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佛罗里达州商业扩繁种鸡场和商业孵化场中检测滑液支原体的诊断程序评估。

Evaluation of diagnostic procedures to detect Mycoplasma synoviae in commercial multiplier-breeder farms and commercial hatcheries in Florida.

作者信息

Ewing M L, Lauerman L H, Kleven S H, Brown M B

机构信息

Department of Pathobiology, College of Veterinary Medicine, University of Florida, Gainesville 32611-0880, USA.

出版信息

Avian Dis. 1996 Oct-Dec;40(4):798-806.

PMID:8980809
Abstract

Sera from 5325 chickens representing 71 commercial poultry flocks were tested for Mycoplasma synoviae (MS) using standard National Poultry Improvement Program (NPIP) testing guidelines. Based on the NPIP guidelines, only sera (N = 195) from flocks that test positive by specific plate agglutination (SPA) were submitted for additional confirmatory tests. Flocks from three multihouse farms were identified as seropositive for MS and confirmed by culture and polymerase chain reaction (PCR). Serum samples (N = 195) from these seropositive flocks were compared by SPA, enzyme-linked immunoassay (ELISA), and hemagglutination-inhibition (HI). Of the 195 sera tested for MS from these flocks, 145 (74%) sera were positive by SPA. Of the 145 SPA-positive sera, the HI test was positive for 127 samples (90.2%), whereas the ELISA was positive for 141 samples (98.6%). This difference between the two tests was significant (P = 0.0006). Significant differences (P = 0.0002) in titer were obtained from paired serum samples that were submitted to three different laboratories for HI analysis. Both the SPA and HI tests failed to detect early infection in newly introduced flocks following depopulation of MS-positive facilities. Both ELISA and PCR detected new infections on these farms. In the MS outbreak described in this study, SPA was not adequate as the sole screening test and HI was not adequate for confirmation of flock infection status. Continued reliance on the same or a similar type of testing could result in missed infections. Confirmation of infection by PCR was preferable to HI and also may be used in place of culture. The findings of this study suggest that ELISA should be considered as a serologic screen in lieu of SPA, screening with SPA may miss MS-infected flocks, and PCR should be considered as a confirmatory test.

摘要

根据美国国家家禽改良计划(NPIP)的标准检测指南,对代表71个商业家禽群的5325只鸡的血清进行了鸡滑液支原体(MS)检测。根据NPIP指南,只有通过特定平板凝集试验(SPA)检测呈阳性的鸡群的血清(N = 195)才会送去进行额外的确诊检测。来自三个多鸡舍农场的鸡群被确定为MS血清阳性,并通过培养和聚合酶链反应(PCR)得到了确认。通过SPA、酶联免疫吸附测定(ELISA)和血凝抑制试验(HI)对这些血清阳性鸡群的血清样本(N = 195)进行了比较。在这些鸡群检测MS的195份血清中,145份(74%)血清通过SPA检测呈阳性。在这145份SPA阳性血清中,HI试验有127份样本呈阳性(90.2%),而ELISA有141份样本呈阳性(98.6%)。这两种检测方法之间的差异具有统计学意义(P = 0.0006)。将配对血清样本送往三个不同实验室进行HI分析,得到的滴度存在显著差异(P = 0.0002)。在MS阳性设施清栏后新引入的鸡群中,SPA和HI试验均未能检测到早期感染。ELISA和PCR均检测到了这些农场中的新感染情况。在本研究描述的MS疫情中,SPA不足以作为唯一的筛查试验,HI也不足以确认鸡群的感染状况。继续依赖相同或类似类型的检测可能会导致漏检感染。通过PCR确认感染比HI更可取,也可用于替代培养。本研究结果表明,应考虑将ELISA作为血清学筛查方法来替代SPA,用SPA进行筛查可能会遗漏感染MS的鸡群,而PCR应作为确诊试验。

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