoside (m/z 493/331); peak 12, malvidin 3-O-glucoside (m/z 493/331); peak 13, peonidin 3-O-arabinoside (m/z 433/301); peak 14, malvidin 3-O-arabinoside (m/z 463/331); peak 15, delphinidin 3-O-(6”-acetylglucoside) (m/z 507/303); peak 16, petunidin 3-O-(6”-acetylglucoside) (m/z 521/317); peak 17, malvidin 3-O-(6”-acetylglucoside) (m/z 535/331).

Typical HPLC chromatogram (Abs 520 nm) of blueberry juice anthocyanins. peak 1, delphinidin 3-O-galactoside (m/z 465/303); peak 2, delphinidin 3-O-glucoside (m/z 465/303); peak 3, cyanidin 3-O-galactoside (m/z 449/287); peak 4, delphinidin 3-O-arabinoside (m/z 435/303); peak 5, cyanidin 3-O-glucoside (m/z 449/287); peak 6, petunidin 3-O-galactoside (m/z 479/317); peak 7, cyanidin 3-O-arabinoside (m/z 419/287); peak 8, petunidin 3-O-glucoside (m/z 479/317); peak 9, peonidin 3-O-galactoside (m/z 463/301); peak 10, petunidin 3-O-arabinoside (m/z 449/317); peak 11, malvidin 3-O-galactoside (m/z 493/331); peak 12, malvidin 3-O-glucoside (m/z 493/331); peak 13, peonidin 3-O-arabinoside (m/z 433/301); peak 14, malvidin 3-O-arabinoside (m/z 463/331); peak 15, delphinidin 3-O-(6”-acetylglucoside) (m/z 507/303); peak 16, petunidin 3-O-(6”-acetylglucoside) (m/z 521/317); peak 17, malvidin 3-O-(6”-acetylglucoside) (m/z 535/331).
Fig.2

Total anthocyanin content (mg/100 mL) and percent polymeric color of blueberry juice before and after pasteurization as affected by pH. Bars represent standard error of the mean (n = 3).

Total anthocyanin content (mg/100 mL) and percent polymeric color of blueberry juice before and after pasteurization as affected by pH. Bars represent standard error of the mean (n = 3).
Fig.3

Total anthocyanin content (mg/100 mL) and percent polymeric color of blueberry juice as affected by pH, storage time and temperature. Bars represent standard error of the mean (n = 3).

Total anthocyanin content (mg/100 mL) and percent polymeric color of blueberry juice as affected by pH, storage time and temperature. Bars represent standard error of the mean (n = 3).
Fig.4

Anthocyanin composition (% of total anthocyanins) of blueberry juice over eight months of storage at 4°C as affected by pH.

Anthocyanin composition (% of total anthocyanins) of blueberry juice over eight months of storage at 4°C as affected by pH.
Fig.5

Anthocyanin composition (% of total anthocyanins) of blueberry juice over eight months of storage at 25°C as affected by pH.

Anthocyanin composition (% of total anthocyanins) of blueberry juice over eight months of storage at 25°C as affected by pH.
Table 1

Anthocyanin composition (mg/100 mL) of blueberry juice before and after pasteurization as affected by pH

Non-pasteurizedPasteurized
AnthocyaninpH 2.1pH 2.5pH 2.9pH 2.1pH 2.5pH 2.9
Dpd 3-galactoside12.7bc113.6a13.1ab11.9 (94)2cd11.2 (82)e11.3 (86)de
Dpd 3-glucoside9.5a9.6a9.7a8.6 (91)b8.0 (84)c7.9 (82)c
Dpd 3-arabinoside11.6a11.8a11.9a9.0 (78)b8.4 (71)c8.5 (71)c
Dpd 3-acetyl-glucoside3.7a3.8a3.8ab3.2 (86)b3.1 (81)b2.8 (74)b
Cyd 3-galactoside1.3bc1.4a1.4a1.4 (108)a1.3 (95)ab1.2 (88)c
Cyd 3-glucoside1.5b1.6b1.6b1.7a (113)1.6 (102)b1.6 (100)a
Cyd 3-arabinoside1.4a1.4a1.5a1.2 (84)b1.2 (85)b1.1 (75)b
Ptd 3-galactoside8.2b8.6a8.4ab7.3 (89)c6.8 (79)d6.9 (83)d
Ptd 3-glucoside8.7a8.8a8.8a7.7 (89)b7.2 (82)c7.2 (82)c
Ptd 3-arabinoside6.2a6.2a6.2a4.7 (76)b4.3 (69)c4.5 (69)bc
Ptd 3-acetyl-glucoside2.3a2.3a2.3a2.1 (93)b2.1 (88)b2.0 (87)b
Pnd 3-galactoside1.3a1.4a1.4a1.4 (108)a1.3 (97)a1.3 (93)a
Mvd 3-galactoside20.6a21.0a21.0a17.3 (83)b16.2 (77)c16.4 (78)c
Mvd 3-glucoside18.4a18.6a18.5a16.3 (89)b15.2 (82)c15.2 (82)c
Mvd 3-arabinoside12.9a13.1a13.1a10.0 (78)b9.3 (71)c9.5 (71)c
Mvd 3-acetyl-glucoside5.1b5.3a5.2ab4.1 (80)e4.4 (83)d4.6 (88)c
Total anthocyanins125.4a128.4a127.9a108.0 (86)b101.6 (79)c102.1 (80)c

1 Mean values (n = 3) within rows with similar letters are not significantly different (P > 0.05). 2 Values in parentheses for pasteurized values represent percent retention compared with corresponding non-pasteurized treatments.