High Antioxidant Action and Prebiotic Activity of Hydrolyzed Spent

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High antioxidant action and prebiotic activity of hydrolyzed spent coffee grounds (HSCG) in a simulated digestion-fermentation model: toward the development of a novel food supplement Lucia Panzella, Sergio Pérez-Burillo, Silvia Pastoriza, María Angeles Martín, Pierfrancesco Cerruti, Luis Goya, Sonia Ramos, José A. Rufián-Henares, Alessandra Napolitano, and Marco d'Ischia J. Agric. Food Chem., Just Accepted Manuscript • DOI: 10.1021/acs.jafc.7b02302 • Publication Date (Web): 10 Jul 2017 Downloaded from http://pubs.acs.org on July 10, 2017

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Journal of Agricultural and Food Chemistry

1 High antioxidant action and prebiotic activity of hydrolyzed spent coffee grounds (HSCG) in a simulated digestion-fermentation model: toward the development of a novel food supplement

Lucia Panzella,*,† Sergio Pérez-Burillo,∞ Silvia Pastoriza,∞ María Ángeles Martín,‡ Pierfrancesco Cerruti,§ Luis Goya,‡ Sonia Ramos,‡ José Ángel Rufián-Henares,# Alessandra Napolitano,† and Marco d’Ischia†



Department of Chemical Sciences, University of Naples “Federico II”, Via Cintia 4, I-80126,

Naples, Italy ∞

Departmento de Nutrición y Bromatología, Facultad de Farmacia, Universidad de Granada,

Campus Universitario de Cartuja, 18071 Granada, Spain ‡

Department of Metabolism and Nutrition, ICTAN, CSIC, José Antonio Novais 10, 28040 Madrid,

Spain §

Institute for Polymers, Composites and Biomaterials (IPCB-CNR), Via Campi Flegrei 34, I-80078

Pozzuoli, Italy #

Departamento de Nutrición y Bromatología, Instituto de Investigación Biosanitaria

ibs.GRANADA, Universidad de Granada, Granada, Spain

*Corresponding author (Tel: +39081674131; Fax: +39081674393; E-mail: [email protected])

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Abstract

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Spent coffee grounds are a by-product with a large production all over the world. The aim of this

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study was to explore the effects of a simulated digestion-fermentation treatment on hydrolyzed

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spent coffee grounds (HSCG) and to investigate the antioxidant properties of the digestion and

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fermentation products in human hepatocellular carcinoma HepG2 cell line. The potentially

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bioaccessible (soluble) fractions exhibited high chemoprotective activity in HepG2 cells against

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oxidative stress. Structural analysis of both the indigestible (insoluble) and soluble material

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revealed partial hydrolysis and release of the lignin components in the potentially bioaccessible

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fraction following simulated digestion-fermentation. A high prebiotic activity as determined from

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the increase in Lactobacillus spp. and Bifidobacterium spp. as well as the production of short chain

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fatty acids (SCFAs) following microbial fermentation of HSCG was also observed. These results

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pave the way toward the use of HSCG as a food supplement.

13 14

Keywords: spent coffee grounds; antioxidant; reactive oxygen species; simulated digestion-

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fermentation; HepG2 cells; short chain fatty acids

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Introduction

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Coffee is by far one of the most consumed beverages in the world and the resulting spent coffee

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grounds (SCG), because of the high content in caffeine, tannins, and polyphenols, can have harmful

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effects on the environment, requiring proper management and disposal.1 Proposed use of SCG

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includes production of biofuel, removal of pollutants from water and as a source of natural phenolic

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antioxidants for use as nutritional supplements, foods, or cosmetic additives.1-9

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SCG contain mainly carbohydrates (38–42%), proteins (8%), and chlorogenic acids (3–4%).10,11 As

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a major outcome of the roasting process, SCG contain also melanoidins, which are usually

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quantified to account for ca. 25% w/w of the dry weight of roasted coffee beans.12,13

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We recently developed an expedient chemical procedure to convert SCG into an all-natural

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biocompatible material, termed hydrolyzed spent coffee grounds (HSCG), involving an hydrolytic

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protocol with 6 M HCl, at 100 °C, overnight. The black powder thus obtained displayed potent

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antioxidant properties for diverse applications, including e.g. cell protection, food lipid preservation

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and thermal and photo-oxidative stabilization of polymers.14

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Yet, simple chemical assays are inadequate to evaluate the actual antioxidant activity of food, and

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the importance of in vitro digestion combined with cellular assays to determine the antioxidant

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activity has been recently emphasized.15-20

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SCG have been found to be good sources of prebiotic compounds following in vitro digestion.12

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The chemical characterization of potentially prebiotic oligosaccharides in SCG have been also

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recently reported.21

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The anti-inflammatory potential of the metabolites produced by colonic fermentation of SCG has

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also been described, supporting the use of SGC in the food industry as dietary fiber source with

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health benefits.12,22 However, the physiological potential and health benefits of HSCG have not yet

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been adequately investigated.

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We report herein the modifications induced by in vitro gastrointestinal digestion followed by a

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fermentation step on the antioxidant activity of HSCG. The potential antioxidant and oxidative ACS Paragon Plus Environment

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stress protection of both the potentially bioaccessible digestion and fermentation products and the

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residual, undigested fraction of HSCG were investigated by validated cellular assays using human

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liver HepG2 cell line. This is generally held as a sensitive model for the determination of the

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chemoprotective potential of antioxidant compounds.23 Preliminary structural investigation on both

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the soluble, potentially bioaccesible, fractions and the residual, indigestible, solid fraction was

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carried out. The prebiotic activity of HSCG was also determined.

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Materials and Methods

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Chemicals. HSCG were prepared from espresso SCG collected from a local coffee shop as

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previously described.14 Salivary α-amylase, pepsin from porcine, bile acids (bile extract porcine),

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tryptone, cysteine, sodium sulphide, resazurin, inulin, o-phthaldialdehyde (OPT), glutathione

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(GSH), and 2,7-dichlorofluorescin diacetate (DCFH-DA) were from Sigma-Aldrich. Pancreatine

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from porcine pancreas was purchased from Alpha Aesar, tert-butylhydroperoxide (t-BOOH) from

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Panreac, Bradford reagent from BioRad.

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General Experimental Methods. FTIR analysis was performed using a Perkin Elmer Spectrum

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100 spectrometer in attenuated total reflectance (ATR) mode, with an average of 32 scans and

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resolution of 4 cm−1, in the range 4000-400 cm−1. UV-vis spectra were recorded on a Agilent/HP

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8453 spectrophotometer. NMR spectra were recorded in D2O or CD3OD on a Bruker 400 MHz

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NMR spectrometer. HPLC analysis was performed with an instrument equipped with a UV-vis

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detector (Agilent, G1314A); a Phenomenex Sphereclone ODS column (250 × 4.60 mm, 5 µm) was

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used, at a flow rate of 0.7 mL/min; a 1% formic acid (solvent A)/methanol (solvent B) gradient

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elution was performed as follows: from 5 to 90% B, 0-45 min; the detection wavelength was 254

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nm. Short chain fatty acid (SCFAs) determination was carried out on Accela 600 HPLC (Thermo

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Scientific) equipped with a pump, an autosampler and a UV-VIS PDA detector set at 210 nm; the

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mobile phase used was 0.1 M phosphate buffer (pH 2.8)/acetonitrile 99:1 v/v delivered at a 1

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mL/min flow rate; the column used was an Aquasil C18 reverse phase (Thermo Scientific) (150 ×

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4.6 mm, 5 µm), with a total run-time of 20 min. ACS Paragon Plus Environment

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In vitro Digestion. The in vitro digestion method followed was an adaptation to the method

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previously described,17,24 composed of an oral phase, a gastric phase and an intestinal one. Briefly,

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for the oral phase, 5 mL of simulated salivary fluid containing α-amylase were added to 0.5 g of

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grinded HSCG. Such mix was incubated at 37 oC for 2 min. Then, 10 mL of simulated gastric fluid

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containing pepsin were added and the pH lowered to 3.0 by adding 1 N HCl. The mixture was

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incubated at 37 oC for 2 h, after that 20 mL of simulated intestinal fluid containing pancreatin and

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bile salts were added and the pH increased to 7.0 with 1 N NaOH. The mixture was then incubated

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at 37 oC for 2 h. In order to stop the enzymatic reactions, the tube was buried in iced water,

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centrifuged at 14000 g for 10 min at 4 oC and the supernatant stored at -80 oC until further analysis.

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A 10% of the liquid fraction was added to the solid residue in order to mimic the fraction that is not

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readily absorbed after digestion.25 Then, the mixed fractions were frozen for further lyophilization.

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When required, the supernatant from the digestion mixture was lyophilized, too, and then subjected

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to chemical extraction: in brief, 300 mg of material were dissolved in 120 mL of water, then the

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solution was taken to pH 1 with 3 M HCl and extracted with ethyl acetate (3 × 100 mL). The

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combined organic layers were dried over Na2SO4 and taken to dryness to give a dark yellow oily

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residue (ca. 30 mg). For comparison ethyl acetate extraction was performed also on the supernatant

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form a control mixture containing enzymes and other ingredients but no HSCG.

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In vitro Fermentation. The method used was adapted from a previously described protocol.26 In

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brief, to 300 mg of lyophilized digestion solid residue, 200 µL of distilled water were added into a

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screw-cap tube to make up the volume up to 0.5 mL. Then, 7.5 mL of fermentation final solution

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(peptone water + resazurine) was added. Finally, 2 mL of inoculum was added being the final

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volume 10 mL. The inoculum consisted of a solution of 32% feces in phosphate buffer 100 mM, pH

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7.0 (fecal content composed of a mixture of equal weight of fresh morning feces of three healthy

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adult human donors, mean body mass index = 21.3). Nitrogen was bubbled in order to reach an

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anaerobic atmosphere and the mixture was incubated at 37 oC for 20 h under oscillation. Right after,

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the sample was buried in ice to stop microbial activity and centrifuged. Supernatant was collected ACS Paragon Plus Environment

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and stored at -80 oC. The solid residue was also stored for direct antioxidant activity measure. Both

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digestion and fermentation were performed in triplicate. When required, the supernatant was

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lyophilized and subjected to chemical extraction: in brief, 100 mg of material were dissolved in 40

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mL of water, then the solution was taken to pH 1 with 3 M HCl and extracted with ethyl acetate (3

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× 30 mL). The combined organic layers were dried over Na2SO4 and taken to dryness to give a dark

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yellow oily residue (ca. 4 mg). For comparison ethyl acetate extraction was performed also on the

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supernatant of a control mixture containing all the ingredients but no HSCG.

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SCFAs Assay. SCFAs determination (acetic, propionic and butyric acids) was carried out by HPLC

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as described in the General Experimental Methods. The sample did not require any pretreatment

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before injection. Briefly, the SCFA standards were prepared in the mobile phase at concentrations

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ranging from 5 to 10000 ppm. After the fermentation process, 1 mL of supernatant was centrifuged

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to remove solid particles, filtered through a 0.22 µm nylon filter and finally transferred to a vial for

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HPLC analysis. A probiotic commercial milk beverage was also analyzed for comparison.

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Prebiotic activity. The ability of bacteria to utilize HSCG as carbon source was performed as

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previously described.12 After the digestion-fermentation step, qRTi-PCR was performed as reported

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previously27 to assess the growth of different bacterial strains. The QIAamp DNA Stool Mini Kit

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(Qiagen) was used for DNA extraction, after diluting the stool contents 1:10 (w/v) in phosphate

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buffer saline (PBS). DNA was eluted in the provided buffer, and purified DNA extracts were stored

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at −20 °C. A series of genus-specific primer pairs were used.27 PCR amplification and detection was

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performed in an Eco Illumina thermocycler as follows. Each reaction mixture (10 µL) was

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composed of 5 µL of KAPA SYBR Fast Master Mix (Kapa Biosystems), 0.25 µL of each specific

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primer (at a concentration of 10 µM) and 2 µL of template DNA. Standard curves were created

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using serial 10-fold dilutions of bacterial DNA extracted from pure cultures with a bacterial

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population ranging from 2 to 9 log10 CFUs, as determined by plate counts. One strain belonging to

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each of the bacterial genera or groups targeted in this study was used to construct the standard

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curve. More specifically, DNA was extracted from the following strains: Bifidobacterium longum ACS Paragon Plus Environment

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CECT 4551, Clostridium coccoides DSMZ 935, Bacteroides fragilis DSMZ 2151, Lactobacillus

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salivarius CECT 2197, obtained from the Spanish Collection of Type Cultures (CECT) or the

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German Collection of Microorganisms and Cell Cultures (DSMZ).

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Cellular Assays. Human hepatoma HepG2 cells were maintained in a humidified incubator

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containing 5% CO2 and 95% air at 37 ºC. They were grown in Dulbecco’s Modified Eagle

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Medium/Nutrient Mixture F-12 (DMEM F-12) from Biowhitaker, supplemented with 2.5%

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Biowhitaker foetal bovine serum (FBS) and 50 mg/L of each of the following antibiotics:

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gentamicin, penicillin and streptomycin.

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To assay direct effect, cells were incubated with doses ranging from 1 to 100 µg/mL (depending of

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the assay) of HSCG, digested HSCG, fermented HSCG or residual fraction from fermented HSCG

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for 20 h. To assay for a protective effect, cells were pre-treated with the noted doses (see Table 1

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and Figures 1 and 2) of the four samples for 20 h, then the medium was removed, cells were washed

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with PBS and 400 µM t-BOOH (dissolved in the medium) was added for 2 h, after which the cell

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cultures were processed as detailed below for each assay.

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Cell viability was measured by the crystal violet assay as previously reported.28 Briefly, HepG2

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cells were seeded at low density (10000 cells per well) in 96-well plates, grown for 20 h under the

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different conditions and incubated with crystal violet (0.2% in ethanol) for 20 min. Plates were

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rinsed with water, allowed to dry, and 1% sodium dodecylsulfate added. The absorbance of each

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well was measured using a microplate reader at 570 nm.

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Cellular reactive oxygen species (ROS) were quantified by the dichlorofluorescein assay as

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previously described.15,29 Briefly, the cells were seeded in 24-well plates (200000 cells per well) in

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medium containing FBS, which was replaced with the FBS-free medium the next day. After 20 h, 5

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µM DCFH-DA was added to the wells which were incubated at 37 ºC for 30 min, after that cells

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were washed with PBS, treated with fresh FBS-free medium with the different concentrations of the

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four HSCG samples and ROS production was monitored for 120 min. For the protection assay, cells

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were seeded and left overnight before treating them with the HSCG samples for 20 h. Then DCFHACS Paragon Plus Environment

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DA was added for 30 min and cells were washed with PBS prior to the addition of 400 µM t-BOOH

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to every well but controls with further incubation for 2 h. Control cells without t-BOOH treatment

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were used as negative control. Multiwell plates were measured in a fluorescent microplate reader at

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excitation wavelength of 485 nm and emission wavelength of 528 nm. Results are expressed as

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percent of fluorescence units.

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GSH content was quantitated by a fluorometric assay as previously described.15 Briefly, HepG2

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cells were plated in 60 mm diameter plates at a concentration of 1.5 × 106 cells/plate. Cells were

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treated with the different quantities of the samples for 20 h, collected by scraping in 1.5 mL of PBS

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and centrifuged (1500 rpm, 4 ºC, 5 min), and lysed by adding 110 µL of 5% w/v trichloroacetic acid

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containing 2 mM EDTA. Protein was measured by the Bradford reagent. After centrifugation of the

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cells (7500 rpm, 4 ºC, 30 min), 50 µL of supernatant were transferred to wells in a 96-well plate.

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Then, 15 µL of 1 M NaOH were added, followed by 175 µL of 0.1 M sodium phosphate buffer (pH

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8.0) containing 5 mM EDTA. 10 µL per well of a 10 mg/mL methanolic solution of OPT were

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finally added. After 15 min at room temperature in the dark, fluorescence was measured (emission

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wavelength: 460 nm; excitation wavelength: 340 nm). The results were expressed as percent related

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to untreated cells.

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Statistical Analysis. Statistical significance of the data was tested by one-way analysis of variance

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(ANOVA), followed by the Duncan test to compare the means that showed significant variation (p

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< 0.05); all the statistical analyses were performed using Statgraphics Plus software, version 5.1.

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For the cellular assays, prior to analysis data were tested for homogeneity of variances by the test of

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Levene; for multiple comparisons, one-way ANOVA was followed by a Bonferroni test when

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variances were homogeneous or by Tamhane test when variances were not homogeneous. The level

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of significance was p < 0.05. A SPSS version 23.0 program was used.

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Results and Discussion

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Determination of Antioxidant Properties of HSCG Following Simulated Digestion and

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Fermentation in HepG2 cells.

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Evaluation of the actual bioavailability of polyphenols in food and food supplements based on data

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concerning their absorption, metabolism, tissue and organ distribution is crucial to establish their

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effects on human body.18,30,31 Drug bioavailability depends on several factors such as administration

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route, phenotype, age, gender, and food interaction,31 however studies carried out on animals or

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human subjects are necessarily complex, expensive, and lengthy. This is the reason why different in

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vitro procedures that mimic the physiochemical and biochemical conditions encountered in the

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gastrointestinal tract have been actively developed and tested, providing preliminary data on the

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potential bioavailability of different components of the food under evaluation.32-37 The importance

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of in vitro digestion combined with cellular assays to determine the antioxidant activity has been

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recently emphasized,15-20 and the HepG2 cell line is widely used to study the biotransformation and

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the chemopreventive potential of different compounds as a model system of the human liver.23,38

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We are aware that i) phase-II metabolism of the phenolic compounds produced after the simulated

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gastrointestinal digestion should be duly considered since it can limit their bioavailability and

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reduce their biological activity,39 and that ii) expression of drug-metabolizing enzymes and drug

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transporters in transformed cell lines is often low and variable. Notwithstanding that, genotyping of

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phase I and phase II enzymes and drug transporter polymorphisms in these cells confirmed HepG2

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as a suitable model for metabolic studies, also because the low levels of sulfotransferase and N-

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acetyltransferase reported in these cells are still high enough to allow metabolism.38

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To test the biocompatibility and cytoprotective properties of both the liquid (potentially

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bioaccessible) fractions from digestion (HSCG-dig) and fermentation (HSCG-ferm) treatment and

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the solid residue after fermentation (HSCG-res), together with raw HSCG for comparison, doses of

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1-20 µg/mL were considered physiological and realistic,14 but higher concentrations were also

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tested in order to ensure that no cytotoxic effect induced by the samples was observed in the cell ACS Paragon Plus Environment

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culture. Thus, crystal violet assay (Table 1) shows that doses up to 100 µg/mL of any of the four

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products did not affect HepG2 cell viability after 20 h.

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Despite a slight increase in ROS observed for HSCG-dig at 1 and 5 µg/mL, no physiologically

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relevant changes in ROS production (Figure 1A) and GSH concentration (Figure 2A) were

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observed after plain treatment of cells with all four samples, indicating no harmful alteration of the

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redox status. Thus, direct treatment with the HSCG products did not induce cellular stress or

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oxidative damage which could impair cell functionality. In order to test the cytoprotective effect of

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the products in a stressful condition, a model of oxidative stress induced by a potent pro-oxidant,

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tert-butylhydroperoxide (t-BOOH) was established.15 In agreement with this model, 400 µM t-

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BOOH evoked a condition of oxidative stress exhibited by decreased cell viability (Table 1) and

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GSH (Figure 2B), as well as overproduction of ROS (Figure 1B). Interestingly, data in Table 1

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show that pre-treatment with 1-10 µg/mL of HSCG-dig and HSCG-ferm and 5-10 µg/mL HSCG

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completely protected HepG2 cell viability from stress-induced death, indicating a clear defense of

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cell integrity by the spent coffee products against a stressful challenge. The antioxidant activity

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observed for HSCG-ferm would indicate that the gut microbiota has a strong metabolic activity

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against HSCG, releasing antioxidant compounds that could be absorbed through the colonic

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intestinal tract.

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The ROS-scavenging effect of HSCG has been recently reported.14 In the present study, Figure 1B

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shows that 1-20 µg/mL of HSCG-dig, HSCG-ferm and raw HSCG significantly reduced ROS

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overproduction evoked by t-BOOH, suggesting a quenching ability of reactive species in a cellular

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environment, which could explain the observed reduced oxidative stress and cell protection. We

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have previously reported a similar ROS reducing effect in this same cell line treated with coffee

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melanoidin15 and with a green coffee bean extract or pure chlorogenic acid.40

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Comparable to what previously reported with HSCG,14 a dose-dependent recovery of the depleted

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GSH was observed with 5-10 µg/mL of HSCG-dig and a complete rescue was confirmed with 5-10

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µg/mL HSCG, whereas the other conditions tested showed no significant recovery of the decreased

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GSH (Figure 2B). GSH is the main non-enzymatic cellular antioxidant attenuating oxidative stress

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by acting as both a reducing agent and a substrate of glutathione peroxidase. Maintaining GSH

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levels above a critical threshold is therefore a crucial issue to guarantee cell survival under

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oxidative stress conditions.

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The present GSH data agree with previous results obtained in the same cell line with other coffee

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constituents,15,40 and clearly indicates that cells exposed to HSCG and HSCG-dig showed a

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protected redox status in a situation of oxidative stress. Thus, the protective mechanism of HepG2

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cell integrity and functionality by HSCG samples can be described in terms of regulation of the

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cellular redox status, as a consequence of the scavenging of ROS by HSCG which would result in

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the recovery of GSH and reduced oxidative damage and cell death.

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Notably, in all the cellular assays performed no significant protective effect was observed for the

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HSCG-res sample, suggesting that most part of the beneficial antioxidant activity exhibited by

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HSCG is transferred to the soluble, potentially bioaccessible fraction. Although much of the

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evidence for bioactivity of polyphenols evaluated on cell lines may be of little significance in vivo,41

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HSCG-ferm containing human gut microbiota derived metabolites may be considered much more

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relevant in this regard.

241 242

Structural Transformations of HSCG Following Simulated Digestion and Fermentation.

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To gain an insight into the structural transformations that occur following simulated digestion-

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fermentation of HSCG, the ATR-FTIR spectra of HSCG and HSCG-res were recorded and are

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shown in Figure 3, together with the subtracted spectrum (HSCGS-res – HSCG). In the high

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frequency region, HSCG and HSCG-res showed similar spectral profiles, with a broad band located

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at 3300 cm-1 and a pattern of signals in the 2900-2800 cm-1 range. These features are due to

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hydroxyl groups of cellulose and hemicellulose10 and to the hydrocarbon moieties of lignins,42

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respectively. A decrease in these latter signals is observed in the subtracted spectrum, indicating ACS Paragon Plus Environment

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partial hydrolysis of lignins following the simulated digestion-fermentation, which could in part

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account for the higher antioxidant activity observed for the soluble, potentially bioaccessible

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fractions compared to HSCG-res. At lower wavenumbers, HSCG shows two absorption bands in

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the carbonyl stretching region, located at 1740 and 1705 cm-1, likely due to acetyl groups of

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hemicellulose and carboxylic acids, respectively.43 The subtracted spectrum shows a remarkable

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reduction of these signals in HSCG-res, likely due to hydrolysis and removal of hemicellulose and

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carboxylic acid constituting HSCG following the enzymatic treatment. No other significant

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differences could be observed among the two samples, either in the cellulose/hemicellulose alcohol

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C-O stretching region (bands at 1160, 1060 and 1034 cm-1)44 or in the aromatic skeleton vibrations

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(1615 ant 1515 cm-1) and C-H bending of aromatic methoxy groups (1461 and 1110 cm-1).45 The

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increase in absorption in the 1600-1500 cm-1 range in the HSCG-res spectrum can be attributed to

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the amide groups of some residual enzymes used for the simulated digestion-fermentation

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treatment.

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To gain information about the nature of the components released from HSCG following simulated

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digestion and fermentation, the soluble fractions HSCG-dig and HSCG-ferm were preliminarily

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analyzed by both HPLC and 1H NMR, but no significant differences were observed compared to

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control mixtures containing enzymes and other ingredients but no HSCG. Accordingly, to avoid

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interferences from these components, in other experiments the HSCG-dig and the HSCG-ferm

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samples were taken to pH 1 and repeatedly extracted with ethyl acetate. HPLC analysis with UV

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detection at 254 nm of the organic extractable fraction from HSCG-dig showed the presence of

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minute amounts of chromatographically defined compounds but significant quantities of organic

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polymeric material eluted as a broad peak at the end of the gradient program. The presence of

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conjugated, aromatic polymer was also well apparent from the UV-vis spectrum of the organic

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extract of HSCG-dig reported in Figure 4, featuring a broadband absorption in the range 200-600

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nm, with maxima at around 280 and 310 nm, typical of lignin moieties with hydroxycinnamic acid

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type structures;46-48 for comparison the UV-vis spectrum of the organic extractable fraction from the ACS Paragon Plus Environment

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control, simulated digestion mixture not containing HSCG is also shown at the same concentration,

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displaying no significant absorption above 300 nm. Unfortunately, all attempts to further

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characterize the main extractable components of HSCG-dig by NMR failed, likely due to the great

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chemical heterogeneity of lignin polymers.

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Very little information could be obtained on the ethyl acetate extractable fraction of HSCG-ferm:

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apparently no polymeric material was present in this case, as highlighed by both HPLC and UV-vis

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analysis, suggesting efficient metabolization of the lignin moieties by the colonic microflora;

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however, not very significant differences could be observed either in the elutoghraphic profiles or in

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the UV-vis or NMR spectra when the extractable fraction of HSCG-ferm was compared with that

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obtained form a control fermentation mixture not containing HSCG.

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Prebiotic Activity of HSCG.

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Given the nutritional composition of SCG,12 and the presence of insoluble components, these by-

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products should have an interesting activity on the gut microbiota. Since it was found that SCG

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increase the levels of Lactobacillus spp. and Bifidobacterium spp. after in vitro fermentation,12 we

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decided to analyze the effect of microbial fermentation over HSCG by determination of changes in

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microbial composition and production of SCFAs, which are known to have healthy properties such

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as immunomodulation through their attachment to the GPR43 receptor.49 Table 2 shows the changes

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in microbial composition after fermentation of HSCG, compared to those produced by a

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commercial milk beverage enriched with a probiotic strain known to produce large amount of

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SCFAs after fermentation, a positive control made of inulin (a commercial prebiotic) and a control

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sample (fermentative medium without any nutrient). HSCG showed a clear prebiotic activity since

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its fermentation increased the population of Bifidobacterium spp. and Lactobacillum spp.

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(compared with the control), which are known microbial species with healthy properties. At the

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same time, a decrease (compared with the control) was observed on Clostridium spp. and

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Bacteroides spp., which are microorganisms related with different pathologies. The same effect was

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also obtained for the milk beverage and inulin (probiotic and prebiotic controls, respectively). ACS Paragon Plus Environment

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However, the amount of Bifidobacterium spp. and Lactobacillum spp. was statistically higher (P