Teses / dissertações sobre o tema "Dairy microbiology"
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McAstocker, Michael. "The effects of dietary dairy products on mammalian cholesterol metabolism". Thesis, Queen's University Belfast, 1992. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.317559.
Texto completo da fonteSarhan, Hassan Raheem. "Rapid fluorogenic methods for the detection of Escherichia coli in dairy products and water supply". Thesis, University of Salford, 1989. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.258363.
Texto completo da fonteCoklin, Tatjana. "Detection and molecular characterization of Giardia and Cryptosporidium in Canadian dairy cattle". Thesis, University of Ottawa (Canada), 2007. http://hdl.handle.net/10393/27823.
Texto completo da fonteDavidse, Elton (Elton Kurt). "Prevention and treatment of mastitis in dairy cows with bacteriocins produced by Enterococcus faecalis". Thesis, Stellenbosch : University of Stellenbosch, 2003. http://hdl.handle.net/10019.1/16296.
Texto completo da fonteENGLISH ABSTRACT: The effect of the bacteriocin-like peptide AS-48, produced by Enterococcus faecalis FAIRE 92, was tested against a mastitis isolate of Staphylococcus aureus in an in vivo and in vitro study. During initial tests peptide AS-48 showed no significant activity towards S. aureus, even with a ten-fold concentrated cell-free supernatant. Activity was obtained only after purification with Triton X-114 phase partitioning, followed by cation exchange chromatography. Titers for the purified peptide varied between 3200 and 12800 AU/ml. The purified peptide also exhibited activity towards Streptococcus agalactiae and Streptococcus dysgalactiae, but not against Escherichia coli. The size of peptide AS-48 was determined at 7150 Da, based on electronspray mass spectrometry and SDS-PAGE. Complete inhibition of cell growth was obtained by adding 1ml of the purified peptide (3200 AU/ml) to 100 ml of cells of S. aureus in the lag growth phase. When the same concentration of peptide AS-48 was added to a culture of S. aureus in mid-exponential growth, a slight decrease in viable cell numbers was recorded, which lasted for only 30 min. Cell growth commenced thereafter. In situ experiments in cows were done with purified peptide AS-48, encapsulated in liposomes. These in vivo studies were conducted by administering peptide AS-48 (6400 AU/ml) to different udder quarters. In a prevention trial, i.e. where quarters were pretreated with peptide AS-48, a reduction close to 90% in the viable cell numbers of S. aureus was recorded relative to the control quarters, which were not treated with the peptide. A 50% reduction in somatic cell count (SCC) was recorded. In the treatment trial, i.e. infected quarters treated with peptide AS-48, a reduction of up to 94% in viable cell numbers of S. aureus was recorded. In the same quarters, a reduction in SCC amounted to almost 80%. A recombinant strain was constructed by conjugating plasmid 92 (p92), encoding peptide AS-48, from Enterococcus faecalis FAIRE 92 to E. faecalis FA2/Ent, which produces enterocins 1071A and 1071B. Southern blot hybridization experiments revealed thepresence of plasmid p92 in the recipient strain without the loss of plasmid pEF1071, which encodes enterocins 1071A and 1071B. All three antimicrobial peptides, i.e. enterocin 1071A, enterocin 1071B and peptide AS-48, were produced in transconjugant FA2/Ent/AS-48. The spectrum of antimicrobial activity of the transconjugant was greater than that recorded for strains FA2/Ent and FAIRE 92, respectively and included E. faecalis, Bacillus cereus, Lactobacillus acidophilus, Lactobacillus casei, Lactobacillus curvatus, Lactobacillus fermentum, Lactobacillus plantarum, Lactobacillus reuteri, Lactobacillus sakei, Leuconostoc cremoris, Leuconostoc pentosaceus, Staphylococcus carnosus and S. aureus. These organisms are not inhibited by strain FA2/Ent. However, low levels of peptide AS-48 was produced by strain FA2/Ent/AS-48. Further research in fermentation and gene expression will be needed before the transconjugant E. faecalis FA2/Ent/AS-48 may be used in the treatment of mastitis.
AFRIKAANSE OPSOMMING: Die effek van die bakteriosien-agtige, peptied AS-48, geproduseer deur Enterococcus faecalis FAIRE 92, is gedurende ‘n in vivo en in vitro studie teen ‘n mastitiese Staphylococcus aureus-isolaat getoets. Aanvanklike toetse met peptied AS-48, selfs tienvoudig gekonsentreerde selvrye supernatant, het geen beduidende aktiwiteit teen S. aureus getoon nie. Aktiwiteit is eers verkry na suiwering met Triton X-114 fase-skeiding gevolg deur katioon uitruilingschromatografie. Titers vir die gesuiwerde peptied het tussen 3200 en 12800 AE/ml gewissel. Die gesuiwerde peptied het ook aktiwiteit teen Streptococcus agalactiae en Streptococcus dysgalctiae getoon, maar nie teen Escherichia coli nie. Peptied AS-48 het ‘n molekulêre massa van 7150 Da, soos bepaal met elektronsproeimassa spektrometrie en SDS-PAGE. Totale inhibisie van selgroei is verkry deur 1 ml gesuiwerde peptied AS-48 (3200 AE/ml) by ‘n 100 ml kultuur van S. aureus in die sloerfase te voeg. Dieselfe konsentrasie peptied AS-48, toegevoeg tydens die mideksponensiële groeifase, het egter slegs ‘n klein vermindering in die aantal lewende selle teweeg gebring en het ook vir slegs ‘n 30 min geduur. Selgroei het hierna weer normaal voort gegaan. In situ eksperimente op koeie is uitgevoer met gesuiwerde peptied AS-48, geenkapsuleerd in liposome. Hierdie In vivo studies is onderneem deur peptied AS-48 (6400 AE/ml) in verskillende kwarte van die uier, kunsmatig of reeds geïnfekteerd met S. aureus, toe te dien. In ‘n voorkomings-eksperiment waar kwarte vooraf met peptied AS- 48 behandel is, is ‘n verlaging van byna 90% in die lewende seltelling van S. aureus relatief tot die kontrole kwarte, sonder behandeling met peptied AS-48, verkry. ‘n 50% verlaging in die somatiese seltelling (SST) is verkry. In die behandelings-eksperiment, waar geïnfekteerde kwarte met peptied AS-48 behandel is, is ‘n verlaging van byna 90% in lewende S. aureus selle gevind. In dieselfde kwarte is ‘n verlaging van byna 80% in die SST genoteer.‘n Rekombinante ras is gekonstrueer deur plasmied 92 (p92), wat kodeer vir peptied AS- 48, vanaf Enterococcus faecalis FAIRE 92 na E. faecalis FA2/Ent, wat enterosien 1071A en 1071B produseer, te konjugeer. Southern-klad hibridisasie het die teenwoordigheid van plasmied p92 in die ontvanger ras, sonder die verlies van plasmied pEF1071 wat enterosien 1071A en 1071B kodeer, getoon. Al drie antimikrobiese peptiede, nl. enterosien 1071A, enterosien 1071B en peptied AS-48, is deur die transkonjugant FA2/Ent/AS-48 geproduseer. Die spektum van antimikrobiese aktiwiteit van die transkonjugant vand die transkonjugant is breër as dié van rasse FA2/Ent en FAIRE 92, onderskeidelik en het ook E. faecalis, Bacillus cereus, Lactobacillus acidophilus, Lactobacillus casei, Lactobacillus curvatus, Lactobacillus fermentum, Lactobacillus plantarum, Lactobacillus reuteri, Lactobacillus sakei, Leuconostoc cremoris, Leuconostoc pentosaceus, Staphylococcus carnosus en S. aureus ingesluit. Hierdie organismes word nie deur ras FA2/Ent geïnhibeer nie. Lae vlakke van peptied AS-48 is egter deur ras FA2/Ent/AS-48 geproduseer. Verdere navorsing in fermentasie en geenuitdrukking is nodig voordat E. faecalis FA2/Ent/AS-48 in die behandeling van mastitis gebruik kan word.
Sanchez, Luis R. "Removal of bacterial indicators and pathogens from dairy wastewater by a treatment system". Diss., The University of Arizona, 1999. http://hdl.handle.net/10150/284075.
Texto completo da fonteManshadi, Faezeh Dehghan. "Occurence of pathogenic and indicator microorganisms on produce irrigated with dairy wastewater". Diss., The University of Arizona, 2003. http://hdl.handle.net/10150/289980.
Texto completo da fonteMosteller, Tracy M. "Sanitizer efficacy towards attached bacteria in a simulated milk pipeline system using pure and mixed cultures". Diss., This resource online, 1993. http://scholar.lib.vt.edu/theses/available/etd-08062007-094410/.
Texto completo da fonteMugabi, Robert. "Genotypes And Phenotypes Of Staphylococci On Selected Dairy Farms In Vermont". ScholarWorks @ UVM, 2018. https://scholarworks.uvm.edu/graddis/844.
Texto completo da fonteYam, Godward Georgia Nga-Mun. "Studies on enhancing the viability and survival of probiotic bacteria in dairy foods through strain selection and microencapsulation". Thesis, View thesis View thesis, 2000. http://handle.uws.edu.au:8081/1959.7/411.
Texto completo da fonteYam, Godward Georgia Nga-Mun, of Western Sydney Hawkesbury University, Faculty of Science and Technology e of Science Food and Horticulture School. "Studies on enhancing the viability and survival of probiotic bacteria in dairy foods through strain selection and microencapsulation". THESIS_FST_SFH_YamGodward_G.xml, 2000. http://handle.uws.edu.au:8081/1959.7/411.
Texto completo da fonteMaster of Science (Hons)
Yam, Godward Georgia Nga-Mun. "Studies on enhancing the viability and survival of probiotic bacteria in dairy foods through strain selection and microencapsulation /". View thesis View thesis, 2000. http://library.uws.edu.au/adt-NUWS/public/adt-NUWS20030428.112849/index.html.
Texto completo da fonteA thesis presented for the fulfilment of Master of Science (Honours), Centre for Advanced Food Research, School of Science, Food and Horticulture, University of Western Sydney, Hawkesbury, December 2000. Spine title : Survival of probiotic bacteria in dairy foods. Bibliography : leaves 228-244.
Pieterse, Renee. "Control of bacterial pathogens associated with mastitis in dairy cows with natural antimicrobial peptides produced by lactic acid bacteria". Thesis, Stellenbosch : Stellenbosch University, 2008. http://hdl.handle.net/10019.1/2323.
Texto completo da fonteMastitis is considered to be the most costly disease affecting the dairy industry. Management strategies involve the extensive use of antibiotics to treat and prevent this disease. Prophylactic dosages of antibiotics used in mastitis control programmes could select for strains with resistance to antibiotics. In addition, a strong drive towards reducing antibiotic residues in animal food products has lead to research in finding alternative antimicrobial agents. Streptococcus macedonicus ST91KM, isolated from bulgarian goat yoghurt, produces the bacteriocin macedocin ST91KM with a narrow spectrum of activity against Grampositive bacteria. These include mastitis pathogens Streptococcus agalactiae, Streptococcus dysgalactiae, Streptococcus uberis, Staphylococcus aureus and Staphylococcus epidermidis as well as Lactobacillus sakei and Micrococcus varians. Macedocin ST91KM is, according to tricine-SDS PAGE, between 2.0 and 2.5 kDa in size. The activity of macedocin ST91KM remained unchanged after 2 h of incubation at pH 2.0 to 10.0 and 100 min at 100 °C. The peptide was inactivated after 20 min at 121 °C and when treated with pronase, pepsin and trypsin. Treatment with α-amylase had no effect on activity, suggesting that the mode of action does not depend on glycosylation. Precipitation with 60 % saturated ammonium sulphate, followed by Sep-Pak C18 separation recovered 43 % of macedocin ST91KM. Amplification of the genome of strain ST91KM with primers designed from the sequence of the macedocin prescursor gene (mcdA) produced two fragments (approximately 375 and 220 bp) instead of one fragment of 150 bp recorded for macedocin produced by S. macedonicus ACA-DC 198. Strain ACA-DC 198 was not available. However, the DNA fragment amplified from strain LMG 18488 (ACA-DC 206), genetically closely related to strain ACADC 198, revealed 99 % homology to the mcdA of S. macedonicus ACA-DC 198 (accession number DQ835394). Macedocin ST91KM may thus be a related bacteriocin described for S. macedonicus. The peptide adsorbed equally well (66 %) to L. sakei LMG13558 and insensitive cells, e.g. Enterococcus faecalis BFE 1071 and FAIR E92, and Streptococcus caprinus ATCC 700066. Optimal adsorption of macedocin ST91KM was recorded at 37 °C and 45 °C and at pH of 8 - 10. Addition of solvents decreased adsorption by 50%, suggesting that the receptors to which the bacteriocin binds have lipid moieties. The addition of MgCl2, KI and Na2CO3 completely prevented adsorption of macedocin ST91KM to the target cells, possibly due to competitive ion adsorption on the bacterial cell surface. The peptide has a bacteriocidal mode of action, resulting in lysis and the release of DNA and β-galactosidase. Atomic force microscopy of sensitive cells treated with macedocin ST91KM have shown deformation of the cell structure and developing of irregular surface areas. Antimicrobial susceptibility patterns were evaluated against eighteen mastitis pathogens. All isolates tested were resistant to methicillin and oxacillin, but had minimum inhibitory concentrations (MICs) falling in the intermediate and susceptible range against erythromycin. S. agalactiae and S. epidermidis had the highest sensitivity to macedocin ST91KM. A teat seal preparation containing macedocin ST91KM effectively released bacteriocin inhibiting the growth of the bacterial pathogen. Macedocin ST91KM could form the basis for an alternative dry cow therapy to prevent mastitis infections in dairy cows, as it is effective against pathogens that display resistance to conventional antibiotic therapy.
Cameron, Michelle. "Impact of low-frequency high-power ultrasound on spoilage and potentially pathogenic dairy microbes". Thesis, Link to the online version, 2007. http://hdl.handle.net/10019/597.
Texto completo da fonteHayward, Stefan. "Partial characterization of a bacterial acyltransferase enzyme for potential application in dairy processing". Thesis, Stellenbosch : Stellenbosch University, 2014. http://hdl.handle.net/10019.1/86636.
Texto completo da fonteENGLISH ABSTRACT: This study describes: the evaluation of the current, and potential assay methods for the quantification of cholesterol, cholesteryl esters and free fatty acids in milk and the application thereof ; an account of the difficulties associated with the usage of FoodPro® Cleanline, an enzyme preparation used as processing aid, during ultra-high temperature processing of milk ; the development of activity assays which can be used for the kinetic characterization of glycerophospholipid cholesterol acyltransferase, the active enzyme in FoodPro® Cleanline ; the development of an accurate and facile activity assay, and the validation thereof, which can be used for the validation of enzyme activity prior to dosage of milk with FoodPro® Cleanline.
AFRIKAANSE OPSOMMING: Hierdie studie beskryf: die evaluering van die huidige, en potensiële, metodes vir die kwantifisering van cholesterol, cholesteriel esters en vryvetsure in melk, sowel as die toepassing van hieridie metodes ; 'n verduideliking van die moeilikhede wat ondervind word gedurende die gebruik van FoodPro® Cleanline, 'n ensiempreparaat vir gebruik as 'n verwerkingshulpmiddel, tydens ultrahoë-temperatuurprosessering van melk ; die ontwikkeling van aktiwiteitsbepalings metodes vir gebruik in kinetiese karakterisering van gliserofosfolipied cholesterol asieltransferase, die aktiewe ensiem in FoodPro® Cleanline ; die ontwikkeling van 'n akkurate, eenvoudige aktiwiteitsbepalings metode, en bevestiging van hierdie metode, wat gebruik kan word vir kwalitieitskontrole alvorens die dosering van melk met FoodPro® Cleanline.
Lippens, Wim. "Rapid Detection of Listeria monocytogenes". DigitalCommons@USU, 2003. https://digitalcommons.usu.edu/etd/5491.
Texto completo da fonteTanih, Godfred Ngu. "Genotypic and phenotypic characterization of enterococci from cow dung and environmental water sources in three selected dairy farms in Amathole District". Thesis, University of Fort Hare, 2016. http://hdl.handle.net/10353/2348.
Texto completo da fonteBorchers, Matthew Richard. "THE EFFECTS OF HOUSING ON DAIRY COW COMFORT, IMMUNE FUNCTION, STRESS, PRODUCTIVITY, AND MILK QUALITY". UKnowledge, 2018. https://uknowledge.uky.edu/animalsci_etds/93.
Texto completo da fonteTomlinson, Dana J. "Effect of nonstructural carbohydrates and rumen undegradable protein on intake, growth, and body condition of dairy heifers". Diss., This resource online, 1990. http://scholar.lib.vt.edu/theses/available/etd-07282008-135549/.
Texto completo da fonteVita. Abstract. No film copy made for this title. Includes bibliographical references (leaves 149-165). Also available via the Internet.
Mackintosh, E. D. "The effect of monensin on in vitro rumen fermentation and in vivo rumen and total tract digestion and milk production in the dairy cow". Thesis, University of Reading, 1998. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.265711.
Texto completo da fonteMussa, Dinna Mathemi. "High pressure processing of milk and muscle foods : evaluation of process kinetics, safety and quality changes". Thesis, McGill University, 1999. http://digitool.Library.McGill.CA:80/R/?func=dbin-jump-full&object_id=35473.
Texto completo da fonteThe application of pressure pulse was explored for pressure destruction of microorganisms as well as changes in physical-chemical characteristics of pork chops. Pork chops (2 days post-rigor) were subjected to HP treatment from 200--350 MPa for 0--120 min. Results showed that pressure changes of pork variables followed a dual effect consisting of an instantaneous pressure kill (IPK) with the application of pressure pulse (no holding) and a subsequent first order rate of destruction during the pressure hold time. The IPK values were pressure dependent and increased with pressure level. Parameters k and D indicated a higher rate of pressure destruction of microorganisms compared to quality attributes.
Kinetics of pressure destruction of Listeria monocytogenes Scott A were studied in relation to those of indigenous microorganism of milk and pork. The IPK was more pronounced with L. monocytogenes than with indigenous microflora. However, the kinetic parameters (k and D values) indicated a larger pressure resistance for L. monoctyogenes. HP processes were developed based on the standard plate count (SPC) kinetic data for indigenous microflora of milk as well as L. monocytogenes in milk and pork. The results showed that SPC kinetics permitted good estimation of microbial destruction in low pressure-lethality processes of milk and pork but its application at higher pressure-lethality levels were inaccurate. On the other hand, processes established based an destruction of L. monocytogenes were more predictable. Pressure pulse application to microbial lethality was also well predicted.
The shelf-life of milk and pork increased with the level of applied pressure lethality, but Q10 values suggested that low storage temperature was nevertheless required to control microbial growth and maintain quality. Storage of HP treated park offered some improvement in the texture but resulted in large color changes and drip losses. L. monocytogenes were not detected in any of the stored milk samples HP treated to achieve a lethality ≥10D.
Cersosimo, Laura Marie. "Rumen Microbial Ecology And Rumen-Derived Fatty Acids: Determinants Of And Relationship To Dairy Cow Production Performance". ScholarWorks @ UVM, 2017. http://scholarworks.uvm.edu/graddis/665.
Texto completo da fonteJawad, Emad. "Technological benefits and potential of incorporation of probiotic bacteria and inulin in soft cheese". Thesis, University of Plymouth, 2016. http://hdl.handle.net/10026.1/4377.
Texto completo da fonteMokoena, Kingsley Katleho. "Airborne microbiota and related environmental parameters associated with a typical dairy farm plant". Thesis, Bloemfontein : Central University of Technology, Free State, 2013. http://hdl.handle.net/11462/160.
Texto completo da fonteFood processing plants and agricultural environments have a long-standing history of being known to provide a conducive environment for the prevalence and distribution of microorganisms which emanate as a consequence of activities undertaken in such premises. Microorganisms in the aforementioned environments may be found in the atmosphere (airborne), and/or on food contact surfaces. Airborne microorganisms from food handlers and in food products and raw materials (as part of bioaerosols) have in the past been implicated as having a potential to cause adverse health effects (especially in indoor environments) and therefore also to have economic implications. Recently their effect on food safety has received increased interest. The recent international interest in bioaerosols in the food industry has played a role in rapidly providing increased understanding of bioaerosols and their effects in different food processing environments. However, there is still a lack of research on the actual impact of bioaerosols over time in most of the food premises especially in Southern Africa and other developing countries. The overall purpose of this dissertation was to assess possible microbial contaminants and the role of selected environmental parameters on these microbes at a dairy farm plant in central South Africa. In relation to the purpose of the study, the objectives of this dissertation were to investigate and establish the food handler’s food safety knowledge, attitude, behaviour and practices. The sub-objective was to investigate the prevalence and distribution of microbial contaminants (both airborne and food contact surface populations), and concomitant environmental parameters. The microbe isolates from both investigations (i.e. air samples and food contact surfaces) were identified to strain level using matrix-assisted laser desorption ionization – time of flight mass spectrometry (MALDI-TOF MS). The findings of this study in relation to food handlers’ food safety knowledge, attitude, behaviour and practices indicated a dire need for training of employees as well as improved health and hygiene measures as emphasised by some of the identified strains. The environmental parameters (both indoor and outdoor) were similar, with no relationship established between airborne microbes’ prevalence and environmental parameters. The samples of the airborne microbial populations in both indoor and outdoor environments were similar. Airborne microbial counts at the dairy farm plant over the entire duration of the study ranged between 1.50 x 101cfu.m-3and 1.62 x 102cfu.m-3. Microbial counts on food contact surfaces ranged between 2.50 x 102 cfu.cm-2 and 1.10 x 105 cfu.cm-2 over the entire duration of the study. A wide variety of microorganisms (from air and food contact surfaces) such as the Gram-positive bacteria, Gram-negative bacteria, as well as fungi were present at the dairy farm plant. A number of the isolated genera have previously been associated with agricultural environments whilst others are associated with hospital environments. The positively identified strains were from genera such as Aeromonas, Arthrobacter, Candida, Pseudomonas, Pantoea, Citrobacter, Staphylococcus, Bacillus, Escherichia, Rhodococcus and Rhodotorula, amongst others. The isolation of microorganisms associated with food spoilage and foodborne disease outbreaks, which are known as indicator organisms such as Escherichia coli, Staphylococcus and Bacillus from both air and surface samples, signified possible faecal contamination and could be attributed to poor health and hygiene practices at the dairy farm plant. Despite the isolation of microorganisms associated with food spoilage and foodborne disease outbreaks, the isolation of microorganisms not usually associated with the food processing industry (usually associated with hospital environments) was an enormous and serious concern which suggested a need for further investigations at dairy farm plants as the implications of these pathogenic microorganisms in food is not known. The isolation of similar microorganisms from both the air samples and surface swabs suggests that airborne microbes have a potential of settling on food contact surfaces, therefore having a potential to contaminate dairy products which are known to be more prone to contamination and which, because of their nutritional status, serve as a good substrate for the growth of microorganisms.
Javorski, Cleovani Rossi. "Utilização de resíduo úmido de fécula de mandioca na dieta de vacas holandesas em lactação". Universidade Estadual do Oeste do Paraná, 2012. http://tede.unioeste.br:8080/tede/handle/tede/1526.
Texto completo da fonteCoordenação de Aperfeiçoamento de Pessoal de Nível Superior
In dairy farming, one of the factors that raise the cost of production is feed, which can reach 70% of the total cost. With this, it is necessary to look for alternatives to reduce these costs without sacrificing productivity. An alternative is to enrich food resources of the animals, through the use of byproducts of industrial manioc starch. These alternative foods may constitute an interesting strategy, because in addition to being acquired by a low commercial value, may have high energy content and can also give an appropriate final destination byproduct of the cassava industry, contributing to the environment. The residue obtained during the processing of cassava has moisture content between 75% and 85%. The animal productivity can be affected negatively, depending on consumption and digestibility of nutrients. This study aimed to evaluate the chemical, microbiological, and detect the presence of mycotoxins in moist residue cassava starch (RMCS), and to evaluate the influence of five levels RMCS on intake and digestibility of nutrients, production and composition milk, and some blood parameters in dairy cows, Holstein, with average initial production of 30.65 kg milk / day. We observed a significant reduction in consumption (EE), and a linear effect for all nutrients studied, except for crude protein. Milk production was negatively affected, with a reduction to include RMCS. The chemical composition of RMCS did not change during storage, only significant variation in dry matter (DM). For populations of microorganisms, there was a significant increase only fungi and yeasts. Zearalenone levels were detected in 100% of the samples analyzed RUFM. The milk was reduced, but the efficiency of feed conversion was not affected, indicating that the residue can be used, however, it is necessary to adjust the levels of inclusion of the diet. The storage of RMCS proved effective under the conditions studied, since there were no changes in the nutritional value of the residue, but high counts of yeasts and fungi, and mycotoxins, may suggest that the material has a high risk of degradation
Na atividade leiteira, um dos fatores que elevam os custos da produção é a alimentação animal, que podem chegar a 70% do custo total. Com isso, é necessário buscar alternativas para redução desses custos, sem prejudicar a produtividade. Uma alternativa é o enriquecimento dos recursos alimentícios dos animais, através da utilização de subprodutos da indústria de fécula de mandioca. Esses alimentos alternativos podem constituir uma estratégia interessante, pois, além de serem adquiridos por um baixo valor comercial, podem apresentar alto teor energético, podem também, dar um adequado destino final ao subproduto da fecularia, contribuindo para preservar o meio ambiente. O resíduo obtido durante o processamento da mandioca apresenta teor de umidade entre 75% e 85%. A produtividade animal pode ser afetada de forma negativa, dependendo do consumo e da digestibilidade dos nutrientes da dieta. Esta pesquisa tem por objetivo avaliar a composição química, microbiológica, e também detectar presença de micotoxinas no resíduo úmido de fécula de mandioca (RUFM), além disso, avaliar a influência de cinco níveis de RUFM sobre o consumo e digestibilidade dos nutrientes, produção e composição do leite, e alguns parâmetros sanguíneos de vacas em lactação, da raça Holandesa, com produção média inicial de 30,65 kg de leite/dia. Nesta pesquisa observou-se a redução significativa no consumo de extrato etéreo (EE), e o efeito linear negativo para todos os nutrientes estudados, exceto para a proteína bruta. A produção de leite foi influenciada de forma negativa, ocorrendo redução com a inclusão de RUFM. A composição química do RUFM não sofreu alterações durante a estocagem, houve variação significativa apenas nos teores de matéria seca (MS). Para as populações de microrganismos, houve elevação significativa apenas de fungos e leveduras. Níveis de Zearalenona foram detectados em 100% das amostras de RUFM analisadas. A produção de leite sofreu redução, mas a eficiência na conversão alimentar não foi alterada, mostrando que o resíduo pode ser utilizado, no entanto, é necessário adequar os níveis de inclusão deste na dieta. A estocagem do RUFM mostrou ser eficiente nas condições estudadas, pois não houve alterações no valor nutricional do resíduo, porém, altas contagens de fungos e leveduras, e a presença de micotoxinas, podem sugerir que o material tenha alto risco de degradação
Thomson, Sean Richard. "Methane Production by a Packed-Bed Anaerobic Digester Fed Dairy Barn Flush Water". DigitalCommons@CalPoly, 2014. https://digitalcommons.calpoly.edu/theses/1329.
Texto completo da fonteMoreno, Izildinha. "Efeito de autólise de culturas lácticas na proteólise do queijo Prato". Universidade de São Paulo, 2003. http://www.teses.usp.br/teses/disponiveis/9/9131/tde-01092016-175444/.
Texto completo da fonteThis paper reports a study aimed at evaluating the variations that occur in the interrelationship between autolysis of lactic starter bacteria and the development of proteolysis in Prato cheese produced in four different regions of Brazil: Santa Catarina (Cheese A), Goiás (Cheese B), São Paulo (Cheese C) and Minas Gerais (Cheese D). Quantitative analysis of microbial population yielded similar microbiological profiles for all the cheese samples investigated. After 5 days ripening, lactococci and streptococci were present in higher numbers than mesophilic and thermophilic lactobacilli, leuconostoc and lactate fermenting bacteria. However, the populations of the latter species had considerably increased by the time the ripening process completed 45 days. Enterococci and citrate fermenting bacteria remained present in relatively low numbers throughout ripening. The findings from qualitative analysis confirmed the predominance of non-starter lactic acid bacteria (NSLAB) in the cheeses from four different origins, especially Lactobacillus sp. Other genera of non-starter lactic acid bacteria (NSLAB) were identified in smaller proportions: Enterococcus sp., Pediococcus sp., Aerococcus sp., Tetragenococcus sp. and Streptococcus sp. Cheese C differed from the cheeses in that it no evidence was found of the presence of Pediococcus sp. and Streptococcus sp. The bacteria of the lactic starter culture Lactococcus lactis sp. and Leuconostoc sp. were also found to be present, although in lower numbers. Autolysis was studied by: (1) determination of aminopeptidase activity; (2) detection of autolysins by zymograms and (3) detection of intracellular enzymes by immunoblotting. The release of aminopeptidase was highest in cheese D, followed by C, B and A. No bands of lytic activity were appeared in the zymograms of Cheeses A and B in all conditions evaluated. At pH 7,4 and 44°C, a low-intensity band of 30 KDa was found in cheeses C e D, whereas another low-intensity band was observed only in cheese D. At pH 6,8 and 42°C, bands of 40KDa were observed in cheese C (low intensity) and cheese D (high intensity), in addition to two more low-intensity bands of 90KDa and 110KDa in cheese D. Immunoblotting with antiserum anti-Lc produced only minor signs of positive reaction, evidenced by the formation of low-intensity bands of 100 Kda in cheeses A and B and two high-intensity bands of 75 Kda and 100 Kda in cheeses C and D. Since these were present in smaller numbers to those revealed with crude cytoplasm of Lac. lactis subsp. lactis, it was concluded that autolysis did practically non occur. Immunoblotting with antiserum anti-D-LDH also detected sings of positive reaction in cheeses A and B, whereas in cheeses C e D positive high-intensity signs of 37Kda were found relative to D-LDH protein, indicating lysis of Lab. helveticus. The evolution of proteolysis was determined quantitatively during the ripening process and evaluated on the basis of the following parameters: NS-pH4,6/NT% and NNP/NT% indexes, tyrosine content, electrophoresis (Urea-PAGE) and quantification of free amino acids. No significant differences were found between cheeses A, B, C and D in the ear1y stages of ripening. However, with the on-going fragmentation of proteins during ripening, a gradual increase of the ripening indexes occurred, with the highest values being observed in cheese D, followed by C, B e A. The electrophoretic profiles were similar for the four cheeses investigated and clear1y showed that the clotting agent or milk coagulant and plasmin were responsible for the initial breakdown of the caseins. The degradation rate of Q.sl- and p-casein followed the following order: D > C ≥ B > A. The buildup of free amino acids was also faster in cheese D, followed by cheeses C, B e A. At the end of the ripening process studied (45 days), the volatile compounds were identified using gas chromatography and mass spectrometry (GC-MS), whereas the instrumental texture profile was measured and evaluated by Texture Profile Analysis (TPA). Cheese samples were evaluated by descriptive and quantitative sensory analysis. With rare exceptions, the cheeses of four different origins contained the same volatile compounds, although in different quantities. Alcohols and esters were the predominant volatile compounds in cheeses A and B and benzaldehyde, 3-methyl-butanal-2 and hexanal in cheeses C and D. Autolysis of Lb. helveticus accelerated proteolysis in cheese D, thereby reducing ripening time by 45% without any negative effect on either flavor or texture development. Cheeses B, C and D exhibited the most typical Prato cheese characteristics, in spite of the fact that the buttery aroma and sweet taste were more pronounced in cheese D. Cheese A was rated as the cheese with the less typical overall Prato cheese profile and was also the one that exhibited the highest degree and number of flavor defects, notably aftertaste and bitterness. The cheeses investigated did not present any significant differences as to elasticity and cohesiveness. Minor changes in the physical-chemical composition of the cheeses - mainly related to the moisture and casein levels - influenced parameters such as firmness and adhesiveness. The present study demonstrates for the very first time the absence of autolysis of Lc. Lactis sp. in Prato cheese from four different origins, as well as the occurrence of autolysis of Lb. helveticus in two of the cheeses analyzed (cheeses C and D). The pronounced autolysis of this species had a positive impact on proteolysis and was responsible for the release of increased quantities of free amino acids in these cheeses. The differences in the evolution of proteolysis observed between cheeses C and D - lower rate of proteolysis in cheese C, in spite of pronounced autolysis of Lb. helveticus - were attributed to poor uniformity of the physical-chemical composition of this cheese, particularly as related to pH and the salt and moisture levels (S/M).
El, Tholth Mahmoud Mohammed El Sayed. "Microbiological risk assessment at the human-animal interface : assessment of human exposure to Mycobacterium avium subspecies paratuberculosis, highly pathogenic avian influenza virus subtype HN51 and Brucella spp". Thesis, Royal Veterinary College (University of London), 2010. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.558962.
Texto completo da fonteBeard, Martin Gale. "The impact of intrinsic and extrinsic factors on the safety and quality of hard and semi-soft natural cheese". Manhattan, Kan. : Kansas State University, 2009. http://hdl.handle.net/2097/1422.
Texto completo da fonteSouto, Luís Ivan Martinhão. "Associação entre o índice de mastite em rebanhos bovinos leiteiros e a qualidade microbiológica do leite cru no Estado de São Paulo, Brasil". Universidade de São Paulo, 2006. http://www.teses.usp.br/teses/disponiveis/10/10134/tde-30052007-152355/.
Texto completo da fonteThe purpose of this research was to investigate the possible correlations between the mastitis rate and raw milk microbiology quality, from 36 dairy farms, in São Paulo State, Brazil. It was investigated 4662 mammary quarters of 1180 lactant animals to examine mastitis cases using Tamis test and CMT. It was collected one sample of each positive mammary quarter in one test at least to microbiological analysis. To estimate the raw milk microbiological quality, it was colected one sample from each farm and realized one aerobic plate count of microorganisms mesophilic, aerobic plate count of microorganisms psychrotrophic, aerobic plate count of microorganisms termophilic, Enterococcus spp. plate count, Stahylococcus spp. plate count, Streptococcus spp. plate count, Corynebacterium spp. plate count, Yeast and Molds plate count, Most Probable Number of coliforms, Most Probable Number of fecal coliforms. It was used Pearson Correlation test and Linear Regression. In order to compare mastitis rates, the best correlation was between positives CMT test rate and the cases of mastitis caused by infections disease (r = 0,920 and R2 = 84,7%). Analysing the mastitis rate and the raw milk microbiological quality, the best result of correlation was between Staphylococcus mastitis rate and the aerobic plate count of microorganisms termophilic (r = 0,522 e R2 = 27,3%). Because of the low number of significant correlation, it was observed that the mastitis heard in dairy bovines herds do not interfere in raw milk microbiological quality, in the condition of this experiment.
Munoz, Vargas Lohendy M. "Impact of Metabolic Stress, Microbiome, and Lymph Node Colonization on Salmonella Shedding in Dairy Cattle". The Ohio State University, 2017. http://rave.ohiolink.edu/etdc/view?acc_num=osu1492625962680584.
Texto completo da fonteLouw, Celmarie. "Factors influencing the bacteriological quality of raw milk produced on dairy farms in Central South Africa". Thesis, Bloemfontein : Central University of Technology, Free State, 2013. http://hdl.handle.net/11462/204.
Texto completo da fonteIntroduction Dairy farms in central South Africa produce a substantial amount of milk, which is sold in Bloemfontein, Free State. Large volumes of unpasteurized (raw) milk is collected on the dairy farms, which undergoes further processing before it reaches the consumer at the end of the production line. There is a large proportion of the population that, in most cases unknowingly, consumes raw milk that has bacterial counts substantially higher than legal standards. Poor quality unpasteurized milk is either sold as fresh milk in the informal market, or as dairy products, such as cheese, manufactured from unpasteurized milk. Consumers are therefore, in most cases, unaware of the poor quality dairy products they consume. Milk quality is usually assessed in terms of bacterial content, which include Escherichia coli, coliforms and total bacterial count. The bacterial quality of milk is influenced by a number of factors, including farming practices, structural design of the milking shed, herd health and quality of water used in the dairy. If the highest level of hygiene practices is maintained, contamination of the milk by pathogenic microorganisms will be controlled, however, any drop in the vigilance of hygiene practices could result in unacceptable high levels of pathogenic microorganisms resulting in poor quality raw milk. Poor quality raw milk will inevitably result in poor quality pasteurized milk, containing unacceptably high levels of pathogenic organisms, which will eventually reach the consumer. Objectives The objectives of this study were to assess the quality of milk and influencing factors of milk produced on 83 dairy farms that supply milk intended for further processing to the greater Mangaung region, Central South Africa. Influencing factors investigated included, water quality and hygiene of milk contact surfaces, namely pulsator surfaces and milk pipeline surfaces. Methods Standard sampling procedures were followed when milk was sampled from bulk milk tanks, water at the point of use in the dairy, as well as collection of surface swabs. Escherichia coli, coliforms, total bacterial counts and somatic cell counts in milk were determined in terms of the regulations relating to milk and dairy products, and for water in terms of drinking water standards. These data were analysed and the factors that directly influence bacterial quality of milk were identified. Results 93% of the dairy farms displayed E. coli in their bulk milk containers, which did not comply with the legal standard. For coliforms, 86% of the milk samples did not comply with the legal standard. The total bacterial count of 85% of the milk samples did comply with the legal standard. The somatic cell count of 42% of the milk samples did not comply with the legal standard. The pulsator surfaces as well as the milk pipeline surfaces of 13% of the dairy farms displayed the presence of E. coli. 80% of the pulsator surfaces and 78% of the milk pipeline surfaces did comply with the legal standard pertaining to coliforms. The total bacterial count of pulsator surfaces revealed that 19% complied, whereas 29% of the milk pipeline surfaces complied with the legal standard. The water data further revealed that 31% of the dairy farms contained E. coli in the water used in the dairies. 63% of the dairy farms contained more than the allowable number of coliforms in their water. Chi-square tests revealed significant differences (p > 0.05) between the presence or absence of E. coli in milk and water; the presence or absence of E. coli in milk and milk pipeline surfaces; the presence or absence of E. coli in milk and pulsator surfaces and the presence or absence of E. coli in milk and the positioning of the cows in the milking shed. When milk quality indexes were calculated for all the farms, only four farms were classified with excellent milk, the remainder were all classified as producing poor quality milk. The hygiene quality indexes revealed that the hygiene practices on all the farms were not up to standard. Discussion and conclusion The study revealed that the milk produced for commercial processing and distribution in the greater Mangaung region of central South Africa was of poor quality. It is often mistakenly believed that the pasteurization process will remove all microorganisms from milk. As this is not the case, it is of major concern that milk delivered commercially is not of acceptable quality. Furthermore, it could be concluded that the quality of milk products from raw milk were also probably not of acceptable quality. The results further revealed that the possible contributing factors to the poor quality milk produced by the 83 commercial dairy farms were; poor quality water used in dairy sheds and contaminated milk contact surfaces. From this study it could be concluded that the overall status of milk production on the 83 commercial dairy farms studied, did not meet the standards required for milk quality, water quality and hygiene practices.
Yohe, Taylor. "Performance and Development of the Rumen in Holstein Bull Calves Fed an Aspergillus oryzae Fermentation Extract". The Ohio State University, 2014. http://rave.ohiolink.edu/etdc/view?acc_num=osu1397769968.
Texto completo da fonteSadik, Mohamad Shabir 1959. "MICROBIAL PROTEIN FLOW TO THE SMALL INTESTINE OF COWS FED DIFFERENT PROTEIN SUPPLEMENTS". Thesis, The University of Arizona, 1987. http://hdl.handle.net/10150/292012.
Texto completo da fonteWinckler, João Pedro Pereira. "Estratégias de vedação e adição de benzoato de sódio no controle de perdas em silagens de milho e desempenho de vacas leiteiras". Universidade de São Paulo, 2015. http://www.teses.usp.br/teses/disponiveis/11/11139/tde-17092015-145557/.
Texto completo da fonteSealing strategies have been adopted to reduce oxygen entrance to silo. Chemical additives such as sodium benzoate have antimicrobial activity and it can also promote an aerobic stability on silage. Nevertheless it is still unknown if sodium benzoate supplementation on silage may affect animal consumption or cause deleterious effect on metabolism with influence on animal performance. The objective of this study was using different sealing strategies to assess dry matter loss and nutritional value on corn silage, and the influence of supplementing sodium benzoate on total mixed ration for dairy cattle. This trial was conducted at Animal Science Department of Luiz de Queiroz College of Agriculture (ESALQ/USP). Corn crop was harvested with 35% of dry matter (DM) and ensiled on horizontal silos (40 t capacity). A factorial design (2x2) for silo sealing and benzoate as an additive on dietary feed were evaluated. Silo sealing strategies were confected as follows: (1) Plastic film doubled-sized 200 μm covered with bagasse (layer thickness 10 cm) (BG) and 2) application of sodium benzoate on top surface of ensiled mass pulverizing 150 g m-2 (dilution of 1:4) sealing it immediately with plastic film double-sided 200 μm (BZ). After 343 days of storage, the silos were open and the lactation trial started. Two dietary treatments evaluated the addition sodium benzoate on feed mixture of total ration. Sodium benzoate was incorporated (+ 0.15 % on total feed) on corn silage from BG and BZ and no incorporation to BG and BZ were used as control treatment. Dietary sodium benzoate was diluted on water (0.3:1 ratio) and pulverized on total ration immediately before each meal. Feed formulation: 8% cottonseed meal, 9.5% citric pulp, 18% soybean meal, 9% dry corn meal, 2.5 % vitamin and mineral premix, and 53% of corn silage. Twenty Holstein cows lactating were allocated in five Latin squares (4 x 4) during 21 days (14 days to acclimate) and fed twice a day. Dry matter intake (DMI), milk yield and quality were recorded between day 15th and 21st from each experimental period. Data were subjected to MIXED procedure from SAS for factorial design (2x2). The silage with sugarcane bagasse coverage was more effective in reducing the oxygen input during the fermentation process and consequently led to lower growth of spoilage microorganisms and better conservation of silage nutrients, resulting in increased digestibility of dry matter. Adding 0.15 % of sodium benzoate on fresh matter diet doesn\'t affect the performance of dairy cows.
Roncatti, Roberta. "Desenvolvimento e caracterização do queijo Santo Giorno, típico do sudoeste do Paraná, produzido com leite cru e fermento endógeno". Universidade Tecnológica Federal do Paraná, 2016. http://repositorio.utfpr.edu.br/jspui/handle/1/1773.
Texto completo da fonteTwo cheese formulations made from raw milk and endogenous yeasts with 30, 60 and 180 days of maturation in two dairy Paraná Southwest were studied to evaluate their quality through physical, physical-chemical, microbiological and sensorial characteristics, as one of the stages of development of a typical regional cheese. The production was accompanied from designing the flowchart processing, where the samples were collected to perform the analysis of proteins, lipids, moisture, ash, carbohydrates, total solids, fat in dry matter, calories; water activity, instrumental texture (hardness, adhesiveness, springiness, cohesiveness, resiliency and chewiness), instrumental color (CIE Lab); microbiological quality was assessed searching for total and thermotolerant coliforms, coagulase positive staphylococci and Salmonella spp.; the acceptance related to sensory characteristics of color, appearance, flavor, texture, taste and purchase intent was evaluated through the structured hedonic scale. This research contributed information relevant to the production process, such as the realization of the viability in freeze-drying lactic acid bacteria yeast isolated from milk in the Southwestern Mesoregion of Parana and the results of the analysis of the cheese showed similarity between formulations, regarding the physical, physical-chemical characterization, moreover good microbiological quality, where the differences between samples of dairy products were not perceived by sensory panelists. Adjustments in standardization related to technological quality control is an extremely important factor for the success of dairy companies and small producers involved in the project and that they have the option of producing the Santo Giorno, a fine cheese, with the great advantage of adding features of region, with high standard of sanitary conditions and with great consumer acceptance of indicative.
Effati, Pedram. "Survey Of Genes Of Escherichia Coli Causing Bovine Mastitis With DNA Microarrays". Thesis, Uppsala universitet, Institutionen för medicinsk biokemi och mikrobiologi, 2011. http://urn.kb.se/resolve?urn=urn:nbn:se:uu:diva-154988.
Texto completo da fonteJaudou, Sandra. "Metadetect : detection of Shiga toxin-producing Escherichia coli with novel metagenomics approaches and its application on dairy farms in France and Germany". Electronic Thesis or Diss., Maisons-Alfort, École nationale vétérinaire d'Alfort, 2023. http://www.theses.fr/2023ENVA0004.
Texto completo da fonteCurrent methodologies for characterization of Shiga toxin-producing Escherichia coli (STEC) require strain isolation, which is complicated by the fact that there is no specific isolation medium that clearly distinguishes STECs from non-pathogenic commensal E. coli. Therefore, obtaining strain information using a metagenomics approach would avoid isolating a strain to fully characterize it. In the framework of the project, in collaboration with the BfR in Germany, we will evaluate whether new, long-read metagenomics approaches could unambiguously determine whether specific markers of typical EHECs (Enterohemorrhagic E. coli) are co-located in the same strain. Third generation hybrid sequencing approaches will be evaluated. Appropriate bioinformatic pipelines developed in collaboration with the BfR will be evaluated to analyze the metagenomic analysis results. These methods will be applied in a pilot study to study the microbiota of raw milk from French and German dairy farms and to tentatively identify a common STEC-associated microbiome. We aim to define a ‘molecular score' based system to identify the status of the farms, in line with the objective to better precise the notion of ‘STEC molecular risk assessment approach' at the farm level
Wetzel, Amy Noel. "Studies in Shiga toxin-producing Escherichia coli O157:H7 determination of factors contributing to the dissemination of Escherichia coli O157:H7 among dairy farms /". Columbus, Ohio : Ohio State University, 2005. http://rave.ohiolink.edu/etdc/view?acc%5Fnum=osu1133239436.
Texto completo da fonteFowler, Colleen Marie. "Evaluation of 2-Hydroxy-4-(methylthio) Butanoic Acid Isopropyl Ester and Methionine Supplementation on Efficiency of Microbial Protein Synthesis and Rumen Bacterial Populations". The Ohio State University, 2009. http://rave.ohiolink.edu/etdc/view?acc_num=osu1248875016.
Texto completo da fonteHolder, Vaughn B. "THE EFFECTS OF SLOW RELEASE UREA ON NITROGEN METABOLISM IN CATTLE". UKnowledge, 2012. http://uknowledge.uky.edu/animalsci_etds/6.
Texto completo da fonteVasconcelos, Bruno Garcia. "Desenvolvimento de mix de açaí probiótico, prebiótico e simbiótico". Universidade de São Paulo, 2010. http://www.teses.usp.br/teses/disponiveis/9/9133/tde-13042010-093047/.
Texto completo da fonteSome studies have been showing that food products supplemented with probiotics and prebiotics, in sufficient amounts, result in benefits to human health. These benefits are related, fundamentally, to their effect on the healthy intestinal microbiota maintenance. Concomitantly, consumption of açai food products, mainly its pulp and derivatives, is increasing in urban centers in Brazil and also abroad. The high caloric value and the presence of antioxidant pigments are responsible for its higher consumption. The main aim of the present study was to develop an açai mix with nutritional and sensory aspects similar to the conventional product, but with a supplementary functional property, by being a probiotic, prebiotic or synbiotic food. Four trials where produced (three times each), all containing frozen açaimix: M1 (control), M2 (supplemented with L. acidophilus La-5 + B. animalis subsp. lactis Bb-12), M3 (supplemented with inulin) and M4 (supplemented with L. acidophilus La-5 + B. animalis subsp. lactis Bb-12 + inulin) and stored at -18 °C for up to 3 months. After 1, 7, 14, 21, 28, 56 and 84 days of storage, the products were analyzed for probiotic microorganisms populations, pH and instrumental color. The moisture content was determined soon after production (on day 0). Additionally, after 7, 42 and 84 days of production, sensory evaluation (acceptability test) was carried out. Finally, compositional analyses proceeded from freeze-dried samples. Results were compared through statistical analysis. Differences in compositional analyses and moisture content between trials were attributed to the presence or absence of inulin. Instrumental color and pH evolution were not influenced by the storage period and also no differences between the different acaimixes studied were observed (p > 0,05). Products were well accepted by the panellists, and mean scores were often above 7. Prebiotic fiber inulin improved overall acceptability of açaimixes and the synbiotic mix obtained higher mean score (p < 0.05) in two storage periods (7 and 84 days), when compared to the others. The storage period did not influence sensory evaluation significantly (p > 0.05). During the storage period studied, probiotics showed a satisfactory survival (viability higher than 108 cfu for the products daily portion), according to the current Brazilian legislation, except for B. animalis subsp. lactis in the mix not supplemented with inulin. The açaimix showed to be a good matrix for the probiotic microorganisms tested and inulin contributed for a higher acceptability of the product.
Sanad, Yasser M. "Molecular Epidemiological and Pathogenesis Studies on Campylobacter Species in Cattle and Sheep". The Ohio State University, 2011. http://rave.ohiolink.edu/etdc/view?acc_num=osu1322032603.
Texto completo da fonteLisita, Milena Olivieri. "Evolução da população bacteriana na linha de produção do queijo minas frescal em uma indústria de laticínios". Universidade de São Paulo, 2005. http://www.teses.usp.br/teses/disponiveis/11/11141/tde-09092005-142314/.
Texto completo da fonteThe evaluation of aerobic mesophilic, of total and fecal coliforms and Staphylococcus positive coagulase microorganisms population in a dairy processing line of "Minas frescal" cheese submitted to inspection of Federal Service was studied. Three processing steps were analysed individually: the pasteurisation through samples of raw and pasteurised milk; the coagulation through samples of pasteurised milk, cut and drained curd; and the salting through samples of cheeses before and after salting and brine itself. The aerobic psichrotrophic microorganims count was made because salting was carried out under refrigeration. After, all the samples of a same allotment were collected. In one year 11 collections were taken and analysed. The results showed that the pasteurisation, the unique control critical point in the process, was not able to ensure the microbial quality of milk in agreement to the microbial standards, due to the bad quality of the raw milk. On curding the aerobic mesophilic population had an average growth of 1.70 cycles log and the fecal coliforms had an average growth of > 3.0 cycles log. On salting the aerobic mesophilic microorganisms had an average growth of 0.73 cycles log as well the aerobic psichrotrophic population had an average growth of 0.37 cycles log. In the processing line, had an average growth of 11.77 cycles log on the population of total coliforms and >9.68 cycles log on the population of fecal coliforms from pasteurised milk until the cheese after salting. An expressive increase of the number of Staphylococcus positive coagulase was not detected. The results indicated that the manufactured "Minas frescal" cheese was improper for consumption even before packing because the high counting of total and fecal coliforms, being harmful to consumers and the processing was responsible for the high contamination, being a potential public health problem.
Moloto, Phuti Gladys. "Identification of the dominant bacteria associated with the spoilage of UHT full cream milk". Thesis, Vaal University of Technology, 2016. http://hdl.handle.net/10352/457.
Texto completo da fonteThe Organization for Economic Co-operation and Development (OECD) and the Food and Agriculture Organization (FAO) of the United Nations predict that milk production and the dairy sector will remain one of the fastest-growing agricultural subsectors over the coming decade. The global milk production is projected to expand over the 2011-2020 period at an annual rate of 2%. In South Africa alone, approximately 14 – 15 million litres of milk are wasted annually due to microbial spoilage. Therefore, the identification of the spoilage microorganisms in the milk products is necessary. This will contribute towards the design of appropriate measures to prevent wastage due to spoilage and in turn contribute towards sustainability of the sector. Accordingly, one hundred samples of spoiled full cream UHT milk were collected from two plants of each of the two largest milk processors. These samples were examined visually, and the pH was measured. A presumptive identification up to genus level was conducted by examining morphological features and conducting Gram-stain, catalase and oxidase tests. Species-specific identification was done by using the Analytical Profile Index and Biolog system. Molecular profiling was done by sequencing the rDNA genes. The main spoilage organisms identified in the samples were Pseudomonas, Micrococcus, Bacillus, Enterococcus and Lactobacillus. All organisms belonging to the five genera were psychrotrophs, which are commonly found in biofilms in UHT milk processing equipment. Therefore, according to the study, the spoilage bacteria apparently entered into the milk due to inadequate cleaning-in-place (CIP) processes. More importantly, further studies should be conducted in order to identify the spoilage microbes and how CIP processes can be improved.
DELLA, SCALA GIULIA. "STREPTOCOCCUS THERMOPHILUS UREASE ACTIVITY: PHYSIOLOGICAL ROLE AND TECHNOLOGICAL RELEVANCE IN DAIRY AND NON-DAIRY APPLICATIONS". Doctoral thesis, Università degli Studi di Milano, 2018. http://hdl.handle.net/2434/604396.
Texto completo da fonteDias, Juliana. "Characterizing the gastrointestinal tract microbiota of dairy calves". Universidade Federal de Viçosa, 2017. http://www.locus.ufv.br/handle/123456789/13065.
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Ao nascimento, os bezerros exibem um trato gastrointestinal subdesenvolvido (TGI) cuja maturação é estritamente relacionada à colonização da microbiota. No entanto, pouco se sabe sobre os fatores que afetam o estabelecimento de comunidades de archaeas, bacterias e de fungos anaeróbicos no TGI dos bezerros, bem como as mudanças na estrutura e abundância desses grupos microbianos durante o período de transição da fase de pré-ruminante para verdadeiro ruminante. Para abordar essas lacunas no conhecimento, este trabalho empregou sequenciamento de próxima geração para caracterizar a microbiota do TGI de bezerros leiteiros mestiços (Holandês-Gir) durante o período pré-desmame. O primeiro estudo avaliou mudanças nas comunidades de archaeas metanogênicas, bacterias e fungos anaeróbicos no rúmen de bezerros leiteiros (n = 45) alimentados com duas dietas diferentes (M: somente leite cru (10% do peso vivo (PV)) e MC: leite cru (10% PV e concentrado ad libitum) e que foram abatidos aos 7, 28, 49, 63 dias de idade. No segundo estudo, caracterizamos as alterações nas comunidades bacterianas entre regiões GIT (rúmen, jejuno, ceco e cólon) de bezerros alimentados com MC (n = 17) que foram abatidos aos 7, 28, 49, 63 dias de idade. Os resultados do primeiro estudo revelaram que as comunidades de archaeas metanogênicas, bacterias e fungos coexistem no rúmen desde a primeira semana de vida, mas são afetadas diferentemente pela dieta e idade. A inclusão de concentrado na dieta de bezerros afetou significativamente a comunidade bacteriana do rúmen: observou-se um aumento na abundância de gêneros relacionados, direta e indiretamente, à degradação de amido (i.e. Megasphaera, Sharpea e Succinivribrio) e um decréscimo acentuado na abundancia de gêneros (i.e. Lactobacillus, Bacteroides e Parabacteroides) relacionados com a degradação de nutrientes do leite. Alterações na comunidade bacteriana, indiretamente afetaram a comunidade de metanogênicas: fermentação de carboidratos não fibrosos alterou padrões de fermentação (acetato:propionato) e disponibilidade de hidrogênio que por sua vez, favoreceu a colonização de Methanosphaera em vez de Methanobrevibacter. Na comunidade de fungos anaeróbicos, a abundância do genêro Caecomyces e família Neocallimastigaceae não variou significativamente com a dieta ou idade, provavelmente devido à alta variação inter-animal e baixo teor de fibra de concentrado usado em nosso estudo. In suma, este estudo mostrou que a manipulação da microbiota no rúmen em desenvolvimento é possível através da intervenção dietética. Nossos resultados podem ser úteis na elaboração de estratégias para promover a colonização de comunidades-alvo (isto é, produtores de butirato e utilizadoras de lactato) que estão ligadas ao desenvolvimento de papilas e equilíbrio do pH ruminal. Em relação ao segundo estudo, as comunidades bacterianas diferem qualitativa e quantitativamente entre os compartimentos (rúmen, jejuno, cécum e colón) do trato gastrointestinal e também respondem diferentemente ao avanço da idade que inclui a substituição progressiva da dieta líquida para a dieta sólida (i.e. aumento do consumo de concentrado). No rúmen, a comunidade bacteriana foi composta em sua maioria pelos gêneros Prevotella, Butyrivibrio e Ruminococcus cuja abundância aumentou proporcionalmente com a idade devido a maior disponibilidade de carboidratos não fibrosos no rúmen. No jejuno, o gênero Lactobacillus foi abundante desde a primeira semana de vida, mas sua dominância foi substituída por membros da família Clostridiaceae em bezerros mais velhos. As comunidades do ceco e do cólon foram compostas pelos gêneros Blautia, Paraprevotella, Prevotella Phascolarctobacterium and Succiniclasticum cuja abundância aumentou com a idade. Em resumo, nossos resultados mostraram que, embora comunidades bacterianas coexistam em regiões distintas do TGI, uma análise mais detalhada da estrutura, abundância e dinâmica dessas comunidades revela uma marcante segregação e sucessão ecológica no TGI de bezerros. Nosso estudo acrescenta novos insights sobre a colonização bacteriana no TGI de pré-ruminantes que podem servir como base para formulação de estratégias para promover a colonização de comunidades-alvo (i.e. bactérias probióticas) para melhorar a saúde e desempenho de bezerros leiteiros no período pré-desmame.
At birth, calves display an underdeveloped gastrointestinal tract (GIT) whose maturation is strictly related to microbiota colonization. However, little is known about the factors that affect the establishment of archaeal, bacterial and fungal communities in the GIT of calves, as well as the changes in their structure and abundance during calf development into a functional ruminant. To address these gaps in knowledge, this work employed next-generation sequencing to characterize the GIT microbiota of Holstein- Gyr crossbred dairy calves across pre-weaning development. The first study aimed to assess changes on the rumen archaeal, bacterial and fungal communities of crossbred dairy calves (n=45) across pre-weaning development (7, 28, 49, 63 days) on two different diets (M: only raw milk at 10% of body weight at birth (BW) and MC: raw milk (10% BW) plus starter concentrate ad libitum). In the second study, we characterized changes in the bacterial communities across GIT regions (rumen, jejunum, cecum and colon) of MC-fed calves (n=17) at 7, 28, 49, 63 days of age. The results of first study revealed that archaeal, bacterial and fungal communities co-occur in the rumen since early calf development but are impacted differently by pre-weaning diet and age. The inclusion of starter concentrate in the calf diet significantly affected rumen bacterial community by promoting increases of genera, direct and indirectly, related to degradation of readily fermentable carbohydrates (i.e. Megasphaera, Sharpea and Succinivribrio) and depressing those reliant on milk nutrients like lactose (i.e. Lactobacillus, Bacteroides and Parabacteroides). These bacterial changes resulted in apparent diet-driven archaeal differences due to altered fermentation patterns and availability of hydrogen in the rumen that favoured the colonization of members from genus Methanosphaera instead of Methanobrevibacter. No such differences were found for fungi community represented by members from genus Caecomyces and family Neocallimastigaceae, likely due to high inter-animal variation and low fibre content of concentrate used our study. Altogether, this study showed that manipulation of the microbiota in the developing rumen is possible through dietary intervention. Our results may be useful in designing strategies to promote colonization of target communities (i.e. butyrate- producers and lactate-utilizing) linked to functional development of the calf. In regards to second study, bacterial communities in the calf GIT differ qualitatively and quantitatively among compartments and respond differently to age advance that encompass the GIT development (i.e. rumen) and progressive replacement of milk- based to grain-diet (i.e. increase of starter concentrate intake). In the rumen, bacterial community was composed majority by members from genera Prevotella, Butyrivibrio and Ruminococcus whose abundance increased proportionally with age possibly due greater availability of readily fermentable carbohydrates in the rumen. Members from genus Lactobacillus were overrepresented in the jejunum but their predominance was replaced by members from Clostridiaceae family in older calves. The cecum and colon displayed similar abundance at taxa level and the abundance of genera Blautia, Paraprevotella, Prevotella, Phascolarctobacterium and Succiniclasticum increased significantly with age. In summary, our results showed that although there are bacterial communities “common” to distinct regions, a closer look at their structure, abundance and dynamic reveals marked segregation and ecological succession in the calf GIT. Our study adds new insights into bacterial colonization across GIT of pre-ruminant that may be considered in formulating strategies to promote the colonization of target communities aiming improve health (i.e. bacteria with probiotic capability) and performance of dairy calves in the pre-weaning period.
CARFORA, VIRGINIA. "Staphylococcus aureus and methicillin resistant staphylococcus aureus (mrsa) in dairy farms of central italy: a characterization of isolates from milk and dairy products and an in-farm epidemiological investigation on mrsa colonization of sheep and in-contact humans". Doctoral thesis, Università degli Studi di Roma "Tor Vergata", 2015. http://hdl.handle.net/2108/203186.
Texto completo da fonteSilvetti, T. "DEVELOPMENT OF INNOVATIVE TECHNIQUES FOR STUDYING MICROBIAL POPULATIONSIN MILK AND DAIRY PRODUCTS". Doctoral thesis, Università degli Studi di Milano, 2010. http://hdl.handle.net/2434/150173.
Texto completo da fonteColombo, Monique. "Beneficial properties and safety of lactic acid bacteria isolated from the dairy production environment". Universidade Federal de Viçosa, 2017. http://www.locus.ufv.br/handle/123456789/11610.
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Coordenação de Aperfeiçoamento de Pessoal de Nível Superior
Bactérias ácido lácticas (BAL) foram isoladas do ambiente de produção de leite e avaliadas quanto ao potencial benéfico. Testes preliminares e análise por PCR foram aplicados para selecionar e identificar através de sequenciamento de rRNA 16S 15 cepas de BAL: Lactobacillus (n = 11; Lb. casei MSI1, Lb. casei MSI5, Lb. casei MRUV1, Lb. casei MRUV6, Lb. acidophilus MVA3, Lb. nagelli MSIV4, Lb. harbinensis MSI3, Lb. harbinensis MSIV2, Lb. fermentum SIVGL1, Lb. plantarum MLE5 e Lb. plantarum MSI2), Pediococcus (n = 2; P. pentosaceus MLEV8 e P. acidilactici MSI7) e Weissella (n = 2; W. paramesenteroides MRUV3 e W. paramesenteroides MSAV5). Todas as linhagens selecionadas apresentaram resistência ao baixo pH e à presença de sais biliares. O teste API ZYM foi realizado para caracterizar a atividade enzimática entre as cepas e foi observada elevada atividade β-galactosidase em 13 delas. Todas as cepas apresentaram alta taxa de sobrevivência ao suco gástrico e as condições intestinais simulados, capacidade de auto-agregação e co- agregação com micro-organismos indicadores e alta hidrofobicidade da superfície celular. A maioria das cepas foi positiva para os genes de adesão map e EFTu. Os resultados de deconjugação de sais biliares mostraram forte desconjugação para todas as cepas. Todas as cepas mostraram bons resultados para assimilar lactose. Após esta etapa de caracterização do potencial benéfico, as 15 BAL foram avaliadas quanto ao potencial de virulência e de resistência antimicrobiana. A produção de fatores de virulência (hemólise, gelatinase, lipase, desoxirribonuclease e aminas biogênicas: lisina, tirosina, histidina e a ornitina) foi avaliada por métodos fenotípicos, a 25 °C e 37 °C, bem como a resistência a 17 antibióticos. Os isolados foram também submetidos à análise de PCR para identificar a presença de 49 genes associados a fatores de virulência. Nenhuma das cepas apresentou atividade hemolítica, produção de gelatinase, lipase, desoxirribonuclease e aminas biogênicas. Das 15 cepas selecionadas, para 12 tipos de antibióticos no método de difusão em disco, todas as amostras foram resistentes à oxacilina e sulfa/trimetoprim, 14 foram resistentes a gentamicina, 11 foram resistentes a clindamicina, nove cepas foram resistentes à vancomicina, oito cepas para rifampicina, cinco foram resistentes a eritromicina, quatro foram resistentes à tetraciclina, duas cepas foram resistentes à ampicilina, uma cepa foi resistente ao cloranfenicol e nenhuma apresentou resistência ao imipenem. Para um teste quantitativo do antibiograma, 5 antibióticos em fitas Etest® (bioMérieux) foram selecionados. Todas as 15 cepas foram resistentes à vancomicina, duas para rifampicina, uma para gentamicina e uma para o cloranfenicol. Em relação aos genes relacionados com virulência, 19 dos 49 genes testados estavam presentes em algumas cepas. Após a caracterização do potencial virulento das 15 BAL, estas foram avaliadas quanto ao potencial tecnológico para aplicação na indústria de laticínios. Todas as cepas apresentaram capacidade de acidificação, atingindo valores de pH entre 0.73 e 2.11 em 24 horas: Lb. casei MRUV6 apresentou maior capacidade de acidificação (pH 2.11 após 24 h). Dez cepas foram capazes de produzir diacetil a 37 °C, com exceção de Lb. casei MSI1, Lb. harbinensis MSI3, Lb. fermentum SIVGL1, Lb. plantarum MLE5 e W. paramesenteroides MRUV3. Todas as cepas foram capazes de produzir exopolissacarídeos, e apenas duas cepas apresentaram atividade proteolítica (Lb. casei MSI5 e W. paramesenteroides MSAV5). Com base nessa caracterização, Lb. casei MRUV6 foi selecionado para produzir o leite fermentado, armazenado a 4 °C e 10 °C e monitorado até 35 dias de vida útil. As amostras foram submetidas a métodos fenotípicos e moleculares para avaliar a presença de Lb. casei MRUV6 (plaqueamento convencional e RT-PCR, verificando a expressão de gapdh, um gene housekeeping) e verificar a expressão do gene bsh, relacionado à resistência à sais biliares (RT-PCR). A população de Lb. casei MRUV6 se apresentou estável durante todo o período de armazenamento a 4 °C e 10 °C a níveis em torno de 9.9 log UFC/g e também pelo monitoramento da expressão do controle endógeno GAPDH. No entanto, o gene bsh não foi expresso durante o período de armazenamento. O estudo demonstrou o potencial uso da cepa de Lb. casei MRUV6 isolada de um ambiente lácteo para a produção de um produto lácteo fermentado e sua estabilidade durante o armazenamento a 4 °C e 10 °C. Todos os isolados do estudo apresentaram características benéficas, segurança para utilização em alimentos e potencial tecnológico para utilização na indústria de laticínios. Além disso, os mesmos podem ainda ser submetidos a estudos adicionais para avaliações in vivo e realizar a caracterização como probióticos.
Lactic acid bacteria isolated from dairy environment were evaluated for beneficial potential. Preliminary screening and PCR analysis were applied to select and identified through 16s rRNA sequencing 15 LAB strains: Lactobacillus (n = 11; Lb. casei MSI1, Lb. casei MSI5, Lb. casei MRUV1, Lb. casei MRUV6, Lb. acidophilus MVA3, Lb. nagelli MSIV4, Lb. harbinensis MSI3, Lb. harbinensis MSIV2, Lb. fermentum SIVGL1, Lb. plantarum MLE5 and Lb. plantarum MSI2), Pediococcus (n = 2; P. pentosaceus MLEV8 and P. acidilactici MSI7) and Weissella (n = 2; W. paramesenteroides MRUV3 and W. paramesenteroides MSAV5). All selected strains showed resistance to acidic pH and to presence of bile salt. API ZYM test characterized enzymatic activity of the strains and high β-galactosidase activity was observed in 13 strains. All strains presented high values for survival rate to simulated gastric and intestinal conditions, ability to auto and co-aggregate with indicators microorganisms and high cell surface hydrophobicity. Most of the strains were positive for map and EFTu beneficial genes. Strong bile salts deconjugation was applied for all strains and all strains showed good results for assimilating lactose. After this first part of the study, the 15 BAL were evaluated for potential virulence and antimicrobial resistance. The production of virulence factors (hemolysis, gelatinase, lipase, deoxyribonuclease and biogenic amines: lysine, tyrosine, histidine and ornithine) was assessed by phenotypic methods at 25 °C and 37 °C, as well as the resistance to 17 antimicrobials. The isolates were also subjected to PCR to identify the presence of 49 genes associated with virulence factors. None of the strains presented hemolytic activity or the production of gelatinase, lipase, deoxyribonuclease and tested biogenic amines. Of the 15 selected cultures, for 12 types of antibiotics in the disc diffusion method, all strains were resistant for oxacillin and sulfa/trimethoprim, 14 were resistant to gentamicin, 11 were resistant to clindamycin, nine strains were resistant to vancomycin, eight strains to rifampicin, five were resistant to erythromycin, four were resistant to tetracycline, two strains were resistant to ampicillin, one strain was resistant to chloramphenicol and none was resistant for imipenem. For a quantitative test of the antibiogram, five antibiotics were selected in Etest ® strips (bioMérieux). All 15 strains were resistant to vancomycin, two for rifampicin, one for gentamicin and one for chloramphenicol. Regarding the virulence related genes, 19 genes from 49 tested were present in some strains. Results showed that five cultures showed the presence of the int gene, four cultures showed the presence of the ant(4')-Ia gene, three cultures were positive for vanC2, cpd and tdc, two cultures for vanA, tet(K), tet(S), ermA, bcrR, mur-2ed, asa1 and ccf, and one culture was positive for vanC1, ermB, aph(3')-IIIa, aac(6’)-le-aph(2”)-Ia, bcrB and hyl. After characterizing the virulent potential of the 15 BAL, these strains were evaluated for the technological potential for application in the dairy industry. All strains presented acidification capacity, reaching pH values between 0.73 and 2.11 in 24 hours: Lb. casei MRUV6 presented the highest acidification ability (pH 2.11 after 24 h). Ten strains were able to produce diacetyl at 37 °C, except by Lb. casei MSI1, Lb. harbinensis MSI3, Lb. fermentum SIVGL1, Lb. plantarum MLE5 and W. paramesenteroides MRUV3. All strains were able to produce exopolysaccharides, and only two strains presented proteolytic activity (Lb. casei MSI5 and W. paramesenteroides MSAV5). Based on this characterization, Lb. casei MRUV6 was selected for producing fermented milk, stored at 4 °C and 10 °C and monitored until 35 days of shelf life. Samples were subjected to phenotypical and molecular methods to quantify the presence of Lb. casei MRUV6 (conventional plating and RT-PCR, by checking the expression of gapdh, a housekeeping gene) and to verify the expression of bsh gene, related to resistance to bile salts (RT-PCR). Lb. casei MRUV6 population was stable during storage period at 4 and 10 °C at levels around 9.9 log CFU/g, and by monitoring the expression of gapdh gene. However, bsh gene was not expressed during storage period. The study demonstrated the potential use of the beneficial strain Lb. casei MRUV6 isolated from a dairy environment for the production of a fermented milk product, and its stability during storage at 4 and 10 °C. All isolates from the study presented beneficial characteristics, safety for use in food and technological potential for use in the dairy industry. In addition, they may further be subjected to further studies for in vivo evaluations and characterization as probiotics.
Arioli, S. "Carbon dioxide metabolism in Streptococcus thermophilus : physiological and ecological importance, and dairy applications". Doctoral thesis, Università degli Studi di Milano, 2008. http://hdl.handle.net/2434/50715.
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