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Heat Resistance in Vegetative Cells and Cysts of AzotobacterRosenthal, Raoul S. 08 1900 (has links)
The purpose of the current study is to determine something of the nature of the heat resistance in Azotobacter, if in fact this is found to exist. An attempt is made to determine the specific physiological state associated with heat resistance as well as to resolve this resistance quantitatively.
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Heat resistance and outgrowth of clostridium perfringens spores as affected by the type of heating medium, and heating and cooling rates in ground porkMarquez Gonzalez, Mayra 15 May 2009 (has links)
The survival and germination of Clostridium perfringens spores in different
heating media and at different heating rates was studied to determine the fate of C.
perfringens spores during abusive cooking and cooling of pork products. The heat
resistance (HR) of C. perfringens spores from three strains that were either previously
heat shocked (HS) or non-heat shocked (NHS) was determined individually and as a
cocktail in phosphate buffer solution (pH 7.4) (PBS), beef gravy (BG), ground pork (GP)
and cured ground pork (CGP) at 75ºC. The effect of the heating rate on HR, germination
and outgrowth of C. perfringens spores in CGP was determined by increasing the
temperature from 20 to 75ºC at a rate of 4, 8, and 12ºC/h prior to heating and holding at
75ºC for 48 h. Heating rates at 4ºC/h in GP and CGP were repeated with additional
cooling from 54.4 to 7.2ºC within 20 h (temperature abuse).
Linear survival curves were observed on NHS spores in the four heating media,
whereas HS spores showed linear curves when heated in PBS and BG, and biphasic
curves when heated in GP and CGP. In general, HS spores were more heat sensitive than NHS spores. NHS spores heated in GP had greater HR than spores heated in CGP, BG
or PBS.
There were no significant differences (P>0.05) on the HR of C. perfringens
spores in CGP heated from 20 to 75ºC at 4, 8, or 12ºC/h. Heating rates of 8 and 12ºC/h
showed no difference in germination and outgrowth of inoculated spores, whereas at
4ºC/h, growth of C. perfringens occurred between 44 and 56ºC.
Temperature abuse during cooling of GP resulted in 2.8 log CFU/g increase of C.
perfringens counts. In CGP, C. perfringens counts decreased by 1.1 log CFU/g during
cooling from 54.4 to 36.3ºC and then increased by 1 log CFU/g until the product reached
7.2ºC. However, with an initial inoculum in raw CGP of 5 log CFU C. perfringens
spores/g, C. perfringens counts did not exceed 3.4 log CFU/g during a 20 h abusive
cooling. These results suggest there is no risk associated with C. perfringens in cured
pork products under the conditions tested. Results from the present study indicate that
different behavior may be expected with different meat products.
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Isolation and characterization of potential indicator bacteria to be used for validation of Escherichia coli O157:H7 reduction in beef slaughter plant critical control pointsMagana Yepez, Maria Belem 01 November 2005 (has links)
Microbiological detection of foodborne pathogens is ineffective for monitoring critical control points (CCP) within a slaughter/processing Hazard Analysis and Critical Control Point (HACCP) system. Pathogens are usually absent from carcass surfaces and their uneven distribution makes it difficult to obtain a representative sample. However, microbiological testing can be applied within a HACCP plan to validate and verify the effectiveness of decontamination procedures designed to control hazards. With proper data collection, the reduction of an indicator group at a point in processing can indicate that a specific pathogen is being effectively controlled, especially when pathogen levels are too low to allow confirmation of process control, as they typically are in beef slaughter processing. Since E. coli O157:H7 has been shown to have some acid resistance, the ability of typical indicator organisms to accurately predict the reduction of this pathogen by carcass decontamination procedures has been a concern. Obtaining potential indicator bacteria from the same environmental reservoir as E. coli O157:H7 may provide non-pathogenic indicators with similar heat- and acid-resistance characteristics suitable for use in processing plant environments for validation and verification of carcass decontamination treatments within HACCP plans.
Potential indicator bacteria were isolated from hides of cattle at slaughter facilities in Arizona, Georgia, and Texas and compared with isolates of E. coli O157:H7 from the same locations to determine similarity in acid- and heat-resistance characteristics. After evaluation at 2 heating temperatures (55 and 65??C) and 3 pH levels (3.0, 4.0, and 5.0), it was determined that several potential indicator bacteria were slightly more resistant than E. coli O157:H7 to heating and acid treatment. The greatest reduction in numbers for E. coli O157:H7 and indicator bacteria occurred at pH 3.0 and temperature of 65??C. Counts of bacteria grown at pH 4.0 and 5.0 were not significantly different.
Testing indicated that several of the isolates from cattle hides would make good process control indicators since the indicator bacteria were reduced by heating or acid conditions at similar or greater rates when compared to E. coli O157:H7, providing an increased level of security that pathogens have been reduced in processing.
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Factors Affecting the Heat Resistance of Clostridium perfringens SporesOrsburn, Benjamin 09 June 2009 (has links)
The bacterium Clostridium perfringens is a gram-positive anaerobe responsible for many diseases in man and other animals, the most common of which is acute food poisoning (AFP). It is estimated that nearly 240,000 cases of AFP occur each year in the U.S. The C. perfringens spore plays an important role in this infection. The heat resistance of the spore allows the organism to survive the cooking process, grow in the cooling food, and infect the victim. Despite the occurrence of this disease and the importance of the spore to this process, little work has been performed to determine how heat resistance is obtained and maintained by C. perfringens spores.
In this work we study the spores and sporulation process of C. perfringens to determine what factors are most important in the formation of a heat resistant spore. We analyzed the spores produced by nine wild-type strains, including five heat-resistant food poisoning isolates and four less heat-resistant environmental isolates. We determined that threshold core density and a high ratio of cortex peptidoglycan relative to germ cell wall were necessary components of a highly heat-resistant spore. In order to test these observations, we constructed two mutant strains. The first could not achieve the necessary level of core dehydration and rapidly lysed in solution. The second mutant had a reduced amount of cortex relative to germ cell wall, and suffered a corresponding decrease in heat resistance as compared to our wild-type strains. The mutant strains supported the observations drawn from our wild-type strains.
Dipicolinic acid is a major component of bacterial spores and is necessary for spore heat resistance. The Cluster I clostridia, including C. perfringens, lack the known DPA synthase operon, spoVF. We developed an in vitro assay for detecting DPA synthetase activity and purified the active enzyme from sporulating C. perfringens crude extract and identified the proteins with mass spectrometry. These results identified the electron transfer flavoprotein alpha chain (EtfA) as the DPA synthase of C. perfringens. Inactivating the etfA gene in C. perfringens resulted in a strain that could begin, but not complete, the sporulation process and produced dramatically lower amounts of DPA than the wild-type. The purified enzyme was shown to produce DPA in vitro and utilized FAD as a preferred cofactor.
The results of this research may lead to future techniques to decrease the occurrence of the diseases caused by C. perfringens spores and treatments which may carry over to the diseases caused by similar organisms. / Ph. D.
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Fire Environments Typical of Navy ShipsLeBlanc, David 01 May 2002 (has links)
Current test methodologies used to evaluate the performance of protective clothing do not adequately determine the provided level of protection. The heat fluxes imposed by current evaluation methods are not specifically related to fire environments typical to those the clothing is designed provide protection against. The U.S. Navy is in the process of developing an improved process for testing the fire resistance of daily wear uniforms and protective gear. The first phase of this project involves evaluating currently used evaluation methods and identifying the severity of fire environments that would be expected aboard Navy ships. The examination of the test protocols currently in use identifies major weaknesses, providing the justification for a new test protocol. The first step in developing an improved test protocol is to determine the types of fire scenarios that would be expected aboard Navy vessels. The nearly infinite number of possible fires are reduced to 6 typical cases involving spray fires, pool fires and furniture fires in both compartmented and unconfined cases. An analysis of the environments produced by these types of fires is presented. The effects of compartmentation parameters are also investigated to determine the critical factors that affect the expected fire environment. Expected heat fluxes for all scenarios are presented at a number of distances from the fire.
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Descrição do comportamento da cepa de Salmonella Enteritidis PT4 frente ao tratamento térmico a 60,0°C por três minutos e meio, em ovo integral pasteurizado desidratado reconstituído / Description the behavior of Salmonella Enteritidis PT4 undergoing thermal treatment at 60°C for 3 ½ minutes, in reconstituted dried-wole eggToledo, Paula Spinha de 03 December 2003 (has links)
O presente trabalho objetivou descrever o comportamento da cepa Salmonella Enteritidis (S. Enteritidis) PT4, frente ao tratamento térmico a 60,0º C por três minutos e meio, em ovo integral pasteurizado desidratado reconstituído, interrelacionando a termorresistência com temperatura prévia de incubação e concentração de microrganismos. Foram realizadas 150 análises, das quais 75 foram trabalhadas com cepa previamente incubada à 35ºC e 75 com cepa incubada à 43ºC. Cada um destes grupos foi subdividido em três subgrupos, inoculado-se as concentrações de 10³, 105 e 108 unidades formadoras de colônia (UFC)/mL de caldo BHI. Após inoculação, foi simulada pasteurização do ovo, a 60,0ºC por 3,5 minutos, em banho-maria, e, posteriormente, realizadas contagem em placa (UFC) e Número Mais Provável (NMP), para verificação da concentração de S. Enteritidis sobrevivente. O tempo de redução decimal (valor D) foi de 2,54 e 2,57 minutos para S. Enteritidis previamente incubada à 35ºC e inoculada nas concentrações de 105 e 108 UFC/mL de caldo BHI, respectivamente. Para S. Enteritidis previamente incubada à 43ºC e inoculada nas concentrações de 105 e 108 UFC/mL de caldo BHI, o valor D foi de 2,58 e 2,40 minutos, respectivamente. Não foi possível o cálculo do valor D para a concentração 10³ UFC/mL de caldo BHI, visto que não houve população sobrevivente. Não houve diferença significativa entre os resultados de contagem e NMP, comparando-se as duas temperaturas de incubação, entretanto, os resultados de contagem e NMP das três concentrações inoculadas foram diferentes entre si. Concluiu-se que a cepa pré incubada a 43ºC não apresentou maior resistência ao calor, em relação à cepa incubada a 35ºC; e não houve maior resistência ao calor, comparando-se as diferentes concentrações. / The purpose of this study was to describe the behavior of Salmonella Enteritidis (S. Enteritidis) PT4 undergoing thermal treatment at 60ºC for 3 ½ minutes in reconstituted dried-whole egg, correlating the heat resistance with a previous temperature of incubation and microrganism concentration. 150 analyses were conducted, 75 with S. Enteritidis PT4 previously incubated at 35ºC and 75 with S. Enteritidis PT4 previously incubated at 43ºC. Each of these two groups was subdivided in 3 sub-groups, adding the inoculum at concentrations of 10³, 105, 108 CFU/mL of BHI broth. After the inoculation, pasteurization of the egg was simulated at 60ºC for 3,5 minutes in a water bath. Then colony count and Most Probable Number (MPN) were carried out to check the concentration of surviving S. Enteritidis. The decimal reduction time (D-value) was 2.54 and 2.57 minutes for S. Enteritidis previously incubated at 35ºC and inoculated in the concentration of 105 and 108 CFU/mL of BHI broth, respectively. Concerning the S. Enteritidis previously incubated at 43ºC and inoculated in concentrations of 105 and 108 CFU/mL of BHI broth, the D-value was 2.58 and 2.40 minutes, respectively. It was not possible to calculate the D-Value for the 10³ CFU/mL concentration of BHI broth, because there was no surviving population. There was no significant difference between the results of colony count and MPN, comparing the two incubation temperatures, however the results of colony count and MPN of the three inoculated concentrations were different from each other. It was possible to conclude that the S. Enteritidis PT4 previously incubated at 43ºC hadn´t shown more heat resistance if compared with the S. Enteritidis PT4 incubated at 35ºC; and there wasnt more heat resistance, comparing the different concentrations.
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Descrição do comportamento da cepa de Salmonella Enteritidis PT4 frente ao tratamento térmico a 60,0°C por três minutos e meio, em ovo integral pasteurizado desidratado reconstituído / Description the behavior of Salmonella Enteritidis PT4 undergoing thermal treatment at 60°C for 3 ½ minutes, in reconstituted dried-wole eggPaula Spinha de Toledo 03 December 2003 (has links)
O presente trabalho objetivou descrever o comportamento da cepa Salmonella Enteritidis (S. Enteritidis) PT4, frente ao tratamento térmico a 60,0º C por três minutos e meio, em ovo integral pasteurizado desidratado reconstituído, interrelacionando a termorresistência com temperatura prévia de incubação e concentração de microrganismos. Foram realizadas 150 análises, das quais 75 foram trabalhadas com cepa previamente incubada à 35ºC e 75 com cepa incubada à 43ºC. Cada um destes grupos foi subdividido em três subgrupos, inoculado-se as concentrações de 10³, 105 e 108 unidades formadoras de colônia (UFC)/mL de caldo BHI. Após inoculação, foi simulada pasteurização do ovo, a 60,0ºC por 3,5 minutos, em banho-maria, e, posteriormente, realizadas contagem em placa (UFC) e Número Mais Provável (NMP), para verificação da concentração de S. Enteritidis sobrevivente. O tempo de redução decimal (valor D) foi de 2,54 e 2,57 minutos para S. Enteritidis previamente incubada à 35ºC e inoculada nas concentrações de 105 e 108 UFC/mL de caldo BHI, respectivamente. Para S. Enteritidis previamente incubada à 43ºC e inoculada nas concentrações de 105 e 108 UFC/mL de caldo BHI, o valor D foi de 2,58 e 2,40 minutos, respectivamente. Não foi possível o cálculo do valor D para a concentração 10³ UFC/mL de caldo BHI, visto que não houve população sobrevivente. Não houve diferença significativa entre os resultados de contagem e NMP, comparando-se as duas temperaturas de incubação, entretanto, os resultados de contagem e NMP das três concentrações inoculadas foram diferentes entre si. Concluiu-se que a cepa pré incubada a 43ºC não apresentou maior resistência ao calor, em relação à cepa incubada a 35ºC; e não houve maior resistência ao calor, comparando-se as diferentes concentrações. / The purpose of this study was to describe the behavior of Salmonella Enteritidis (S. Enteritidis) PT4 undergoing thermal treatment at 60ºC for 3 ½ minutes in reconstituted dried-whole egg, correlating the heat resistance with a previous temperature of incubation and microrganism concentration. 150 analyses were conducted, 75 with S. Enteritidis PT4 previously incubated at 35ºC and 75 with S. Enteritidis PT4 previously incubated at 43ºC. Each of these two groups was subdivided in 3 sub-groups, adding the inoculum at concentrations of 10³, 105, 108 CFU/mL of BHI broth. After the inoculation, pasteurization of the egg was simulated at 60ºC for 3,5 minutes in a water bath. Then colony count and Most Probable Number (MPN) were carried out to check the concentration of surviving S. Enteritidis. The decimal reduction time (D-value) was 2.54 and 2.57 minutes for S. Enteritidis previously incubated at 35ºC and inoculated in the concentration of 105 and 108 CFU/mL of BHI broth, respectively. Concerning the S. Enteritidis previously incubated at 43ºC and inoculated in concentrations of 105 and 108 CFU/mL of BHI broth, the D-value was 2.58 and 2.40 minutes, respectively. It was not possible to calculate the D-Value for the 10³ CFU/mL concentration of BHI broth, because there was no surviving population. There was no significant difference between the results of colony count and MPN, comparing the two incubation temperatures, however the results of colony count and MPN of the three inoculated concentrations were different from each other. It was possible to conclude that the S. Enteritidis PT4 previously incubated at 43ºC hadn´t shown more heat resistance if compared with the S. Enteritidis PT4 incubated at 35ºC; and there wasnt more heat resistance, comparing the different concentrations.
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Heat tolerance mechanisms of an exceptional strain of Escherichia coliPleitner, Aaron M. Unknown Date
No description available.
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Testování tepelných vlastností rukavic pomocí tepelného manekýna / Determination of thermal properties of gloves by means of thermal manikinPidrová, Kateřina January 2016 (has links)
This diploma thesis is focused on determination of thermal properties of gloves by means of thermal manikin. The background research with relation to this topic together with derivation of the computational equations used for the following measurement are presented in the first part. The most significant part of this work is suggestion of procedure for measuring the heat resistance of gloves with thermal manikin based on procedure from ČSN EN 511. This methodics was verificated with 5 pairs of gloves together with analysing the uncertainties and testing the repeatability of this measurement. This work also contains the outline for all of the measured pairs with posibilities of their usage in specific situations and surrounding air temperatures. At the end of this work is mentioned brief summary of achieved results.
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Разработка технологии получения кордиеритовой керамики : магистерская диссертация / Development of technology for obtaining cordierite ceramicsГиренко, Г. С., Girenko, G. S. January 2021 (has links)
В результате проведенных исследований подобраны и исследованы отечественные сырьевые материалы, рассчитан и разработан состав массы прекурсора и синтезирован композитный материал для производства кордиеритовой керамики. Разработаны составы масс для производства кордиеритовой керамики различными способами формования: шликерным литьем, пластическим и полусухим формованием. Проведенные исследования показывают возможность получения кордиеритовой керамики на основе сырья отечественных месторождений с высоким содержанием α-кордиерита. / As a result of the conducted research, domestic raw materials were selected and studied, the composition of the precursor mass was calculated and developed, and a composite material for the production of cordierite ceramics was synthesized. Mass compositions for the production of cordierite ceramics by various molding methods have been developed: by slip casting, plastic and semi-dry molding. The results of investigation show the possibility of obtaining cordierite ceramics based on the raw materials of domestic deposits with a high content of α-cordierite.
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