Development of a coagglutination kit as a rapid test for diagnosing Newcastle disease in poultry

Naf’an, Muhammad Kholish; Kurniasih, Kurniasih; Untari, Tri; Prakoso, Yos Adi

doi:10.14202/vetworld.2020.1719-1724

Cited by 3 publications

(4 citation statements)

References 23 publications

(22 reference statements)

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“…The previous study described that utilization of polyclonal antibody produced by rabbit vaccination could be used as coagglutination kit with high sensitivity for diagnosing ND in poultry (Naf'an et al, 2020) and diagnosing viral nervous necrosis in fish (Sulistiyono et al, 2020). The findings of the present study indicated that ND polyclonal antibodies produced by vaccination can be used as the primary polyclonal antibody in chickens' tissue staining.…”

Section: Resultssupporting

confidence: 49%

Production of Newcastle Disease Polyclonal Antibody as the Alternative of Immunohistochemistry Primary Antibody against Newcastle Disease in Poultry

Naf’an¹,

Kurniasih²,

Untari³

et al. 2021

WVJ

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Newcastle disease (ND) is the most pathogenic viral infection in poultry. Furthermore, the availability of laboratories that support the molecular diagnosis of ND is still limited in Indonesia. The present study aimed to produce ND polyclonal antibody as the alternative of immunohistochemistry primary antibody against ND in poultry. Two adult male New Zealand White rabbits weighed 2.5 kg were vaccinated seven days after the adaptation using intraperitoneal injection of the ND live vaccine at multilevel doses weekly. The serum was collected inactivated, and purified in the sixth week. A total number of 31 chicken samples were collected and their samples of brain, lung, spleen, and intestine were tested using immunohistochemistry and Reverse Transcription Polymerase Chain reaction (RT-PCR). The result showed that 19/31 (61%) were positive against immunohistochemistry and RT-PCR and a total of 12/31 (39%) were negative. Based on the obtained results, immunohistochemistry using ND polyclonal antibody had a similar accuracy with RT-PCR. It can be concluded that ND polyclonal antibody produced by vaccination in the rabbit could be used as the alternative immunohistochemistry primary antibody for diagnosing ND in poultry.

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Section: Resultssupporting

confidence: 49%

Production of Newcastle Disease Polyclonal Antibody as the Alternative of Immunohistochemistry Primary Antibody against Newcastle Disease in Poultry

Naf’an¹,

Kurniasih²,

Untari³

et al. 2021

WVJ

Self Cite

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“…Briefly, S. aureus was incubated using 5-cyano-2,3-ditolyl tetrazolium chloride (CTC) and thermally treated at 65 °C for 30 min to reach an unculturable red-fluorescent state. − The anti-GCA mAb was conjugated onto the red-colored S. aureus by the binding between the Fc fragment of the mAb and protein A on S.…”

Section: Methodsmentioning

confidence: 99%

Rapid Naked-Eye Detection of a Liver Disease Biomarker by Discovering Its Monoclonal Antibody to Functionalize Engineered Red-Colored Bacteria Probes

Shen

Zhao

et al. 2021

ACS Omega

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Glycocholic acid (GCA) is a biomarker for liver diseases, but few facile naked-eye detection methods have been reported to detect it till now. To tackle this challenge, we first prepared a novel monoclonal mouse antibody (mAb) of GCA by a hybridoma technique. The anti-GCA mAb exhibited high specificity, making its cross-reactivity with seven structurally and functionally related GCA analogs negligible. Using this anti-GCA mAb and an engineered red-colored bacterial strain (Staphylococcus aureus, S. aureus), we developed a simple naked-eye visualized method for GCA detection. Toward this goal, S. aureus bacteria were turned red by 5-cyano-2,3-ditolyl tetrazolium chloride treatment and heat treated to an unculturable state, rendering the bacteria as an optical detection probe powerful in in vitro diagnostics. Through the natural binding ability of protein A on the surface of S. aureus and the Fc fragment of a mouse antibody, the anti-GCA antibody was simply conjugated onto S. aureus. Then, the engineered S. aureus served as a red-colored bioprobe for detecting GCA through a coagglutination test. In the presence of GCA, the bioprobes aggregated into dense red-colored eye-visible clusters, enabling the sensitive detection of GCA with a concentration of 0.05−0.10 μg/mL. This naked-eye visualization method only takes a few minutes to detect GCA and avoids the use of expensive equipment. It represents a rapid, convenient, and simple method for detecting GCA to diagnose liver diseases.

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“…When designing an RT-PCR technique, it's crucial to keep in mind a number of critical processes. A first step is the isolation of RNA (Naf'an et al, 2020). Using polymerase enzymes, PCR works on the premise that it can simultaneously amplify and distinguish between many target nucleic acids.…”

Section: Introductionmentioning

confidence: 99%

“…However, the viruses of interest in this research contain RNA as their nucleic acid, thus PCR cannot be used. Since viral RNA serves as a template for reverse transcription, a particular Alyaa Mohson Reda, et al: Analysis of a Fragment of the Fusion Gene for Newcastle Disease by DNA Sequencing oligonucleotide primer and viral RNA must be used to generate single-stranded complementary DNA (cDNA) (Naf'an et al, 2020). Due to the rapid turnaround time, molecular methods have become more popular for identifying NDV infection.…”

Section: Introductionmentioning

confidence: 99%

Analysis of a Fragment of the Fusion Gene for Newcastle Disease by DNA Sequencing

2022

pnr

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Newcastle disease is caused by Avian Paramyxovirus Type 1 (APMV-1), which is found in the genus Avulavirus and family Paramyxoviridae (Suarez et al., 2020). Mild to severe respiratory, visceral, and central nervous system lesions contribute to the illness's devastating impact on vulnerable flocks.The purpose of this study to analysis of a fragment of the fusion Gene for Newcastle disease virus by DNA sequencing.Three representative Fusion gene for Newcastle disease virus isolates were sequenced by Macrogen, Korea.Alignment of the sequences of the three isolated (AN02, AN03 and AN07) against the registered sequences of Newcastle viruses in the database of NCBI were studied, and the result showed that, 94% identity with avian orthoavulavirus 1 isolate By Ck/IR/MAME96/2017, 99% identity with avian orthoavulavirus 1 isolate INDTNC22020 and 86% identity with avian orthoavulavirus 1 isolate INDTNC22020 respectively.Virulent strain-specific motifs were found in the majority of circulating strains, as shown by partial sequencing of the F gene cleavage site.

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Development of a coagglutination kit as a rapid test for diagnosing Newcastle disease in poultry

Cited by 3 publications

References 23 publications

Production of Newcastle Disease Polyclonal Antibody as the Alternative of Immunohistochemistry Primary Antibody against Newcastle Disease in Poultry

Production of Newcastle Disease Polyclonal Antibody as the Alternative of Immunohistochemistry Primary Antibody against Newcastle Disease in Poultry

Rapid Naked-Eye Detection of a Liver Disease Biomarker by Discovering Its Monoclonal Antibody to Functionalize Engineered Red-Colored Bacteria Probes

Analysis of a Fragment of the Fusion Gene for Newcastle Disease by DNA Sequencing

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