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Physicochemical properties of apple juice during sequential steps of the industrial processing and functional properties of pectin fractions from the generated pomace
Accepted Manuscript Physicochemical properties of apple juice during sequential steps of the industrial processing and functional properties of pectin fractions from the generated pomace Ana L. Ramos-Aguilar, Claudia I. Victoria-Campos, Emilio Ochoa-Reyes, José de Jesús Ornelas-Paz, Paul B. Zamudio-Flores, Claudio Rios-Velasco, Jaime ReyesHernández, Jaime D. Pérez-Martínez, Vrani Ibarra-Junquera PII:
S0023-6438(17)30600-X
DOI:
10.1016/j.lwt.2017.08.030
Reference:
YFSTL 6452
To appear in:
LWT - Food Science and Technology
Received Date: 16 March 2017 Revised Date:
9 August 2017
Accepted Date: 10 August 2017
Please cite this article as: Ramos-Aguilar, A.L., Victoria-Campos, C.I., Ochoa-Reyes, E., de Jesús Ornelas-Paz, José., Zamudio-Flores, P.B., Rios-Velasco, C., Reyes-Hernández, J., Pérez-Martínez, J.D., Ibarra-Junquera, V., Physicochemical properties of apple juice during sequential steps of the industrial processing and functional properties of pectin fractions from the generated pomace, LWT Food Science and Technology (2017), doi: 10.1016/j.lwt.2017.08.030. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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Physicochemical properties of apple juice during sequential steps of the
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industrial processing and functional properties of pectin fractions from the
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generated pomace
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Ana L. Ramos-Aguilar a, Claudia I. Victoria-Campos a, Emilio Ochoa-Reyes a,
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José de Jesús Ornelas-Paz
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Velasco a, Jaime Reyes-Hernández b, Jaime D. Pérez-Martínez c, Vrani Ibarra-
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Junquera d
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a
*, Paul B. Zamudio-Flores a, Claudio Rios-
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a,
Centro de Investigación en Alimentación y Desarrollo A.C.-Unidad Cuauhtémoc,
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Av. Río Conchos S/N, Parque Industrial, C.P. 31570, Cd. Cuauhtémoc,
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Chihuahua, México.
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b
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artillero No. 138, Zona Universitaria, C.P. 78210, San Luis Potosí, México.
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c
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Manuel Nava 6 Zona Universitaria, C.P. 78210, San Luis Potosí, México.
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d
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Colima, C.P. 28400, Coquimatlán, Colima, México.
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Universidad Autónoma de San Luis Potosí, Facultad de Ciencias Químicas,
Universidad de Colima, Bioengineering Laboratory, Km. 9 carretera Coquimatlán-
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Universidad Autónoma de San Luis Potosí, Facultad de Enfermería, Av. Niño
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Short running head: Quality of apple juice and pectin
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*Corresponding
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[email protected] (J. J. Ornelas-Paz).
author.
Tel/Fax:
+52-625-5812920.
E-mail
address:
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Abstract
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The impact of processing at industrial scale on properties of apple juice and pectin
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fractions extracted from the generated pomace is scarcely known. In this study,
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apple juice was collected at selected steps of the industrial production process and
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evaluated for physical and chemical properties. The generated pomace was
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recovered and subjected to extraction of pectins according to their solubility. They
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were evaluated for their physicochemical and functional properties. The
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transmittance for color and clearness of juice increased during clarification step but
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decreased during concentration. The sugar content was not altered by any step.
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The content of individual acids showed some changes during the pasteurization.
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The levels of total and individual phenols tended to increase during the production
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process. Low levels of 5-HMF (4.0 mg/L) were detected only in the concentrated
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juice while patulin was absent. The pomace contained only chelator and alkali
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soluble pectin. In comparison to commercial apple pectin, extracted pectins were of
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low degree of esterification (67% vs 22.8– 44.6%), GalA (654.1 vs 393.5–436.6
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mg/g) and Gal (228.6 vs 71.3–115.0 mg/g) content but rich in Ara (27.5 vs 103.4–
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166.3 mg/g) and of high molecular weight (644.5 vs 1559.6-2360.6 kDa). Their
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viscosity was lower than that of commercial apple pectin (k values of 0.03–0.05 vs
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0.14 Pa·sn, respectively). They showed lower thermal stability than commercial
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apple pectin. The production steps involving high temperature or enzymes effected
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the properties of apple juice and extracted pectins.
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Keywords: Industrial
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Functional properties
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processing;
Nutrients;
Antioxidants; Polysaccharides;
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1. Introduction
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Clarified apple juice is one of the most popular processed foods in the world.
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Several chemical components (i.e. sugars, acids, phenolic compounds, pigments,
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safety-related compounds, etc.) are involved in juice quality; however, the levels of
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these compounds are highly influenced by the production process (Kadakal & Nas,
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2003; Suárez-Jacobo et al., 2011). The apple pulp and juice are exposed to
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exogenous enzymes, adsorbent materials, high temperatures, and high osmotic
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pressure during the production process (Eisele & Drake, 2005). These conditions
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favor the release, degradation, transformation, and generation of compounds
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involved in juice quality (Markowski, Baron, Le Quéré, & Płocharski, 2015;
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Onsekizoglu, Bahceci, & Acar, 2010). The production process determines the color
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and turbidity as well as the levels of phenols, sugars, acids, the mycotoxin patulin
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and 5-hydroxymethylfurfural (5-HMF) of clarified juice, among other compounds
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(He, Ji, & Li, 2007; Onsekizoglu et al., 2010; Markowski et al., 2015; Gökmen et al.,
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2001; Welke, Hoeltz, Dottori, & Noll, 2009). However, these processing effects
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have mainly been determined under laboratory or pilot plant conditions (Gökmen,
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Artık, Acar, Kahraman, & Poyrazoğlu, 2001; Kadakal & Nas, 2003; Onsekizoglu et
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al., 2010; Spanos, Wrolstad, & Heatherbell, 1990; Suárez-Jacobo et al., 2011).
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The effect of apple juice processing at industrial scale has been scarcely studied
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and limited to a few processing steps and juice attributes (Welke et al., 2009).
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Further information in this regard is required to be used as a basis for the
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improvement of the quality of clarified apple juice.
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The pomace is the main waste product generated by the apple juice industry. It
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represents 25% of fruit weight and its disposal involves costs and environmental
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pollution (O’Shea et al., 2015). However, it also is an important source of
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commercial pectin, which is a heteropolysaccharide widely used in many industrial
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sectors for its functional properties (gelling, stabilizing, emulsifying and thickening
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agent) (Wang, Chen, & Lü, 2014). The functionality of this type of apple pectin
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depends of its physicochemical characteristics, which are highly influenced by
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apple variety and ripening stage as well as the using of enzymes during juice
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production (Canteri-Schemin, Fertonani, Waszczynskyj, & Wosiacki, 2005; Fischer,
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Arrigoni, & Amadò, 1994). The physicochemical properties of total pectin from
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apple pomace have extensively been studied (Kammerer, Kammerer, Valet, &
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Carle, 2014; Kosmala et al., 2010; Min et al., 2010; O’Shea et al., 2015; Wang et
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al., 2014). However, the physicochemical and functional properties of pectin
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fractions from apple pomace have received scarce attention (Kosmala et al., 2010).
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The objective of this work was to determinate the impact of selected steps of the
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production process at industrial scale in apple juice quality as well as to evaluate
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the physicochemical and functional properties of different pectin fractions obtained
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from the generated pomace.
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2. Materials and methods
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2.1. Apple juice and pomace
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The samples of juice and pomace from ‘Golden Delicious’ apples were obtained
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under industrial scale conditions. Triplicate samples of juice (1L) and pomace (3 4
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Kg) were weekly collected during four weeks. Juice was collected at the pressing,
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pasteurization, clarification, and concentration step while pomace only at pressing
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step. The first step consisted in pressing apple cubes (2 mm) previously treated
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with pectin lyase for 60 min at 25 °C. The pomace was collected at this step and
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stored at -70 °C until pectin extraction. The juice was pasteurized at 90 °C for 60 s
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and then quickly cooled (50°C). The clarification step involved the treatment with a
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mixture of polygalacturonases, pectinase and glucoamylase for 100 min at 55 °C
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followed by ultrafiltration (UF) with tubular membranes of molecular weight cut-off
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(MWCO) of 100 kDa. The concentration consisted of two heating steps, one at 55
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°C (23 min) and other at 70 °C (60 min). The average production flow was 3000
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L/h. The juice samples were immediately stored at -70 °C until analysis. The juice
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samples were analyzed for total soluble solids content (TSS %) to determine the
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dehydration level during the production process and then adjusted to 11.2 °Brix
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before analysis of the physicochemical attributes. Several pectins were
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sequentially obtained from the apple pomace according to their solubility and
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evaluated for physicochemical and functional properties.
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2.2. Miscellaneous evaluations in juice
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The content of TSS (%) was determined in three subsamples (0.5 mL) of each
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juice using an automatic digital refractometer RX 5000 (ATAGO, Tokyo, Japan).
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The titratable acidity was determined in tree subsamples (5 mL) of each juice
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according to Eisele and Drake (2005). The total phenolic content was determined
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three times in each juice by the Folin Ciocalteu method at 750 nm, according to
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Spanos et al. (1990), and expressed as mg of chlorogenic acid equivalent per L of
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juice. Three subsamples (8 mL) of each juice were evaluated for color and
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clearness using a Thermo Spectronic 20D+ spectrophotometer (Thermo Scientific,
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Wisconsin, USA) at 440 and 625 nm (transmittance), respectively. These
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measurements were performed according to Kadakal and Nas (2003).
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2.3. Individual sugars and organic acids
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The evaluation of sugars and organic acids was performed according to Ornelas-
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Paz et al. (2017), with slight modifications. For sugars, three subsamples of each
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juice were centrifuged (24652 g/ 20 min/ 4 °C) and then diluted ten times with
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water. The pH of diluted juice was adjusted at 7 with 10% NaOH, filtered and
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manually injected (20 µL) into a HPLC system (Varian Inc., CA, USA), which was
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equipped with a refractive index detector (Star Model 9040). The sugars were
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separated in a SUGAR SC 1821 (8.0 x 300 mm) (SHODEX, Tokyo, Japan) ion
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exchange column at 70 °C. The mobile phase was HPLC grade water at a flow rate
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of 0.6 mL/min. For organic acids, three subsamples of each juice were filtered and
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directly injected (20 µL) into the HPLC system described above but fitted to a UV-
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Vis detector (Model 9050). Acids were separated in an Aminex HPX-87H (7.78 x
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300 mm) ion exchange column (Bio-Rad Laboratories., CA, USA). The separation
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was performed at 60 °C using 5mM H2SO4 as mobile phase at a flow rate of 0.4
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mL/min. The organic acids were monitored at λ=210 nm. The identification and
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quantification of sugars and acids were performed using standard compounds.
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2.4. Analysis of phenolic compounds
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The extraction and chromatographic separation of phenolic compounds were
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based in the methodology described by Ornelas-Paz et al. (2017). Three
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subsamples of each juice were centrifuged (24652 g/ 20 min/ 4 °C), filtered and
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manually injected (20 µL) into an Agilent 1200 series HPLC system (Agilent Inc.,
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CA, USA) equipped with a diode array detector. The separation of phenolic
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compounds was performed in a ZORBAX XDB-C18 column (4.6 x 150 mm)
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(Agilent Inc., CA, USA) at 30 °C. The phenolic compounds were monitored at λ=
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280, 320, 350 and 520 nm. The mobile phase consisted of 2% acetic acid (A) and
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acetonitrile (B), according to the following gradient: 100% A at 0 min, 93% A at 12
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min, 89% A at 20 min, 86%A at 35 min, 84% A at 36 min, 82% A at 41 min, 76% A
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at 48 min, 70% A at 54 min, and 65% A at 59 min. The flow rate was 1 mL/min.
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Reference compounds were used for identification and quantification purposes.
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2.5. Analysis of patulin and 5-HMF
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Three subsamples (10 mL) of each juice were individually placed in a separatory
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funnel, vigorously mixed with ethyl acetate (20 mL), and kept in repose until
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separation of phases. The organic phase was recovered while the aqueous phase
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was extracted two times more with ethyl acetate (20 mL each time), recovering the
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organic phase after each washing. The organic phases were pooled and washed
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two times with 1.5% Na2CO3 (10 mL). The organic phase was recovered and
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evaporated at reduced pressure at 40 °C. The residue was dissolved in 1 mL of
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water at pH 4 (adjusted with acetic acid), filtered, and manually injected (100 µL) in
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the Agilent 1200 series HPLC system described above. The separation of patulin
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and 5-HMF was performed according to Gökmen and Acar (1999), using a
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ZORBAX XDB-C18 (4.6 x 150 mm) (Agilent Inc., CA, USA) column at 30 °C. The
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patulin and 5-HMF were monitored at 276 and 284 nm, respectively. The mobile
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phase consisted of water (pH 4, A) and acetonitrile (B) according to the following
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gradient: 99% A at 0 min, 95% A at 10 min, 90% A at 15 min, 50% A at 20 min,
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100% B from 25 to 35 min. The flow rate was 1 mL/min. The qualitative and
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quantitative analyses were performed using reference compounds.
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2.6. Extraction of pectin
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Triplicate samples of apple pomace (500 g each) were used as pectin source. The
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extraction of alcohol-insoluble residues (AIR) and pectins was performed according
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to Ramos-Aguilar et al. (2015). The AIR was subjected to sequential extraction of
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pectin with hot water (95 °C) for 5 min, 0.05M CDTA in 0.1 M potassium acetate at
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pH 6.5 for 6 h at 28 °C, and 0.05 M Na2CO3 containing 0.02 M NaBH4 for 16 h at 4
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°C and then for 6 h at 28 °C. The ratio of AIR to extraction solution was 1:100 (w/v)
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in all cases. The pectin was precipitated with ethanol and recovered by
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centrifugation (12, 000 g/5 min/ 4 °C) and filtration (Whatman paper No. 541). The
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recovered pectins were named as water, chelator, and alkali soluble pectin (WSP,
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CSP, and NSP, respectively). Triplicate samples of these pectins as well as of
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commercial apple pectin (CAP) were evaluate for physicochemical and rheological
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properties.
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2.7. Degree of esterification of pectin
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The GalA was liberated from pectins and colorimetrically quantified at 525 nm
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according to Ramos-Aguilar et al. (2015). The methanol was liberated from pectins
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according to Voragen, Schols, & Pilnik (1986). The extract was filtered and
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manually injected (20 µL) to the Varian HPLC system described above (refractive
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index detection). The methanol was separated in a TSKGel SCX H+ (7.8 x 300
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mm) ion exchange column (Tosoh Bioscience LLC, Tokyo, Japan) at 30 °C.
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Deionized water was used as mobile phase at a flow rate of 1 mL/min. The degree
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of esterification (DE) was calculated according to Voragen et al. (1986).
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2.8. Monosaccharide composition of pectin
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Pectin was sequentially subjected to acid and enzymatic hydrolysis according to
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Ramos-Aguilar et al. (2015). Each hydrolysate was analyzed under two different
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HPLC conditions using the Varian system described above (refractive index
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detection). The Glu, Ara, Rha, Gal, and Fuc were separated at 58 °C in a Metacarb
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H+ (7.8 x 300 mm; Varian Inc., CA, USA) ion-exchange column, using 0.0085N
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H2SO4 as mobile phase at a flow rate of 0.4 mL/min. Xyl and Man were separated
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in a Supelcogel Pb (7.8 x 300 mm; Sigma-Aldrich., MO, USA) ion exchange
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column at 70°C using water as mobile phase at a flow rate of 0.5 mL/min. The
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qualitative and quantitative analyses were performed using reference compounds.
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2.9. Molecular weight distribution of pectin
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The molecular weight (MW) distribution was determined by high performance size-
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exclusion chromatographic, according to Pérez-Martínez et al. (2013). Pectins
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were solubilized in water (5 g/L). The solutions were filtered through a polyethylene
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membrane of 0.45 µm of pore size (Millipore Corp., MA, USA) and manually
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injected (20 µL) into the Varian HPLC system described above (refractive index
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detection). Separation was performed using a series of TSK-GEL columns
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(GMPW XL, G5000PW XL, and G4000PW XL; 7.8 x 300 mm each) (Tosoh Bioscience;
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Tokyo, Japan) at 40° C. Phosphate buffer (0.2 M; pH= 6.9) was used as mobile
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phase at a flow rate of 0.4 mL/min. The MW was determined relative to dextrans of
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known MW (1-670 kDa) (Sigma-Aldrich., MO, USA).
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2.10. Other evaluations of pectin
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The FT-IR spectra (4000 to 450 cm−1) were collected using a Spectrum Two FT-IR
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spectrometer (Perkin Elmer Inc., MA, USA). Triplicate samples of each pectin were
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analyzed and applied on the Attenuated Total Reflection crystal as powder. For
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each sample, 34 scans were averaged with a spectral resolution of 4 cm−1. Spectra
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analyses and baseline corrections were performed using the Spectra software ver.
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10.4.4.449 (Perkin Elmer Inc., MA, USA). The viscosity of pectin solutions (1%)
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was determined according to Ramos-Aguilar et al. (2015) but using a stainless
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steel cone geometry (4°, 40 mm diameter) and a gap size of 90 µm. Pectin thermal
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stability was analyzed with a Q500 thermogravimetric analyzer (TA Instruments.,
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DE, USA). Ten milligrams of pectin powder were weighted in aluminum pans and
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heated from 30 to 600 °C at 10 °C/min under nitrogen flow (15 mL/min). The
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thermogravimetric curves were analyzed with Universal Analysis 2000 software
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(ver. 4.5A). The tristimulus color (L*, a* and b*) was determined on pectin samples
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(powder) using Minolta colorimeter (CR-300 model, Minolta Co. Ltd, Osaka,
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Japan).
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2.11. Statistical analysis
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The values obtained weekly for each measurement were averaged and considered
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as a single value. Data were analyzed by an analysis of variance under a
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completely randomized design with a limit of significance of 0.05. The comparison
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of means was performed using the Tukey-Kramer post hoc test. The analysis data
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was performed using JMP statistical software (SAS Institute, Inc., NC, USA).
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3. Results and discussion
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3.1. Juice color and clearness
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The pasteurization and clarification steps sequentially increased the transmittance
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of the freshly pressed juice at both wavelengths (Table 1). He et al. (2007) also
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observed that the transmittance of apple juice at 440 nm increased from 53.7% to
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66.7% after pasteurization. Vladisavljević, Vukosavljević, & Bukvić (2003) observed
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increases of transmittance after juice clarification that varied between 30 and 21%,
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depending of the clarification method. The increase of transmittance during the first
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steps of juice processing might be attributed to the hydrolysis of pectin and starch
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by added enzymes as well as by removal of these polysaccharides by UF
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membranes (He et al., 2007). In our study, the transmittance of juice at both
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wavelengths was reduced 6-8.7% after concentration (Table 1). Others are also
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observed a slight decrease (4.4-7.7%) in the transmittance of apple juice at both
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wavelengths after concentration (Kadakal & Nas, 2003; Garza, Giner, Martín,
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Costa, & Ibarz, 1996). The decrease of transmittance at the concentration step
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might be consequence of phenol oxidation, the suspension of particles formed by
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residues of depolymerized pectin and denaturalized proteins that crossed the UF
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membrane at the clarification step, and formation of Maillard’s reaction products
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(Garza et al., 1996; He et al., 2007; Kadakal & Nas, 2003; Onsekizoglu et al.,
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2010; Vladisavljević et al., 2003). The 5-HMF might contribute to juice color
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because it was detected in concentrated juice at a concentration of 4.0 ± 0.6 mg/L.
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Similar contents of 5-HMF (up to 7.9 mg/L) have been reported in apple juices after
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thermal concentration in a rotavapor
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patulin was not detected.
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3.2. Effect of processing on sugars and acids
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The TSS content in freshly pressed juice did not changed during pasteurization
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and clarification steps (Table 1). Others have reported similar findings at laboratory
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and pilot plant scale (Gökmen et al., 2001; Suárez-Jacobo et al., 2011;
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Vladisavljević et al., 2003). In our study, the juice was concentrated 5.2 times
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during the evaporation step. Similar changes of concentration (4.8 times) have
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been reported for apple juice under industrial-scale conditions (Welke et al., 2009).
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Fructose was the main sugar in tested juices, followed by sucrose and glucose
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(Table 2). The content of individual sugars was not significantly altered by any
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processing step, as reported in some studies at laboratory and pilot plant scale
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(Onsekizoglu et al., 2010; Suárez-Jacobo et al., 2011).
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The TA of juice was similar during the first three steps of the production process
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(Table 1). Previous studies at laboratory scale with juice from ‘Golden Delicious’
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apples demonstrated that the TA was not significantly altered by both thermal or
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non-thermal pasteurization and clarification by UF (Aguilar-Rosas, Ballinas-
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Casarrubias, Nevarez-Moorillon, Martin-Belloso, & Ortega-Rivas, 2007; Youn,
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Hong, Bae, Kim, & Kim, 2004). In this study, a slight decrease (11%) of TA was
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observed after evaporation. Onsekizoglu et al. (2010) observed under laboratory
283
conditions a decrease of 4.7% in acid concentration of juice from the clarification to
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the evaporation step. The malic and ascorbic acids were the most abundant in
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tested juices (Table 2). The concentration of each acid in freshly pressed juice was
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statistically similar to that of the concentrated juice (final juice). However,
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temporary alterations in acid content were observed at pasteurization step.
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Interestingly, the highest or lowest concentration of each one of tested acids were
289
observed after pasteurization (Table 2). The effect of this step on acids has not
290
been clearly studied; however, the high temperatures used for pasteurization could
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improve the release of organic acids from apple particles and the dehydration of
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some of them, altering consequently their concentrations (Gökmen & Acar, 1998).
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3.3. Phenolic compounds in apple juice
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Tested juices were rich in phenolic compounds, as judged by the total phenolic
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content (Table 1). Interestingly, such content increased (100%) during the
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production process. This might be a consequence of the thermal and enzymatic
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release of phenols from fibers during the production process (Kammerer et al.,
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2014). Eleven phenolic compounds were identified and quantified in tested juices,
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with chlorogenic acid, procyanidin B2, phloridzin and epicatechin being the most
301
abundant (Table 3). The concentration of these compounds was into the range
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reported for raw and processed juices (chlorogenic acid, 3.4-113.7 mg/L; caffeic
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acid, 0.7-8.7 mg/L; p-coumaric acid, 0.1-3.0 mg/L; epichatequin, 0-71.8 mg/L;
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procyanidin B2, 0-121 mg/L; quercertin-3-galactoside, 0-14.4 mg/L; quercetin-3-
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glucoside, 0-9.1 mg/L; phloridzin, 1.3-56.0 mg/L) (Gliszczynska-Swiglo &
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Tyrakowska, 2003; Oszmiański, Wojdyło, & Kolniak, 2011; Spanos et al., 1990).
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In general, the content of individual phenolic compounds continuously increased
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from the pressing to the clarification step (Table 3). Some studies at laboratory
309
scale demonstrated the reduction of the phenolic content (4-45%) in apple juice
310
during juice clarification with membranes of MWCO from 10 to 30 kDa (Gökmen et
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al., 2001; Onsekizoglu, 2013). The membrane used in this study was of a MWCO
312
considerably higher (100 kDa), explaining the low impact of such step on phenols.
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The concentration step did not alter the levels of phenolic compounds.
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Substantial increases (34-109%) in chlorogenic, caffeic and p-coumaric acids were
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observed during the pasteurization and clarification steps. Spanos et al. (1990)
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demonstrated at pilot plant scale that the juice production at elevated temperatures
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(55-73 °C) improved the extractability (3-222%) of cinnamic acids and decreased
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their degradation due to the inactivation of polyphenol oxidase. Oszmiański et al.
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(2011) also observed at laboratory scale increases (4-14%) in the content of
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chlorogenic acid in apple juice after treatment with pectolytic and cellulolytic
321
enzymes. The changes in the content of flavan-3-ols during pasteurization and
322
clarification were higher than those for cinnamic acids (Table 3). The increase in
323
the content of epicatechin and procyanidin B2 ranged from 52 to 163% during
324
pasteurization and clarification steps. Similar increases (109-286%) have been
325
observed for these flavan-3-ols during such steps at laboratory scale (Spanos et
326
al., 1990). The high temperature could induce the hydrolysis of inter-flavonoid
327
linkages in procyanidins, increasing the concentration of their monomeric and
328
dimeric structures, epicatechin and procyanidin B2, while the enzymatic treatment
329
might favor the liberation of procyanidins linked to cell-wall polysaccharides,
330
especially pectin (De Paepe et al., 2014; Oszmiański et al., 2011). The content of
331
quercetin glycosides did not show significant changes during the apple juice
332
processing (Table 3). However, the quercetin aglycone was detected in clarified
333
and evaporated juices, probably as a consequence of the hydrolysis of glycosidic
334
forms during the enzymatic clarification. The effect of processing steps in free and
335
glycosylated quercetin of apple juice has been previously reported under laboratory
336
and pilot scale conditions with contradictory results (increases of up to 300% and
337
reductions of up to 75%), depending of the apple variety, enzymatic treatment, and
338
clarification and concentration methods (Gökmen et al., 2001; Markowski et al,
339
2015; Onsekizoglu et al., 2010; Spanos et al., 1990).
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3.4. Properties of pectin
342
The total pectin content of apple pomace was 9% (Table 4). Similar content of
343
pectin (7.8%) in apple pomace was recently reported by O’Shea et al. (2015). The
344
FT-IR spectra showed the two characteristic absorption bands for polysaccharides,
345
a strong and wide absorption band at 3100-3700 cm-1 for O-H stretching vibrations
346
and a weak absorption peak of about 2800-3000 cm-1 for C-H stretching vibrations
347
(Fig. 1) (Qiao et al., 2009). It also showed the peaks at 882 and 1273 cm-1, which
348
are characteristic of the pyranose ring of pectin and the C-O dilatation and vibration
349
(Kačuráková, Capek, Sasinkova, Wellner, & Ebringerova, 2000; Wang et al.,
350
2014). In this study, the pomace contained only CSP and NSP, while the WSP was
351
missing. The yield for CSP was 30% higher than that of NSP. These findings differ
352
from those of Kosmala et al. (2010), who observed that content of pectin types in
353
apple pomace followed the order of NSP˃CSP˃WSP (49.9–107.3, 18.9–26.0, 9.4–
354
20.0 mg/g, respectively). This difference might be a consequence of the high
355
activity of the pectin lyase at the pressing step and the using of overripe fruit in the
356
present study. The pectinolytic activity of this enzyme is particularly high for highly
357
esterified pectins and WSP use to show the highest DE (Yadav, Yadav, Yadav, &
358
Yadav, 2009). Laboratory-scale studies conducted in our laboratory with the same
359
apples demonstrated the existence of WSP in apple pomace obtained without the
360
using of enzymes (data not shown). Thus, pectin lyase might hydrolysate all of the
361
WSP as well as high amounts of CSP and NSP. The using of overripe fruit might
362
exacerbate this effect. Recently, Ramos-Aguilar et al. (2015) demonstrated that
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the yield of pectin from ripe green peppers follow the order of NSP˃CSP˃WSP but
364
this order was inverted with red peppers (WSP˃ CSP ˃NSP).
365
The extracted pectins were of low DE (Table 4). The DE decreased 49% from CSP
366
to NSP. CAP showed the highest DE (67%), which was virtually identical to that
367
provided by the supplier (70-75%). CSP and NSP from other plant sources have
368
also been described as lowly esterified pectins (DE= 11.2-14.8%) (Sila et al., 2006;
369
Sila et al., 2009). The FT-IR spectra confirmed the high difference of DE for tested
370
pectins (Fig. 1). The absorption peaks at 1750-1730 cm-1 indicated the presence of
371
carbonyl esters (C=O) (Wang et al., 2014) and their intensity and area agreed with
372
the obtained DE values, especially with those of CAP and CSP (Fig. 1, Table 4).
373
The composition of neutral sugars was different for tested pectins (Table 4). The
374
content of GalA was 10% higher in CSP than in NSP; however, CAP showed the
375
highest GalA content, which was up to 40% higher than that of the other pectins.
376
Similarly, Kosmala et al. (2010) observed that the GalA content was 49-74% higher
377
in chelator soluble pectin from apple pomace than in alkali soluble pectin. The
378
content of Man and Ara in CSP and NSP was 68-83% higher than in CAP while
379
CAP was especially rich in Gal and Glu, showing a content of these sugars 50–
380
71% higher than that of the other pectins. Interestingly, the content of almost all of
381
the tested sugars was higher (17-40%) in NSP than in CSP. This finding indicates
382
that NSP was more branched and intact than CSP (Sila et al., 2009). This was
383
supported by the MW distribution of tested pectins. They contained up to three
384
fractions but the first of them was substantially abundant. The peak MW of such
385
fraction is shown in Table 4. First fraction showed the highest MW in NSP, followed
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by CSP and CAP. In general, the MW found in this study for the most abundant
387
fractions was into the range reported for apple pectin (100-10000 kDa) (Fischer et
388
al., 1994).
389
The pectin solutions showed a pseudoplastic behavior, especially whiting the range
390
from 50 to 100 s-1 (Fig. 2). The flow behavior showed high correlation values (R2=
391
0.989–0.999) with the power law model. The k values of tested pectins were
392
significantly different, with viscosity of CSP (k= 0.053 Pa.sn) being almost twice
393
than that NSP (k= 0.027 Pa.sn). CAP showed the highest viscosity (k= 0.143
394
Pa.sn). The viscosity of tested pectins showed an inverse relationship with MW of
395
the main fractions (Table 4). The viscosity of pectin solutions is highly influenced
396
by sugar composition, DE and MW. In this study, the content of GalA and Glu and
397
the DE were directly related with viscosity. Wang et al. (2014) demonstrated that
398
the viscosity of apple pectin increased with the GalA content. Liu, Cao, Huang, Cai,
399
and Yao (2010) demonstrated that the gellification and viscosity of pectin increased
400
with the content of GalA and DE.
401
The thermogravimetric analysis showed that the tested pectins released moisture
402
(∼6%) with a maximum derivative of weight loss peak (Pk) at 80°C. The CSP
403
showed a low thermal stability fraction (Pk ≈ 200 °C). The highest degradation
404
amount for all pectins was observed at Pk between 238 and 245 °C (Fig. 3), which
405
has been associated to the pyrolytic decomposition of homogalacturonans (Combo
406
et al., 2013). Accordingly, the pectin with the higher GalA content and viscosity
407
(CAP) had the highest degradation in this region (Table 4; Figs. 2 and 3). At
408
temperatures above 350 °C, the CSP and the NSP showed degradation, which
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probably was associated to lignocellulosic materials (Yang et al., 2006). Thus, we
410
could assume that CSP contained a relatively higher content of cellulosic material
411
than NSP. NSP probably contained more lignin-associated polysaccharides
412
because it showed a higher stability at temperature above 350 °C. These
413
compositional changes were probably responsible for the absence of the direct
414
relationship between MW and viscosity and thermogravimetric properties of tested
415
pectins.
416
The color of pectins is not usually reported; however, it is an important property of
417
pectin because it may determine its use in food formulations. In this study, the CSP
418
and CAP showed similar color values, although their L* values were statistically
419
different (Table 4). The color values of these pectins (L*= 72.7- 74.1, a*= 4.1-3.9,
420
b*= 12.9-12.3) were within the ranges reported for pectin from other sources, such
421
as mango, citrus, beet and peppers (L*= 67.5–93.5, a*= -0.6–3.5 and b*= 9.38–
422
20.2) (Berardini, Knödler, Schieber, & Carle, 2005; Mesbahi, Jamalian, &
423
Farahnaky, 2005; Ramos-Aguilar et al., 2015). The NSP was darker than CSP and
424
CAP, according to its significantly lower values of L* and b*, and the higher value
425
of a* (Table 4). The darkness of pectin is highly related with their phenol content
426
(Ramos-Aguilar et al., 2015), thus, the oxidation of phenols during the extraction of
427
NSP might explain the color of this pectin type. However, the extraction conditions
428
can also influence the structure of pectin and these alterations can influence the
429
color of pectin (Pérez-Martínez et al., 2013; Einhorn-Stoll, Kastner, & Drusch,
430
2014).
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4. Conclusions
433
The steps of the juice production process involving high temperature and enzymes
434
had a significant effect on key components of apple juice (organic acids, phenolics,
435
and 5-HMF). Some effects of the processing coincided with those observed
436
previously at laboratory or pilot plant scale. Tested pomace contained CSP and
437
NSP but not WSP. These pectins differed from CAP in terms of their high MW,
438
Man and Ara content as well as for their low DE, GalA and Gal content. This
439
resulted in lower viscosity and different thermal stability, as compared with the
440
functional properties observed for CAP. The ripening, type of fruit and use of
441
enzymes during the process of juice production were probably involved in the
442
physical and chemical properties of extracted pectins, compromising their
443
functionality.
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Acknowledgements
446
This research was funded by the Fondo Mixto CONACYT- Gobierno del Estado de
447
Chihuahua (Project Clave: CHIH-2012-C03-194579).
448
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Figure captions
588
Fig. 1. FT-IR spectra of commercial apple pectin (CAP, ─) and chelator- and alkali-
589
soluble pectin fractions (CSP, ─; NSP, ─) from apple pomace.
590
Fig. 2. Flow curves and parameters of power law model obtained from solutions of
591
commercial apple pectin (CAP, ⚫) and chelator- and alkali-soluble pectin fractions
592
(CSP, ⚪; NSP, ▼) from apple pomace. n, flow behavior. k, consistency index.
593
Fig. 3. Thermogravimetric analysis (A) and derivative thermogravimetric (B) curves
594
for commercial apple pectin (CAP, ─) and chelator- and alkali-soluble pectin
595
fractions (CSP, ─; NSP, ─) from apple pomace.
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Table captions
599
Table 1. Effect of industrial processing on color, clearness, total soluble solids,
600
titratable acidity, and total phenolic content in apple juice
601
Table 2. Concentration of sugars and organic acids in apple juice at selected steps
602
of the industrial production process.
603
Table 3. The effect of the industrial processing on the content of phenolic
604
compounds in of apple juice.
605
Table 4. Yield and physicochemical characteristics of commercial apple pectin
606
(CAP) and chelator- and alkali-soluble pectin fraction (CSP and NSP) from
607
enzyme-treated apple pomace.
AC C
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598
27
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Table 1.
0.1 ± 0.0 c
0.8 ± 0.2 c
4.9 ± 0.46 d
10.7 ± 1.5 c
11.2 ± 0.4 b
7.0 ± 0.1 ab
Color a
(440 nm)
Clearness
10.7 ± 0.7 b
11.6 ± 0.5 b
69.0 ± 0.6 a
7.8 ± 0.4 a
7.3 ± 0.2 ab
6.5 ± 0.2 b
0.35 ± 0.0 ab
0.4 ± 0.0 a
M AN U
(%)
AC C
equivalents /L)
0.3 ± 0.0 b
EP
0.2 ± 0.0 c
TE D
Titratable acidity
(g chlorogenic acid
47.6 ± 0.3 b
90.1 ± 0.5 b
Total soluble solids
Total phenols
53.8 ± 2.4 a
Concentration
98.8 ± 2.6 a
(625 nm )a
(g malic acid/ L)
Clarification
RI PT
Pasteurization
SC
Pressing
The juice was adjusted at 11.2 °Brix before color, clearness, acidity, and total phenolic content measurements. Values represent the mean of 12 individual measurements ± the standard error. Data in the same row connected by different letters are significant different (p ≤ 0.05). a Values are given % transmittance.
ACCEPTED MANUSCRIPT
Table 2. Pasteurization
Fructose
56.8 ± 2.2 a
64.0 ± 3.5 a
Sucrose
32.0 ± 1.8 a
35.9 ± 1.0 a
Glucose
16.1 ± 0.8 a
16.5 ± 0.8 a
Malic
2732.4 ± 185.7 b
Ascorbic
Clarification
RI PT
Pressing Sugars (g/L)
Concentration
58.6 ± 1.4 a
33.0 ± 1.6 a
31.4 ± 1.0 a
16.0 ± 0.6 a
17.2 ± 0.6 a
3653.8 ± 387.2 a
3137.7 ± 98.7 ab
2953.4 ± 95.3 ab
935.6 ± 121.3 a
722.7 ± 64.6 a
820.6 ± 80.5 a
808.7 ± 170.4 a
Succinic
555.0 ± 52.7 b
707.3 ± 57.2 a
526.1 ± 48.3 b
465.9 ± 27.5 b
Oxalic
196.7 ± 40.0 a
95.3 ± 16.4 b
151.6 ± 13.7 ab
201.0 ± 18.8 a
3.6 ± 0.5 c
5.3 ± 0.4 bc
8.3 ± 0.3 a
7.1 ± 2.9 a
1.9 ± 0.3 a
3.1 ± 0.3 a
Fumaric
4.2 ± 0.5 a
M AN U
AC C
EP
6.8 ± 1.3 ab
TE D
Organic acids (mg/L)
Tartaric
SC
57.7 ± 1.7 a
The juice was adjusted at 11.2 °Brix before analysis. Values represent the mean of 12 individual measurements ± the standard error. Data in the same row connected by different letters are significant different (p ≤ 0.05).
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Table 3. Compound (mg/L)
Pressing
Pasteurization
Clarification
Concentration
Chlorogenic acid
18.5 ± 1.3 c
31.7 ± 2.4 b
38.8 ± 2.0 a
37.2 ± 1.1 ab
Caffeic acid
0.9 ± 0.0 b
1.0 ± 0.1 b
1.2 ± 0.0 a
1.2 ± 0.0 a
ND
ND
0.04 ± 0.00
ND
0.5 ± 0.0 b
0.5 ± 0.0 b
0.9 ± 0.1 a
0.8 ± 0.1 a
0.2 ± 0.0 a
0.2 ± 0.0 ab
0.1 ± 0.0 b
0.1 ± 0.0 b
6.6 ± 0.8 a
8.4 ± 0.6 a
8.9 ± 0.8 a
15.4 ± 1.5 a
16.9 ± 2.0 a
15.1 ± 0.2 ab
ND
ND
0.3 ± 0.1 a
0.3 ± 0.1 a
Quercetin 3-D-galactoside
1.5 ± 0.1 a
1.8 ± 0.2 a
1.5 ± 0.1 a
1.6 ± 0.1 a
Quercetin 3-β-glucoside
0.5 ± 0.0 a
0.5 ± 0.0 a
0.6 ± 0.0 a
0.6 ± 0.0 a
4.8 ± 0.5 b
6.3 ± 0.9 b
10.7 ± 0.9 a
9.7 ± 0.6 a
p-Coumaric acid
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Cinnamic acid
Flavan-3-ols Epicatechin
3.2 ± 0.4 b
Procyanidin B2
10.1 ± 0.8 b
Phloridzin
EP
Dihydrochalcones
AC C
Quercetin
TE D
Flavonols
M AN U
Hydroxybenzoic acid Protocatechuic acid
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Hydroxycinnamic acids
The juice was adjusted at 11.2 °Brix before analysis. Values represent the mean of 12 individual measurements ± the standard error. Data in the same row connected by different letters are significant different (p ≤ 0.05). ND, not detected.
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Table 4. Pectin type CSP
NSP
-
5.3 ± 0.1 a
3.7 ± 0.1 b
L*
72.7 ± 0.1 b
74.1 ± 0.4 a
54.6 ± 0.1 c
a*
4.1 ± 0.0 b
3.9 ± 0.1 b
5.3 ± 0.1 a
b*
12.9 ±0.1 a
12.3 ± 0.1 b
11.0 ± 0.1 c
436.6 ± 8.0 b
393.5 ± 5.2 c
Galacturonic acid (mg/g)
654.1 ± 5.7 a
Monosaccharides (mg/g)
M AN U
Tristimulus color
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Yield (%)
RI PT
CAP
Mannose Arabinose Galactose
Xylose Rhamnose Fucose
EP
Degree of esterification (%)
132.9 ± 3.0 b
198.3 ± 5.0 a
27.5 ± 0.3 c
103.4 ± 1.9 b
166.3 ± 1.9 a
228.6 ± 2.2 a
71.3 ± 1.8 c
115.0 ± 1.8 b
45.5 ± 0.3 a
16.1 ± 0.2 b
13.4 ± 0.1 c
13.0 ± 0.3 a
11.7 ± 0.5 b
14.0 ± 0.2 a
9.0 ± 0.1 a
4.8 ± 0.2 c
7.9 ± 0.3 b
2.8 ± 0.1 a
2.5 ± 0.1 b
ND
67.4 ± 3.4 a
44.6 ± 2.9 b
22.8 ± 2.4 c
644.5 ± 8.9 c
1559.6 ± 49.6 b
2360.6 ± 38.3 a
TE D
Glucose
42.1 ± 0.5 c
AC C
Peak molecular weight (kDa)
Values represent the mean of at least three individual measurements ± the standard error. Values in the same row with different letters are significantly different (p < 0.05). ND, not detected.
SC
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3000-2800
100
96 3700-3100
92 90
86
Fig. 1.
1273-882
EP
88
84 4000
1750-1730
TE D
94
3500
AC C
Transmittance (%)
98
M AN U
102
3000
2500 2000 Wavenumber (cm-1)
1500
1000
500
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0.10
M AN U
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0.08
n
k (Pa·s ) a 0.143 ± 0.003 b 0.053 ± 0.001 c 0.027 ± 0.001
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CAP CSP NSP
0.06
0.04
0.00 100
200
EP
0
TE D
0.02
AC C
Apparent viscosity (Pa.s)
0.12
n a 0.919 ± 0.004 b 0.891 ± 0.004 c 0.852 ± 0.006
Fig. 2.
300
Shear rate (1/s)
400
500
600
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Fig. 3.
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-The impact of industrial processing on properties of apple juice is scarcely known -Few pectin fractions from apple pomace have been characterized
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-The sugar content in apple juice was not altered by any processing step
-The pasteurization step altered the levels of individual phenols and acids -Concentration step favored the formation of 5-HMF
AC C
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-Pomace pectins showed less functionality than commercial apple pectin
S0023-6438(17)30600-X
DOI:
10.1016/j.lwt.2017.08.030
Reference:
YFSTL 6452
To appear in:
LWT - Food Science and Technology
Received Date: 16 March 2017 Revised Date:
9 August 2017
Accepted Date: 10 August 2017
Please cite this article as: Ramos-Aguilar, A.L., Victoria-Campos, C.I., Ochoa-Reyes, E., de Jesús Ornelas-Paz, José., Zamudio-Flores, P.B., Rios-Velasco, C., Reyes-Hernández, J., Pérez-Martínez, J.D., Ibarra-Junquera, V., Physicochemical properties of apple juice during sequential steps of the industrial processing and functional properties of pectin fractions from the generated pomace, LWT Food Science and Technology (2017), doi: 10.1016/j.lwt.2017.08.030. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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1
Physicochemical properties of apple juice during sequential steps of the
2
industrial processing and functional properties of pectin fractions from the
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generated pomace
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4 5
Ana L. Ramos-Aguilar a, Claudia I. Victoria-Campos a, Emilio Ochoa-Reyes a,
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José de Jesús Ornelas-Paz
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Velasco a, Jaime Reyes-Hernández b, Jaime D. Pérez-Martínez c, Vrani Ibarra-
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Junquera d
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a
*, Paul B. Zamudio-Flores a, Claudio Rios-
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a,
Centro de Investigación en Alimentación y Desarrollo A.C.-Unidad Cuauhtémoc,
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Av. Río Conchos S/N, Parque Industrial, C.P. 31570, Cd. Cuauhtémoc,
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Chihuahua, México.
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b
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artillero No. 138, Zona Universitaria, C.P. 78210, San Luis Potosí, México.
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c
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Manuel Nava 6 Zona Universitaria, C.P. 78210, San Luis Potosí, México.
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d
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Colima, C.P. 28400, Coquimatlán, Colima, México.
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Universidad Autónoma de San Luis Potosí, Facultad de Ciencias Químicas,
Universidad de Colima, Bioengineering Laboratory, Km. 9 carretera Coquimatlán-
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Universidad Autónoma de San Luis Potosí, Facultad de Enfermería, Av. Niño
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Short running head: Quality of apple juice and pectin
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*Corresponding
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[email protected] (J. J. Ornelas-Paz).
author.
Tel/Fax:
+52-625-5812920.
address:
1
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Abstract
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The impact of processing at industrial scale on properties of apple juice and pectin
24
fractions extracted from the generated pomace is scarcely known. In this study,
25
apple juice was collected at selected steps of the industrial production process and
26
evaluated for physical and chemical properties. The generated pomace was
27
recovered and subjected to extraction of pectins according to their solubility. They
28
were evaluated for their physicochemical and functional properties. The
29
transmittance for color and clearness of juice increased during clarification step but
30
decreased during concentration. The sugar content was not altered by any step.
31
The content of individual acids showed some changes during the pasteurization.
32
The levels of total and individual phenols tended to increase during the production
33
process. Low levels of 5-HMF (4.0 mg/L) were detected only in the concentrated
34
juice while patulin was absent. The pomace contained only chelator and alkali
35
soluble pectin. In comparison to commercial apple pectin, extracted pectins were of
36
low degree of esterification (67% vs 22.8– 44.6%), GalA (654.1 vs 393.5–436.6
37
mg/g) and Gal (228.6 vs 71.3–115.0 mg/g) content but rich in Ara (27.5 vs 103.4–
38
166.3 mg/g) and of high molecular weight (644.5 vs 1559.6-2360.6 kDa). Their
39
viscosity was lower than that of commercial apple pectin (k values of 0.03–0.05 vs
40
0.14 Pa·sn, respectively). They showed lower thermal stability than commercial
41
apple pectin. The production steps involving high temperature or enzymes effected
42
the properties of apple juice and extracted pectins.
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Keywords: Industrial
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Functional properties
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processing;
Nutrients;
Antioxidants; Polysaccharides;
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1. Introduction
47
Clarified apple juice is one of the most popular processed foods in the world.
48
Several chemical components (i.e. sugars, acids, phenolic compounds, pigments,
49
safety-related compounds, etc.) are involved in juice quality; however, the levels of
50
these compounds are highly influenced by the production process (Kadakal & Nas,
51
2003; Suárez-Jacobo et al., 2011). The apple pulp and juice are exposed to
52
exogenous enzymes, adsorbent materials, high temperatures, and high osmotic
53
pressure during the production process (Eisele & Drake, 2005). These conditions
54
favor the release, degradation, transformation, and generation of compounds
55
involved in juice quality (Markowski, Baron, Le Quéré, & Płocharski, 2015;
56
Onsekizoglu, Bahceci, & Acar, 2010). The production process determines the color
57
and turbidity as well as the levels of phenols, sugars, acids, the mycotoxin patulin
58
and 5-hydroxymethylfurfural (5-HMF) of clarified juice, among other compounds
59
(He, Ji, & Li, 2007; Onsekizoglu et al., 2010; Markowski et al., 2015; Gökmen et al.,
60
2001; Welke, Hoeltz, Dottori, & Noll, 2009). However, these processing effects
61
have mainly been determined under laboratory or pilot plant conditions (Gökmen,
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Artık, Acar, Kahraman, & Poyrazoğlu, 2001; Kadakal & Nas, 2003; Onsekizoglu et
63
al., 2010; Spanos, Wrolstad, & Heatherbell, 1990; Suárez-Jacobo et al., 2011).
64
The effect of apple juice processing at industrial scale has been scarcely studied
65
and limited to a few processing steps and juice attributes (Welke et al., 2009).
66
Further information in this regard is required to be used as a basis for the
67
improvement of the quality of clarified apple juice.
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The pomace is the main waste product generated by the apple juice industry. It
69
represents 25% of fruit weight and its disposal involves costs and environmental
70
pollution (O’Shea et al., 2015). However, it also is an important source of
71
commercial pectin, which is a heteropolysaccharide widely used in many industrial
72
sectors for its functional properties (gelling, stabilizing, emulsifying and thickening
73
agent) (Wang, Chen, & Lü, 2014). The functionality of this type of apple pectin
74
depends of its physicochemical characteristics, which are highly influenced by
75
apple variety and ripening stage as well as the using of enzymes during juice
76
production (Canteri-Schemin, Fertonani, Waszczynskyj, & Wosiacki, 2005; Fischer,
77
Arrigoni, & Amadò, 1994). The physicochemical properties of total pectin from
78
apple pomace have extensively been studied (Kammerer, Kammerer, Valet, &
79
Carle, 2014; Kosmala et al., 2010; Min et al., 2010; O’Shea et al., 2015; Wang et
80
al., 2014). However, the physicochemical and functional properties of pectin
81
fractions from apple pomace have received scarce attention (Kosmala et al., 2010).
82
The objective of this work was to determinate the impact of selected steps of the
83
production process at industrial scale in apple juice quality as well as to evaluate
84
the physicochemical and functional properties of different pectin fractions obtained
85
from the generated pomace.
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2. Materials and methods
88
2.1. Apple juice and pomace
89
The samples of juice and pomace from ‘Golden Delicious’ apples were obtained
90
under industrial scale conditions. Triplicate samples of juice (1L) and pomace (3 4
ACCEPTED MANUSCRIPT
Kg) were weekly collected during four weeks. Juice was collected at the pressing,
92
pasteurization, clarification, and concentration step while pomace only at pressing
93
step. The first step consisted in pressing apple cubes (2 mm) previously treated
94
with pectin lyase for 60 min at 25 °C. The pomace was collected at this step and
95
stored at -70 °C until pectin extraction. The juice was pasteurized at 90 °C for 60 s
96
and then quickly cooled (50°C). The clarification step involved the treatment with a
97
mixture of polygalacturonases, pectinase and glucoamylase for 100 min at 55 °C
98
followed by ultrafiltration (UF) with tubular membranes of molecular weight cut-off
99
(MWCO) of 100 kDa. The concentration consisted of two heating steps, one at 55
100
°C (23 min) and other at 70 °C (60 min). The average production flow was 3000
101
L/h. The juice samples were immediately stored at -70 °C until analysis. The juice
102
samples were analyzed for total soluble solids content (TSS %) to determine the
103
dehydration level during the production process and then adjusted to 11.2 °Brix
104
before analysis of the physicochemical attributes. Several pectins were
105
sequentially obtained from the apple pomace according to their solubility and
106
evaluated for physicochemical and functional properties.
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2.2. Miscellaneous evaluations in juice
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The content of TSS (%) was determined in three subsamples (0.5 mL) of each
110
juice using an automatic digital refractometer RX 5000 (ATAGO, Tokyo, Japan).
111
The titratable acidity was determined in tree subsamples (5 mL) of each juice
112
according to Eisele and Drake (2005). The total phenolic content was determined
113
three times in each juice by the Folin Ciocalteu method at 750 nm, according to
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Spanos et al. (1990), and expressed as mg of chlorogenic acid equivalent per L of
115
juice. Three subsamples (8 mL) of each juice were evaluated for color and
116
clearness using a Thermo Spectronic 20D+ spectrophotometer (Thermo Scientific,
117
Wisconsin, USA) at 440 and 625 nm (transmittance), respectively. These
118
measurements were performed according to Kadakal and Nas (2003).
119
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2.3. Individual sugars and organic acids
121
The evaluation of sugars and organic acids was performed according to Ornelas-
122
Paz et al. (2017), with slight modifications. For sugars, three subsamples of each
123
juice were centrifuged (24652 g/ 20 min/ 4 °C) and then diluted ten times with
124
water. The pH of diluted juice was adjusted at 7 with 10% NaOH, filtered and
125
manually injected (20 µL) into a HPLC system (Varian Inc., CA, USA), which was
126
equipped with a refractive index detector (Star Model 9040). The sugars were
127
separated in a SUGAR SC 1821 (8.0 x 300 mm) (SHODEX, Tokyo, Japan) ion
128
exchange column at 70 °C. The mobile phase was HPLC grade water at a flow rate
129
of 0.6 mL/min. For organic acids, three subsamples of each juice were filtered and
130
directly injected (20 µL) into the HPLC system described above but fitted to a UV-
131
Vis detector (Model 9050). Acids were separated in an Aminex HPX-87H (7.78 x
132
300 mm) ion exchange column (Bio-Rad Laboratories., CA, USA). The separation
133
was performed at 60 °C using 5mM H2SO4 as mobile phase at a flow rate of 0.4
134
mL/min. The organic acids were monitored at λ=210 nm. The identification and
135
quantification of sugars and acids were performed using standard compounds.
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2.4. Analysis of phenolic compounds
138
The extraction and chromatographic separation of phenolic compounds were
139
based in the methodology described by Ornelas-Paz et al. (2017). Three
140
subsamples of each juice were centrifuged (24652 g/ 20 min/ 4 °C), filtered and
141
manually injected (20 µL) into an Agilent 1200 series HPLC system (Agilent Inc.,
142
CA, USA) equipped with a diode array detector. The separation of phenolic
143
compounds was performed in a ZORBAX XDB-C18 column (4.6 x 150 mm)
144
(Agilent Inc., CA, USA) at 30 °C. The phenolic compounds were monitored at λ=
145
280, 320, 350 and 520 nm. The mobile phase consisted of 2% acetic acid (A) and
146
acetonitrile (B), according to the following gradient: 100% A at 0 min, 93% A at 12
147
min, 89% A at 20 min, 86%A at 35 min, 84% A at 36 min, 82% A at 41 min, 76% A
148
at 48 min, 70% A at 54 min, and 65% A at 59 min. The flow rate was 1 mL/min.
149
Reference compounds were used for identification and quantification purposes.
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2.5. Analysis of patulin and 5-HMF
152
Three subsamples (10 mL) of each juice were individually placed in a separatory
153
funnel, vigorously mixed with ethyl acetate (20 mL), and kept in repose until
154
separation of phases. The organic phase was recovered while the aqueous phase
155
was extracted two times more with ethyl acetate (20 mL each time), recovering the
156
organic phase after each washing. The organic phases were pooled and washed
157
two times with 1.5% Na2CO3 (10 mL). The organic phase was recovered and
158
evaporated at reduced pressure at 40 °C. The residue was dissolved in 1 mL of
159
water at pH 4 (adjusted with acetic acid), filtered, and manually injected (100 µL) in
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the Agilent 1200 series HPLC system described above. The separation of patulin
161
and 5-HMF was performed according to Gökmen and Acar (1999), using a
162
ZORBAX XDB-C18 (4.6 x 150 mm) (Agilent Inc., CA, USA) column at 30 °C. The
163
patulin and 5-HMF were monitored at 276 and 284 nm, respectively. The mobile
164
phase consisted of water (pH 4, A) and acetonitrile (B) according to the following
165
gradient: 99% A at 0 min, 95% A at 10 min, 90% A at 15 min, 50% A at 20 min,
166
100% B from 25 to 35 min. The flow rate was 1 mL/min. The qualitative and
167
quantitative analyses were performed using reference compounds.
168
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2.6. Extraction of pectin
170
Triplicate samples of apple pomace (500 g each) were used as pectin source. The
171
extraction of alcohol-insoluble residues (AIR) and pectins was performed according
172
to Ramos-Aguilar et al. (2015). The AIR was subjected to sequential extraction of
173
pectin with hot water (95 °C) for 5 min, 0.05M CDTA in 0.1 M potassium acetate at
174
pH 6.5 for 6 h at 28 °C, and 0.05 M Na2CO3 containing 0.02 M NaBH4 for 16 h at 4
175
°C and then for 6 h at 28 °C. The ratio of AIR to extraction solution was 1:100 (w/v)
176
in all cases. The pectin was precipitated with ethanol and recovered by
177
centrifugation (12, 000 g/5 min/ 4 °C) and filtration (Whatman paper No. 541). The
178
recovered pectins were named as water, chelator, and alkali soluble pectin (WSP,
179
CSP, and NSP, respectively). Triplicate samples of these pectins as well as of
180
commercial apple pectin (CAP) were evaluate for physicochemical and rheological
181
properties.
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2.7. Degree of esterification of pectin
184
The GalA was liberated from pectins and colorimetrically quantified at 525 nm
185
according to Ramos-Aguilar et al. (2015). The methanol was liberated from pectins
186
according to Voragen, Schols, & Pilnik (1986). The extract was filtered and
187
manually injected (20 µL) to the Varian HPLC system described above (refractive
188
index detection). The methanol was separated in a TSKGel SCX H+ (7.8 x 300
189
mm) ion exchange column (Tosoh Bioscience LLC, Tokyo, Japan) at 30 °C.
190
Deionized water was used as mobile phase at a flow rate of 1 mL/min. The degree
191
of esterification (DE) was calculated according to Voragen et al. (1986).
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2.8. Monosaccharide composition of pectin
194
Pectin was sequentially subjected to acid and enzymatic hydrolysis according to
195
Ramos-Aguilar et al. (2015). Each hydrolysate was analyzed under two different
196
HPLC conditions using the Varian system described above (refractive index
197
detection). The Glu, Ara, Rha, Gal, and Fuc were separated at 58 °C in a Metacarb
198
H+ (7.8 x 300 mm; Varian Inc., CA, USA) ion-exchange column, using 0.0085N
199
H2SO4 as mobile phase at a flow rate of 0.4 mL/min. Xyl and Man were separated
200
in a Supelcogel Pb (7.8 x 300 mm; Sigma-Aldrich., MO, USA) ion exchange
201
column at 70°C using water as mobile phase at a flow rate of 0.5 mL/min. The
202
qualitative and quantitative analyses were performed using reference compounds.
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2.9. Molecular weight distribution of pectin
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The molecular weight (MW) distribution was determined by high performance size-
206
exclusion chromatographic, according to Pérez-Martínez et al. (2013). Pectins
207
were solubilized in water (5 g/L). The solutions were filtered through a polyethylene
208
membrane of 0.45 µm of pore size (Millipore Corp., MA, USA) and manually
209
injected (20 µL) into the Varian HPLC system described above (refractive index
210
detection). Separation was performed using a series of TSK-GEL columns
211
(GMPW XL, G5000PW XL, and G4000PW XL; 7.8 x 300 mm each) (Tosoh Bioscience;
212
Tokyo, Japan) at 40° C. Phosphate buffer (0.2 M; pH= 6.9) was used as mobile
213
phase at a flow rate of 0.4 mL/min. The MW was determined relative to dextrans of
214
known MW (1-670 kDa) (Sigma-Aldrich., MO, USA).
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2.10. Other evaluations of pectin
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The FT-IR spectra (4000 to 450 cm−1) were collected using a Spectrum Two FT-IR
218
spectrometer (Perkin Elmer Inc., MA, USA). Triplicate samples of each pectin were
219
analyzed and applied on the Attenuated Total Reflection crystal as powder. For
220
each sample, 34 scans were averaged with a spectral resolution of 4 cm−1. Spectra
221
analyses and baseline corrections were performed using the Spectra software ver.
222
10.4.4.449 (Perkin Elmer Inc., MA, USA). The viscosity of pectin solutions (1%)
223
was determined according to Ramos-Aguilar et al. (2015) but using a stainless
224
steel cone geometry (4°, 40 mm diameter) and a gap size of 90 µm. Pectin thermal
225
stability was analyzed with a Q500 thermogravimetric analyzer (TA Instruments.,
226
DE, USA). Ten milligrams of pectin powder were weighted in aluminum pans and
227
heated from 30 to 600 °C at 10 °C/min under nitrogen flow (15 mL/min). The
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thermogravimetric curves were analyzed with Universal Analysis 2000 software
229
(ver. 4.5A). The tristimulus color (L*, a* and b*) was determined on pectin samples
230
(powder) using Minolta colorimeter (CR-300 model, Minolta Co. Ltd, Osaka,
231
Japan).
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232
2.11. Statistical analysis
234
The values obtained weekly for each measurement were averaged and considered
235
as a single value. Data were analyzed by an analysis of variance under a
236
completely randomized design with a limit of significance of 0.05. The comparison
237
of means was performed using the Tukey-Kramer post hoc test. The analysis data
238
was performed using JMP statistical software (SAS Institute, Inc., NC, USA).
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3. Results and discussion
241
3.1. Juice color and clearness
242
The pasteurization and clarification steps sequentially increased the transmittance
243
of the freshly pressed juice at both wavelengths (Table 1). He et al. (2007) also
244
observed that the transmittance of apple juice at 440 nm increased from 53.7% to
245
66.7% after pasteurization. Vladisavljević, Vukosavljević, & Bukvić (2003) observed
246
increases of transmittance after juice clarification that varied between 30 and 21%,
247
depending of the clarification method. The increase of transmittance during the first
248
steps of juice processing might be attributed to the hydrolysis of pectin and starch
249
by added enzymes as well as by removal of these polysaccharides by UF
250
membranes (He et al., 2007). In our study, the transmittance of juice at both
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wavelengths was reduced 6-8.7% after concentration (Table 1). Others are also
252
observed a slight decrease (4.4-7.7%) in the transmittance of apple juice at both
253
wavelengths after concentration (Kadakal & Nas, 2003; Garza, Giner, Martín,
254
Costa, & Ibarz, 1996). The decrease of transmittance at the concentration step
255
might be consequence of phenol oxidation, the suspension of particles formed by
256
residues of depolymerized pectin and denaturalized proteins that crossed the UF
257
membrane at the clarification step, and formation of Maillard’s reaction products
258
(Garza et al., 1996; He et al., 2007; Kadakal & Nas, 2003; Onsekizoglu et al.,
259
2010; Vladisavljević et al., 2003). The 5-HMF might contribute to juice color
260
because it was detected in concentrated juice at a concentration of 4.0 ± 0.6 mg/L.
261
Similar contents of 5-HMF (up to 7.9 mg/L) have been reported in apple juices after
262
thermal concentration in a rotavapor
263
patulin was not detected.
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3.2. Effect of processing on sugars and acids
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The TSS content in freshly pressed juice did not changed during pasteurization
267
and clarification steps (Table 1). Others have reported similar findings at laboratory
268
and pilot plant scale (Gökmen et al., 2001; Suárez-Jacobo et al., 2011;
269
Vladisavljević et al., 2003). In our study, the juice was concentrated 5.2 times
270
during the evaporation step. Similar changes of concentration (4.8 times) have
271
been reported for apple juice under industrial-scale conditions (Welke et al., 2009).
272
Fructose was the main sugar in tested juices, followed by sucrose and glucose
273
(Table 2). The content of individual sugars was not significantly altered by any
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processing step, as reported in some studies at laboratory and pilot plant scale
275
(Onsekizoglu et al., 2010; Suárez-Jacobo et al., 2011).
276
The TA of juice was similar during the first three steps of the production process
277
(Table 1). Previous studies at laboratory scale with juice from ‘Golden Delicious’
278
apples demonstrated that the TA was not significantly altered by both thermal or
279
non-thermal pasteurization and clarification by UF (Aguilar-Rosas, Ballinas-
280
Casarrubias, Nevarez-Moorillon, Martin-Belloso, & Ortega-Rivas, 2007; Youn,
281
Hong, Bae, Kim, & Kim, 2004). In this study, a slight decrease (11%) of TA was
282
observed after evaporation. Onsekizoglu et al. (2010) observed under laboratory
283
conditions a decrease of 4.7% in acid concentration of juice from the clarification to
284
the evaporation step. The malic and ascorbic acids were the most abundant in
285
tested juices (Table 2). The concentration of each acid in freshly pressed juice was
286
statistically similar to that of the concentrated juice (final juice). However,
287
temporary alterations in acid content were observed at pasteurization step.
288
Interestingly, the highest or lowest concentration of each one of tested acids were
289
observed after pasteurization (Table 2). The effect of this step on acids has not
290
been clearly studied; however, the high temperatures used for pasteurization could
291
improve the release of organic acids from apple particles and the dehydration of
292
some of them, altering consequently their concentrations (Gökmen & Acar, 1998).
294
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3.3. Phenolic compounds in apple juice
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Tested juices were rich in phenolic compounds, as judged by the total phenolic
296
content (Table 1). Interestingly, such content increased (100%) during the
297
production process. This might be a consequence of the thermal and enzymatic
298
release of phenols from fibers during the production process (Kammerer et al.,
299
2014). Eleven phenolic compounds were identified and quantified in tested juices,
300
with chlorogenic acid, procyanidin B2, phloridzin and epicatechin being the most
301
abundant (Table 3). The concentration of these compounds was into the range
302
reported for raw and processed juices (chlorogenic acid, 3.4-113.7 mg/L; caffeic
303
acid, 0.7-8.7 mg/L; p-coumaric acid, 0.1-3.0 mg/L; epichatequin, 0-71.8 mg/L;
304
procyanidin B2, 0-121 mg/L; quercertin-3-galactoside, 0-14.4 mg/L; quercetin-3-
305
glucoside, 0-9.1 mg/L; phloridzin, 1.3-56.0 mg/L) (Gliszczynska-Swiglo &
306
Tyrakowska, 2003; Oszmiański, Wojdyło, & Kolniak, 2011; Spanos et al., 1990).
307
In general, the content of individual phenolic compounds continuously increased
308
from the pressing to the clarification step (Table 3). Some studies at laboratory
309
scale demonstrated the reduction of the phenolic content (4-45%) in apple juice
310
during juice clarification with membranes of MWCO from 10 to 30 kDa (Gökmen et
311
al., 2001; Onsekizoglu, 2013). The membrane used in this study was of a MWCO
312
considerably higher (100 kDa), explaining the low impact of such step on phenols.
313
The concentration step did not alter the levels of phenolic compounds.
314
Substantial increases (34-109%) in chlorogenic, caffeic and p-coumaric acids were
315
observed during the pasteurization and clarification steps. Spanos et al. (1990)
316
demonstrated at pilot plant scale that the juice production at elevated temperatures
317
(55-73 °C) improved the extractability (3-222%) of cinnamic acids and decreased
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their degradation due to the inactivation of polyphenol oxidase. Oszmiański et al.
319
(2011) also observed at laboratory scale increases (4-14%) in the content of
320
chlorogenic acid in apple juice after treatment with pectolytic and cellulolytic
321
enzymes. The changes in the content of flavan-3-ols during pasteurization and
322
clarification were higher than those for cinnamic acids (Table 3). The increase in
323
the content of epicatechin and procyanidin B2 ranged from 52 to 163% during
324
pasteurization and clarification steps. Similar increases (109-286%) have been
325
observed for these flavan-3-ols during such steps at laboratory scale (Spanos et
326
al., 1990). The high temperature could induce the hydrolysis of inter-flavonoid
327
linkages in procyanidins, increasing the concentration of their monomeric and
328
dimeric structures, epicatechin and procyanidin B2, while the enzymatic treatment
329
might favor the liberation of procyanidins linked to cell-wall polysaccharides,
330
especially pectin (De Paepe et al., 2014; Oszmiański et al., 2011). The content of
331
quercetin glycosides did not show significant changes during the apple juice
332
processing (Table 3). However, the quercetin aglycone was detected in clarified
333
and evaporated juices, probably as a consequence of the hydrolysis of glycosidic
334
forms during the enzymatic clarification. The effect of processing steps in free and
335
glycosylated quercetin of apple juice has been previously reported under laboratory
336
and pilot scale conditions with contradictory results (increases of up to 300% and
337
reductions of up to 75%), depending of the apple variety, enzymatic treatment, and
338
clarification and concentration methods (Gökmen et al., 2001; Markowski et al,
339
2015; Onsekizoglu et al., 2010; Spanos et al., 1990).
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3.4. Properties of pectin
342
The total pectin content of apple pomace was 9% (Table 4). Similar content of
343
pectin (7.8%) in apple pomace was recently reported by O’Shea et al. (2015). The
344
FT-IR spectra showed the two characteristic absorption bands for polysaccharides,
345
a strong and wide absorption band at 3100-3700 cm-1 for O-H stretching vibrations
346
and a weak absorption peak of about 2800-3000 cm-1 for C-H stretching vibrations
347
(Fig. 1) (Qiao et al., 2009). It also showed the peaks at 882 and 1273 cm-1, which
348
are characteristic of the pyranose ring of pectin and the C-O dilatation and vibration
349
(Kačuráková, Capek, Sasinkova, Wellner, & Ebringerova, 2000; Wang et al.,
350
2014). In this study, the pomace contained only CSP and NSP, while the WSP was
351
missing. The yield for CSP was 30% higher than that of NSP. These findings differ
352
from those of Kosmala et al. (2010), who observed that content of pectin types in
353
apple pomace followed the order of NSP˃CSP˃WSP (49.9–107.3, 18.9–26.0, 9.4–
354
20.0 mg/g, respectively). This difference might be a consequence of the high
355
activity of the pectin lyase at the pressing step and the using of overripe fruit in the
356
present study. The pectinolytic activity of this enzyme is particularly high for highly
357
esterified pectins and WSP use to show the highest DE (Yadav, Yadav, Yadav, &
358
Yadav, 2009). Laboratory-scale studies conducted in our laboratory with the same
359
apples demonstrated the existence of WSP in apple pomace obtained without the
360
using of enzymes (data not shown). Thus, pectin lyase might hydrolysate all of the
361
WSP as well as high amounts of CSP and NSP. The using of overripe fruit might
362
exacerbate this effect. Recently, Ramos-Aguilar et al. (2015) demonstrated that
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the yield of pectin from ripe green peppers follow the order of NSP˃CSP˃WSP but
364
this order was inverted with red peppers (WSP˃ CSP ˃NSP).
365
The extracted pectins were of low DE (Table 4). The DE decreased 49% from CSP
366
to NSP. CAP showed the highest DE (67%), which was virtually identical to that
367
provided by the supplier (70-75%). CSP and NSP from other plant sources have
368
also been described as lowly esterified pectins (DE= 11.2-14.8%) (Sila et al., 2006;
369
Sila et al., 2009). The FT-IR spectra confirmed the high difference of DE for tested
370
pectins (Fig. 1). The absorption peaks at 1750-1730 cm-1 indicated the presence of
371
carbonyl esters (C=O) (Wang et al., 2014) and their intensity and area agreed with
372
the obtained DE values, especially with those of CAP and CSP (Fig. 1, Table 4).
373
The composition of neutral sugars was different for tested pectins (Table 4). The
374
content of GalA was 10% higher in CSP than in NSP; however, CAP showed the
375
highest GalA content, which was up to 40% higher than that of the other pectins.
376
Similarly, Kosmala et al. (2010) observed that the GalA content was 49-74% higher
377
in chelator soluble pectin from apple pomace than in alkali soluble pectin. The
378
content of Man and Ara in CSP and NSP was 68-83% higher than in CAP while
379
CAP was especially rich in Gal and Glu, showing a content of these sugars 50–
380
71% higher than that of the other pectins. Interestingly, the content of almost all of
381
the tested sugars was higher (17-40%) in NSP than in CSP. This finding indicates
382
that NSP was more branched and intact than CSP (Sila et al., 2009). This was
383
supported by the MW distribution of tested pectins. They contained up to three
384
fractions but the first of them was substantially abundant. The peak MW of such
385
fraction is shown in Table 4. First fraction showed the highest MW in NSP, followed
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by CSP and CAP. In general, the MW found in this study for the most abundant
387
fractions was into the range reported for apple pectin (100-10000 kDa) (Fischer et
388
al., 1994).
389
The pectin solutions showed a pseudoplastic behavior, especially whiting the range
390
from 50 to 100 s-1 (Fig. 2). The flow behavior showed high correlation values (R2=
391
0.989–0.999) with the power law model. The k values of tested pectins were
392
significantly different, with viscosity of CSP (k= 0.053 Pa.sn) being almost twice
393
than that NSP (k= 0.027 Pa.sn). CAP showed the highest viscosity (k= 0.143
394
Pa.sn). The viscosity of tested pectins showed an inverse relationship with MW of
395
the main fractions (Table 4). The viscosity of pectin solutions is highly influenced
396
by sugar composition, DE and MW. In this study, the content of GalA and Glu and
397
the DE were directly related with viscosity. Wang et al. (2014) demonstrated that
398
the viscosity of apple pectin increased with the GalA content. Liu, Cao, Huang, Cai,
399
and Yao (2010) demonstrated that the gellification and viscosity of pectin increased
400
with the content of GalA and DE.
401
The thermogravimetric analysis showed that the tested pectins released moisture
402
(∼6%) with a maximum derivative of weight loss peak (Pk) at 80°C. The CSP
403
showed a low thermal stability fraction (Pk ≈ 200 °C). The highest degradation
404
amount for all pectins was observed at Pk between 238 and 245 °C (Fig. 3), which
405
has been associated to the pyrolytic decomposition of homogalacturonans (Combo
406
et al., 2013). Accordingly, the pectin with the higher GalA content and viscosity
407
(CAP) had the highest degradation in this region (Table 4; Figs. 2 and 3). At
408
temperatures above 350 °C, the CSP and the NSP showed degradation, which
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probably was associated to lignocellulosic materials (Yang et al., 2006). Thus, we
410
could assume that CSP contained a relatively higher content of cellulosic material
411
than NSP. NSP probably contained more lignin-associated polysaccharides
412
because it showed a higher stability at temperature above 350 °C. These
413
compositional changes were probably responsible for the absence of the direct
414
relationship between MW and viscosity and thermogravimetric properties of tested
415
pectins.
416
The color of pectins is not usually reported; however, it is an important property of
417
pectin because it may determine its use in food formulations. In this study, the CSP
418
and CAP showed similar color values, although their L* values were statistically
419
different (Table 4). The color values of these pectins (L*= 72.7- 74.1, a*= 4.1-3.9,
420
b*= 12.9-12.3) were within the ranges reported for pectin from other sources, such
421
as mango, citrus, beet and peppers (L*= 67.5–93.5, a*= -0.6–3.5 and b*= 9.38–
422
20.2) (Berardini, Knödler, Schieber, & Carle, 2005; Mesbahi, Jamalian, &
423
Farahnaky, 2005; Ramos-Aguilar et al., 2015). The NSP was darker than CSP and
424
CAP, according to its significantly lower values of L* and b*, and the higher value
425
of a* (Table 4). The darkness of pectin is highly related with their phenol content
426
(Ramos-Aguilar et al., 2015), thus, the oxidation of phenols during the extraction of
427
NSP might explain the color of this pectin type. However, the extraction conditions
428
can also influence the structure of pectin and these alterations can influence the
429
color of pectin (Pérez-Martínez et al., 2013; Einhorn-Stoll, Kastner, & Drusch,
430
2014).
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4. Conclusions
433
The steps of the juice production process involving high temperature and enzymes
434
had a significant effect on key components of apple juice (organic acids, phenolics,
435
and 5-HMF). Some effects of the processing coincided with those observed
436
previously at laboratory or pilot plant scale. Tested pomace contained CSP and
437
NSP but not WSP. These pectins differed from CAP in terms of their high MW,
438
Man and Ara content as well as for their low DE, GalA and Gal content. This
439
resulted in lower viscosity and different thermal stability, as compared with the
440
functional properties observed for CAP. The ripening, type of fruit and use of
441
enzymes during the process of juice production were probably involved in the
442
physical and chemical properties of extracted pectins, compromising their
443
functionality.
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Acknowledgements
446
This research was funded by the Fondo Mixto CONACYT- Gobierno del Estado de
447
Chihuahua (Project Clave: CHIH-2012-C03-194579).
448
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stages of apple juice concentrate on patulin levels. Food Control, 20, 48–52.
576
Yadav, S., Yadav, P. K., Yadav, D., & Yadav, K. D. S., 2009. Pectin lyase: A
577 578
TE D
574
review. Process Biochemistry, 44, 1–10. Yang, H., Yan, R., Chen, H., Zheng, C., Lee, D. H., & Liang, D. T. (2006). In-Depth investigation
of
biomass
pyrolysis
based
on
three
major
580
components: hemicellulose, cellulose and lignin. Energy & Fuels, 20, 398-
581
393.
AC C
EP
579
582
Youn, K. S., Hong, J. H., Bae, D. H., Kim, S. J., & Kim, S. D. (2004). Effective
583
clarifying process of reconstituted apple juice using membrane filtration with
584
filter-aid pretreatment. Journal of Membrane Science, 228, 179-186.
585 586 26
ACCEPTED MANUSCRIPT
Figure captions
588
Fig. 1. FT-IR spectra of commercial apple pectin (CAP, ─) and chelator- and alkali-
589
soluble pectin fractions (CSP, ─; NSP, ─) from apple pomace.
590
Fig. 2. Flow curves and parameters of power law model obtained from solutions of
591
commercial apple pectin (CAP, ⚫) and chelator- and alkali-soluble pectin fractions
592
(CSP, ⚪; NSP, ▼) from apple pomace. n, flow behavior. k, consistency index.
593
Fig. 3. Thermogravimetric analysis (A) and derivative thermogravimetric (B) curves
594
for commercial apple pectin (CAP, ─) and chelator- and alkali-soluble pectin
595
fractions (CSP, ─; NSP, ─) from apple pomace.
M AN U
SC
RI PT
587
596
597
Table captions
599
Table 1. Effect of industrial processing on color, clearness, total soluble solids,
600
titratable acidity, and total phenolic content in apple juice
601
Table 2. Concentration of sugars and organic acids in apple juice at selected steps
602
of the industrial production process.
603
Table 3. The effect of the industrial processing on the content of phenolic
604
compounds in of apple juice.
605
Table 4. Yield and physicochemical characteristics of commercial apple pectin
606
(CAP) and chelator- and alkali-soluble pectin fraction (CSP and NSP) from
607
enzyme-treated apple pomace.
AC C
EP
TE D
598
27
ACCEPTED MANUSCRIPT
Table 1.
0.1 ± 0.0 c
0.8 ± 0.2 c
4.9 ± 0.46 d
10.7 ± 1.5 c
11.2 ± 0.4 b
7.0 ± 0.1 ab
Color a
(440 nm)
Clearness
10.7 ± 0.7 b
11.6 ± 0.5 b
69.0 ± 0.6 a
7.8 ± 0.4 a
7.3 ± 0.2 ab
6.5 ± 0.2 b
0.35 ± 0.0 ab
0.4 ± 0.0 a
M AN U
(%)
AC C
equivalents /L)
0.3 ± 0.0 b
EP
0.2 ± 0.0 c
TE D
Titratable acidity
(g chlorogenic acid
47.6 ± 0.3 b
90.1 ± 0.5 b
Total soluble solids
Total phenols
53.8 ± 2.4 a
Concentration
98.8 ± 2.6 a
(625 nm )a
(g malic acid/ L)
Clarification
RI PT
Pasteurization
SC
Pressing
The juice was adjusted at 11.2 °Brix before color, clearness, acidity, and total phenolic content measurements. Values represent the mean of 12 individual measurements ± the standard error. Data in the same row connected by different letters are significant different (p ≤ 0.05). a Values are given % transmittance.
ACCEPTED MANUSCRIPT
Table 2. Pasteurization
Fructose
56.8 ± 2.2 a
64.0 ± 3.5 a
Sucrose
32.0 ± 1.8 a
35.9 ± 1.0 a
Glucose
16.1 ± 0.8 a
16.5 ± 0.8 a
Malic
2732.4 ± 185.7 b
Ascorbic
Clarification
RI PT
Pressing Sugars (g/L)
Concentration
58.6 ± 1.4 a
33.0 ± 1.6 a
31.4 ± 1.0 a
16.0 ± 0.6 a
17.2 ± 0.6 a
3653.8 ± 387.2 a
3137.7 ± 98.7 ab
2953.4 ± 95.3 ab
935.6 ± 121.3 a
722.7 ± 64.6 a
820.6 ± 80.5 a
808.7 ± 170.4 a
Succinic
555.0 ± 52.7 b
707.3 ± 57.2 a
526.1 ± 48.3 b
465.9 ± 27.5 b
Oxalic
196.7 ± 40.0 a
95.3 ± 16.4 b
151.6 ± 13.7 ab
201.0 ± 18.8 a
3.6 ± 0.5 c
5.3 ± 0.4 bc
8.3 ± 0.3 a
7.1 ± 2.9 a
1.9 ± 0.3 a
3.1 ± 0.3 a
Fumaric
4.2 ± 0.5 a
M AN U
AC C
EP
6.8 ± 1.3 ab
TE D
Organic acids (mg/L)
Tartaric
SC
57.7 ± 1.7 a
The juice was adjusted at 11.2 °Brix before analysis. Values represent the mean of 12 individual measurements ± the standard error. Data in the same row connected by different letters are significant different (p ≤ 0.05).
ACCEPTED MANUSCRIPT
Table 3. Compound (mg/L)
Pressing
Pasteurization
Clarification
Concentration
Chlorogenic acid
18.5 ± 1.3 c
31.7 ± 2.4 b
38.8 ± 2.0 a
37.2 ± 1.1 ab
Caffeic acid
0.9 ± 0.0 b
1.0 ± 0.1 b
1.2 ± 0.0 a
1.2 ± 0.0 a
ND
ND
0.04 ± 0.00
ND
0.5 ± 0.0 b
0.5 ± 0.0 b
0.9 ± 0.1 a
0.8 ± 0.1 a
0.2 ± 0.0 a
0.2 ± 0.0 ab
0.1 ± 0.0 b
0.1 ± 0.0 b
6.6 ± 0.8 a
8.4 ± 0.6 a
8.9 ± 0.8 a
15.4 ± 1.5 a
16.9 ± 2.0 a
15.1 ± 0.2 ab
ND
ND
0.3 ± 0.1 a
0.3 ± 0.1 a
Quercetin 3-D-galactoside
1.5 ± 0.1 a
1.8 ± 0.2 a
1.5 ± 0.1 a
1.6 ± 0.1 a
Quercetin 3-β-glucoside
0.5 ± 0.0 a
0.5 ± 0.0 a
0.6 ± 0.0 a
0.6 ± 0.0 a
4.8 ± 0.5 b
6.3 ± 0.9 b
10.7 ± 0.9 a
9.7 ± 0.6 a
p-Coumaric acid
SC
Cinnamic acid
Flavan-3-ols Epicatechin
3.2 ± 0.4 b
Procyanidin B2
10.1 ± 0.8 b
Phloridzin
EP
Dihydrochalcones
AC C
Quercetin
TE D
Flavonols
M AN U
Hydroxybenzoic acid Protocatechuic acid
RI PT
Hydroxycinnamic acids
The juice was adjusted at 11.2 °Brix before analysis. Values represent the mean of 12 individual measurements ± the standard error. Data in the same row connected by different letters are significant different (p ≤ 0.05). ND, not detected.
ACCEPTED MANUSCRIPT
Table 4. Pectin type CSP
NSP
-
5.3 ± 0.1 a
3.7 ± 0.1 b
L*
72.7 ± 0.1 b
74.1 ± 0.4 a
54.6 ± 0.1 c
a*
4.1 ± 0.0 b
3.9 ± 0.1 b
5.3 ± 0.1 a
b*
12.9 ±0.1 a
12.3 ± 0.1 b
11.0 ± 0.1 c
436.6 ± 8.0 b
393.5 ± 5.2 c
Galacturonic acid (mg/g)
654.1 ± 5.7 a
Monosaccharides (mg/g)
M AN U
Tristimulus color
SC
Yield (%)
RI PT
CAP
Mannose Arabinose Galactose
Xylose Rhamnose Fucose
EP
Degree of esterification (%)
132.9 ± 3.0 b
198.3 ± 5.0 a
27.5 ± 0.3 c
103.4 ± 1.9 b
166.3 ± 1.9 a
228.6 ± 2.2 a
71.3 ± 1.8 c
115.0 ± 1.8 b
45.5 ± 0.3 a
16.1 ± 0.2 b
13.4 ± 0.1 c
13.0 ± 0.3 a
11.7 ± 0.5 b
14.0 ± 0.2 a
9.0 ± 0.1 a
4.8 ± 0.2 c
7.9 ± 0.3 b
2.8 ± 0.1 a
2.5 ± 0.1 b
ND
67.4 ± 3.4 a
44.6 ± 2.9 b
22.8 ± 2.4 c
644.5 ± 8.9 c
1559.6 ± 49.6 b
2360.6 ± 38.3 a
TE D
Glucose
42.1 ± 0.5 c
AC C
Peak molecular weight (kDa)
Values represent the mean of at least three individual measurements ± the standard error. Values in the same row with different letters are significantly different (p < 0.05). ND, not detected.
SC
RI PT
ACCEPTED MANUSCRIPT
3000-2800
100
96 3700-3100
92 90
86
Fig. 1.
1273-882
EP
88
84 4000
1750-1730
TE D
94
3500
AC C
Transmittance (%)
98
M AN U
102
3000
2500 2000 Wavenumber (cm-1)
1500
1000
500
ACCEPTED MANUSCRIPT
0.10
M AN U
SC
0.08
n
k (Pa·s ) a 0.143 ± 0.003 b 0.053 ± 0.001 c 0.027 ± 0.001
RI PT
CAP CSP NSP
0.06
0.04
0.00 100
200
EP
0
TE D
0.02
AC C
Apparent viscosity (Pa.s)
0.12
n a 0.919 ± 0.004 b 0.891 ± 0.004 c 0.852 ± 0.006
Fig. 2.
300
Shear rate (1/s)
400
500
600
AC C
EP
TE D
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
Fig. 3.
ACCEPTED MANUSCRIPT
-The impact of industrial processing on properties of apple juice is scarcely known -Few pectin fractions from apple pomace have been characterized
RI PT
-The sugar content in apple juice was not altered by any processing step
-The pasteurization step altered the levels of individual phenols and acids -Concentration step favored the formation of 5-HMF
AC C
EP
TE D
M AN U
SC
-Pomace pectins showed less functionality than commercial apple pectin