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Research Note: Repetitive element–based polymerase chain reaction genotyping improves efficiency of Salmonella surveillance in a model broiler production system

机译:研究注意:重复的元素的聚合酶链反应基因分型提高了模型肉鸡生产系统中的沙门氏菌监测的效率

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摘要

The genetic relatedness and antimicrobial susceptibility profiles of Salmonella isolated from poultry and their environment were determined. One broiler breeder flock (BBF1) and 2 broiler flocks (BF1 and BF2) were reared over a 1.75-year period on the same poultry research farm. Hatching eggs were obtained from BBF1 to produce BF1 chicks, while BF2 chicks were progeny of a separate, unsampled broiler breeder flock. BF1 and BF2 were reared in the same housing facilities but 6 mo apart. Salmonella isolates were collected via litter sock sampling (BF1), cecal excision (BF1 and BF2), or cloacal swabs (BBF1). Serotyping identified Salmonella enterica subsp. enterica serovar Altona (SA) in BBF1 and S. enterica subsp. enterica serovar Senftenberg (SS) in BF1 and BF2. Genotypic fingerprinting was achieved with Rep-PCR using the (GTG)5 primer and revealed sequence homology among Senftenberg isolates from BF1 and BF2. For each isolate, the minimum inhibitory concentration was determined for 27 antimicrobial agents using Sensititre plates with formularies specific to antimicrobials used in poultry production or those used to control gram negative pathogens. Isolates from the 3 flocks were resistant to clindamycin, erythromycin, novobiocin, penicillin, and tylosin tartrate and demonstrated intermediate resistance to azithromycin, florfenicol, and spectinomycin. These data demonstrated that serovar Altona and Senftenberg were harbored by poultry, the latter appeared to persist in broiler flocks, and both serotypes shared similar patterns of antimicrobial susceptibility in an integrated research operation. In the case of multiple Salmonella isolates, combining genotypic fingerprinting methods with serotyping of representative isolates would reduce the number of samples required for serotyping and more clearly identify relatedness of isolates. These methods facilitate effective surveillance in poultry production systems, thus allowing for implementation of precise Salmonella control measures.
机译:确定了从家禽和环境中分离的沙门氏菌的遗传相关性和抗微生物敏感性谱。在同一家禽研究场的1.75年期间,饲养一个肉鸡繁殖群(BBF1)和2个肉鸡群(BF1和BF2)。从BBF1获得孵化蛋以产生BF1雏鸡,而BF2雏鸡是单独的,未加注的肉鸡繁殖者的后代。 BF1和BF2被饲养在相同的住房设施中,但6 Mo分开。通过垃圾袜采样(BF1),肠切除(BF1和BF2)或癌拭子(BBF1)收集沙门氏菌分离株。血清型鉴定了Salmonella entenica subsp。 BBF1和S. enteica Subsp的Entenica Serovar Altona(SA)。 BF1和BF2中的Enteica Serovar Senftenberg(SS)。使用(GTG)5引物通过Rep-PCR实现基因型指纹识别,并在来自BF1和BF2的Senftenberg分离株中揭示了序列同源物。对于每种分离物,使用具有特异于家禽生产的抗微生物或用于控制革兰阴性病原体的抗微生物的抗微生物的敏感剂或用于控制革兰阴性病原体的抗微生物的抗微生物剂的最小抑制浓度。来自3群的分离物对Clindamycin,红霉素,Novociocin,青霉素和Tylosin Tartrate,并表现出对阿奇霉素,氟芬辛醇和透明霉素的中间抗性。这些数据表明,塞洛达拉和森林培尔特被家禽覆盖,后者似乎持续存在于肉鸡羊群中,两种血清型都在综合研究操作中共享了类似的抗菌易患模式。在多种沙门氏菌分离物的情况下,组合具有代表性分离物的血清型的基因型指纹方法将减少血清型化所需的样品的数量,并且更明显地识别分离物的相关性。这些方法有助于在家禽生产系统中进行有效监测,从而允许实施精确的沙门氏菌控制措施。

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