The Responses of Bioactive Betanin Pigment and Its Derivatives from a Red Beetroot (Beta vulgaris L.) Betalain-Rich Extract to Hypochlorous Acid

Neutrophils produce hypochlorous acid (HOCl) as well as other reactive oxygen species as part of a natural innate immune response in the human body; however, excessive levels of HOCl can ultimately be detrimental to health. Recent reports suggest that betacyanin plant pigments can act as potent scavengers of inflammatory factors and are notably effective against HOCl. Comparison of the in vitro anti-hypochlorite activities of a novel betalain-rich red beetroot (Beta vulgaris L.) extract with its pure betalainic pigments revealed that the extract had the highest anti-hypochlorite activity, far exceeding the activity of all of the betalainic derivatives and selected reference antioxidants. This suggests that it may be an important food-based candidate for management of inflammatory conditions induced by excessive HOCl production. Among all pigments studied, betanidin exhibited the highest activity across the pH range.

The attributes of betalains as natural colorants provide a wide spectrum of applications as natural additives in the food industry [1][2][3]. It is worth noting that no adverse effects have ever been reported due to the ingestion of betalains by living organisms [4]. Betalain pigments have the ability to bioaccumulate in blood and yet are generally excreted from the body via the urine within a few hours after ingestion [3,4]. Besides being extensively used in the food industry as natural food colorants, betalains exhibit strong antioxidant and chemopreventive activities [1][2][3][4]. These characteristics contribute to the increased interest in betacyanins, especially from B. vulgaris root, in oncology applications [3,4]. Furthermore, recent studies indicate that betalains can act as potent scavengers of inflammatory factors [5,6] and may improve various health conditions related to inflammation [7,8]. Hypochlorous acid (HOCl) is an important reactive oxygen species (ROS) that causes oxidation and chlorination reactions. It is produced by activated neutrophils and monocytes via the reaction of H 2 O 2 with Cl − ions catalyzed by the heme enzyme myeloperoxidase [9,10]. In living systems, HOCl can react at the molecular level with primary amines and other N-compounds, leading to the formation of chloramines and N-Cl derivatives [11]. The presence of HOCl and its derivatives in intercellular spaces can lead to the local irritation of epithelial tissue cells, damage of proteins, nucleotides, DNA, RNA, fatty acids, or cholesterol [11][12][13][14][15].
Although neutrophilic production of HOCl is part of a natural innate immune response, excessive HOCl levels can ultimately be detrimental to health. The harmful impact of hypochlorite derivatives occurs in people suffering from chronic inflammation, e.g., joints. Overproduction of HOCl during inflammation may also cause or enhance the pathogenesis of various diseases including Alzheimer's disease, cardiovascular disease, atherosclerosis, organ transplant rejection, and even certain cancers [11]. In individuals with joint distress, locally elevated concentrations of hypochlorous acid and other ROS contribute to the stimulation of the immune system and to the increased production of antibacterial compounds [7,8,12]. Allegra et al. reported the effectiveness of betanin and indicaxanthin in scavenging hypochlorous acid [16].
Previously, a novel betalain-rich extract/concentrate (BRE) was tested in a pilot clinical study that reported short-term treatment with BRE improved the function and comfort of knee joints in individuals with knee distress [7,8]. Said BRE was designed to deliver the benefits of betalains without the accompanying sugars, nitrates, and calories from beetroot, and is currently being used as a dietary supplement [17]. During extraction, naturally occurring sugar derivatives and nitrates are selectively eliminated in order to yield a standardized minimum weight content of 25% betalain. BRE contains mainly betanin, neobetanin, and some decarboxylated derivatives [17].
Another study indicated that betalains are readily chlorinated in the presence of HOCl at pH 3-5; however, when the pH of the reaction mixture is increased, the oxidation of betalains prevails [5,6]. Therefore, the ability of betalains to react with hypochlorous acid within a wide pH range [5,6] suggests the possible use of BRE as a dietary supplement for the support of healthy scavenging of HOCl in vivo. Recently, we worked to prove the hypothesis of the betacyanin chlorination mechanism by HOCl [5,6,18]. This was accomplished by LCMS-IT-TOF and NMR analyses of the resultant chlorination products [18].
In this contribution, we used fluorescent methods that employed two novel HOClspecific BODIPY-based HCSe and HCS probes [19,20] to study the in vitro anti-hypochlorite activities of selected purified betacyanins and their derivatives as well as the BRE, considering the reactivity of particular betalainic pigments depending on the structures of the active compounds.
HCSe and HCS are novel, fluorescent probes based on the BODIPY skeleton. They are sensitive to hypochlorous acid. These probes produce no fluorescence in acetonitrile/aqueous solutions in the absence of hypochlorous acid. The addition of HOCl to a reaction mixture induces a selective oxidation of the probes, leading to the formation of strong fluorescent derivatives HCSeO or HCSO, respectively [19,20]. An important characteristic of the probes is that they are highly sensitive to hypochlorous acid at pH 7.4 and are able to penetrate the membranes of living cells. This allows for their utilization in in vitro assays that simulate inflammatory processes due to the presence of HOCl and OClat a physiological pH of 7.4 [19,20].

Results and Discussion
Our previous studies on the mechanism of betacyanin chlorination indicated that the formation of monochlorinated betanin and betanidin (as well as their respective decarboxylated derivatives) resulted from the reaction of betacyanins with HOCl or Cl 2 O. Cl 2 O is a potent chlorinating agent and coexists with HOCl in equilibrium, especially in acidic conditions [5,6,18]. The experiments were monitored by HPLC with low-resolution mass spectrometric detection. These chemical changes were studied also by the enzymatic chlorination of betacyanins catalyzed by MPO at NaCl concentration (150 mM-typical to normal physiological levels), enabling a slow and continuous production of HOCl from Cl − [5]. The chlorination mechanism and the position of the electrophilic substitution in betacyanins (Figure 2), as well as their molecular formulas, were studied using detailed mass spectrometric experiments on the fragmentation of the chlorinated pigments performed by the high-resolution IT-TOF technique [5,6,18]. The reactions with HOCl and Cl 2 O were proposed ( Figure 2) according to an electrophilic mechanism based upon the departing group ability from Cl + in HOCl (-OH − ) and in Cl 2 O (-OCl − ) [5,18]. This is also supported by the inactivity of neobetanin towards chlorination. Neobetanin is an aromatized betanin with a pyridine ring resulting from betanin oxidation. The fact that this ring cannot be chlorinated suggests that in betacyanins, only the unsaturated bond is attacked, preferably at C-18 due to its partial negative charge [5]. The mass spectrometric studies were further supported by additional structural analyses using NMR techniques that completed the identification of the chlorinated betacyanins [18]. In this study, a comparison of chlorination kinetics was conducted during measurements of the in vitro anti-hypochlorite activity of pure isolated betalainic pigments from BRE. Earlier comprehensive characterization of the BRE [17,21] enabled isolation of betalainic pigments and further study on the chlorination/oxidation of betanin as well as its derivatives for elucidation of different reaction mechanisms [5,6,18]. As mentioned previously [17], the Nilsson calculation method [22] of betalain total concentration is related to betacyanins and betaxanthins only when there is a lack of their derivatives in the formulations. Therefore, the calculated results for the yellow components of the BRE roughly represent the following group of betalains: betaxanthins, neobetanin as well as decarboxylated betacyanins, neobetacyanins, and xanneobetacyanins [17]. This is important when establishing correlations between concentrations of betalains in complex mixtures and their respective activities, such as anti-hypochlorite activity or free-radical scavenging capacity as measured in this study.
This contribution reports on their anti-hypochlorite activity also compared to their antioxidant activity [23].

No.
Compound In order to simplify the nomenclature, we propose the substitution of the phrase "xan" instead of "2,3-dehydro" in the trivial name of the 2,3-dehydrogenated betacyanins in accordance with our previous contribution [26]. Such a simplification is similar to the "neo" prefix used for several decades to replace the cumbersome "14,15-dehydro". The "xan" prefix underlines the hypsochromic effect observed after dehydrogenation of betacyanins that leads to the formation of yellow pigments. Therefore, because betacyanins can appear as both 2,3-and 14,15-dehydrogenated, there is a group of pigments formed that can be called "xanneobetacyanins". In the BRE, three compounds from such a group were tentatively detected, together with four neobetacyanins [17].
The single chromatographic peak of 15-decarboxy-betanin 3 ( Figure 1) with an absorption maximum at λ max 528 nm is very well separated from 17-decarboxy-betanin/isobetanin 2/2 and 2-decarboxy-betanin/-isobetanin 4/4 also present in the extract [17]. The enrichment of 15-decarboxy-betanin 3 in the BRE is at a similar level as for 2/2 , suggesting the same formation rate; therefore, it is one of the main decarboxylation derivatives of betanin formed during the preparation of the extract. The most hydrophobic product of betanin degradation/oxidation is 2-decarboxy-xanneobetanin 8, characterized by a single chromatographic peak, indicating the lack of chirality at carbon C-15, and by the absorption maximum at λ max 422 nm. From the point of view of oxidation studies, this is an important compound because it is generated from betanin, most likely via an unstable quinone methide intermediate and the fairly stable 2-decarboxy-2,3-dehydro-betanin (2decarboxy-xanbetanin) [24,25], which is oxidized in the second step to a much more stable 2-decarboxy-xanneobetanin 8 ( Figure 1).

Chlorination of Betanin by Sodium Hypochlorite
The results obtained after 10 min spectrophotometric tracing of betanin 1, betanidin 5, and neobetanin 7 reaction progress induced by NaClO (Table 2, Figure 3) reveal the differences between the partially oxidized betacyanin (neobetanin 7) which does not undergo chlorination [5] and non-oxidized betacyanins (1 and 5) which are easily chlorinated at pH 3. The chlorination effects are detected by the hypsochromic shift of absorption maximum λ max from ca. 538-540 nm (for 1 and 5) to 522-524 nm typical of chlorinated betacyanins. This effect is not observed for neobetanin 7 and is also diminished at higher pH (5 and 7.4) for 1 and 5 ( Figure 3). In those cases, the main reaction processes involve oxidation of the pigments, presumably by HClO or other chlorine species being in equilibrium in the reacting solution [5].
Therefore, interpretation of the results of the anti-hypochlorite activity measurements should take into account that scavenging of hypochlorous acid by betalains proceeds according to different mechanisms and is especially different at pH 3 and at 7.4. Betalains exhibit a high tendency to be chlorinated at pH 3 but at pH 7.4, their rapid oxidation by hypochlorous acid is observed [5]. In addition, according to the presented results on chlorination and oxidation of betanin by NaOCl at pH 7.4 (Table 2, Figure 4), a multipath of the reactions can be deduced ( Figure 5). The chromatograms of selected ions corresponding to the products of betanin chlorination and oxidation are depicted in Figure 4A,B and support the presence of oxidized derivatives not only of betanin but also of betanidin in the reaction mixtures at pH 7.4. Therefore, oxidation of betanin 1 results in the formation of 2-decarboxy-xanbetanin 16 at the first typical step observed for betacyanins [24] but at the same time, generation of the deglucosylated derivative 2-decarboxy-xanbetanidin 18 is detected. The deglucosylation of 1 presumably results from the formation of the quinonoid system during the oxidation of betanin which influences the stability of the 5-O-glucosidic bond. This phenomenon is analogous to the deglucosylation of gomphrenin during its oxidation by ABTS cation radicals [27]. As in the case of gomphrenin oxidation [27], this should be taken into account during the anti-hypochlorite activity measurements since the occurrence of betanidin or its derivatives as potent antioxidants in the reaction mixtures may be responsible for increasingly potentiating the high overall activity of betalains.  Proposed mechanism of betanin oxidation by NaOCl with subsequent alternate pathways of deglucosylation, decarboxylation, and chlorination steps based on this contribution and previous study [5].
The detected ions fit to the oxidation pathway of betanidin 7 studied previously [24]; however, in this case, it is implemented in the whole representative reaction scheme for betanin 1 transformations ( Figure 5).

Determination of Betalainic Reactivity against Hypochlorites by Measurements of Anti-Hypochlorite Activity with the Use of HCSe and HCS Fluorescent Probes
Further study on the chlorination kinetics was possible to perform using in vitro anti-hypochlorite activity measurements of pure isolated betalainic pigments from the red beetroot extract (BRE). This gave a detailed insight to the differences of the chlorination ability of HOCl towards different pigments at selected pHs of the tested solutions but also into the combined effect with oxidation.
Due to the fact that HOCl may be associated with various diseases, there is a growing need to develop a rapid and effective method for its detection and determination. Unfortunately, the development of novel methods for the detection of HOCl in vivo remains challenging due to its short half-life and the concurrent existence of various antioxidants within cells such as glutathione (GSH) and cysteine (Cys) [11,12]. In recent years, various analytical and bioanalytical methods, including traditional detection approaches such as chemiluminescence, colorimetric, electrochemical, and chromatographic techniques have been applied [11,12]. Among them, fluorescent methods exhibit more advantages in terms of selectivity, sensitivity, and spectral resolution. Fluorescent probes have shown promise as analytical tools for rapid and specific detection of HOCl/OCl − [28,29]. Commonly utilized fluorescent probes for sensing HOCl are based on the skeleton of fluorescein [29][30][31][32], rhodamine [32][33][34], BODIPY (boron-dipyrromethene) [19,20,[35][36][37], or coumarin [38,39]. Recently, HOCl fluorescent probes based on 1,8-naphthalimide [40] or phenothiazine [41] have also been designed and synthesized.
The HCSe and HCS probes' high sensitivity to hypochlorous acid encouraged us to investigate their respective applicability in determination of betalains' anti-hypochlorite activities. According to our results, these probes remained active, even when utilized within a more acidic environment ( Figure 6). Consequently, in this study, our intention was to expand the working range of the probes to pH 3-7.4 in order to make it possible to test the anti-hypochlorite activity even when pH was as low as 3 when high chlorinating activity of NaOCl against betacyanins is observed [5,6]. Due to a much lower HOCl reaction rate observed for the HCS probe [19,20], the HCSe probe was selected for further studies wherein ca. 95 and 99.9% completion of the oxidation by HOCl was observed after 5 and 10 min, respectively. According to recent results [19,20], strong decreases in the emission of both the probes at higher pH (8)(9)(10) can be attributed to nearly complete ionization of HOCl, indicating that the reactive moiety for oxidation of the probes is HOCl but not OCl − [9]. As mentioned above, this was at least partially confirmed in this study due to the fact that at more acidic pH, these probes are still active against HOCl ( Figure 6). The studies on betalain anti-hypochlorite activity using the HCSe probe were performed for the BRE, its isolated betacyanins, betanin derivatives, and other selected antioxidants such as quercetin, catechin, caffeic acid, and ascorbic acid. The sensing performance of the HCSe probe was tested towards 150 µM NaOCl across a wide pH range. The fluorescence intensity of the reaction between HOCl and the HCSe is linear in the NaOCl concentration range of 0 to 200 µM ( Figure 6). Therefore, the anti-hypochlorite activity tests related to 150 µM NaOCl were performed at pH 3, 5, and 7.4 in order to generate a comparison of the activities of the tested compounds in solutions containing meaningfully different composition of chlorine entities [5,6,9]. Based on previous results, partial conversion of HOCl to Cl 2 O in acidic conditions as well as the greater ability of Cl 2 O to chlorinate even at lower concentrations than HOCl should also be considered [9].
As a result of the scavenging of hypochlorous acid by the selected pigments, a decrease in the intensity of fluorescence emission was observed for all of the reaction mixtures along with the increase in the analytes' concentrations. The concentrations (C 50 ) of the measured anti-hypochloric agents required for a 50% decrease in fluorescent emission of the 150 µM HCSe probe after 5 min of incubation with a reaction mixture of 150 µM NaOCl and the anti-hypochloric agent at 25 • C are presented in Table 3. Despite the betalains exhibiting significantly lower tendency of being chlorinated under physiological conditions compared to pH ranging from 3 to 5, a rapid elimination of hypochlorous acid at pH 7.4 was also noticed, presumably by betalains' oxidation [5]. Fluorescence quenching for micro-molar concentrations of betalains as well as selected antioxidants is shown in Figure 7A-E. Based on the results of initial slope "a" factors' measurements (Table 3) for fluorescence intensity-compound concentration dependence, the anti-hypochlorite activity (anti-HA) of the analytes related to Trolox (the water-soluble analogue of vitamin E), having a wellknown antioxidant capacity and frequently used as a reference, was calculated ( Figure 8, Table 3). The first inspection of the results (Figures 7 and 8A, Table 3) enables us to conclude that the reactivity of Trolox with hypochlorous acid at pH 3 ( Figure 7A,B) is much lower than at pH 5 ( Figure 7C,D) and 7.4 ( Figure 7E,F); therefore, relating the analytes' activity to Trolox for comparison reasons in a wide pH range misleadingly increases the anti-HA values for all the tested compounds. Therefore, for this aim, a comparison of the analyte initial slope "a" factors to ascorbic acid (another antioxidant that exhibits the lowest activity) was also performed ( Figure 8B) resulting in a decrease in anti-HA values at pH 3 to the levels observed at pH 5 and 7.4 for all the samples. The data suggest that all the tested compounds except Trolox can be applied as a reference in similar studies. In Figure 8A, the anti-HA values of the analytes were additionally compared to the antioxidant capacity for ABTS cation radicals determined at pH 7.4 as Trolox equivalent antioxidant capacity (TEAC). Comparison of these results allows for a conclusion that they all reasonably correlate even at pH 3; therefore, it more generally supports the oxidizing action of the hypochlorous acid rather than chlorination as a means of their scavenging by the analytes.
Betanin 1 is capable of suppressing the fluorescence of the 150 µM HCSe probe at physiological pH 7.4 and phagosomal pH 5 in the presence of 150 µM NaOCl after 5 min of incubation at room temperature (Figures 7 and 8A). It is worth noting that the required concentration of betanin pigment for complete removal of 150 µM OCl − ranges from 0 to 20 µM at any tested pH (Figure 7). This indicates the high capability of betanin to scavenge hypochlorous acid well beyond the consequence of pigment chlorination even at pH 3 [5]. Betanidin 2 is even more effective in the removal of HOCl than 1 as a result of its reactive catechol moiety which is confirmed by the TEAC value. Betanidin 2 concentration, required for complete suppression of the fluorescence at pH 7.4, is almost two times lower than in the case of its glycosylated derivative 1 (Figures 7 and 8A). The anti-hypochlorite activity of 17-decarboxy-betanin 2, 2-decarboxy-betanin 4, 2,17-bidecarboxy-betanin 6/6 , and 2-decarboxy-xanneobetanin 8 are at similar levels and are slightly lower in relation to betanin 1 in contrast to 15-decarboxy-betanin 3. Lower activity was observed for neobetanin 7, which may result from the partial oxidation of the molecule (Figure 1) at carbons C-14,15 and thus, may lead to a completely different mechanism of chlorination/oxidation reaction as compared to the one previously stated in studies with NaOCl [5], where the neo-derivative 7 of betanin did not undergo chlorination. As a consequence, the antihypochlorite activity of 7 should be attributed to other chemical transformations.
For comparative purposes, four well-known antioxidants were also analyzed under the same reaction conditions. In comparison to betanidin 5, much lower activity for ascorbic acid 9 and caffeic acid 10 was observed, while catechin 11 and quercetin 12 exhibit similar or slightly lower anti-hypochlorite and antioxidant properties (Figures 7 and 8B, Table 3). The highest anti-hypochlorite activity and antioxidant capacity, and far exceeding the activity all of the betalain derivatives and selected antioxidants, were determined for the BRE. Its ability to scavenge hypochlorous acid is approximately twice the activity of the strongest pigment, betanidin 5, at all of the tested pH values (Figures 7 and 8, Table 3). A precise explanation of such high BRE activity requires further analytical research. Its higher activity could possibly be due to the composition of the extract containing some synergistic group of betalain derivatives that influences the overall activity of BRE. Additionally, other still unidentified or unknown compounds that occur naturally in red beetroot may be present in the extract. In any event, the superior anti-HOCl activity of BRE reported here must be ascribed to inherent structures present in BRE that possess rapid electron exchange potential with reducing agents such as HOCl or other ROS. In our previous studies, we have demonstrated that the metabolism of betalains in the human body results in structures with similar potential to the ones elucidated in this study. Logically, it follows that BRE and/or its fractions may serve as readily oxidizable decoys that could potentially be employed to protect biological tissues and cells from inflammatory insult from HOCl generated by chronic inflammation. Table 3. Anti-hypochloric activity (Anti-HA) of betanidin (Bd), betanin (Bt), and its derivatives (17-decarboxy-betanin (17-dBt), 15-decarboxy-betanin (15-dBt), 2-decarboxy-betanin (2-dBt), betanidin (Bd), 2,17-decarboxy-betanin (2,17-dBt), neobetanin (NeoBt), and 2-decarboxy-xanneobetanin (2-dXNBt)) and selected antioxidants (ascorbic acid (ASC), caffeic acid (CAF), catechin (CAT) and quercetin (QUE)) related to Trolox (TROL) based on measurements of initial slope "a" factors for fluorescence intensity-compound concentration dependence at selected pH. C50-concentration of the measured anti-hypochloric agent required for a 50% decrease in the fluorescence emission of the 150 mM HCSe probe after 5 min of its incubation with reaction mixture of 150 mM NaOCl and the anti-hypochloric agent at 25 • C. The measurements were performed in triplicate.
For the direct isolation of pigments from BRE, 10 g of the extract was dissolved in 10 L of water and was initially purified by ion-exchange chromatography. Obtained fractions were subjected to further semi-preparative HPLC purification. In order to obtain betanidin 5, purified betanin was subjected to enzymatic deglycosylation catalyzed by almond β-glycosidase and further preparative fractionation in accordance with previously developed protocols [24]. 2-decarboxy-betanin 4 and 2,17-bidecarboxy-betanin/-isobetanin 6/6 were obtained by thermal degradation of aqueous and ethanolic solutions of purified betanin acidified with glacial acetic acid at 85 • C (aqueous solution) and 75 • C (ethanolic solution) in a water bath for 40 min according to a previously published procedure [21].

Preparative Oxidation of Betanin and Neobetanin by ABTS Cation Radicals
In order to obtain 2-decarboxy-xanneobetanin 8, ABTS cation radicals generated from ABTS salt were gradually added to 500 mL of solution containing 50 mg of betanin 1 in 10 mM acetate buffer of pH 5. The solution was stirred on a magnetic stirrer and the absorption at λ max 538 nm was measured until it was diminished three times. After the next 10 min, the mixture was subjected to isolation and purification using the ion-exchange chromatographic system and semipreparative HPLC.

Semi-Preparative HPLC Purification of Betalain Fractions
Preliminary purification of the pigments was performed by flash chromatography on a column 30 × 40 mm filled with Sepra™ ZT-SAX 30 µm polymer, 85 Å (Phenomenex, Torrance, CA, USA). Further separation and isolation of pigments were performed on a HPLC semipreparative column Luna C18(2) 250 × 20 mm i.d., 10 µm (Phenomenex) with a 20 × 25 mm i.d. guard column of the same material (Phenomenex). A gradient system consisting of 1% aqueous formic acid (solvent A) and acetone (solvent B) for semisynthesized betanidin 5 was used as follows: 0 min, 10% B; increasing to 10 min, 12% B; increasing to 20 min, 14% B; increasing to 30 min, 70% B and for betanin was used as follows: 0 min, 10% B; increasing to 10 min, 11% B; increasing to 20 min, 12% B; increasing to 30 min, 13% B; increasing to 40 min; 70% B. The injection volume was 15 mL with a flow rate of 20 mL/min. Detection was performed using a PDA UV/Vis detector at 538, 505, 480, and 440 nm, at a column temperature of 22 • C. The eluates were pooled and concentrated under reduced pressure at 25 • C and finally, freeze-dried. All the solutions were concentrated in rotary evaporators at 25 • C under reduced pressure to remove the organic solvent and stored at −20 • C for further assays.

Chromatographic Analysis by LC-DAD-ESI-MS/MS System
For the chromatographic and mass spectrometric analyses, an LCMS-8030 mass spectrometric system (Shimadzu, Kyoto, Japan) coupled to LC-20ADXR HPLC pumps, an SIL-20ACXR injector model, and a PDA (photo diode array) detector model SPD-M20A, all controlled with LabSolutions software version 5.60 SP1 (Shimadzu) was used. The samples were eluted through a 150 × 4.6 mm i.d., 5.0 µm, Kinetex C18 chromatographic column preceded by a guard column of the same material (Phenomenex, Torrance, CA, USA). The injection volume was 20 µL and the flow rate was 0.5 mL/min. The column was thermostated at 40 • C. The separation of the analytes was performed with a binary gradient elution. For the separation, a gradient system consisting of 2% aqueous formic acid (solvent A) and pure methanol (solvent B) was used as follows: 0 min, 5% B; increasing linearly to 12 min, 30% B; increasing linearly to 15 min, 80% B. The full range of PDA signals was recorded and chromatograms were individually displayed at 538, 505, 490, and 440 nm. Positive ion electrospray mass spectra were recorded on the LC-MS system, which was controlled with LabSolutions software for registration of total ion chromatograms, mass spectra, and ion chromatograms in selected ion monitoring mode (SIM) as well as the fragmentation spectra. The ionization electrospray source was operated in positive mode (ESI+), at an electrospray voltage of 4.5 kV and capillary temperature at 250 • C, using N 2 as a gas for the spray. Argon was used as the collision gas for the collision-induced dissociation (CID) experiments. The relative collision energies for MS/MS analyses were set at −35 V.

HCSe and HCS Assays for Determination of Anti-Hypochlorite Activity
For determination of the ability of betalains and BRE to scavenge hypochlorous acid, pigment solutions of gradually increasing concentrations were dosed to wells of the black 96-well plate (Nunc™ F96 MicroWell™ Black Polystyrene Plate, Thermo Scientific™, Waltham, MA, USA) buffered with 25 mM acetate (pH 3 and 5) and phosphate (pH 7.4) buffers. Afterwards, an acetonitrile/aqueous solution of NaOCl was added to the wells and the final concentration was 150 µM in 200 µL of the total sample volume. After 5 min of chlorination reaction, 60 µL of 500 µM HCSe or HCS acetonitrile solution was dosed into the wells for their final concentration of 150 µM. Then, the plate was shaken for 20 s and the fluorescence was measured in a Tecan Infinite 200 microplate reader (Tecan Austria GmbH, Grödig/Salzburg, Austria). The HCSe and HCS probes were excited at λ Exc 480 nm and the emission signal was monitored at λ Em 536 and 515 nm, respectively. Then, fluorescence spectra were recorded for all wells at the range of λ 500-650 nm, excited by light of λ Exc 480 nm. Similar measurements were performed for selected, commonly known antioxidants including: ascorbic acid 9 (ASC), caffeic acid 10 (CAF), catechin 11 (CAT), and quercetin 12 (QUE). The concentrations of measured pigments as well as selected antioxidants were individually set for each sample so that the fluorescence decrease in the probes was in the range of 10-90% of their initial value in the sample without tested analytes. The results for all tested compounds were referenced to a standard of Trolox as well as ascorbic acid. All measurements were repeated in triplicate.

Measurement of Antioxidant Activity with ABTS Cation Radicals
The antioxidant activity of the tested BRE and isolated compounds was measured by the Trolox equivalent antioxidant capacity (TEAC) assay based on their reaction with ABTS cation radicals [23] in 96-well plates of a Tecan Infinite 200 microplate reader (Tecan Austria GmbH, Grödig/Salzburg, Austria). ABTS cation radicals were generated from ABTS salt by reaction of 2.45 mM potassium persulfate with 7 mM ABTS salt in 0.002 M phosphate-buffered saline at pH 7.4 for 16 h at room temperature in the dark. The resultant ABTS cation radical solution was diluted with water and adjusted to absorption of 0.7 at 734 nm for the experiments. Just before the measuring step, 10 µL of the measured sample dilutions were individually loaded into wells containing 190 µL of ABTS cation radicals. Then, the mixtures were shaken for 20 s by a shaker within the reader. The absorption measurement at 734 nm was performed after 30 min of reaction at 25 • C. All experiments were performed in triplicate.

Conclusions
The results of this study show that all of the tested betalainic pigments are efficient in the removal of hypochlorous acid; however, betanidin exhibited the highest activity. Additionally, the fact that betalains as well as the BRE inactivated HOCl within a few minutes, even at micro-molar concentrations, emphasizes their highly efficient anti-hypochlorite activity and possibility for applications in physiological conditions wherein HOCl has a very short half-life. In combination with the ability of fluorescent probes to penetrate cell membranes, BRE may also be used as a scavenging factor to remove HOCl in future in vitro trials. Finally, and of special interest, is the fact that BRE significantly and unexpectedly outperformed any of the individual pigments in terms of HOCl scavenging ability. As such, these results further support the use of BRE as a natural dietary supplement that may provide support against chronic inflammation.

Conflicts of Interest:
The authors declare no conflict of interest.