**2. Results and Discussion**

#### *2.1. Polyphenolic Content and Chemical Profile*

In the present study, polyphenolic compounds were determined using UPLC-PDA-ESI-MS/MS in Saskatoon berry powders with carriers considering the type of the material subjected to drying (whole fruit, juice, pomace), the drying method, and the type of carrier and its concentration (Table 1 and Tables S1–S4). Detailed analyses allowed identifying 42 compounds classified to four main groups as anthocyanins, phenolic acids, flavonols, and flavan-3-ols. Their presence in powders obtained from Saskatoon berry fruits was also confirmed in earlier works [1,2,4,6,17,18].

The most abundant group belonging to polyphenolic compounds was represented in the analyzed powders by flavan-3-ols (monomers, oligomers, and polymeric procyanidins). These compounds were previously identified in fruits by Lachowicz et al. [6,17]. This group accounted for 35% of total polyphenolic compounds in fruit powder, for 33% in juice powder, and for 39% in pomace powder. Among the monomers and oligomers, the presence of 14 compounds was identified; they accounted for 36% of total flavan-3-ols in fruit powder, for 67% in juice powder, and for 20% in pomace powder. In addition, the presence of polymeric procyanidins was determined by phloroglucinolysis (they accounted for 64% of total flavan-3-ols in fruit powder, for 33% in juice powder, and for 80% in pomace powder) (Table S1). In this research two monomers (main ion at *m*/*z* 289), two dimers (main ion at *m*/*z* 577), five trimers (main ion at *m*/*z* 863), and five tetramers (main ion at *m*/*z* 1153) were identified based on MS data and available literature [1,17].

Anthocyanins were the second abundant group determined in the powders [1] and constituted 26% of total polyphenolic compounds in fruit powder, 5% in juice powder, and 34% in pomace powder. Furthermore, six cyanidins were identified including four glycosides of cyanidins (cyanidin-3- *O*-galactoside: *m*/*z* 449, -3- *O*-glucoside: *m*/*z* 499, -3- *O*-xyloside: *m*/*z* 419, -3- *O*-arabinoside: *m*/*z* 419) and two cyanidin aglycons ( *m*/*z* 287). Among the 6 identified compounds, the major compound belonging to anthocyanins was cyanidin-3- *O*-galactoside (it accounted for 69.9% of all anthocyanins). This was confirmed in earlier reports [2].

Phenolic acids were the next group of polyphenols that accounted for 33% of total polyphenolic compounds in fruit powder, for 55% in juice powder, and for 20% in pomace powder. According to the MS spectra, standards, and literature, eight hydroxycinnamic acids were determined, including: three isomers of ca ffeoylquinic acid ( *m*/*z* 353), two coumaroylquinic acids ( *m*/*z* 353), and three isomers of ca ffeic acids ( *m*/*z* 341), as well as one hydroxybenzoic acid identified as protocatechuic acid ( *m*/*z* 153). The major phenolic acids were 5- *O*-ca ffeoylquinic acid (56% of all phenolic acids), and 4- *O*-ca ffeoylquinic acid (19%). The mass noted on the negative mode was *m*/*z* 353 with similar MS spectra to those reported in literature [1,2].

The last and the smallest group of phenolic compounds was constituted by flavonols [17]. This group accounted for 6% of total flavonols in fruit powder, for 6% in juice powder, and for 7% in pomace powder; and the major compound was quercetin-3- *O*-galactoside [1,2] which represented 46% of all flavonols. In this work, thirteen flavonols were identified including ten glycosides of kaempferol and quercetin (based on ion at *m*/*z* 285 and 301, respectively), two acetylated compounds ( *m*/*z* 507), and one quercetin aglycon ( *m*/*z* 301) [1,2].

The average total content of identified polyphenols was 6535 mg/100 g d.m. in pomace powders. Their content was lower by 38% and 70% in fruit and juice powders, respectively (Table 1 and Tables S1–S4). This is due to the accumulation location of these constituents in the outer layer of the fruit that remains in the pomace during pressing [19,20]. In addition, the highest antioxidant capacity was found in pomace powders and was 3.4-fold (ABTS assay) and 3-fold (FRAP assay) higher when compared to the fruit powders as well as 7-fold (ABTS assay) and 6-fold (FRAP assay) compared to juice powders (Table 2). These relationships were also confirmed during the drying of chokeberry [21] and cranberry fruits [22] and can be explained by distribution of phenols, because they are not equally distributed in the plant material [22]. Anthocyanins and flavonols are mostly presented in the peel of berry, also polymeric procyanidins, monomers, and oligomers of flavan-3-ols are essentially located in the peel, but some content of these compounds occur in the pulp thus in the juice [21,22]. In addition, conditions of juice processing, mash maceration, and the type of enzymatic preparation may significantly impact the content of polyphenols in the juice and pomace of product [21,22]. This fact is widely known in the literature, but there is little information on the impact of carriers and their quantity and drying methods on the individual matrix, especially of Saskatoon berry. What is more, according to literature [1–3,17,23,24], the Saskatoon berry fruits are an excellent source of polyphenolic compounds and antioxidant properties responsible for their proved anti-inflammatory, antidiabetic, and chemo-protective e ffects. They have more bioactive compounds than e.g., blueberry, blackberry, bilberry, raspberry, and strawberry [25,26]. However, little is known about the use of this raw material as a functional additive. Available data relate only to Saskatoon berry supplements and used the accumulation of plasma levels of anthocyanins [27]. *Amelanchier alnifolia* Nutt. (90 g) were administered immediately after every low antioxidant meal. The authors noted plasma concentrations of cyanidin-3- *O*-xyloside and cyanidin-3- *O*-galactoside were significantly increased following 3 consecutive supplements 4 h apart. Therefore, they recommend that anthocyanin supplements with every meal would higher their plasma concentrations [27]. Another work concerned the prevention of diabetes in obese mice by consuming Saskatoon berry [28]. Male mice were served a control diet, high fat and high sucrose diet, and high fat and high sucrose with 5% of Saskatoon berry powder (weight/weight) diet for 15 weeks. The results showed that Saskatoon berry powder suppressed high fat, high sucrose diet-induced hyperglycemia, hyperlipidemia, insulin resistance, and vascular inflammation [28]. Therefore, research was undertaken to obtain new functional additives (powders) from various Saskatoon berry matrices with the highest possible content of antioxidant compounds.

#### *2.2. Influence Type of Carriers on Polyphenolic Compounds and Antioxidant Capacity in Dependence on the Matrix*

The principal component analysis (PCA) was used to study the impact of the type of carriers on the protection of polyphenolic compounds and their antioxidant activity depending on the matrix tested (Figure 1). It showed that in the case of fruit powders, drying in the presence of inulin was associated with a higher concentration and protection of flavan-3-ols group and their individual compounds ((+)-catechin, B-type procyanidin: dimer, and tetramer, and A-type procyanidin dimer), 3 and 4- *O*-ca ffeoylquinic acids, di-ca ffeoylquinic acid, and cyanidin-3- *O*-arabinoside. While maltodextrin caused the higher retention and ensured protection of polymeric procyanidins, total phenolic acids and their derivatives, total flavonols and their derivatives, total anthocyanins and their derivatives, and total phenolic acids and their antioxidant activity (strong correlation with the ferric reducing antioxidant potential (FRAP)) and positive correlation with the radical scavenging capacity (ABTS)). Bakowska-Barczak and Kołodziejczyk [29] also reported that the use of maltodextrin resulted in the highest contents of anthocyanins and polyphenols in black currant powders. The higher retention of polyphenolic compounds was also noted in cactus pear with maltodextrin when compared to inulin [30]. In turn, PCA analysis showed that in the case of juice powders, inulin had a stronger impact on total flavonols and their main derivatives, (+)-catechin, (−)-epicatechin, B-type procyanidin dimer, polymeric procyanidins, cyanidin-3- *O*-arabinoside, and 3- *O*-ca ffeoylquinic acid; while, maltodextrin led to the higher retention of total phenolic acid, total anthocyanins, total flavan-3-ols. What is more, the ability to scavenge the ABTS radicals was higher in the case of the juice powders with maltodextrin addition, whereas higher FRAP values were noted for the powders prepared with inulin. The addition of maltodextrin into juice powders a ffected the release of free cyanidin and quercetin aglycons. Whereas, in black currant juice powder, the use of inulin resulted in a 9% higher anthocyanin retention compared to the use of maltodextrin [16]. Furthermore, the PCA analysis of pomace powders showed that the product with inulin had higher contents of total of polyphenolic compounds, A and B-type procyanidin dimer, polymeric procyanidin, and quercetin-3- *O*-robinobioside, and also a higher degree of polymerization. This product had higher antioxidant potency, while maltodextrin was responsible for the protection of total anthocyanins and their derivatives, total flavan-3-ols and their derivatives, total phenolic acids and their derivatives, and total flavonols and their derivatives. Thus, the type of carrier and its impact on antioxidant compounds depended mainly on the analyzed matrix. The high antioxidant power of the juice and pomace powders with inulin and also of the fruit powders with maltodextrin can be a ffected by polymerized compounds. This can also be confirmed by a strong correlation between the polymerized compounds and antioxidant activity i.e., *r* = 0.997 for FRAP and 0.430 for ABTS (for fruit powders), *r* = 0.995 and 0.998 for FRAP and ABTS assay (juice powders), and *r* = 0.997 and 0.998 for FRAP and ABTS assay (pomace powders). Therefore, the choice of a carrier will largely depend on the desired composition of bioactive compounds with antioxidant activity for the functional additive regardless of the Saskatoon berry matrix tested.

**A** 

 

187

**Figure 1.** *Cont.*

3&

**C** 

**Figure 1.** Principal component analysis (PCA) of the impact of type of carrier to phytochemical parameter in fruit ( **A**), juice (**B**), pomace ( **C**) powders. *Abbreviations:* ANT—sum of anthocyanins; FL—sum of flavonols; PA—sum of phenolic acid; PP—polymeric procyanidins; F3O—sum of flavan-3-ols (monomers and oligomers); DP—degree of polymerization; PC—sum of polyphenolic compounds; **<sup>1</sup>**—cyanidin-3- *O*-galactoside; **<sup>2</sup>**—cyanidin-3- *O*-glucoside; **<sup>3</sup>**—cyanidin-3- *O*-arabinoside; **<sup>4</sup>**—cyanidin-3- *O*-xyloside; **<sup>5</sup>**—cyanidin; **<sup>6</sup>**—protocatechuic acid; **7**—caffeic acid glucoside; **8**—caffeoylhexose; **9**—acid isomers; **10**—3- *O*-caffeoylquinic acid; **11**—5- *O*-caffeoylquinic acid; **12**—4- *O*-caffeoylquinic acid; **13**—3- *O*-*p*-coumaroylquinic acid; **14**—di-caffeoylquinic acid; **15**—di-caffeoylquinic acid; **16**—kaempferol-3- *O*-galactoside; **<sup>17</sup>**—quercetin-3- *O*-arabinobioside; **18**—kampferol-3- *O*-glucoside; **19**—quercetin; **<sup>20</sup>**—quercetin-3- *O*rutinoside; **<sup>21</sup>**—quercetin-3- *O*-robinobioside; **<sup>22</sup>**—quercetin-3- *O*-galactoside; **<sup>23</sup>**—quercetin-3- *O*-glucoside; **<sup>24</sup>**—quercetin-3- *O*-arabinoside; **<sup>25</sup>**—quercetin-3- *O*-xyloside; **<sup>26</sup>**—quercetin-3- *O*-(6"-acetyl)glucoside; **<sup>27</sup>**—quercetin-3- *O*-(6"-acetyl)galactoside; **<sup>28</sup>**—quercetin-deoxyhexo-hexoside; **29**—sum of B-type procyanidin tetramer; **30**—sum of B-type procyanidin trimer; **31**—sum of B-type procyanidin dimer; **32**—A-type procyanidin dimer; **33**—(-)-epicatechin; **34**—(+)-catechin.

#### *2.3. Impact of the Amount of Added Carriers' on Polyphenols Content and Antioxidant Capacity in Dependence on the Matrix*

The concentration of carriers had a stronger impact on the retention of polyphenolic compounds than the type of carrier or drying method. A similar observation was made for black currant powders with the use of the mentioned-above carriers for drying [16]. In turn, addition of maltodextrin at the level of 15% was found to protect the bioactive compounds from thermal degradation [31]. The principal component analysis (PCA) was used to evaluate the influence of the concentration of carriers on the protection of antioxidant compounds depending on the matrix tested (Figure 2). PCA graph for powders with 30% of carriers showed by 20% and 37% higher content of total polyphenols, and by 29% and 47% higher antioxidant potential determined with ABTS and FRAP assays compared

to the powders obtained with 40% and 50% of carriers, respectively, regardless of the matrix tested. Probably, the content of phenolics was a ffected by the dilution e ffect with the carrier; the higher the carrier concentration, the lower the content of bioactive compounds. A similar observation was made in the case of *Eugenia dysenterica* DC. powders pointing to a concentration of a carrier on the content of polyphenols. Samples obtained using 10% of carriers showed the highest content of polyphenols, while the powders with 30% of carrier presenting the lowest amount of phenols [32]. This can also be confirmed by a strong positive correlation between individual polyphenolic compounds (anthocyanins, phenolic acids, flavonols, flavan-3-ols) and antioxidant activity (ABTS assay) of *r* = 0.979, 0.999, 0.998, 0.992 (for fruit powders), *r* = 0.993, 0.974, 0.998, 0.999 (juice powders), and *r* = 0.958, 0.993, 0.994, 0.998 (pomace powders). Depending on the matrix, the lowest loss of polyphenolic compounds was noted in juice powders and it was 17% and 21% with 40% and 50% of carriers compared to the powders with 30% of carriers. While in fruit and pomace powders losses were 11% and 18% higher. Greater degradation of flavan-3-ols (monomers and oligomer) and polymeric procyanidin was found in the fruit and pomace powders than in the juice powders; it reached ca. 24% and 30%. As for the anthocyanins, the greatest degradation was found in fruit powder (ca. 43% in product with 50% of carrier) > pomace powder (around 40%) > juice powders (38%). While, the smallest degradation of phenolic acids and flavonols was found in the pomace powders—around 15% and 26% and 12% and 28% in products with 40% and 50% of carriers, respectively, compared to the final product with 30% of carrier. Probably high stability can be due to presence of cell wall polysaccharide compounds e.g., pectins, whether lower water activity [21,22]. Additionally, it might be due to the better encapsulation process of these samples, which is confirmed by Daza et al. [32] who followed the highest retentions of bioactive compounds in cagaita powders with 20%–30% of carriers. However, the higher carrier concentration a ffected the protection of individual compounds, e.g., in the case of fruit powders—40% of carrier influenced higher protection of cyanidin-3-O-arabinose and a higher degree of polymerization, but 50% of carrier a ffected the B-type procyanidin tetramer. Whereas in the case of juice powders—40% of carrier caused high retention of quercetin-3-O-robinobioside, -3-O-arabinoside, -3-O-glucoside, and protocatechuic acid, but 50% of carrier caused a high degree of polymerization. Finally, in the case of pomace powders—40% of carrier caused a high degree of polarization just like in the fruit powders. Indicating that might have led to a release of the compounds from more polymerized structures. Similarly as with pulp and juice powders made from cagaita and plum, the concentration of carriers had a strong influence on the decrease of total polyphenolic compounds [32,33]. Thus, the higher carrier concentration led to a lower polyphenol content and lower antioxidant activity, indicating the strong e ffect of the initial composition of the matrix tested. Moreover, dried products with carriers showed a 1.6 and 1.9, and 1.5 times higher protection of the antioxidant capacity and phenolic compounds, than the products without carriers [17]. Which is also confirmed by other authors who confirmed that the use of carriers affects the protection of bioactive compounds [32,33]. Di fferent interactions between the powders compounds and the carrier might also occur compared to the powders without a carrier [32].

**A** 

**Figure 2.** *Cont.*

**C** 

**Figure 2.** Principal component analysis (PCA) of the impact of carriers' concentration on phytochemicals in fruit (**A**), juice (**B**), pomace (**C**) powders. *Abbreviations:* 30%, 40%, 50%, concentration; ANT—sum of anthocyanins; FL—sum of flavonols; PA—sum of phenolic acid; PP—polymeric procyanidins; F3O—sum of flavan-3-ols (monomers and oligomers); DP—degree of polymerization; PC—sum of polyphenolic compounds; **<sup>1</sup>**—cyanidin-3-*O*-galactoside; **<sup>2</sup>**—cyanidin-3-*O*-glucoside; **<sup>3</sup>**—cyanidin-3-*O*-arabinoside; **<sup>4</sup>**—cyanidin-3-*O*-xyloside; **<sup>5</sup>**—cyanidin; **<sup>6</sup>**—protocatechuic acid; **7**—caffeic acid glucoside; **8**—caffeoylhexose; **9**—trihydroxycinnamoylquinic acid isomers; **10**—3-*O*-caffeoylquinic acid; **11**—5-*O*-caffeoylquinic acid; **12**—4-*O*-caffeoylquinic acid; **<sup>13</sup>**—3-*O*-*p*-coumaroylquinic acid; **14**—di-caffeoylquinic acid; **15**—di-caffeoylquinic acid; **<sup>16</sup>**—kaempferol-3-*O*-galactoside; **<sup>17</sup>**—quercetin-3-*O*-arabinobioside; **<sup>18</sup>**—kaempferol-3-*O*-glucoside; **19**—quercetin; **<sup>20</sup>**—quercetin-3-*O*rutinoside; **<sup>21</sup>**—quercetin-3-*O*-robinobioside; **<sup>22</sup>**—quercetin-3-*O*-galactoside; **<sup>23</sup>**—quercetin-3-*O*-glucoside; **<sup>24</sup>**—quercetin-3-*O*-arabinoside; **<sup>25</sup>**—quercetin-3-*O*-xyloside; **<sup>26</sup>**—quercetin-3-*O*-(6"-acetyl)glucoside; **<sup>27</sup>**—quercetin-3-*O*-(6"-acetyl)galactoside; **<sup>28</sup>**—quercetin-deoxyhexo-hexoside; **29**—sum of B-type procyanidin tetramer; **30**—sum of B-type procyanidin trimer; **31**—sum of B-type procyanidin dimer; **32**—A-type procyanidin dimer; **33**—(-)-epicatechin; **34**—(+)-catechin.

#### *2.4. Impact of the Type of Drying Method on Polyphenolic Compounds and Antioxidant Capacity in Dependence on the Matrix*

The PCA analyses showed that the powders produced after the freeze-drying process had the highest content of almost all polyphenolic compounds and antioxidant activity, regardless of the matrix tested (Figure 3). Similar observations were made during drying Averrhoa carambola pomace. The freeze-drying with carriers was more effective in ensuring the retention of polyphenolic compounds when compared to spray drying [12]. Moreover, after freeze-drying Averrhoa carambola pomace, it was noted that the higher the drying process temperature, the lower the antioxidant activity, while opposite observation was made for the juice powder. The higher the vacuum drying temperature, the stronger the degradation of anthocyanins in juice powders made from black currant. However, vacuum drying at 50 ◦C affected high retained phenolic acids and flavonols [16]. The best effect of drying cranberry products was obtained after spray-drying and freeze-drying, while an increase in aglycon of quercetin after vacuum-drying at 60 ◦C was observed [31]. Therefore, it can be concluded that the antioxidant activity of the tested material was dependent on the content of polyphenolic compounds, which did not degrade under mild freeze-drying conditions.

**Figure 3.** *Cont.*

**C** 

**Figure 3.** Principal component analysis (PCA) of the impact of drying method on phytochemicals in fruit (**A**), juice (**B**), pomace (**C**) powders. *Abbreviations:* FD, freeze-drying; VD/50, vacuum-drying in 50 ◦C; VD/60, vacuum-drying in 60 ◦C; ANT—sum of anthocyanins; FL—sum of flavonols; PA—sum of phenolic acid; PP—polymeric procyanidins; F3O—sum of flavan-3-ols (monomers and oligomers); DP—degree of polymerization; PC—sum of polyphenolic compounds; **<sup>1</sup>**—cyanidin-3-*O*-galactoside; **<sup>2</sup>**—cyanidin-3-*O*-glucoside; **<sup>3</sup>**—cyanidin-3-*O*-arabinoside; **<sup>4</sup>**—cyanidin-3-*O*-xyloside; **<sup>5</sup>**—cyanidin; **<sup>6</sup>**—protocatechuic acid; **7**—caffeic acid glucoside; **8**—caffeoylhexose; **9**—trihydroxycinnamoylquinic acid isomers; **10**—3-*O-*caffeoylquinic acid; **11**—5*-O*-caffeoylquinic acid; **12**—4*-O*-caffeoylquinic acid; **<sup>13</sup>**—3-*O*-*p*-coumaroylquinic acid; **14**—di-caffeoylquinic acid; **15**—di-caffeoylquinic acid; **<sup>16</sup>**—kaempferol-3-*O*-galactoside; **<sup>17</sup>**—quercetin-3-*O*-arabinobioside; **<sup>18</sup>**—kampferol-3-*O*-glucoside; **19**—quercetin; **<sup>20</sup>**—quercetin-3-*O*xrutinoside; **<sup>21</sup>**—quercetin-3-*O*-robinobioside; **<sup>22</sup>**—quercetin-3-*O*-galactoside; **<sup>23</sup>**—quercetin-3-*O*-glucoside; **<sup>24</sup>**—quercetin-3-*O*-arabinoside; **<sup>25</sup>**—quercetin-3-*O*-xyloside; **<sup>26</sup>**—quercetin-3-*O*-(6"-acetyl)glucoside; **<sup>27</sup>**—quercetin-3-*O*-(6"-acetyl)galactoside; **<sup>28</sup>**—quercetin-deoxyhexo-hexoside; **29**—sum of B-type procyanidin tetramer; **30**—sum of B-type procyanidin trimer; **31**—sum of B-type procyanidin dimer; **32**—A-type procyanidin dimer; **33**—(-)-epicatechin; **34**—(+)-catechin.

Vacuum drying method affected the retention of individual compounds: for fruit powders, vacuum drying at 50 ◦C resulted in a higher retention of hydroxybenzoic acid (protocatechuic acid), and hydroxycinnamic acid (caffeic acid) in powders whereas drying at 60 ◦C had an impact on B-type procyanidin dimer, and tetramer, 4, 3-*O*-caffeoylquinic acids, di-caffeoylquinic acid, free cyanidin, and quercetin aglycon. In the case of juice powders, application of the temperature of 50 ◦C during vacuum drying resulted in a higher retention of quercetin-3-*O*-robinobioside, -3-*O*-arabinoside, and quercetin aglycon. Drying at 60 ◦C influenced a higher content of total flavonols and their derivatives, flavan-3-ols and their monomers and oligomers, and free cyanidin aglycon. However, in blackcurrant juice powders, the vacuum drying at 50 ◦C and 70 ◦C caused a higher retention of anthocyanins, and according to the authors, this could be due to the inactivation of polyphenol oxidase [16]. In the

present study, the higher temperature contributed only to the release of free aglycon of anthocyanins. As far as the pomace powders are concerned, the vacuum drying at 50 ◦C had a strong impact on the content of free aglycon, and quercetin-3- *O*-rutinoside. The drying at 60 ◦C influenced the retention of monomers ((−)-epicatechin) and oligomers of flavan-3-ols, and total flavonols and their derivatives. On the other hand, among all compounds identified in flavan-3-ols group, (−)-epicatechin content in juice powders was 2.8 times higher after vacuum drying at 60 ◦C when compared to the freeze-drying. This suggests the temperature-depended release of this compound from polymerized structures. A similar observation was made for blackcurrant juice the vacuum drying of which at 90 ◦C resulted in 130 times higher (+)-catechin content compared to vacuum drying at 50 ◦C. The authors concluded that the controlled release of compounds from polymerized structures during drying may be helpful in obtaining the desired content of polyphenolic compounds in the powders [16]. In turn, a similar increase of flavonols aglycon content under the influence of high temperature as a result of the deglycosylation of flavonol glycosides was observed in cranberry products [31,34]. In addition, similarly to cranberry juice powders [31], the temperature influenced the retention of total flavonols in juice and pomace powders made from Saskatoon berry. This can also be confirmed by negative correlation between flavonols and antioxidant activity of *r* = −0.265 for ABTS assay, and *r* = −0.253 for FRAP assay (for juice powders), and *r* = −0.925 for ABTS assay, and *r* = −0.890 for FRAP assay (pomace powders). Moreover, the increased content of flavonols and their derivatives was also observed upon vacuum drying of juice and pomace powders made of black currant at 50 ◦C and 70 ◦C [16,35]; however, the authors observed that an increase of temperature above 80 ◦C and 90 ◦C decreased flavonols content. Among all of the compounds tested, anthocyanins were the most unstable constituents when the higher temperature of drying was applied. Their average amount after vacuum drying at 50 ◦C was 42% lower when compared to the freeze-drying. Moreover, the increase of the temperature during vacuum drying by 10 ◦C caused their 13% loss. Bakowska-Barczak and Kołodziejczyk [29] reported that the higher the temperature during drying black current powder, the stronger the degradation of anthocyanins. Cai and Corke [36] also noted that a higher drying temperature had a stronger e ffect on amaranthus betacyanins degradation. On the other hand, depending on the matrix tested, the smallest degradation of anthocyanins was noted in the pomace powder after freeze-drying and it was 1.4 and 1.7 times lower when compared to vacuum drying at 50 and 60 ◦C, respectively. While, degradation of anthocyanins in the fruit and juice powder after vacuum drying at 50 and 60 ◦C was 56% and 65%. Probably the highest retention of compounds from pomace can be due to lower water activity, and also with location of compounds because most of them are distributed in berry skin which does not lead to their complete degradation during heat conditions [21,22]. Thus, the research confirmed that mild conditions of freeze-drying ensured the protection of anthocyanins, and this was in line with the previous reports showing that the temperature strongly a ffected their degradation [37–39]. Moreover, the higher the drying temperature is, the greater the degradation of the polyphenolic compounds and their antioxidant activity. The temperature of 50 ◦C influenced the release of quercetin aglycon. Regardless of the matrix tested, the temperature of 60 ◦C used for vacuum drying resulted in greater retention of phenolic acid derivatives as well as flavan-3-ols monomers ((−)-epicatechin) and oligomers. It could be due to the partial inactivation of polyphenol oxidase, because Siddiq et al. [40] noted that PPO lost about partial inactivation during thermal treatment of blueberry at 55 and 65 ◦C [40]. Therefore, the selection of drying technique for the preparation of Saskatoon berry powders is highly important when the retention of bioactive compounds is concerned.




**Table 2.** Antioxidant activity [mmol Trolox/100 g d.m.] of the fruit, juice, and pomace powders made from Saskatoon berry.



**Table 2.** *Cont.*

1 Values are expressed as the mean (*n* = 3) ± standard deviation. ND, not detected; FD, freeze-drying; VD/50, vacuum-drying at 50 ◦C; VD/60, vacuum-drying at 60 ◦C.
