| Literature DB >> 36242690 |
S Santhosh Kumar1, Snehal Jamalpure2,3, A Nafeez Ahmed1, G Taju1, S Vimal4, S Abdul Majeed1, S Suryakodi1, Syed Rahamathulla5, Kishore M Paknikar2,6, Jyutika M Rajwade7,8, A S Sahul Hameed9.
Abstract
Shrimp farming is an important socioeconomic activity worldwide. Infectious myonecrosis virus (IMNV) is an important shrimp virus responsible for significant mortality (up to 70%) in Litopenaeus vannamei. We produced recombinant capsid protein (r-IMNV31) and obtained a highly specific antibody, anti-r-IMNV31, which was used in WOAH-approved ELISA and Western blot to detect IMNV. Further, anti-r-IMNV31 was employed in an indigenously developed lateral flow immunoassay (LFA) with gold nanoparticles as a visual label. Using LFA, IMNV could be detected rapidly (20 min) from tissue homogenate with high specificity, reproducibility, and sensitivity (LOD = 103 viral particles). LFA was validated with "gold standard" qRT-PCR using 60 samples with high sensitivity (100%), specificity (86%). A Cohen's kappa coefficient of 0.86 suggested "good agreement" between LFA and qRT-PCR. With a shelf-life of ~ 1 year at ambient temperature, the use of LFA in the on-site detection of IMNV by shrimp farmers will be a reality.Entities:
Keywords: Antibody; IMNV; Immunodetection; LFIA; Recombinant capsid protein
Year: 2022 PMID: 36242690 DOI: 10.1007/s10126-022-10172-6
Source DB: PubMed Journal: Mar Biotechnol (NY) ISSN: 1436-2228 Impact factor: 3.727