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Caracterização molecular de cepas de Listeria monocytogenes de casos clínicos e alimentos no BrasilCOSTA, Ana Paula Rocha da 28 February 2013 (has links)
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Previous issue date: 2013-02-28 / FACEPE / Listeria monocytogenes é um bacilo gram-positivo, intracelular facultativo, transmitido por
alimentos, que pode causar doença, a listeriose, em indivíduos susceptíveis. Embora rara, a
listeriose tem grande importância para a saúde pública pela sua alta letalidade. Este trabalho
teve como objetivo, identificar marcadores moleculares para utilização no desenvolvimento
de nova técnica de diagnóstico molecular da listeriose. Os estudos envolveram sorotipagem,
tipagem molecular pela amplificação das sequências 23S, 16S-23S e RAPD, pesquisa de
plasmídios e de genes de virulência (inlA, inlB, inlC, inlJ, hly, iap, plcA, actA) em 135 cepas
de L. monocytogenes de casos humanos e alimentos isoladas no Brasil no período de 1975 a
2001; infecção experimental em camundongos com cepas portando ausência ou alterações em
genes de virulência; e a caracterização de isolados de um caso de endocardite atendido numa
unidade de emergência cardiológica em Recife, PE, em 2010. Nenhuma relação foi
encontrada entre a origem das cepas, sorotipos, perfis genéticos, conteúdo plasmidial e
distribuição dos genes de virulência. Os ensaios de infecção experimental em camundongos
também não permitiram estabelecer uma relação entre a presença dos marcadores de
virulência considerados no estudo e as respostas dos animais inoculados. Seis isolados de
hemocultura de um caso de endocardite com identificação presuntiva de Listeria spp. foram
classificados como L. monocytogenes sorotipo 4b pela amplificação por PCR dos genes 23S,
lmo2243 e ORF2210 específicos do gênero Listeria, espécie L. monocytogenes e sorotipo b
respectivamente. Todos os genes de virulência pesquisados foram detectados por PCR nas
amostras e a análise do perfil de amplificação da sequência 16S-23S revelou que os seis
isolados são uma mesma cepa. Embora esses estudos não tenham revelado nenhum marcador
molecular de patogenicidade, a alta frequência de genes de virulência observada entre cepas
dos sorotipos mais patogênicos (1/2a, 1/2b, 4b) evidencia o potencial patogênico nas cepas
brasileiras de L. monocytogenes e a necessidade de incrementar a vigilância e diagnóstico
dessa bactéria. Considerando a prevalência dos sorotipos 1/2a, 4b nas amostras clinicas e dos
sorotipos 1/2a, 1/2b, 4b em alimentos, desenvolvemos e padronizamos um procedimento
baseado em LAMP (loop-mediated isothermal amplification) para identificação desses
sorotipos. A técnica é rápida e de fácil operacionalização, utiliza um bloco de aquecimento ou
banho-maria e o produto da reação pode ser visualizado a olho nu mediante adição de
reagentes fluorescentes. O procedimento padronizado mostrou-se sensível, capaz de detectar
100pg de DNA ou 104 UFC, e espécie - específica, capaz de diferenciar L. monocytogenes de
espécies intimamente relacionadas geneticamente. Outros sorotipos intimamente relacionados
(3a, 3b, 4e e 4d) foram amplificados sem detrimento da técnica porque são raramente
encontrados em amostras humanas e animais. A técnica LAMP se apresenta como uma
alternativa fácil e rápida para diagnóstico e tipagem de L. monocytogenes especialmente para
os programas de vigilância e investigação epidemiológica.
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Contagem de listeria spp pelo metodo do numero mais provavel (NMP), avaliação de sua ocorrencia em carnes de frango e da eficiencia de sanitizantes na redução da contaminação por Listeria monocytogenesKabuki, Dirce Yorika, 1964- 31 October 1997 (has links)
Orientador: Arnaldo Yoshiteru Kuaye / Dissertação (mestrado) - Universidade Estadual de Campinas, Faculdade de Engenharia de Alimentos / Made available in DSpace on 2018-07-22T23:06:06Z (GMT). No. of bitstreams: 1
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Previous issue date: 1997 / Resumo: Atualmente a L. monocytogenes é considerada um patógeno de importância em alimentos, pois vários surtos e casos de listeriose associados ao consumo de alimentos têm sido relatados, incluindo os produtos de frango. O aumento da produção brasileira de carnes de aves, a redução de preço no mercado interno e conseqüente aumento do consumo e a falta de métodos oficiais para a quantificação de L. monocytogenes em alimentos, principalmente os in natura, levaram ao desenvolvimento deste projeto numa tentativa de quantificá-la para que limites máximos de tolerância possam ser propostos. Amostras resfriadas de peito e de frango inteiro obtidas no comércio varejista, foram submetidas a quantificação de Listeria spp pelo método do Número Mais Provável (NMP) utilizando-se: a) caldo Fraser modificado (MdFB) contendo 20 mg de acriflavina/L a 35°C/48h; b) caldo de enriquecimento para Listeria (LEB) (USDA) a 30°C/48h e c) caldo LEB a 30°C/24h seguido do caldo Fraser modificado (MFB) (USDA) a 35°C/24-48h. No isolamento foram utilizados os ágares cloreto de lítio feniletanol moxalactam (LPM) e Oxford modificado (MOX) e na identificação as provas bioquímicas padrão ou o kit API-Listeria. Os resultados revelaram: i) a viabilidade do emprego do meio MdFB na técnica do NMP; ii) valores de NMP para Listeria sp e L. monocytogenes entre <0,3 a 93/g para peitos e entre <9 a 2,8x103/carcaça ou <0,005 a 1,943/g de frango; iii) predomínio de L. innocua, L. monocytogenes, L. welshimeri e L. seeligeri. Em estudo paralelo com as mesmas amostras, verificou-se ocorrência elevada de Listeria sp e L. monocytogenes, com índices de 96,7% e 90,0% respectivamente e pequena diferença entre carcaças e peitos de frango. O ágar LPM apresentou desempenho melhor que o MOX no isolamento de L. monocytogenes. Em outro estudo, empregando-se a técnica do NMP proposta, verificou-se a ineficiência de hipoclorito de sódio e de fosfato trissódico na redução de L. monocytogenes em coxas de frango artificialmente contaminadas; os níveis de redução obtidos foram ? 0,42 ciclos log, os quais não foram considerados estatisticamente significantes / Abstract: L. monocytogenes is currently considered to be an important food pathogen, since various outbreaks and cases of listeriosis have been related to the consumption of foods, including some chicken products. The increase in the production of fowl meats in Brazil, the reduction of the price on the internal market and consequent increase in consumption by the population and the lack of official methods for the quantification of L. monocytogenes in foods, principally in raw foods, are the factors which led to the development of this project, aimed at quantifying the problem and subsequently proposing maximum tolerance limits. Thus refrigerated samples of chicken breast and whole chickens, ali obtained on the retail market, were quantified for Listeria spp by the Most Probable Number (MPN) method, using a) modified Fraser broth (MdFB) containing 20 mg acriflavine/L at 35°C/48h; b) Listeria enrichment broth (LEB) (USDA) at 30°C/48h and c) LEB broth at 30°C/24h followed by modified Fraser broth (MFB) (USDA) at 35°C/2448h. For the isolation procedure, lithium chloride phenylethanol moxalactam agar (LPM) and modified Oxford agar (MOX) were used, and the standard biochemical test or API Listeria kit used for identification. The results showed the following: i) the viability of using the medium MdFB in the MPN technique; ii) MPN values for Listeria spp and L. monocytogenes between <0.3 and 93/g for breasts and between <9 and 2.8x103/carcass or <0.005 to 1.943/g chicken and iii) predominance of L. innocuti, L. monocytogenes, L. welshimeri and L. seeligeri. In a parallel study with the same samples, an elevated occurrence of Listeria spp and L. monocytogenes was determined, with indices of 96.7% and 90.0% respectively, the difference between the carcasses and breasts being relatively small. LPM agar was shown to be a better isolation media for L. monocytogenes than MOX. In another study using the proposed MPN technique, the inefficiency of sodium hypochlorite and of trisodium phosphate in the reduction of L. monocytogenes in artificially contaminated chicken legs was shown, the reduction levels being ?0.42 log cycles, and not therefore statistically significant / Mestrado / Mestre em Tecnologia de Alimentos
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Development of Monoclonal Antibodies that Recognize a Wide Spectrum of Listeria Monocytogenes StrainsO'Neill, Teela January 2013 (has links)
Listeria monocytogenes is a bacterial pathogen that is typically transmitted to humans through consumption of contaminated foods. Infection with this organism can lead to a severe and life-threatening illness referred to as listeriosis. The goal of this study was to develop monoclonal antibodies (MAbs) with high specificity and affinity to proteins found on the surface of all strains of L. monocytogenes while not cross-reacting with non-pathogenic Listeria spp. or other major bacterial pathogens commonly found in foods. A literature search was conducted to identify ten candidate surface proteins involved or putatively involved in the virulence of L. monocytogenes. Bioinformatics analyses using BLAST on the NCBI website showed that five of the ten candidate proteins were potentially present in L. monocytogenes strains but absent from strains of other Listeria spp. Genes encoding for these five proteins, ActA, InlA, InlC2, InlJ and LapB, were cloned and expressed in Escherichia coli. MAbs were raised against recombinant LapB, InlJ and InlC2 proteins using hybridoma technology. A total of 48 anti-LapB, 33 anti-InlJ and 37 anti-InlC2 MAbs were developed. Based on the comparison of IFM signal of each MAb against L. monocytogenes cells, seven anti-LapB MAbs and six anti-InlC2 MAbs were selected for further characterization. All of the anti-InlJ MAbs showed weak IFM signals and negative reactivity in ELISA against L. monocytogenes cells. The selected anti-LapB and anti-InlC2 MAbs were further characterized by assessing their ability to bind to cells of 51 strains representing 11 L. monocytogenes serotypes using ELISA. Six anti-LapB MAbs (M3484, M3495, M3500, M3509, M3517, M3519) reacted strongly with 44 of 51 strains representing 9 of the 11 L. monocytogenes serotypes tested. Five anti-InlC2 MAbs (M3607, M3618, M3630, M3633, M3636) reacted strongly with 47 strains representing 10 of the 11 L. monocytogenes serotypes tested. These results indicate that anti-LapB and anti-InlC2 MAbs could potentially be used as diagnostic reagents for isolation and detection of almost all L. monocytogenes strains in contaminated foods.
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Identification of Genetic Determinants Associated with Biofilm Formation Capacity of Listeria MonocytogenesSoosai, Diana Margaret January 2016 (has links)
Persistence of Listeria monocytogenes in food processing plants is a huge health and economic burden. Biofilms are considered to be one of the major mechanisms by which this pathogen persists within these environments. Studies so far have mostly used optimal growth conditions in their investigations which may not provide a realistic understanding of the biofilm forming abilities of L. monocytogenes in food processing plants. Therefore the aim of this study was to 1) establish a model (12 ºC, Beef Broth) that closely relates to the food processing environment 2) screen 66 isolates of L. monocytogenes from food and clinical sources and determine their biofilm forming phenotypes (non-, weak, moderate and strong formers) and 3) analyze the correlation between biofilm formation phenotypes and biofilm associated genes detected using polymerase chain reaction (PCR) and Basic Local Alignment Search Tool (BLAST) for whole genome sequences. Biofilm formation established at 12 ºC in Beef Broth was the most consistent and quantifiable at day 9 of incubation. Subsequently, 66 isolates were screened using this model, resulting in 60 isolates being identified as strong biofilm formers, 5 isolates as moderate biofilm formers and 1 isolate as a weak biofilm former. Twenty biofilm associated genes were analyzed using PCR in 27 representative isolates. Out of the 20 genes, at least 17 of them were detected in all the tested isolates. Out of the 106 biofilm associated genes analyzed using BLAST, all the isolates were found to show the presence of at least 92 genes. In conclusion, there was no obvious correlation between the presence/absence of the genes selected for analysis and the ability to form biofilms using approaches performed in this study. However, the model established in the study will be useful in further analysis (transcription and translation studies) of genetic markers responsible for biofilm formation of L. monocytogenes under food processing conditions.
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Impact of Parkinson’s Disease- Linked- Lrrk2 Mutation (Lrrk2G2019S) on the Innate Immune Response During Infection with Listeria Monocytogenes.Sam, Leila 06 October 2020 (has links)
Mutations in the Leucine-rich repeat kinase 2 (Lrrk2) gene are associated with familial and sporadic cases of Parkinson’s disease but are also found in inflammatory-related disorders such as Crohn’s disease, systemic lupus erythematosus, tuberculosis and leprosy. There is also evidence that LRRK2 is highly expressed in immune cells, particularly in macrophages, and has been functionally linked to pathways pertinent to immune cell function such as modulating the course of infections, cytokine release, autophagy and phagocytosis. Indeed, G2019S mutation in Lrrk2 is the most common mutation in Parkinson’s disease. Accordingly, we hypothesized that G2019S mutation in Lrrk2 might enhance the activation of the innate immune system. We tested our hypothesis by performing challenge experiments in a mouse model of Listeria monocytogenes, and by measuring the activation of bone marrow derived macrophages (BMDMs) following in vitro infection with the bacterium.
We found that Lrrk2G2019S mutant mice controlled L. monocytogenes better than WT mice. The mechanism behind the better control of L. monocytogenes by the G2019S mutation of Lrrk2 was investigated in BMDMs following in vitro infection with L. monocytogenes. Interestingly, we found that Lrrk2G2019S mutation enhances the production of TNF-α, IL-1β and IL-10 by infected BMDMs. The impact on TNF-α and IL-1β was specifically due to the G2019S mutation of Lrrk2 since there was no impact on the expression of these cytokines in Lrrk2 knockout macrophages. Western blotting experiments revealed that the G2019S mutation of Lrrk2 enhances MAPK signaling (TAK1, p38 and ERK). Modulation of the expression of the pro-inflammatory cytokines, TNF-α and IL-1β by G2019S mutation of Lrrk2 occurred via p38 MAPK activation. The impact on IL-10 expression occurred through increased ERK activation by the G2019S mutation of Lrrk2. We did not observe any impact of G2019S mutation of Lrrk2 on the activation of NF-κB and JNK MAPK pathways.
Increased expression of IL-1β by G2019S mutation of Lrrk2 revealed increased inflammasome signaling. Inflammasome signaling in response to L. monocytogenes was mainly mediated by the AIM2- and partly by NLRP3- inflammasome and was dependent on activation of caspase-1. We found that Lrrk2G2019S mutation enhanced the expression of NLRP3 and caspase-1.
Finally, we found that the expression of reactive oxygen species (ROS) following infection with L. monocytogenes was augmented by G2019S mutation of Lrrk2, and this can be an important mechanism that promotes the enhanced clearance of the bacterium in vivo.
Overall, these results present new insights into the signaling mechanisms through which the G2019S mutation of Lrrk2 augments innate immune response which leads to better control of infection.
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The effect of liquid smoke on Listeria monocytogenesMessina, Maria Cipolla, 1961- January 1988 (has links)
Four strains of Listeria monocytogenes (LCDC 81-861, ATCC 19115, M1 and M2) examined in pure culture behaved similarly when exposed to a concentration of 0.5% CharSol C-10 liquid smoke by reducing Listeria numbers to an undetectable level within 4 hours post treatment. However, at the lower concentration of 0.25% liquid smoke, differences in resistance to the antimicrobial properties of smoke components become evident among these strains indicating that a level of 0.5% liquid smoke is more effective in controlling this organism. CharSol C-10 liquid smoke was used as a full strength dip treatment for beef franks surface inoculated with six strains of L. monocytogenes (LCDC 81-861, ATCC 19115, M1, M2, M5, and C6) then vacuum packaged and stored at 4 ± 1°C for 72 hours. Beef franks dipped in CharSol C-10 liquid smoke exhibited a significant (P < 0.001) reduction in L. monocytogenes numbers after 72 hours of storage at both inoculum levels of 1 x 10³ cells/ml and 1 x 10⁵ cells/ml.
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Changes in cell surface and metabolism associated with strains of Listeria monocytogenes displaying different sensitivities to class IIa bacteriocinsVadyvaloo, Viveka 12 1900 (has links)
Thesis (PhD)--Stellenbosch University, 2003. / ENGLISH ABSTRACT: The possible use of the bacterially produced antimicrobial peptides, and in particular class IIa
bacteriocins as food preservatives is a motivating factor in studies on resistance to them by
food-borne pathogens like Listeria monocytogenes. The high frequencies of resistance to class
Ha bacteriocins have however sparked concern regarding their adequacy as potential biopreservatives.
Activity of these cationic peptides was reported to occur by membrane
permeabilisation due to pore formation, which results in the leakage of the intracellular
contents followed by cell death. The cell envelope (cell wall and cell membrane) is therefore
envisaged as a key site of modification in suscepti bility of bacteria to class Ha bacteriocins.
Mutants of the L. monocytogenes 873 isolate, resistant to the class IIa bacteriocin, leucocin A,
were generated at the start of the study to complement the existing array of L. monocytagenes
wild-type and resistant isolates obtained from other sources. The fifty percent inhibitory
concentrations using a highly sensitive and reproducible bioassay were determined. This
allowed categorisation of the mutants into intermediate and highly resistant phenotypes.
Analysis of the growth patterns of all these strains showed decreased growth rates and higher
growth yields for all the resistant strains in general. This provided evidence for possible
effects of membrane adaptation and metabolic changes in the resistant strains and prompted
further investigation. The major focus of the study on the class Ha resistant mutants were: (1)
analysis of membrane compositional changes and factors influencing cell surface charge; (2)
assessment of physical changes in the membrane and bacteriocin itself using circular
dichroism and fourier transform infrared spectroscopy; (3) and, determination of changes in
glucose metabolism.
Electrospray mass spectrometry analysis of the major listerial phospholipid,
phosphatidylglycerol, revealed that membranes of resistant strains had increased levels of
unsaturated and short-acyl-chain phosphatidylglycerol molecular species, indicating more
fluid membranes. In addition, treatment with a desaturase inhibitor resulted in increased
sensitivity of only the intermediate resistant strains to the class na bacteriocin, leucocin A.
This indicated the influence of membrane adaptation in only lower levels of resistance. It is
conceivable that more fluid membranes could also impact on decreased stability of pore
formation by the bacteriocin.
Complementary biophysical studies using fourier transform infrared spectroscopy indicated
the possible occurrence of greater membrane fluidity of resistant cells, by the notable shift in the anti symmetric CH2 stretching vibration from 2921 cm-I to 2922 cm-I. Additionally,
circular dichroism revealed a decreased a-helical and increased random structure of leucocin
A in the presence of listerial liposomes derived from highly resistant cell membrane extracts.
It is possible that this may result in reduced activity of the bacteriocin in resistant cell
membranes as a-helical stucture is a critical feature for membrane insertion of cationic
antimicrobial peptides.
Cell surface charge was determined by quantification of alanine and lysine esterification of
the anionic cell surface polymer, teichoic acid, and membrane phospholipids respectively.
Increased D-alanine, which causes neutralisation of the cell surface, was observed in all
resistant cells. A tendency for greater lysine content in membrane phospholipids, which also
impacts on neutralisation of the anionic phospholipid of listerial membranes, was observed in
highly resistant strains only. This neutralisation of the negative charge of the cell surface may
interfere with initial electrostatic interaction of bacteriocin with the cell, and subsequent
interactions required for permeabilisation of the cell membrane. These differences in alanine
and lysine esterification were not the result of increased expression of certain associated genes
(d/tA and /mo1695) and may be the result of post-transcriptional regulation. It was, however,
found that all resistant L. monocytogenes strains, including the intermediate resistant strains,
exhibited decreased expression of a putative docking molecule, the mannose-specific
phosphotransferase system EIIAB subunit (EIlABMan).A clear correlation existed between the
levels of resistance and EIIABMandown-regulation.
Finally, analysis of the glucose metabolism in highly resistant and wild-type strains, indicated
a more efficient metabolism with regards to higher growth yields and ATP yield, in contrast to
a lower specific growth rate in a spontaneous and genetically defined (EIlABMan inactivated)
highly resistant mutant. The switch in metabolic end-product observed, was attributed to the
loss of the glucose transporter, EIlABMan,and may cast doubts on the feasibility of the use of
class Ha bacteriocins as food preservatives in light of a stable and efficient resistant
phenotype. / AFRIKAANSE OPSOMMING:
Sien volteks vir opsomming
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Antimicrobial activity of nisin and hen lysozymeJaczynski, Jacek 16 November 1998 (has links)
Varying concentrations of the food preservatives nisin and lysozyme were
adsorbed onto glass surfaces chemically modified to exhibit different degrees of
hydrophobicity. The antimicrobial activity of the adsorbed preservatives was evaluated
by documenting the ability of Listeria monocytogenes to adhere and grow on the glass
surfaces. A bioluminescence protocol was developed to effectively enumerate bacterial
cells adhered to glass. Lysozyme adsorption onto glass surfaces was monitored by
labeling with ¹²⁵I.
Results indicated that synergy was present for 0.9/0.1 molecular ratio of
nisin/lysozyme. Synergistic effect was increasing gradually with the increase of nisin in
the ratios tested. This trend was observed on both surface types. However, the magnitude
of synergy was more pronounced on hydrophobic surfaces than on hydrophilic ones.
Results from protein radiolabeling showed that lysozyme was adsorbed with higher mass
to hydrophilic surfaces than to hydrophobic ones. / Graduation date: 1999
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Prevalencia de Listeria Monocytogenes en salchichas tipo Huacho provenientes de los mercados de abastos del Cercado de LimaPérez Alarcón, María Elizabeth January 2013 (has links)
Se analizaron 60 muestras de Salchicha tipo Huacho de los Mercados de Abastos del Cercado de Lima, con la finalidad de determinar la incidencia de Listeria monocytogenes. Estas muestras se llevaron al Laboratorio de Microbiología de la Facultad de Farmacia y Bioquímica de la Universidad Nacional Mayor de San Marcos, en recipientes estériles, refrigerados y se procesaron dentro de las 24 horas de colectadas.
Para el análisis microbiológico se utilizó la técnica según USDA- FSIS, que consta de tres fases: Pre-enriquecimiento, Enriquecimiento de la muestra y siembra en agares selectivos, pruebas Bioquímicas, Catalasa, Gram positivos y la prueba del CAMP para su confirmación.
La incidencia de L. monocytogenes en Salchicha tipo Huacho, en los Mercados de Abastos del Cercado de Lima es de 78%, siendo un valor considerable y que supera a los valores reportados en estudios a nivel internacional. Estos resultados permiten considerar que la Salchicha tipo Huacho se constituye como un alimento de riesgo potencial para la Salud Pública. / --- 60 samples of the Huacho Sausage from the Food Markets in Cercado de Lima, in Lima, Peru, were analyzed in order to determine the incidence of Listeria monocytogenes.
These samples were taken to the Laboratory of Microbiology to the Faculty of Pharmacy and Biochemistry at the National University of San Marcos. They were taken in sterile containers for being refrigerated. Then they were processed within 24 hours of being collected.
The USDA-FSIS technique was used for microbiological analysis, which consists of three phases: Pre-enrichment of the sample, Sample Enrichment and Reseeding on selective agars. At the same time, some biochemical tests were applied, such as the positive Catalase test, the test of Great Positive, and CAMP test to confirm the results.
The incidence of the Listeria monocytogenes in the Huacho Sausage, from the Food Markets in Cercado de Lima, is 78%. This is quite high, as it exceeds the values reported in international studies.
These results support the conclusion that the Huacho Sausage is a food with a potential risk to the public health.
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Capacidad de formación de biopelículas de cepas de Listeria monocytogenes aisladas de quesos frescos procedentes de mercados del Cercado de LimaVillanueva Durand, Diego Armando January 2015 (has links)
Se analizaron 75 muestras de quesos frescos de diferentes mercados del
Cercado de Lima, con la finalidad de aislar e identificar Listeria monocytogenes,
además de determinar su capacidad para formar biopelículas. El análisis
microbiológico se realizó empleando las metodologías recomendadas por el
Manual de Bacteriología Analítica de la Food and Drug Administration (BAM -
FDA). El procedimiento para determinar la capacidad de formación de biopelículas
fue el método de microplaca de 96 pocillos descrito por Djordjevic con las
modificaciones recomendadas por Borucki. El estudio microbiológico permitió
aislar Listeria monocytogenes en 14 muestras de quesos frescos (18,67%), siendo
un valor elevado representando un riesgo potencial para la población
consumidora. La capacidad de las cepas de Listeria monocytogenes para producir
biopelículas en microplaca de poliestireno fue clasificada según la densidad óptica
obtenida a 595 nm. Se obtuvo que el 64,29 % (9/14) de las cepas de Listeria
monocytogenes tienen capacidad de formar biopelículas, distinguiéndose entre
formadores débiles y moderadas dependiendo del medio de enriquecimiento
estudiado, los cuales fueron caldo tripticasa de soya (TSB) e Infusión cerebro
corazón (BHI). El medio BHI fue el más efectivo en promover la formación de
biopelículas de Listeria monocytogenes en microplaca de poliestireno.
Palabras clave: Listeria monocytogenes, quesos frescos, Cercado de Lima,
biopelículas, microplaca. / --- A total of 75 samples of fresh cheese from different markets in Cercado de Lima, were analyzed in order to isolate and identify Listeria monocytogenes and also determine its ability to produce biofilms. The microbiological analysis was performed using the methodologies recommended by FDA’s Bacteriological Analytical Manual (BAM – FDA). The methodology for assessment of Listeria monocytogenes biofilm formation was the 96-well microtiter plate method
described by Djordjevic with the modifications recommended by Borucki. The microbiological study allowed identifying Listeria monocytogenes in 14 samples of fresh cheese (18,67%), being a high value and which means a potential risk for the
consumer population. The assessment of Listeria monocytogenes strains to produce biofilm in microtiter polystyrene plate was classified according to optical density at 595 nm. It was found that 64,29% (9/14) of Listeria monocytogenes
strains have the ability to produce biofilms, distinguishing between weak and moderate biofilm producers depending of the type of enrichment medium used, which were Trypticase Soy Broth (TSB) and Brain Heart Infusion (BHI). BHI medium was the most effective in promoting the Listeria monocytogenes biofilm formation in polystyrene microtiter plate.
Key words: Listeria monocytogenes, fresh cheese, Cercado de Lima, biofilm, microtiter plate.
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