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1.
Ch. Fablet C. Robinault J.P. Jolly M. Collet M. Chemaly A. Labb F. Madec Ph. Fravalo 《Livestock Science》2006,102(3):216-225
The study aimed to (1) validate the mini-MSRV-MPN method to quantify Salmonella enterica in pig slurry, (2) estimate the effect and interaction on temperature, time and initial Salmonella load on the survival of the 2 strains of Salmonella typhimurium (PF 1690 and DT104 100/706/037) during slurry storage and (3) identify Salmonella contaminated finishing pig batches and assess the level of contamination of their slurry. The mini-MSRV-MPN method was compared to direct isolations on brilliant green agar supplemented with rifampicin to quantify Salmonella in pig slurry. Doelhert uniform shell design was used to study the effect of different parameters on the survival of the 2 strains of Salmonella in pig slurry. Environmental samples of faecal material and a sample of the slurry of 50 batches of finishing pigs were analysed by bacteriological classical method to identify Salmonella. Quantification was performed on pools of faeces and in slurry using the mini-MSRV-MPN technique. This method proved to be suited to quantify Salmonella in pig slurry. Temperature, time of slurry storage and their interaction influenced Salmonella decrease. 12 batches of pigs tested Salmonella positive. Quantification was possible in 5 batches of faecal samples (2.4–350 MPN g− 1 of Salmonella). Quantification was achieved in 2 out of 6 positive samples of slurry (1.6 and 110 MPN mL− 1 of Salmonella). 相似文献
2.
Zhu YM Miao JF Zhang YS Li Z Zou SX Deng YE 《Veterinary immunology and immunopathology》2007,120(3-4):168-176
Seven healthy native goats in early lactation, weighing 30–40 kg, were used in this study. The right mammary gland of the seven does were infused with CpG-ODN at a dosage of 100 μg kg−1 body weight on the day 5 postpartum (PP). The left glands were used as controls and infused with sterile phosphate-buffered saline (PBS). On day 8 PP, the same dosage of CpG-ODN or PBS was again infused. On day 9 PP, the mammary glands (both right and left) of the seven does were infused with 6 × 106 colony-forming units (CFU) Escherichia coli and, at 0, 8, 16, 24, 48 and 72 h postinfection (PI), milk samples were collected from all glands. Goats were euthanized at 72 h PI and the mammary tissue harvested. Infusion with 6 × 106 CFU ml−1 E. coli induced acute mastitis. Histopathological evaluations showed that polymorphonuclear neutrophils (PMNs) were still present in alveoli at 72 h PI, but PMNs in the CpG-ODN-treated glands has disappeared. Bacteria counts in milk peaked at 16 h PI and CpG-ODN induced a significant decrease in viable bacteria from 16 h PI until the end of the experiment. This study showed that CpG-ODN promoted the expression of its specific receptor (TLR-9 mRNA) in mammary tissue, stimulated IL-6 production, reduced bacteria counts in milk, attenuated the impact of inflammation mediators on cells and significantly shortened the inflammation course. These results suggest that the CpG-ODN improved mammary gland defense and, thereby, had a beneficial effects against mastitis caused by E. coli infection in goats. 相似文献
3.
Estimating the number of undetected multi-resistant Salmonella Typhimurium DT104 infected pig herds in Denmark 总被引:1,自引:0,他引:1
Rugbjerg H Wingstrand A Hald T Andersen JS Lo Fo Wong DM Korsgaard H 《Preventive veterinary medicine》2004,65(3-4):147-171
In Denmark, the detection of multi-resistant Salmonella Typhimurium DT104 (MRDT104)-infected pig herds relies on the national Salmonella surveillance programme at the farm and slaughterhouse levels of production. With the surveillance sampling protocol and the diagnostic methods currently used, some herds might remain undetected. The number of undetected Danish pig herds infected with MRDT104 in the period 1 August 2001–31 July 2002 was estimated and compared with the number of culture-confirmed detected herds. A flow chart was constructed to illustrate where infected herds will go undetected in the surveillance system and Monte Carlo simulation was used to model the actual number of pig herds infected with MRDT1104. We estimated that 52 (90% CI [28, 178]) finisher herds were infected with MRDT104 compared to 23 (44%) detected. Among sow herds with production of weaners or growers, we estimated that 38 (90% CI [23, 74]) were infected with MRDT104 compared to 7 (18%) actually detected. Among breeder and multiplier herds, we estimated that five (90% CI [3, 8]) herds were infected with MRDT104 compared to three (60%) detected. In total, we estimated that 102 pig herds were infected with MRDT104 from 1 August 2001 till 31 July 2002 (90% CI [63, 228]). In comparison, 33 (32%) infected herds were detected in this period. The predicted proportion of undetected herds varied considerably with herd type. We infer that the proportion of detected MRDT104 infected herds depended on the intensity of the combined serological and bacteriological testing. 相似文献
4.
Salmonella Typhimurium DT104 (DT104) is unwanted in products for human consumption due to its antibiotic resistance and ability to cause disease. We intended to set up an improved monitoring and management program to aid in deciding when to use pork contaminated with DT104 for production of sausages without jeopardizing consumer safety. We started by carrying out two assessments of the risk for human health associated with consumption of sausages produced by: (1) Danish pork from average slaughter days; (2) imported pork (IMP) with average prevalence of DT104. The assessments showed that, if Salmonella is present, it is usually in lower numbers (≤50 per 400 cm2 surface). Additionally, during processing, the numbers will be reduced by at least 2 log-units. In Danish (DK) pork, DT104 constitutes 0.2–1.0% of the Salmonella isolates reported, while in imported pork (IMP), 18%. We estimated that out of one million, 25 g servings of DK dry-cured sausages, up to two DT104 bacteria could be found in each of 245 servings. Out of one million servings of 25 g IMP dry-cured sausages, up to two DT104 bacteria would occur in each of 19,260 servings. 相似文献
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为探究撒坝猪源大肠杆菌(E.coli)高致病性毒力岛(HPI)诱导小鼠病理损伤的超微结构特征,本研究将实验室保存的E.coli HPI阳性株(HPI+)和E.coli HPI基因缺失株(ΔHPI)进行复苏和培养,分别用E.coli HPI+、E.coli ΔHPI菌株以腹腔接种的方式感染昆明小鼠,检测菌株的半数致死量(50% lethal dose,LD50),通过HE染色和透射电镜观察并分析菌株对小鼠病理损伤的超微结构特征,利用免疫组织化学标记白细胞介素-1β(interleukin-1β,IL-1β)阳性细胞在被感染小鼠肝脏和肾脏组织中的分布,以反映E.coli HPI+及E.coli ΔHPI菌株所引起炎症水平的差异。结果显示,E.coli HPI+和E.coli ΔHPI菌株的半数致死量分别为1×107.39和1×108.62 CFU/mL;HE染色显示,E.coli感染小鼠后,可见肝脏细胞肿胀、变性,肝窦淤血,肾脏间质淤血,肾小管上皮细胞变性脱落等病理变化;超微结构变化显示,肝脏细胞的完整形态消失,胞核呈不规则形态,线粒体畸形,粗面内质网上核糖体脱落,滑面内质网增生;多数肾小管上皮细胞出现胞核固缩,部分细胞核核仁边移、体积增大,足突融合,系膜细胞间隙变宽。此外,E.coli HPI+感染组小鼠于肝脏、肾脏的水肿现象较E.coli ΔHPI菌株感染的小鼠更为明显。免疫组化结果显示,大肠杆菌感染小鼠后,IL-1β蛋白主要表达于肝细胞、中央静脉周围、肾间质细胞和肾小管上皮细胞,且E.coli HPI+感染组的IL-1β表达量高于E.coliΔHPI感染组。综上所述,撒坝猪源E.coli HPI能够调控E.coli对小鼠的致病性,HPI的调控作用可使E.coli对小鼠肝脏、肾脏造成的病变及超微结构变化更明显,并且能够增加小鼠的炎症反应。 相似文献
7.
Inhibition of adhesion of F18+ Escherichia coli to piglet intestinal villous enterocytes by monoclonal antibody against blood group H-2 antigen 总被引:3,自引:0,他引:3
Enterotoxigenic and verotoxigenic F18+ Escherichia coli colonising the pig small intestine, adhere to receptors on intestinal villous enterocytes by F18 fimbriae. The aim of the present study was to define the F18R nature. The knowledge on the nature of this receptor could be important for the development of receptor-based treatments against F18+ E. coli-induced disease. The adhesion of F18+ E. coli to pig intestinal villous enterocytes was analysed in an in vitro assay. The adhesion of F18+ E. coli but not of F4ac+ E. coli was strongly inhibited by monoclonal antibodies (mAb) with blood group H-2 specificity. Conversely, blood group H-1 specific mAb could not inhibit the adhesion of F18+ E. coli nor F4ac+ E. coli. Moreover, the blood group H-2 trisaccharide strongly inhibited the adhesion of F18+ E. coli, but only partially the adhesion of F4ac+ E. coli. These data demonstrate that the F18 receptor contains the blood group antigen H-2 (-fuc-(1-2)-β-Gal-(1-4)-GlcNAc) as major carbohydrate. 相似文献
8.
试验旨在研究大肠杆菌(E.coli)对奶牛子宫内膜上皮细胞(bovine endometrial epithelial cells,BEECs)的体外炎性损伤,探究大肠杆菌引发炎性反应的最佳浓度、作用时间及机制。首先,用不同浓度的大肠杆菌(5×104、5×105、1×106、2.5×106、5×106 CFU/mL)诱导刺激细胞3、6和9 h,通过倒置显微镜观察细胞形态、CCK-8法测D450 nm值,检测大肠杆菌对细胞活性的影响;其次,用不同浓度的大肠杆菌(5×104、5×105 CFU/mL)处理细胞3、6和9 h,用ELISA方法检测细胞上清液中白介素-1β(IL-1β)、IL-6、IL-8和肿瘤坏死因子-α(TNF-α)的分泌量;最后,用不同浓度的大肠杆菌(5×104、5×105 CFU/mL)处理细胞6和9 h,用Western blotting检测核因子κB抑制蛋白α(IκBα)和p65蛋白的磷酸化水平。结果显示,与对照组相比,大肠杆菌感染细胞9 h后,1×106、2.5×106和5×106 CFU/mL大肠杆菌组细胞活性均极显著降低(P<0.01),5×105 CFU/mL大肠杆菌组显著降低(P<0.05);大肠杆菌感染细胞9 h后,5×105 CFU/mL大肠杆菌组IL-1β、IL-6、IL-8和TNF-α极显著升高(P<0.01);大肠杆菌感染细胞6 h后,5×105 CFU/mL大肠杆菌组IκBα、p65蛋白磷酸化水平和IL-6均极显著升高(P<0.01),5×104 CFU/mL大肠杆菌组IκBα和p65蛋白磷酸化水平显著升高(P<0.05)。结果表明,大肠杆菌可以刺激奶牛子宫内膜上皮细胞产生炎性反应,且当细胞与5×105 CFU/mL大肠杆菌作用6 h或与5×104 CFU/mL大肠杆菌作用9 h为最佳。 相似文献
9.
Ravi M Ngeleka M Kim SH Gyles C Berthiaume F Mourez M Middleton D Simko E 《Veterinary microbiology》2007,120(3-4):308-319
In order to evaluate the role of the AIDA-I of porcine diarrheagenic Escherichia coli strain PD20 serogroup O143 (AIDA-I+, STb+), a mutant strain PD20M (AIDA-I−, STb+) was generated from strain PD20 by an allelic exchange procedure. In addition, the full-length aidA gene was reintroduced into strain PD20M to generate the complemented strain PD20C (pTaidA, AIDA-I+, STb+). A non-pathogenic E. coli strain PD71 was used as negative control. Each strain was inoculated to newborn pigs via stomach tube. Severity of diarrhea was evaluated clinically and intestinal colonization was assessed by histology, immunohistochemistry (IHC), and transmission electron microscopy (TEM) including immunogold electron microscopy (IGEM). The adhesion pattern to HeLa cells, bacterial auto-aggregation and biofilm formation were evaluated in vitro. Pigs infected with strains PD20 or PD20C developed diarrhea 16 and 28 h after inoculation, respectively, in contrast to pigs infected with strains PD20M or PD71. Histology, IHC, TEM and IGEM examinations showed heavy bacterial colonization with biofilm formation in the large intestine, and marked in vivo expression of AIDA-I protein in pigs infected with strains PD20 or PD20C in contrast to pigs infected with strains PD20M or PD71. The in vitro assays showed marked diffuse adherence to HeLa cells, enhanced bacterial auto-aggregation and significant biofilm formation (p < 0.05) by the AIDA-I+ strains, when compared to AIDA-I− strains. These results demonstrate that expression of AIDA-I is essential for intestinal colonization and in vitro bacterial autoaggregation and biofilm formation. Thus, AIDA-I may be considered a significant virulence determinant in development of diarrhea caused by porcine diarrheagenic AIDA-I+ E. coli PD20 in piglets. 相似文献
10.
甜叶菊绿原酸增强大肠杆菌感染蛋雏鸡免疫力研究 总被引:1,自引:0,他引:1
旨在评价甜叶菊绿原酸增强人工腹气囊感染大肠杆菌O78蛋雏鸡免疫力的作用效果,为功能性抗生素替代品研发提供基础参数支持。本试验随机将1日龄、体重无显著差异的健康海兰蛋鸡360只分为6组:空白对照组(C)、大肠杆菌O78处理组(EC0)、1.0 g·L-1杜仲素+大肠杆菌O78处理组(ED1)、1.0 g·L-1甜叶菊绿原酸+大肠杆菌O78处理组(EC1)、2.0 g·L-1甜叶菊绿原酸+大肠杆菌O78处理组(EC2)、4.0 g·L-1甜叶菊绿原酸+大肠杆菌O78处理组(EC4),预饲7 d后开始正式试验。第7天时将大肠杆菌O78通过腹气囊感染蛋雏鸡,饮水投喂药物,每天1次,连用3 d。随后通过ELISA法检测血清IL-1β、IL-2、IL-6、IgM、IgA、TNF-α水平;RT-qPCR检测空肠和回肠IL-1β、IL-2、TNF-α、Claudin-1和ZO-1基因表达;高通量测序分析盲肠内容物微生物种类。结果显示:1)腹气囊感染大肠杆菌O78显著增加了蛋雏鸡死亡率(P<0.05),而甜叶菊绿原酸处理组(EC2、EC4)蛋雏鸡的死亡率显著降低(P<0.05)。2)甜叶菊绿原酸对大肠杆菌O78感染蛋雏鸡血清IgA和IgM含量有提高趋势,可不同程度降低血清炎性因子含量,其中EC1、EC2、EC4组血清TNF-α含量显著降低(P<0.05);EC2显著降低大肠杆菌O78感染蛋雏鸡回肠促炎细胞因子IL-1β、IL-2、TNF-α的基因表达(P<0.05)。3)甜叶菊绿原酸可促进蛋雏鸡空肠紧密连接蛋白基因表达,改善腹气囊感染大肠杆菌O78对肠道屏障的损伤。4)腹气囊感染大肠杆菌O78导致鸡肠道特有OTUs增加,增加肠道拟杆菌门、变形菌门和梭杆菌门的相对丰度,降低厚壁菌门的相对丰度;而甜叶菊绿原酸处理组(EC2)蛋雏鸡盲肠厚壁菌门的相对丰度升高,拟杆菌门和变形菌门的相对丰度降低。甜叶菊绿原酸可增强腹气囊感染大肠杆菌O78蛋雏鸡机体的免疫功能,抵御大肠杆菌O78对蛋雏鸡的侵袭,其中应用剂量为2.0 g·L-1甜叶菊绿原酸的效果较好。这预示绿原酸具有抗生素替代品的功效,其对大肠杆菌感染蛋雏鸡机体免疫力的积极作用可能是通过调控免疫相关基因和维持盲肠微生物菌群稳态达到的,但其作用机制仍需深入的研究。 相似文献
11.
Twenty four, 21-d-old female pigs were fed diets containing either skim milk powder (CON+), spray-dried bovine colostrum (7.5%, BC+) or spray-dried bovine plasma (7.5%, BP+) and were dosed orally with 1 × 109 CFU of E. coli O149:K88. Another group of 8 unchallenged pigs was fed the skim milk powder diet (CON−). On d 19 of the experiment all piglets were euthanased. Adverse effects of the E. coli challenge were observed variously throughout the small intestine in pigs consuming either the BC+ or BP+ diets. In this experiment, similar responses to the E. coli challenge were observed in both plasma and colostrum fed pigs, which suggests that spray-dried bovine colostrum may be a potential alternative to spray-dried bovine plasma. 相似文献
12.
Quantitative risk assessment of human listeriosis from consumption of soft cheese made from raw milk 总被引:1,自引:0,他引:1
N. Bemrah M. Sanaa M. H. Cassin M. W. Griffiths O. Cerf 《Preventive veterinary medicine》1998,37(1-4):129-145
Microbial hazards have been identified in soft cheese made from raw milk. Quantification of the resulting risk for public health was attempted within the frame of the Codex Alimentarius Commission, 1995 approach to quantitative risk assessment, using Monte Carlo simulation software. Quantitative data could only be found for Listeria monocytogenes. The complete process of cheese making was modeled, from milking to consumption. Using data published on the different sources of milk contamination (environment and mastitis) and bacterial growth, distributions were assumed for parameters of the model. Equations of Farber, J.M., Ross, W.H., Harwing, J. (1996) for general and at-risk populations were used to link the ingested dose of L. monocytogenes to the occurrence of listeriosis. The probability of milk contamination was estimated to be 67% with concentration ranging from 0 to 33 CFU ml−1. The percentage of cheese with a predicted concentration of L. monocytogenes greater than 100 CFU g−1 was low (1.4%). The probability of consuming a contaminated cheese serving was 65.3%. Individual annual cumulative risk of listeriosis, in a population each consuming 50 servings of 31 g, ranged from 1.97 × 10−9 to 6.4 × 10−8 in a low-risk sub-population and 1.04 10−6 to 7.19 10−5 in a high-risk sub-population. The average number of expected cases of listeriosis per year was 57 for a high-risk sub-population and one for a low-risk healthy sub-population. When the frequency of environmental milk contamination was reduced in the model and L. monocytogenes mastitis was eliminated, the expected incidence of listeriosis decreased substantially; the average number of expected cases was reduced by a factor of 5. Thus the usefulness of simulation to demonstrate the efficiency of various management options could be demonstrated, even if results should be interpreted with care (as many assumptions had to be made on data and their distributions). 相似文献
13.
Pathogenic microorganisms in manure represents a potential hazard to human and animal. Few data describing the microbiological content of liquid hog manure intended for spreading are available in the scientific literature. The objective of this project was to verify the presence and estimate the persistence of Escherichia coli, Salmonella spp., Yersinia enterocolitica and Cryptosporidium spp. in liquid hog manure from storages under conditions typical of commercial swine production in Québec. E. coli content of liquid hog manure taken during the spreading period in the 32 hog operations varied between 0 and 5.52 log10 CFU/g with a 95% confidence interval of 3.16–4.23 log10 CFU/g. Salmonella spp., Y. enterocolitica and Cryptosporidium spp. were detected in 37%, 9% and 3% samples, respectively. Under the conditions of this experiment, the predicted number of days required to obtain a 90% reduction of E. coli populations varied between 15 and 26 days, while the predicted storage period necessary to reach undetectable levels was 54–114 days. The maximal persistence of Salmonella observed in this study was 88 days. A 73-day storage time was insufficient for the elimination of Y. enterocolitica. 相似文献
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为了研究前列腺素D2(prostaglandin D2,PGD2)/DP1受体途径对大肠杆菌(Escherichia coli)和金黄色葡萄球菌(Staphylococcus aureus)感染奶牛子宫内膜组织中炎症介质HMGB-1和PAFR的表达及对组织损伤程度的影响,试验以体外培养奶牛子宫内膜组织为研究对象,应用1×10-6 mol/L DP1受体激动剂(BW-245C和15d-PGJ2)和等量(1×106 CFU/mL)大肠杆菌、金黄色葡萄球菌共同处理奶牛子宫内膜组织,采用实时荧光定量PCR、免疫组化和HE染色法检测奶牛子宫内膜组织中HMGB-1和PAFR的表达并评价组织损伤情况。结果显示,与空白对照组相比,大肠杆菌和金黄色葡萄球菌感染奶牛子宫内膜组织中HMGB-1和PAFR表达量显著升高(P<0.05),而DP1受体激动剂与大肠杆菌和金黄色葡萄球菌共处理奶牛子宫内膜组织中DP1受体激动剂显著抑制奶牛子宫组织中HMGB-1和PAFR的表达(P<0.05)。HE染色结果显示,大肠杆菌与金黄色葡萄球菌感染的奶牛子宫内膜组织上皮细胞和腺上皮细胞完全脱落、坏死、崩解;而DP1受体激动剂、大肠杆菌、金黄色葡萄球菌共同处理奶牛子宫内膜组织中,DP1受体激动剂的加入显著减轻奶牛子宫内膜组织的损伤程度(P<0.05)。免疫组化染色法结果与以上两种方法结果一致。结果表明,PGD2能够抑制大肠杆菌与金黄色葡萄球菌感染的奶牛子宫内膜组织中损伤相关因子HMGB-1、PAFR的表达,减轻组织损伤程度,这一作用可能是由DP1受体所介导的。 相似文献
16.
The F18 fimbrial adhesin FedF is highly conserved among F18+Escherichia coli isolates 总被引:2,自引:0,他引:2
F18+ Escherichia coli cause postweaning diarrhoea and oedema disease in newly weaned piglets. Protection against these diseases can be established by preventing the fimbrial adhesion of these bacteria to the enterocytes of the porcine intestine. To test a vaccine against F18+ E. coli consisting of the adhesin of F18 fimbriae, FedF, the conservation of the FedF subunit had to be examined. Therefore, the fedF sequence of 37 F18+ E. coli isolates from different countries was determined and compared to the fedF gene of the F18ab reference strain F107/86. The amino acid sequence of the mature FedF from the individual F18+ E. coli isolates was 96–100% identical to that from E. coli F107/86, but the overall homology was 90.4%. Hyper variable regions were not found in the FedF sequence. The FedF sequence was conserved over the different countries and between the two antigenic variants, F18ab and F18ac, suggesting that F18ab and F18ac strains have the same receptor. Furthermore, the conserved C-terminal region in the FedF adhesin suggests that the F18 fimbriae, in analogy with type 1 and P pili, are assembled by a donor strand mechanism. In conclusion, the reported conservation of FedF supports the usefulness of the fimbrial adhesin as a subunit vaccine against F18+ E. coli infection. 相似文献
17.
In a study of diarrhoeic and non-diarrhoeic livestock (cattle, pigs and sheep) from 50 farms in Trinidad, the prevalence of bacterial (Campylobacter, Salmonella, Yersinia and Escherichia coli), parasitic (coccidia, Cryptosporidium and enteric helminths) and viral (rotavirus) enteropathogens in faeces or rectal swabs was determined. Occurrence of the enteropathogens was tested for association with age, health status, animal species and mixed infections.
Of 423 diarrhoeic animals tested, Salmonella was isolated from 21 (5.0%), Campylobacter from 191 (45.2%) and Yersinia from three (0.7%), while the corresponding prevalence from 270 non-diarrhoeic controls was eight (3.0%) (χ2 1.19, P = 0.28), 119 (44.1%) (χ2 0.04, P = 0.85) and four (1.5%) (χ2 0.8, P = 0.39), respectively. Verocytotoxigenic E. coli and heat-labile toxin-producing E. coli were isolated from 51 (13.7%) and five (1.3%), respectively, of 373 diarrhoeic animals but the corresponding prevalence from 258 non-diarrhoeic animals was 39 (15.1%) (χ2 0.15, P = 0.7) and five (1.9%) (χ2 0.07, P = 0.8), respectively. Cryptosporidium oocytes were detected in 67 (16.5%) of 406 diarrhoeic animals and from 31 (12.1%) of 257 non-diarrhoeic animals (χ2 2.13, P = 0.15). For 147 diarrhoeic animals tested for coccidia, 64 (43.5%) were positive compared with 34 (37.8%) of 90 non-diarrhoeic animals (χ2 0.54, P = 0.49).
The prevalence of rotavirus infection was significantly (P 0.001, χ2 37.8) higher in diarrhoeic animals (39.9%, 112 of 281) than in non-diarrhoeic animals (13.4%, 26 of 194). 相似文献
18.
本试验旨在建立一种乳品中大肠杆菌PMA-qPCR活菌检测方法.优化qPCR检测方法,探究菌浓度为1×108 CFU/mL的大肠杆菌活菌悬液、热致死菌悬液细胞数来确定不同的PMA剂量、暗孵育时间、曝光时间对死菌抑制效果的影响,确定最佳PMA处理方案.结果表明,qPCR检测可特异性扩增大肠杆菌,1×108 CFU/mL的大肠杆菌经90 ℃水浴30 s全部致死后,采用10 μg/mL的 PMA暗孵育15 min后冰上曝光10 min为最佳处理方案,这种处理方案可最大程度抑制死细胞信号,而对活细胞几乎没有影响,样品中微生物初始浓度不低于1×108 CFU/mL时较稳定,得到标准曲线回归方程y=-3.356x+47.413,R2=0.9989,最低检测限为103 CFU/mL,加标样本检测结果与实际相符.该方法为利用PMA-qPCR检测食品中的活大肠杆菌杆菌奠定了基础. 相似文献
19.
GAI Dong-xue REN Hong-lin LU Shi-ying HU Pan MENG Xian-mei LIU Xi SONG De-gang JIN Wen ZHANG Song CHANG Jiang LIU Yan-yan LIU Zeng-shan 《中国畜牧兽医》2016,43(2):493-498
In order to detect viable E.coli in milk,a new PMA-qPCR method was established.The influences of different PMA concentration,dark incubation time,exposure time on dead bacteria inhibition effect were determined by detection of the cell numbers of viable and heat-killed E.coli suspensions at concentration of 1×108 CFU/mL through fluorescence quantitative PCR (qPCR) method.The results showed that qPCR assay could specifically detect E.coli,and the viable E.coli must be exposed to 90 ℃ for 30 s in water bath to be lethal.The best treatment was 10 μg/mL PMA with 15 min of dark incubation time and 10 min of exposure time.This treatment could inhibit dead cell signals to a largest extend,while had little impact on aviable cells.The stability of PMA-qPCR assay was kept while the concentration of bacteria was more than 1×108 CFU/mL.The regression equation of standard curve was y=-3.356x+47.413,R2=0.9989,the lowest detection limit was 103 CFU/mL.The result of adding assay was agreed with the actual situation.This study laid a foundation for using of PMA-qPCR to detect the viable E.coli in food. 相似文献
20.
试验旨在探索革兰氏阴性菌大肠杆菌(Escherichia coli,E.coli)及其表面分子脂多糖(LPS)诱导胰腺再生蛋白Ⅲγ(RegⅢγ)表达调控的机制。首先,用不同浓度灭活E.coli(109、108、107、106、105、104 CFU/mL)和LPS (0.01、0.1、1、5、10、20、40、80 μg/mL)诱导猪肠黏膜上皮细胞(IPEC-JⅡ),用MTT法测D490 nm值,检测E.coli和LPS对IPEC-JⅡ细胞活力的影响;其次,用不同浓度灭活E.coli(107、106、105 CFU/mL)和LPS (0.01、0.1、1、5 μg/mL)处理IPEC-JⅡ细胞24 h,用实时荧光定量PCR和Western blotting检测RegⅢγ mRNA和蛋白的表达;最后,用1 μg/mL LPS处理IPEC-JⅡ细胞24 h,用实时荧光定量PCR和Western blotting检测p65、p38、JNK、ERK mRNA和蛋白表达及磷酸化水平。结果显示,除0.01 μg/mL LPS不抑制IPEC-JⅡ细胞活力外,其他浓度的灭活E.coli和LPS均可抑制IPEC-JⅡ细胞活力,且109、108 CFU/mL E.coli和10、20、40、80 μg/mL LPS组细胞活力极显著下降(P<0.01);与对照组相比,107、106和105 CFU/mL E.coli均能诱导RegⅢγ表达增加,且105 CFU/mL E.coli组RegⅢγ mRNA表达量极显著高于对照组(P<0.01),蛋白表达量显著高于对照组(P<0.05);0.01、0.1、1和10 μg/mL LPS均能诱导RegⅢγ表达增加,且0.1和1 μg/mL LPS组RegⅢγ mRNA表达量极显著高于对照组(P<0.01),RegⅢγ蛋白表达虽有增加趋势,但差异不显著(P>0.05);与对照组相比,1 μg/mL LPS组p65、p38 mRNA表达量极显著增加(P<0.01),JNK、ERK mRNA表达量显著增加(P<0.05);同时,p38、JNK蛋白表达量和磷酸化水平均极显著增加(P<0.01),p65蛋白磷酸化水平显著增加(P<0.05),ERK蛋白和磷酸化水平均增加,但差异不显著(P>0.05)。以上结果表明,灭活E.coli和LPS均可诱导RegⅢγ表达,1 μg/mL LPS可增加p65、p38和JNK蛋白的磷酸化水平。 相似文献