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Development of a lateral flow test for the rapid detection of <Emphasis Type="Italic">Avibacterium paragallinarum</Emphasis> in chickens suspected of having infectious coryza
Authors:Sandra Morales Ruiz  Jorge Bendezu  Ricardo Choque Guevara  Ricardo Montesinos  David Requena  Luz Choque Moreau  Ángela Montalván Ávalos  Manolo Fernández-Díaz
Institution:1.Laboratorios de Investigación y Desarrollo,FARVET SAC,Chincha Alta,Peru;2.Laboratorio de Bioinformática y Biología Molecular, Laboratorio de Investigación y Desarrollo,Universidad Peruana Cayetano Heredia,Lima,Peru;3.FARVET SPF SAC,Chincha Alta,Peru
Abstract:

Background

Infectious coryza (IC) is an acute respiratory disease of growing chickens and layers caused by Avibacterium paragallinarum. The development of tools that allow rapid pathogen detection is necessary in order to avoid disease dissemination and economic losses in poultry. An Av. paragallinarum-specific Ma-4 epitope of the TonB-dependent transporter (TBDT) was selected using bioinformatic tools in order to immunize a BalbC mouse and to produce monoclonal antibodies to be used in a lateral flow test (LFT) developed for Av. paragallinarum detection in chicken nasal mucus samples.

Results

The 1G7G8 monoclonal antibody was able to detect TBDT in Av. paragallinarum cultures (serogroups: A, B and C) by Western blot and indirect ELISA assay. Consequently, we developed a self-pairing prototype LFT. The limit of detection of the prototype LFT using Av. paragallinarum cultures was 1?×?104 colony-forming units (CFU)/mL. Thirty-five nasal mucus samples from chickens suspected of having infectious coryza were evaluated for the LFT detection capacity and compared with bacterial isolation (B.I) and polymerase chain reaction (PCR). Comparative indicators such as sensitivity (Se), specificity (Sp), positive predictive value (PPV), negative predictive values (NPV) and the kappa index (K) were obtained. The values were 100.0% Se, 50% Sp, 65.4% PPV, 100% NPV, and 0.49?K and 83.9% Se, 100% Sp, 100% PPV, 44.4% NPV, and 0.54?K for the comparison of the LFT with B.I and PCR, respectively. Additionally, the LFT allowed the detection of Av. paragallinarum from coinfection cases of Av. paragallinarum with Gallibacterium anatis.

Conclusions

The results indicate that the self-pairing prototype LFT is suitable for the detection of TBDT in Av. paragallinarum cultures as well as in field samples such as nasal mucus from Av. paragallinarum-infected chickens. Therefore, this prototype LFT could be considered a rapid and promising tool to be used in farm conditions for Av. paragallinarum diagnosis.
Keywords:
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