Your search keyword '"Sforza S"' showing total 18 results

1. Polar Lipid Profile of Nannochloropsis oculata Determined Using a Variety of Lipid Extraction Procedures.

Author

Servaes, K., Maesen, M., Prandi, B., Sforza, S., and Elst, K.

Published

2015

2. Assessment of Protein Quality and Digestibility in Plant-Based Meat Analogues.

Author

Cutroneo S, Prandi B, Pellegrini N, Sforza S, and Tedeschi T

Subjects

Child, Animals, Humans, Meat analysis, Proteins, Amino Acids metabolism, Meat Substitutes, Digestion

Abstract

In this first work, commercial steak-like ( n = 3) and cured meat ( n = 3) analogues with different legume and cereal formulations were studied and compared to their animal-based ( n = 3) counterparts. Plant-based products showed lower protein content than meat controls but a good amino acidic profile even though the sum of essential amino acids of plant-cured meats does not fulfill the requirements set by the Food and Agriculture Organization for children. A comparable release of soluble proteins and peptides in the digestates after in vitro digestion was observed in meat analogues as meat products, whereas the digestibility of proteins was lower in plant-based steaks and higher in plant-based cured meats than their counterparts. The overall protein quality and digestibility of products are related to both the use of good blending of protein sources and processes applied to produce them. An adequate substitution of meat with its analogues depends mostly on the quality of raw materials used, which should be communicated to consumers.

Published

2024

3. Label-Free Quantification by Liquid Chromatography-Tandem Mass Spectrometry of the Kunitz Inhibitor of Trypsin KTI3 in Soy Products.

Author

Prandi B, Vacca C, Sforza S, and Tedeschi T

Subjects

Animals, Humans, Trypsin, Trypsin Inhibitors, Chromatography, Liquid, Trypsin Inhibitor, Kunitz Soybean, Tandem Mass Spectrometry

Abstract

The greater awareness of consumers regarding the sustainability of food chains has shifted part of the consumption from animal protein sources to vegetable sources. Among these, of relevance both for human food use and for animal feed, is soy. However, its high protein content is unfortunately accompanied by the presence of antinutritional factors, including Kunitz's trypsin inhibitor (KTI). Now there are few analytical methods available for its direct quantification, as the inhibitory activity against trypsin is generically measured, which however can be given by many other molecules and undergo numerous interferences. Therefore, in this work, a direct label-free liquid chromatography-mass spectrometry (LC-MS) method for the identification and quantification of trypsin Kunitz inhibitor KTI3 in soybean and derivative products has been developed. The method is based on the identification and quantification of a marker peptide, specific for the protein of interest. Quantification is achieved with an external calibration curve in the matrix, and the limit of detection and the limit of quantification of the method are 0.75 and 2.51 μg/g, respectively. The results of the LC-MS method were also compared with trypsin inhibition measured spectrophotometrically, highlighting the complementarity of these two different pieces of information.

Published

2023

4. Technological Quality and Nutritional Value of Two Durum Wheat Varieties Depend on Both Genetic and Environmental Factors.

Author

Graziano S, Marando S, Prandi B, Boukid F, Marmiroli N, Francia E, Pecchioni N, Sforza S, Visioli G, and Gullì M

Subjects

Amino Acids chemistry, Environment, Italy, Nutritive Value, Phenols chemistry, Quality Control, Triticum classification, Triticum growth & development, Triticum chemistry, Triticum genetics

Abstract

Durum wheat ( Triticum turgidum L. subsp. durum (Desf.) Husn) is a major food source in Mediterranean countries since it is utilized for the production of pasta, leavened and unleavened breads, couscous, and other traditional foods. The technological and nutritional properties of durum wheat semolina depend mainly on the type of gluten proteins and on their amount, which is a genotype- and environment-dependent trait. Gluten proteins are also responsible for celiac disease (CD), an autoimmune enteropathy with a prevalence of about 0.7-2% in the human population. At this purpose, two Italian durum wheat cultivars, Saragolla and Cappelli, currently used for monovarietal pasta, were chosen to compare (i) the reserve and embryo proteome, (ii) the free and bound phenolics, antioxidant activity, and amino acid composition, and (iii) the content of immunogenic peptides produced after a simulated gastrointestinal digestion. The results obtained from 2 years of field cultivation on average showed a higher amount of gluten proteins, amino acids, and immunogenic peptides in Cappelli. Saragolla showed a higher abundance in bound phenolics, antioxidant enzymes, and stress response proteins in line with its higher antioxidant activity. However, the impact of the year of cultivation, largely depending on varying rainfall regimes through the wheat growth cycle, was significant for most of the parameters investigated. Differences in technological and nutritional characteristics observed between the two cultivars are discussed in relation to the influence of genetic and environmental factors.

Published

2019

5. Effectiveness of Germination on Protein Hydrolysis as a Way To Reduce Adverse Reactions to Wheat.

Author

Boukid F, Prandi B, Buhler S, and Sforza S

Subjects

Electrophoresis, Polyacrylamide Gel, Glutens chemistry, Glutens immunology, Hydrolysis, Plant Proteins adverse effects, Plant Proteins immunology, Seeds chemistry, Seeds immunology, Spectrometry, Mass, Electrospray Ionization, Triticum adverse effects, Triticum growth & development, Triticum immunology, Celiac Disease immunology, Germination, Plant Proteins chemistry, Seeds growth & development, Triticum chemistry

Abstract

In this work, the aim is to study the effectiveness of germination on wheat protein degradation, with a specific focus on proteins involved in adverse reactions to wheat. The effects of 8 days of germination at 25 °C on the chemical composition and the protein profile were determined. Germination did not have a significant effect on starch, protein, lipid, and ash contents. General protein profile, as indicated by SDS-PAGE analysis, revealed that germination induced a relevant degradation in protein fraction. After in vitro gastrointestinal digestion, gluten peptides involved in celiac disease (CD) were identified and quantified using UPLC/ESI-MS technique. Also, CM3 protein, involved in baker's asthma and intestinal inflammation, was quantified by measuring a marker peptide. Statistical analysis underlined that germination and genotype had significant impact on the amount of both components. Regarding gluten peptides related to CD, germination enabled an average reduction of 47% in peptides eliciting adaptive immune response and 46% in peptides eliciting innate immune response. CM3 protein showed also a high average reduction (56%). Thus, this study suggests that germination might be a good bioalternative to provide a low "impact" raw ingredient for special wheat-based foodstuffs.

Published

2017

6. Understanding the Effects of Genotype, Growing Year, and Breeding on Tunisian Durum Wheat Allergenicity. 1. The Baker's Asthma Case.

Author

Boukid F, Prandi B, Sforza S, Sayar R, Seo YW, Mejri M, and Yacoubi I

Subjects

Breeding, Genotype, Humans, Plant Proteins genetics, Plant Proteins immunology, Time Factors, Triticum chemistry, Triticum growth & development, Triticum immunology, Tunisia, Asthma immunology, Plant Proteins analysis, Triticum genetics, Wheat Hypersensitivity immunology

Abstract

Baker's asthma is a serious airway disease triggered by wheat protein CM3 α-amylase/trypsin inhibitor. The purpose of the present study was to investigate the impact of genotype and crop year on allergen CM3 α-amylase/trypsin inhibitor associated with baker's asthma. A historical series of Tunisian durum wheat (100 accessions), derived from three crop years, was used to compare the amount of CM3 from landraces to advanced cultivars. CM3 protein quantification was assessed after an enzymatic cleavage of the soluble protein extracts on a UPLC/ESI-MS system, using a marker peptide for its quantification. Combined data analysis of variance revealed an important effect of genotype, crop year, and their interaction. The CM3 allergenic proteins were found to significantly vary among studied genotypes, as confirmed by genetic variability, coefficient of variance, heritability, and genetic advance.

Published

2017

7. Understanding the Effects of Genotype, Growing Year, and Breeding on Tunisian Durum Wheat Allergenicity. 2. The Celiac Disease Case.

Author

Boukid F, Prandi B, Sforza S, Sayar R, Seo YW, Mejri M, and Yacoubi I

Subjects

Breeding, Genotype, Humans, Plant Proteins genetics, Plant Proteins immunology, Seasons, Time Factors, Triticum growth & development, Triticum immunology, Tunisia, Celiac Disease immunology, Plant Proteins analysis, Triticum chemistry, Triticum genetics

Abstract

The aim of this study was to compare immunogenic and toxic gluten peptides related to celiac disease (CD). 100 accessions of genotypes selected during the 20th century in Tunisia were in vitro digested and then analyzed by UPLC/ESI-MS technique using an isotopically labeled internal standard. The first MANOVA confirmed a high variability in the content of immunogenic and toxic peptides reflecting high genetic diversity in the germplasm released during the past century in Tunisia, consistently with PCA and clustering analysis results. Our finding showed also important variability in CD epitopes due to growing season's climate scenarios. Moreover, the second MANOVA revealed significant differences between abandoned and modern cultivars' CD-related peptide amounts. Although we could not conclude that there was an augment of allergens in newly selected durum wheat lines compared to abandoned ones, we demonstrated that modern genotype peptides were less sensitive to climate variation, which is a useful indicator for wheat breeders.

Published

2017

8. O-Methylisourea Can React with the α-Amino Group of Lysine: Implications for the Analysis of Reactive Lysine.

Author

Hulshof TG, Rutherfurd SM, Sforza S, Bikker P, van der Poel AF, and Hendriks WH

Subjects

Animal Feed analysis, Animals, Digestion, Homoarginine chemistry, Homoarginine metabolism, Lysine metabolism, Methylurea Compounds metabolism, Chickens metabolism, Lysine chemistry, Methylurea Compounds chemistry, Swine metabolism

Abstract

The specificity of O-methylisourea (OMIU) to bind to the ε-amino group of Lys, an important supposition for the OMIU-reactive Lys analysis of foods, feeds, ingredients, and digesta, was investigated. Crystalline l-Lys incubated under standard conditions with OMIU resulted in low homoarginine recoveries. The reaction of OMIU with the α-amino group of Lys was confirmed by MS analysis, with double derivatized Lys being identified. None of the changes in reaction conditions (OMIU pH, OMIU to Lys ratio, and reaction time) with crystalline l-Lys resulted in 100% recovery of homoarginine. The average free Lys content in ileal digesta of growing pigs and broilers was found to be 13% of total Lys, which could result in a significant underestimation of the reactive Lys content. The reaction of OMIU with α-amino groups may necessitate analysis of free Lys to accurately quantify reactive lysine in samples containing a large proportion of Lys with a free α-amino group.

Published

2017

9. Purification and Characterization of Anacardium occidentale (Cashew) Allergens Ana o 1, Ana o 2, and Ana o 3.

Author

Reitsma M, Bastiaan-Net S, Sforza S, van der Valk JP, van Gerth van Wijk R, Savelkoul HF, de Jong NW, and Wichers HJ

Subjects

Amino Acid Sequence, Anacardium genetics, Anacardium immunology, Antigens, Plant genetics, Antigens, Plant immunology, Epitope Mapping, Molecular Sequence Data, Plant Proteins genetics, Anacardium chemistry, Antigens, Plant chemistry, Antigens, Plant isolation & purification, Plant Proteins chemistry, Plant Proteins immunology, Plant Proteins isolation & purification

Abstract

In this study a fast and simple purification procedure for the three known allergens from cashew (7S globulin Ana o 1, 11S globulin Ana o 2, and 2S albumin Ana o 3) is described. The purified allergens are characterized by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE), Western blot, glycoprotein stain, and protein identification. The purified proteins still bind IgE, and this IgE binding varied between different pools of patient serum. Ana o 1 was found to be a glycoprotein. Ana o 3 has been studied more in detail to identify both the small and large subunits, both displaying microheterogeneity, and epitope mapping of Ana o 3 has been performed.

Published

2016

10. Effect of Extraction Conditions on the Saccharide (Neutral and Acidic) Composition of the Crude Pectic Extract from Various Agro-Industrial Residues.

Author

Babbar N, Roy SV, Wijnants M, Dejonghe W, Caligiani A, Sforza S, and Elst K

Subjects

Agrochemicals chemistry, Agrochemicals isolation & purification, Molecular Structure, Pectins chemistry, Chemical Fractionation methods, Crops, Agricultural chemistry, Pectins isolation & purification

Abstract

The influence of different extraction methodologies was assessed on the composition of both neutral (arabinose, rhamnose, galactose) and acidic (galacturonic acid) pectic polysaccharides obtained from four agro-industrial residues, namely, berry pomace (BP), onion hulls (OH), pressed pumpkin (PP), and sugar beet pulp (SBP). For acidic pectic polysaccharides, the extraction efficiency was obtained as BP (nitric acid-assisted extraction, 2 h, 62.9%), PP (enzymatic-assisted extraction, 12 h, 75.0%), SBP (enzymatic-assisted extraction, 48 h, 89.8%; and nitric acid-assisted extraction, 4 h, 76.5%), and OH (sodium hexametaphosphate-assisted extraction, 0.5 h, 100%; and ammonium oxalate-assisted extraction, 0.5 h, 100%). For neutral pectic polysaccharides, the following results were achieved: BP (enzymatic-assisted extraction, 24 h, 85.9%), PP (nitric acid-assisted extraction, 6 h, 82.2%), and SBP (enzymatic assisted extraction, 48 h, 97.5%; and nitric acid-assisted extraction, 4 h, 83.2%). On the basis of the high recovery of pectic sugars, SBP and OH are interesting candidates for the further purification of pectin and production of pectin-derived products.

Published

2016

11. Determination of the influence of substrate concentration on enzyme selectivity using whey protein Isolate and Bacillus licheniformis protease.

Author

Butré CI, Sforza S, Gruppen H, and Wierenga PA

Subjects

Bacillus chemistry, Bacterial Proteins metabolism, Biocatalysis, Hydrolysis, Kinetics, Milk Proteins metabolism, Peptide Hydrolases metabolism, Whey Proteins, Bacillus enzymology, Bacterial Proteins chemistry, Milk Proteins chemistry, Peptide Hydrolases chemistry

Abstract

Increasing substrate concentration during enzymatic protein hydrolysis results in a decrease in hydrolysis rate. To test if changes in the mechanism of hydrolysis also occur, the enzyme selectivity was determined. The selectivity is defined quantitatively as the relative rate of hydrolysis of each cleavage site in the protein. It was determined from the identification and quantification of the peptides present in the hydrolysates. Solutions of 0.1-10% (w/v) whey protein isolate (WPI) were hydrolyzed by Bacillus licheniformis protease at constant enzyme-to-substrate ratio. The cleavage sites were divided into five groups, from very high (>10%) to very low selectivity (<0.1%). The selectivity toward cleavage sites after Glu 62 and 134 was 2 times higher at 10% (w/v) WPI than at the lower protein concentrations. This finding shows that both the rate of hydrolysis and the enzyme selectivity were influenced by the substrate concentration.

Published

2014

12. Simple and validated quantitative ¹H NMR method for the determination of methylation, acetylation, and feruloylation degree of pectin.

Author

Müller-Maatsch J, Caligiani A, Tedeschi T, Elst K, and Sforza S

Subjects

Acetic Acid analysis, Acetylation, Coumaric Acids analysis, Dopamine analogs & derivatives, Esterification, Hydrolysis, Methanol analysis, Methylation, Molecular Structure, Reproducibility of Results, Magnetic Resonance Spectroscopy methods, Pectins chemistry

Abstract

The knowledge of pectin esterification degree is of primary importance to predict gelling and other properties of pectin from different sources. This paper reports the development of a simple and rapid (1)H NMR-based method for the simultaneous quantitative determination of methylation, acetylation, and feruloylation degree of pectin isolated from various food sources. Pectin esters are hydrolyzed in NaOH/D2O, and the obtained methanol, acetic acid, and ferulic acid are directly measured by (1)H NMR. High accuracy, repeatability, and reproducibility of the method were obtained, and the analysis time is reduced as compared to conventional chromatography- or titration-based methods.

Published

2014

13. Patterning of peptide nucleic acids using reactive microcontact printing.

Author

Calabretta A, Wasserberg D, Posthuma-Trumpie GA, Subramaniam V, van Amerongen A, Corradini R, Tedeschi T, Sforza S, Reinhoudt DN, Marchelli R, Huskens J, and Jonkheijm P

Subjects

Microscopy, Fluorescence, Peptide Nucleic Acids chemistry

Abstract

PNAs (peptide nucleic acids) have been immobilized onto surfaces in a fast, accurate way by employing reactive microcontact printing. Surfaces have been first modified with aldehyde groups to react with the amino end of the synthesized PNAs. When patterning fluorescein-labeled PNAs by reactive microcontact printing using oxygen-oxidized polydimethylsiloxane stamps, homogeneous arrays were fabricated and characterized using optical methods. PNA-patterned surfaces were hybridized with complementary and mismatched dye-labeled oligonucleotides to test their ability to recognize DNA sequences. The stability and selectivity of the PNA-DNA duplexes on surfaces have been verified by fluorescence microscopy, and the melting curves have been recorded. Finally, the technique has been applied to the fabrication of chips by spotting a PNA microarray onto a flat PDMS stamp and reproducing the same features onto many slides. The chips were finally applied to single nucleotide polymorphism detection on oligonucleotides.

Published

2011

14. New uracil dimers showing erythroid differentiation inducing activities.

Author

Accetta A, Corradini R, Sforza S, Tedeschi T, Brognara E, Borgatti M, Gambari R, and Marchelli R

Subjects

Alkylation, Cell Line, Tumor, Cell Proliferation drug effects, Dimerization, Drug Design, Drug Screening Assays, Antitumor, Humans, Models, Molecular, Molecular Structure, Structure-Activity Relationship, Uracil chemical synthesis, Cell Differentiation drug effects, Erythroid Cells cytology, Erythroid Cells drug effects, Uracil chemistry, Uracil pharmacology

Abstract

The synthesis of C5 linked uracil dimers was carried out according to a model developed in order to bind adenine in DNA. N1-Alkylated uracil derivatives were synthesized from isoorotic acid (uracil-5-carboxylic acid) or thymine. The carboxylic acid derivatives were condensed with diamines in order to produce dimeric compounds or with monoamines in order to obtain reference monomeric compounds. Some of the derivatives, in particular the uracil dimers, showed antiproliferative and erythroid differentiation induction properties towards human chronic myelogenous leukemia K562 cells, thus indicating that these compounds could represent a new class of drugs useful for the development of antitumor therapy based on the ability to induce terminal differentiation.

Published

2009

15. Isolation and identification of two lipid transfer proteins in pomegranate (Punica granatum).

Author

Zoccatelli G, Dalla Pellegrina C, Consolini M, Fusi M, Sforza S, Aquino G, Dossena A, Chignola R, Peruffo A, Olivieri M, and Rizzi C

Subjects

Antigens, Plant chemistry, Beverages analysis, Carrier Proteins chemistry, Electrophoresis, Polyacrylamide Gel, Fruit chemistry, Immunoblotting, Plant Proteins chemistry, Spectrometry, Mass, Electrospray Ionization, Antigens, Plant analysis, Antigens, Plant isolation & purification, Carrier Proteins analysis, Carrier Proteins isolation & purification, Lythraceae chemistry, Plant Proteins analysis, Plant Proteins isolation & purification

Abstract

Lipid transfer proteins (LTPs) are a family of low molecular mass (7-9 kDa) polypeptides, the members of which share 35-95% sequence homology. These proteins are widely distributed throughout the plant kingdom and are receiving attention for their biochemical characteristics and biological activity. LTPs are indeed studied in different research fields varying from allergy to food technology, and numerous molecules belonging to this class are progressively being identified and investigated. Proteins from pomegranate juice were fractioned by cation exchange chromatography and analyzed by SDS-PAGE. Two proteins were identified as putative LTPs on the basis of their molecular weights and their electrophoretic behaviors under reducing and nonreducing conditions. Finally, proteins were purified and characterized by mass spectrometry. This analysis confirmed that the two polypeptides are LTPs on the basis of an amino acid sequence common to LTPs from other plant sources and cysteine content. The two proteins, named LTP1a and LTP1b, showed similar molecular masses but different immunological profiles when immunodetected with rabbit antibodies specific for Pru p 3 and human IgE from a patient suffering from pomegranate allergy. The demonstration of the existence of two immunologically unrelated LTPs in pomegranate confirms the variability and the complexity of the plant LTP family. This should be taken into account when the role of these proteins as elicitors of allergies to fruits is investigated and could help to explain the contradictory literature data on pomegranate allergy.

Published

2007

16. Identification of PCR-amplified genetically modified organisms (GMOs) DNA by peptide nucleic acid (PNA) probes in anion-exchange chromatographic analysis.

Author

Rossi S, Lesignoli F, Germini A, Faccini A, Sforza S, Corradini R, and Marchelli R

Subjects

Anions, Chromatography, High Pressure Liquid, Nucleic Acid Probes, Glycine max genetics, Zea mays genetics, Chromatography, Ion Exchange, DNA analysis, Plants, Genetically Modified genetics, Polymerase Chain Reaction

Abstract

PCR products obtained by selective amplification of transgenic DNA derived from food samples containing Roundup Ready soybean or Bt-176 maize have been analyzed by anion-exchange HPLC. Peptide nucleic acids (PNAs), oligonucleotide analogues known to bind to complementary single-stranded DNA with high affinity and specificity, have been used as specific probes in order to assess the identity of the peaks observed. Two different protocols were adopted in order to obtain single-stranded DNA: amplification with an excess of one primer or digestion of one DNA strand. The single-stranded DNA was mixed with the PNA probe, and the presence of a specific sequence was revealed through detection of the corresponding PNA:DNA peak with significantly different retention time. Advantages and limits of this approach are discussed. The method was tested with reference materials and subsequently applied to commercial samples.

Published

2007

17. Effect of extended aging of parma dry-cured ham on the content of oligopeptides and free amino acids.

Author

Sforza S, Galaverna G, Schivazappa C, Marchelli R, Dossena A, and Virgili R

Subjects

Animals, Chromatography, High Pressure Liquid, Food Preservation methods, Spectrometry, Mass, Electrospray Ionization, Swine, Taste, Time Factors, Amino Acids analysis, Food Handling methods, Meat analysis, Oligopeptides analysis

Abstract

The effect of the dry-curing processing time on the release of oligopeptides and amino acids was evaluated with 158 Parma hams subdivided into three groups: (1) traditional processing (450 days); (2) extended processing (570 days); and (3) extended aging (690 days). Most of the oligopeptides and free amino acids detected increased up to the last deadline (690 days); a sharp increase of peptides below 400 Da was the main change in most aged hams. In particular, gamma-glutamyl dipeptides showed a remarkable increase during ham extended aging, acting like permanent taste-active compounds, being unsuitable for further enzymatic breakdown. The pH of fresh hams showed negative relationships (P < 0.001) with most peptides. With regard to free amino acids, the pattern was modified by different processing lengths, together with their taste categories, so that the amino acids having monosodium glutamate-like and bitter tastes were enhanced in more aged hams.

Published

2006

18. Extraction, semi-quantification, and fast on-line identification of oligopeptides in Grana Padano cheese by HPLC-MS.

Author

Sforza S, Ferroni L, Galaverna G, Dossena A, and Marchelli R

Subjects

Molecular Weight, Time Factors, Cheese analysis, Chromatography, High Pressure Liquid methods, Oligopeptides analysis, Spectrometry, Mass, Electrospray Ionization

Abstract

Sixteen samples of Grana Padano cheese aged from 2 to 33 months were analyzed by HPLC-MS. The extraction process involved the use of diluted HCl, thus avoiding a strong deproteinizing agent (TCA), and allowing to maintain in solution also very lipophilic peptides. The molecular mass of the most abundant peptides were determined by electrospray ionization (ESI) mass spectrometry. A new method was developed based on the small fragmentation peaks arising from in-source fragmentation and from software analysis of the known casein sequences, which in many cases allowed the direct on-line identification of the oligopeptide sequences. Several new peptides never previously reported were identified, some of which containing bioactive sequences, consistently with what was described in the literature. Semiquantification of peptides at the different stages of aging was also performed by using a suitable internal standard, providing new insights into the evolution of the oligopeptide fraction during aging.

Published

2003