The influence of surface characteristics on adhesion to enamel and dentine

Adebayo, Olabisi

January 2009

This body of research investigated the bonding efficiency of self-etching primer adhesives to enamel and dentine with various surface characteristics. A series of preliminary experiments was carried out to determine the effect of operator experience, dentine tubule orientation, bond strength test method and resin composite material used on bond strengths. The results of the preliminary tests concluded that it is essential to develop skills in material handling and the test methods used; 2-step self-etching primer adhesives exhibit higher but more variable microshear bond strengths (µSBS) than ‘all-in-one’ adhesives on dentine at different depths and tubule orientations; fracture toughness and bond strength test results suggest that the fracture toughness of a resin composite may not be of significant influence on microtensile and µSBS tests outcomes for nano-filled hybrid materials. / An investigation of the bonding ability of self-etching primer adhesives under various tooth preparation conditions was carried out. Enamel and dentine specimens were prepared from human teeth and finished with various rotary cutting instruments and the erbium, chromium:yttrium, scandium, gallium, garnet laser. Specimens were bonded with two 2-step self-etching primer adhesives and two ‘all-in-one’ adhesives with a resin composite. The results showed that one of the 2-step adhesives exhibited higher but more variable µSBS than the ‘all-in-one’ adhesives and a silorane-based self-etching primer adhesive system to enamel and dentine. / The relationship between enamel microhardness and µSBS was evaluated. Enamel specimens were prepared and finished with one half of the surface tested for hardness using the Vickers test. The other half of the enamel surface was bonded using either a 2-step self-etching primer adhesive or an ‘all-in-one’ adhesive and a hybrid resin composite. Mean Vickers hardness numbers and µSBS for each enamel surface were calculated. Analysis using Pearson’s parametric test for regression analysis evaluated the correlation between Vickers hardness and µSBS. The results revealed a weak negative insignificant correlation between VHN and µSBS for the 2-step adhesive and no correlation for the ‘all-in-one’ adhesive. / The effect of conditioning and casein phosphopeptide-amorphous calcium phosphate (CPP-ACP) on bonding to bleached and unbleached enamel was investigated. Four groups of enamel specimens: untreated control; bleaching with 16% carbamide peroxide gel for 90 min daily x 14 days; treated with CPP-ACP paste (Tooth Mousse, GC Corp., Japan) for 60 min daily x 7 days and bleached and CPP-ACP-treated were used. The specimens were divided into a further two groups and bonded with a total-etch adhesive or a 2-step self-etching primer adhesive. Specimens bonded with the self-etching primer adhesive were sub-divided into four conditioning subgroups before bonding: no conditioning; 30 – 40% phosphoric; 15% EDTA; 20% polyacrylic acid. Specimens were tested in shear mode until failure and analysed by 2-way ANOVA, one-way ANOVA and Tukey’s post-hoc test. The µSBS of the total-etch adhesive was not affected by enamel treatment. Bleaching reduced the µSBS of the self-etching primer adhesive but preconditioning with phosphoric acid and polyacrylic acid improved bond strengths after CPP-ACP application. Bond failure analysis revealed a predominance of adhesive failures after bleaching, but prior conditioning reduced the proportion of adhesive failures. Scanning electron microscopy (SEM) revealed that the interfacial morphology produced by the 2-step self-etching primer adhesive was independent of enamel treatment except after bleaching. Phosphoric acid etching was not inhibited by CPP-ACP treatment. Resin tag formation was observed with prior phosphoric acid and polyacrylic acid conditioning. / The effect of conditioning and CPP-ACP application on dentine bonding was also investigated. Dentine specimens with and without the smear layer were prepared and divided into a further two groups, CPP-ACP paste applied to one group for 60 min daily x 7 days and the other group was untreated. The two groups were divided into three subgroups for conditioning: no conditioning; 30 - 40% phosphoric acid; 20% polyacrylic acid. The dentine was bonded using a 2-step self-etching primer adhesive and an ‘all-in-one’ adhesive, and tested as previously described. Statistical analysis was carried out using one-way ANOVA and Tukey’s post-hoc test at α = 0.05. The results showed that the µSBS of both adhesives were not significantly affected on smear-covered dentine but was affected on smearless dentine. Conditioning did not improve bond strengths. Bond failure analysis showed more adhesive failures for the ‘all-in-one’ adhesive, particularly on smearless dentine and with prior polyacrylic acid conditioning. SEM revealed a similar morphology of the bonded interface for the 2-step self-etching primer adhesive regardless of conditioning; and areas of bond failures for the ‘all-in-one’ adhesive. / The 2-step self-etching primer adhesives exhibited higher bond strength and more regular bond integrity than the ‘all-in-one’ adhesives, as shown on the SEM observations. However, the ‘all-in-one’ adhesives exhibited less variability in bond strengths to tooth surface characteristics.

Studies of UHT-plant fouling by fresh, recombined and reconstituted whole milk : a thesis presented in partial fulfilment of the requirements for the degree of Doctor of Philosophy in Food Engineering

Srichantra, Arunee

January 2008

The objective of this study was to investigate the effects of preheat treatments on fouling by fresh whole milk (FWM), recombined whole milk (RCB) and reconstituted whole milk (Recon) in the high-temperature heater of indirect UHT plants. Various preheat treatments prior to evaporation during milk powder manufacture were applied to skim milk powder (SMP, 75 °C 2 s, 85 °C, 155 s and 95 °C, 155 s) and whole milk powder (WMP, 95 °C, 33 s). These preheat treatments were so-called “evaporator preheat treatments”. Skim milk powder (SMP) and whole milk powder (WMP) were derived from the same original batch of pasteurised FWM to remove the effects of the variation in milk composition between different milk batches. These SMPs were recombined with anhydrous milk fat and water to prepare RCB, and WMPs were reconstituted with water to prepare Recon. Then, (homogenized) FWM, RCB and Recon were subjected to various preheat treatments (75 °C, 11 s, 85 °C, 147 s and 95 °C, 147 s) prior to UHT processing. These preheat treatments were so-called “UHT preheat treatments”. Temperature difference (hot water inlet temperature – milk outlet temperature) was taken as a measure of the extent of fouling in the high-temperature heater. The slope of the linear regression of temperature difference versus time (for two hours of UHT processing) was taken as fouling rate (°C/h). Increasing both evaporator and UHT preheat treatments resulted in increasing fouling rate and total deposit weight for all three whole milk types for several milk batches. In the case of FWM, there was no reduction in fouling rate with increasing UHT preheat treatment whether FWM was homogenized then preheated, preheated then homogenized or not homogenized at all. These findings, which are wholly consistent and well replicated, are in apparent conflict with the results of most previous comparable studies. Possible reasons for this are explained. Further investigations of the effects of homogenization relating to the role of whey protein on the surface of the fat globules showed that whey protein associated with the membrane covering the surface of fat globules for homogenized then preheated FWM, RCB and Recon and that association increased with increasing heating process stage. The increasing association of whey protein with the milk fat globules membrane with increasing severity of heating process stage became faster when preheat treatment was more severe: the association of whey protein plateaued on intermediate temperature heating when the milks were preheated at 75°C, 11 s and on preheating when the milks were preheated at 95°C, 147 s. In the case of FWM, the thickness of the membrane covering the surface of fat globules for homogenized then preheated FWM, which increased with the severity of heating process stage, was greater than the thickness of the membrane in preheated then homogenized FWM. Preheating then homogenization resulted in the greater interfacial spreading of small molecules on the surface of fat globules, i.e. whey protein or small molecules from the disintegration of casein micelles during preheating. Possible basic mechanisms for UHT fouling in the high-temperature heater include: the reduction in the solubility of calcium phosphate and the deposition of protein as fat-bound protein and non-fat-bound protein. When non-fat-bound protein in milk plasma deposited, it could be a carrier for the deposition of mineral, such as, the precipitate of calcium phosphate in the casein micelles or the deposition of complexes between whey protein and casein micelles.

milk powder manufacture

evaporator pre-heat treatments

UHT processing

casein micelles

milk protein

NMR investigation on molecular mobility of poly(ethylene glycol / oxide) and dendrimer probes in casein dispersions and gels

Salami, Souad

21 February 2013

The aim of this study was to investigate the impact of the casein microstructure on the molecular diffusion of probes with different sizes and deformabilities. The mobility of molecular flexible ('PEG') and rigid (dendrimer) probes of various sizes was studied in suspensions and gels of NPC and SC at various protein concentrations. Measurements were carried out by NMR, which makes it possible to probe translational mobilities over a distance of 1.5 microns, as well as local mobilities at the molecular scale (several nanometers) through the relaxation times, T2. A coherent model was used and the same mechanism was proposed to describe the diffusion of small probes in both casein dispersions. It is the combination of different factors that should be considered: the ratio of the probe size to the distance between the obstructing particles or the entanglement points, as well as the flexibility of the probe. The rotational diffusion of PEG and dendrimer probes was less hindered than translational diffusion in both casein systems. Different relaxation behaviors were observed between the two casein systems and retardation in T2 relaxation times was highlighted in rennet and acid casein gels. These results are probably related to the local mobility of the matrix. The overall results of this project led to a better understanding of probe mobility in casein systems and made it possible to propose a new model that challenges the previous one proposed by Le Feunteun et al. to describe the diffusion of probes in casein systems.

[CHIM:OTHE] Chemical Sciences/Other

[CHIM:OTHE] Chimie/Autre

Nmr

Diffusion

Relaxation

Poly(ethylene glycol/oxide)

dendrimer

Casein micelle

Sodium caseinate

Rennet coagulation

Acid coagulation

Downstream purification and analysis of the recombinant human myelin basic protein produced in the milk of transgenic cows : a thesis presented in partial fulfillment of the requirements for the degree of Doctor of Philosophy in Chemistry, Massey University (Palmerston North) New Zealand. EMBARGOED till 28 July 2011

Al-Ghobashy, Medhat Ahmed Abdel-Hamid

Unknown Date

Downstream purification and analysis of a model biopharmaceutical protein (recombinant human myelin basic protein) is described. The recombinant protein was expressed in the milk of transgenic cows and was found exclusively associated with the casein micellar phase. Binding of milk calcium to the active sites of a cation exchanger resin was used beneficially in this study in order to gently disrupt the casein micelles and liberate the recombinant protein. This approach was found superior to the conventional micelle disruption procedures with respect to product recovery, resin fouling due to milk components and column hydrodynamic properties. Further purification was carried out using Ni2+ affinity chromatography and resulted in purity more than 90% and a total recovery of 78%. A capillary electrophoresis total protein assay employing large volume sample stacking and a microsphere-based, sandwich-type immunoassay were developed and validated. Both methods were successfully integrated with the downstream purification protocol in order to evaluate various quality attributes of the recombinant protein. A onestep capillary isoelectric focusing protocol was developed in order to monitor the recombinant protein in milk samples. The results showed extra protein bands in the transgenic milk that had isoelectric points significantly lower than the theoretically calculated one which indicated that the protein had been modified during expression. The association between the recombinant protein and bovine milk caseins was explored at the molecular level using the surface plasmon resonance technique. Results showed a calciummediated interaction between the recombinant protein and the phosphorylated caseins. This selective interaction was not noted between the human myelin basic protein and milk caseins which indicated mammary gland-related posttranslational modifications, most likely phosphorylation. The co-expression of the recombinant protein and caseins in the mammary gland, along with the ability of the recombinant protein to form calcium bridges with caseins explained its association with the casein micellar phase in the transgenic milk. Despite this and owing to the low expression levels of the recombinant protein in milk, light scattering investigations using diffusing wave spectroscopy showed no significant differences between the transgenic and the non-transgenic milk samples with respect to the average micelle size and the micelle surface charges.

myelin basic protein

transgenic cows

genetic recombination

casein

milk proteins analysis

Studies of UHT-plant fouling by fresh, recombined and reconstituted whole milk : a thesis presented in partial fulfilment of the requirements for the degree of Doctor of Philosophy in Food Engineering

Srichantra, Arunee

January 2008

The objective of this study was to investigate the effects of preheat treatments on fouling by fresh whole milk (FWM), recombined whole milk (RCB) and reconstituted whole milk (Recon) in the high-temperature heater of indirect UHT plants. Various preheat treatments prior to evaporation during milk powder manufacture were applied to skim milk powder (SMP, 75 °C 2 s, 85 °C, 155 s and 95 °C, 155 s) and whole milk powder (WMP, 95 °C, 33 s). These preheat treatments were so-called “evaporator preheat treatments”. Skim milk powder (SMP) and whole milk powder (WMP) were derived from the same original batch of pasteurised FWM to remove the effects of the variation in milk composition between different milk batches. These SMPs were recombined with anhydrous milk fat and water to prepare RCB, and WMPs were reconstituted with water to prepare Recon. Then, (homogenized) FWM, RCB and Recon were subjected to various preheat treatments (75 °C, 11 s, 85 °C, 147 s and 95 °C, 147 s) prior to UHT processing. These preheat treatments were so-called “UHT preheat treatments”. Temperature difference (hot water inlet temperature – milk outlet temperature) was taken as a measure of the extent of fouling in the high-temperature heater. The slope of the linear regression of temperature difference versus time (for two hours of UHT processing) was taken as fouling rate (°C/h). Increasing both evaporator and UHT preheat treatments resulted in increasing fouling rate and total deposit weight for all three whole milk types for several milk batches. In the case of FWM, there was no reduction in fouling rate with increasing UHT preheat treatment whether FWM was homogenized then preheated, preheated then homogenized or not homogenized at all. These findings, which are wholly consistent and well replicated, are in apparent conflict with the results of most previous comparable studies. Possible reasons for this are explained. Further investigations of the effects of homogenization relating to the role of whey protein on the surface of the fat globules showed that whey protein associated with the membrane covering the surface of fat globules for homogenized then preheated FWM, RCB and Recon and that association increased with increasing heating process stage. The increasing association of whey protein with the milk fat globules membrane with increasing severity of heating process stage became faster when preheat treatment was more severe: the association of whey protein plateaued on intermediate temperature heating when the milks were preheated at 75°C, 11 s and on preheating when the milks were preheated at 95°C, 147 s. In the case of FWM, the thickness of the membrane covering the surface of fat globules for homogenized then preheated FWM, which increased with the severity of heating process stage, was greater than the thickness of the membrane in preheated then homogenized FWM. Preheating then homogenization resulted in the greater interfacial spreading of small molecules on the surface of fat globules, i.e. whey protein or small molecules from the disintegration of casein micelles during preheating. Possible basic mechanisms for UHT fouling in the high-temperature heater include: the reduction in the solubility of calcium phosphate and the deposition of protein as fat-bound protein and non-fat-bound protein. When non-fat-bound protein in milk plasma deposited, it could be a carrier for the deposition of mineral, such as, the precipitate of calcium phosphate in the casein micelles or the deposition of complexes between whey protein and casein micelles.

milk powder manufacture

evaporator pre-heat treatments

UHT processing

casein micelles

milk protein

Molecular mechanisms of nuclear factor-erythroid-2 related factor 2 (Nrf2) regulation phosphorylation by casein kinase 2 (CK2) and interaction with proto-oncogene N-Myc in neuroblastoma cells /

Apopa, Patrick L.,

January 2007

Thesis (Ph. D.)--West Virginia University, 2007. / Title from document title page. Document formatted into pages; contains vi, 130 p. : ill. (some col.). Includes abstract. Includes bibliographical references.

Texturization of dairy protein systems with whey protein isolate aggregates / Texturer des matrices laitières avec des agrégats de protéines laitières

Kharlamova, Anna

15 November 2017

Dans le lait on peut distinguer les protéines sériques et les caséines. Les protéines sériques sont des protéines globulaires qui se trouvent dans le sérum du lait et elles sont connues pour leurs propriétés fonctionnelles exceptionnelles. Quand une solution de protéines sériques est chauffée, elles perdent leur structure native et peuvent s'agréger. Elles forment des agrégats de différentes formes, tailles et densités : des cylindres, des agrégats fractals, des microgels et des agrégats fibrillaires. De l'autre côté, les caséines sont organisées dans des micelles de caséine d'un rayon environ 100-200 nm stabilisées par du phosphate de calcium colloïdal.Au cours de ce travail, nous avons cherché à comprendre comment les agrégats de protéines sériques pouvaient être utilisés en mélange avec les micelles de caséine pour obtenir et contrôler la texture de produits laitiers. Dans un premier temps, nous avons étudié le processus de « cold gelation » induit par ajout de calcium et/ou acidification d'agrégats et de microgels de protéines sériques seuls. Dans une deuxième partie, nous nous sommes intéressés à la fonctionnalité des agrégats dans les mélanges plus complexes avec les autres protéines laitières et en présence de minéraux. L'addition de petites quantités d'agrégats fractals dans des suspensions de micelles diminuait leur température critique de gélification, augmentait le module élastique et diminuait la synérèse des gels.Les agrégats de protéines sériques peuvent être utilisés pour modifier la viscosité des mélanges, comme gélifiant ou pour enrichir la teneur en protéine du milieu sans en augmenter la viscosité. / The proteins of milk can be divided into whey proteins and caseins. Whey proteins are compact globular proteins that are found in the aqueous phase of milk. They are well-known for their exceptional functional properties. Upon heating, individual whey proteins denature and aggregate, forming aggregates of different morphologies and sizes, such as strands, fractal aggregates, microgels and fibrillar aggregates, depending on the heating conditions. On the other hand, the caseins in milk are organized in complex protein units with a diameter of 100-200 nm called casein micelles stabilized by colloidal calcium phosphate (CCP).The current work is an endeavor to understand how whey protein aggregates might be used in mixtures with other dairy proteins, such as casein micelles, in order to get a particular texture in a dairy product. We first extended the understanding of so-called “cold gelation” of pure WPI aggregates induced by calcium and acidification and then studied how the aggregates work in more complex mixtures of proteins and minerals. Interestingly, addition of small amounts of fractal aggregates to suspensions of casein micelles has been demonstrated to decrease the critical gelation temperature, increase the elastic modulus and decrease the syneresis of the gels.The aggregates are to be used to modify the viscosity of dairy products, as a gelling agent and for protein enrichment. The properties of strands, fractal aggregates and microgels have been studied and compared. WPI aggregates might be considered as “clean label” texturizing ingredients that do not require approval from the European Food Safety Authority (EFSA).

Agrégats de protéines sériques

Micelles de caséines

Microgels

Gélification

Viscosité

Texture

Clean label

Mélanges des protéines laitières

WPI aggregates

Casein micelles

Cold gelation

Viscosity

Dairy protein mixtures

664.024

Avaliação de hidrolisados de caseína como antioxidantes em produtos cárneos e chocolate branco

Rossini, Karina

January 2008

Estudos recentes indicam que os peptídeos obtidos pela hidrolise enzimática da caseína podem apresentar atividades antioxidantes. Neste trabalho, previamente obteve-se os peptídeos através de hidrolise da caseína utilizando as enzimas Alcalase e Flavourzyme (4h, a 50ºC e pH 8), selecionando os que apresentaram as melhores características, in vitro, relativas à atividade antioxidante. A hidrolise enzimática utilizando a enzima Flavourzyme mostrou melhores resultados, com alto valor de proteína solúvel e conteúdo de aminoácidos livres, além de peptídeos de menor peso molecular do que com a Alcalase, como observado nas análises de cromatografia de permeação em gel e eletroforese em gel de poliacrilamida. Os peptídeos de caseína obtidos com a Flavourzyme também apresentaram melhores resultados utilizando o método ABTS na determinação da capacidade antioxidante. O hidrolisado obtido a partir da enzima Flavourzyme foi aplicado em produtos cárneos e em chocolate branco. Em produtos cárneos, os peptídeos de caseína (2.0%) inibiram, efetivamente, a peroxidação lipídica em carne moída (100%) e em carne mecanicamente separada de ave (CMS) (cerca de 20%) indicando que estes peptídeos podem ser utilizados nestes produtos, auxiliando na prevenção da formação de flavor desagradável e aumentando sua vida útil. Relativamente a sua aplicação em chocolate branco, esta adição teve o intuito de inibir escurecimento deste produto, fator considerado como limitante na sua vida-útil sendo conseqüência tanto de reações de escurecimento não enzimático quanto da oxidação de lipídeos. Os parâmetros que indicaram alteração lipidica e reações não enzimáticas foram mensurados em três diferentes amostras de chocolate branco: uma amostra com 0,2%, de manteiga de cacau, de antioxidante sintético Grindox 562, outra com 0,2%, de manteiga de cacau, dos peptídeos de caseína e a terceira amostra sem qualquer tipo de antioxidante. As amostras foram expostas a duas temperaturas diferentes: 20 ± 2 e 28 ± 2ºC. Os resultados das análises realizadas indicaram que as amostras armazenadas à temperatura de 20ºC apresentaram resultados significativamente melhores àqueles das amostras armazenadas à temperatura de 28ºC, relativos ao índice de acidez, à atividade de água, ao índice de peróxido, à cor e às substâncias reativas ao ácido tiobarbitúrico (TBARS), indicando melhor conservação deste produto. Também foi observado que a adição de quaisquer dos antioxidantes empregados não influenciou de forma significativa os resultados obtidos, evidenciandose assim, que o principal parâmetro responsável pelas alterações do chocolate branco em sua vida útil refere-se à temperatura de armazenamento a qual as amostras foram submetidas. / Recent studies indicate that peptides obtained by casein hydrolysis may have antioxidant activity. In this work, previous casein peptides were obtained by enzymatic hydrolysis using Alcalase and Flavourzyme (4h, at 50ºC and pH 8), selecting the ones that showed the best characteristics in vitro, related to the antioxidant activity. The enzymatic hydrolysis using Flavourzyme showed the best results, with higher soluble protein and free amino acid content and producing lower molecular weight peptides than Alcalase, as observed by gel permeation chromatography and polyacrylamide gel electrophoresis. Related to its application in meat products, casein peptides obtained with Flavourzyme also exhibited greater antioxidant capacity using the ABTS method. The casein hydrolyzed from Flavourzyme enzyme was applicated in ground beef homogenates, mechanically deboned meat (MDM) of poultry and white chocolate. In meat products, casein peptides (2.0%) effectively inhibited lipid peroxidation in ground beef homogenates (100%) and mechanically deboned meat (about 20%) of poultry. Casein peptides may be useful in meat processing as another naturally occurring antioxidant, helping to prevent off-flavor formation in meat products and increasing shelf life. In the use for white chocolate, the goal was to inhibit its browning, the main problems that limit the white chocolate’s shelf-life. Non-enzymatic browning reaction and lipid oxidation were involved directly in the browning of white chocolate. Thus, parameters which indicated fat alteration and non-enzymatic reactions were measured in three different samples of white chocolate. One sample with 0,2% of cocoa butter, with the synthetic antioxidant Grindox 562, other with 0,2% of cocoa butter, with the natural antioxidant and the third sample without any kind of antioxidant. The samples were exposed to two different temperatures: 20 ± 2 and 28 ± 2ºC. The results of the analysis made indicated that the samples stored at the temperature of 20ºC showed results significantly better to those samples stored at the temperature of 28ºC, related to the conservation of the white chocolate. Besides, the results indicated that the addition of any antioxidants employees has not influenced in a significant way the results obtained. Thus, it was evidenced that the main responsible parameter for the alterations of the white chocolate’s shelf-life is related to the storage temperature to which the samples were submitted.

Caseina

Peptidio

Carne mecanicamente separada

Hidrolise enzimatica

Antioxidante

Chocolate branco

Oxidação lipídica

Reacao de maillard

Casein peptides

Enzymatic hydrolysis

Antioxidant

Ground beef

MDM

White chocolate

Lipid oxidation

Maillard reaction

Avaliação de hidrolisados de caseína como antioxidantes em produtos cárneos e chocolate branco

Rossini, Karina

January 2008

Estudos recentes indicam que os peptídeos obtidos pela hidrolise enzimática da caseína podem apresentar atividades antioxidantes. Neste trabalho, previamente obteve-se os peptídeos através de hidrolise da caseína utilizando as enzimas Alcalase e Flavourzyme (4h, a 50ºC e pH 8), selecionando os que apresentaram as melhores características, in vitro, relativas à atividade antioxidante. A hidrolise enzimática utilizando a enzima Flavourzyme mostrou melhores resultados, com alto valor de proteína solúvel e conteúdo de aminoácidos livres, além de peptídeos de menor peso molecular do que com a Alcalase, como observado nas análises de cromatografia de permeação em gel e eletroforese em gel de poliacrilamida. Os peptídeos de caseína obtidos com a Flavourzyme também apresentaram melhores resultados utilizando o método ABTS na determinação da capacidade antioxidante. O hidrolisado obtido a partir da enzima Flavourzyme foi aplicado em produtos cárneos e em chocolate branco. Em produtos cárneos, os peptídeos de caseína (2.0%) inibiram, efetivamente, a peroxidação lipídica em carne moída (100%) e em carne mecanicamente separada de ave (CMS) (cerca de 20%) indicando que estes peptídeos podem ser utilizados nestes produtos, auxiliando na prevenção da formação de flavor desagradável e aumentando sua vida útil. Relativamente a sua aplicação em chocolate branco, esta adição teve o intuito de inibir escurecimento deste produto, fator considerado como limitante na sua vida-útil sendo conseqüência tanto de reações de escurecimento não enzimático quanto da oxidação de lipídeos. Os parâmetros que indicaram alteração lipidica e reações não enzimáticas foram mensurados em três diferentes amostras de chocolate branco: uma amostra com 0,2%, de manteiga de cacau, de antioxidante sintético Grindox 562, outra com 0,2%, de manteiga de cacau, dos peptídeos de caseína e a terceira amostra sem qualquer tipo de antioxidante. As amostras foram expostas a duas temperaturas diferentes: 20 ± 2 e 28 ± 2ºC. Os resultados das análises realizadas indicaram que as amostras armazenadas à temperatura de 20ºC apresentaram resultados significativamente melhores àqueles das amostras armazenadas à temperatura de 28ºC, relativos ao índice de acidez, à atividade de água, ao índice de peróxido, à cor e às substâncias reativas ao ácido tiobarbitúrico (TBARS), indicando melhor conservação deste produto. Também foi observado que a adição de quaisquer dos antioxidantes empregados não influenciou de forma significativa os resultados obtidos, evidenciandose assim, que o principal parâmetro responsável pelas alterações do chocolate branco em sua vida útil refere-se à temperatura de armazenamento a qual as amostras foram submetidas. / Recent studies indicate that peptides obtained by casein hydrolysis may have antioxidant activity. In this work, previous casein peptides were obtained by enzymatic hydrolysis using Alcalase and Flavourzyme (4h, at 50ºC and pH 8), selecting the ones that showed the best characteristics in vitro, related to the antioxidant activity. The enzymatic hydrolysis using Flavourzyme showed the best results, with higher soluble protein and free amino acid content and producing lower molecular weight peptides than Alcalase, as observed by gel permeation chromatography and polyacrylamide gel electrophoresis. Related to its application in meat products, casein peptides obtained with Flavourzyme also exhibited greater antioxidant capacity using the ABTS method. The casein hydrolyzed from Flavourzyme enzyme was applicated in ground beef homogenates, mechanically deboned meat (MDM) of poultry and white chocolate. In meat products, casein peptides (2.0%) effectively inhibited lipid peroxidation in ground beef homogenates (100%) and mechanically deboned meat (about 20%) of poultry. Casein peptides may be useful in meat processing as another naturally occurring antioxidant, helping to prevent off-flavor formation in meat products and increasing shelf life. In the use for white chocolate, the goal was to inhibit its browning, the main problems that limit the white chocolate’s shelf-life. Non-enzymatic browning reaction and lipid oxidation were involved directly in the browning of white chocolate. Thus, parameters which indicated fat alteration and non-enzymatic reactions were measured in three different samples of white chocolate. One sample with 0,2% of cocoa butter, with the synthetic antioxidant Grindox 562, other with 0,2% of cocoa butter, with the natural antioxidant and the third sample without any kind of antioxidant. The samples were exposed to two different temperatures: 20 ± 2 and 28 ± 2ºC. The results of the analysis made indicated that the samples stored at the temperature of 20ºC showed results significantly better to those samples stored at the temperature of 28ºC, related to the conservation of the white chocolate. Besides, the results indicated that the addition of any antioxidants employees has not influenced in a significant way the results obtained. Thus, it was evidenced that the main responsible parameter for the alterations of the white chocolate’s shelf-life is related to the storage temperature to which the samples were submitted.

Caseina

Peptidio

Carne mecanicamente separada

Hidrolise enzimatica

Antioxidante

Chocolate branco

Oxidação lipídica

Reacao de maillard

Casein peptides

Enzymatic hydrolysis

Antioxidant

Ground beef

MDM

White chocolate

Lipid oxidation

Maillard reaction

Dinâmica de degradação in vitro da fibra em detergente neutro de forragens tropicais em função de suplementação protéica e/ou energética / In vitro degradation dynamics of tropical forages neutral detergent fiber according to protein and/or energy supplementation

Costa, Viviane Aparecida Carli

02 October 2006

Made available in DSpace on 2015-03-26T13:55:14Z (GMT). No. of bitstreams: 1 texto completo.pdf: 338504 bytes, checksum: 1d5ec3b26be107cc6435dba9aa861024 (MD5) Previous issue date: 2006-10-02 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior / The current thesis was based on two in vitro trials aiming at assessing the effect of protein and/or energy supplementation on ruminal degradation of fibrous carbohydrates of tropical forages. At Experiment 1, it was evaluated the effect of protein and/or energy supplementation on the utilization of fibrous carbohydrates from low quality forage by ruminal microorganisms. The experiment simulated the supplementation of finishing cattle grazing low quality Brachiaria decumbens pasture during the dry season (70:30 forage to concentrate ratio, as dry matter basis). The concentrate used was formulated to contain 30% of crude protein, using starch as the energetic source and casein as the proteic source. The treatments were established by omission of the proteic and/or energetic source of the supplement, associated with the total substitution of starch by pectin. In that way, six treatments were evaluated: 1. Forage; 2. Forage plus Starch; 3. Forage plus Pectin; 4. Forage plus Casein, 5. Forage plus Casein plus Starch and 6. Forage plus Casein plus Pectin. The treatments were evaluated under ruminal environment, simulated by in vitro incubation, where the experimental diets were submitted to different incubation periods: 0, 3, 6, 9, 12, 24, 36, 48, 72 and 96 hours. The incubation procedure was repeated four times in a way that four evaluations within each incubation time were done for each treatment. The incubation residues were evaluated according to its content of neutral detergent fiber (NDF) and interpreted using a non-linear logistic model. It was observed that the degradation rate of the potentially degradable NDF (pdNDF) increased almost 46% with casein supplementation (0.0261 and 0.0381 h-1), resulting in an increment of 14.6% in the effective degraded fraction. A minor effect was observed with the inclusion or substitution of the supplemental carbohydrate source. The starch supplementation resulted in reduction on the degradation rate of pdNDF, whereas pectin supplementation did not affect this parameter, when compared to the treatment without carbohydrate supplementation. In the presence of casein, the starch supplementation raised the discrete lag time of NDF degradation. At Experiment 2, it was evaluated the effect of protein and/or energy supplementation on ruminal degradation of fibrous carbohydrates from high quality forage. The evaluation procedures and the forage to concentrate ratio were similar to those used at Experiment 1. Instead of Brachiaria decumbens, samples of elephant-grass (pennisetum purpureum, 21 days of regrowth) were used as basal forage. The treatments were established by omission of the proteic and/or energetic source of the supplement, associated with total substitution of starch by pectin and of crude protein from casein by crude protein from the mixture urea:ammonium sulfate (9:1). The nine treatments were: 1. Forage; 2. Forage plus Starch; 3. Forage plus Pectin; 4.Forage plus Casein; 5. Forage plus Casein plus Starch; 6. Forage plus Casein plus Pectin; 7. Forage plus Urea; 8. Forage plus Urea plus Starch and 9. Forage plus Urea plus Pectin. When submitted to exclusive supplementation of protein or energy, it was detected a reduction in the pdNDF degradation rate. On the other hand, the negative effects of the individual supplementation with protein or energy were or not eliminated according to the final composition of the supplement. The negative effects of the individual supplementation on the pdNDF degradation rate were maintained when casein and pectin or starch and urea were used concomitantly. Conversely, similar degradation rates to that of the basal forage were obtained with the combinations pectin and urea, and starch and casein. / A presente tese foi elaborada com base em dois experimentos in vitro com o objetivo de avaliar o efeito da suplementação protéica e/ou energética sobre a degradação ruminal dos carboidratos fibrosos de forragens tropicais. No Experimento 1, objetivou-se avaliar o efeito da suplementação protéica e/ou energética sobre a utilização dos carboidratos fibrosos de forragem de baixa qualidade. O experimento simulou a suplementação de bovinos em terminação sob pastejo em Brachiaria decumbns de baixa qualidade durante o período seco (70% de forragem e 30% de concentrado, com base na matéria seca). O concentrado referente ao tratamento base foi formulado de forma a apresentar 30% de proteína bruta (PB), utilizando-se amido, como componente energético, e caseína, como componente protéico. Os tratamentos foram construídos a partir da omissão do fornecimento das fontes protéica e/ou energética do suplemento, associando-se, ainda, a substituição total do amido por pectina. Desta forma, seis foram os tratamentos avaliados: 1.Forragem; 2.Forragem + Amido; 3.Forragem + Pectina; 4.Forragem + Caseína; 5.Forragem + Caseína + Amido ; e 6.Forragem + Caseína + Pectina. Os tratamentos foram avaliados em ambiente ruminal simulado por incubação in vitro sendo submetidos a diferentes tempos de incubação: 0, 3, 6, 9, 12, 24, 36, 48, 72 e 96 horas. O procedimento de incubação foi repetido quatro vezes, perfazendo-se o total de quatro avaliações por tempo de incubação para cada tratamento. Os resíduos de incubação foram avaliados quanto ao teor de fibra em detergente neutro (FDN), e interpretados por intermédio de modelo nãolinear logístico . Observou-se que a taxa de degradação da FDN potencialmente degradável (FDNpd) foi ampliada em cerca de 46% com a suplementação com caseína (0,0261 e 0,0381 h-1), resultando em incrementos da ordem de 14,6% sobre a fração efetivamente degradada. Observou-se efeito de menor amplitude com a inclusão ou alteração da fonte de carboidrato suplementar. A suplementação com amido causou redução na taxa de degradação da FDNpd, ao passo que a suplementação com pectina não afetou este parâmetro em comparação à ausência de carboidratos. Na presença de caseína, a suplementação com amido elevou o tempo de latência discreta para início do processo de degradação da FDN. No Experimento 2 objetivou-se avaliar o efeito da suplementação protéica e/ou energética sobre a degradação ruminal dos carboidratos fibrosos de forragem de alta qualidade. Os procedimentos de avaliação e a relação forragem:concentrado e o teor de PB no suplemento foram similares ao experimento 1, utilizando-se contudo amostras de capim-elefante (Pennisetum purpureum) com 21 dias de rebrotação como forragem basal. Os tratamentos foram construídos a partir da omissão do fornecimento da fonte protéica e/ou energética do suplemento, associando-se ainda a substituição total do amido por pectina e da proteína bruta oriunda da caseína por proteína bruta oriunda da mistura uréia:sulfato de amônio (9:1). Desta forma, nove foram os tratamentos avaliados: 1.Forragem; 2.Forragem + Amido; 3.Forragem + Pectina; 4.Forragem + Caseína; 5.Forragem + Caseína + Amido; e 6.Forragem + Caseína + Pectina; 7. Forragem + Uréia; 8.Forragem + Uréia + Amido; e 9.Forragem + Uréia + Pectina. Observou-se decréscimo na taxa de degradação FDNpd, quando essa foi submetida a suplementação exclusiva com fontes energéticas ou protéicas. Por outro lado, os efeitos deletérios individuais das suplementações protéica ou energética foram ou não eliminados de acordo com a composição final dos suplementos. Os efeitos deletérios individuais sobre a taxa de degradação da FDNpd foram mantidos pela utilização concomitante de caseína e pectina ou amido e uréia . Por outro lado, taxas de degradação similares ao tratamento basal (forragem) foram obtidas com as combinações pectina e uréia ou amido e caseína.

Bovino de corte

Nutrição

Suplementos dietéticos

Fibras

Degradabilidade

Caseína

Amido

Beef cattle

Nutrition

Diet supplements

Fibers

Degradation

Casein

Starch