Inhibition of Infectious Bursal Disease Virus by Vector Delivered SiRNA in Cell Culture.

In this study, IBDV was isolated from field cases and confirmed by RT-PCR. The virus was then adapted on chicken embryo fibroblast cells (CEF) in which it showed severe cytopathic effects (CPE). The short hairpin RNA (shRNAs) constructs homologous to the VP2 gene were designed and one, having maximum score and fulfilling maximum Reynolds criteria, was selected for evaluation of effective inhibition. Selected shRNA construct (i.e., VP2-shRNA) was observed to be the most effective for inhibiting VP2 gene expression. Real time PCR analysis was performed to measure the relative expression of VP2 gene in different experimental groups. The VP2 gene was less expressed in virus infected cells co-transfected with VP2-shRNA as compared to mock transfected cells and IBDV+ cells (control) at dose 1.6 µ g. The result showed ∼95% efficient down regulation of VP2 gene mRNA in VP2-shRNA treated cells. These findings suggested that designed shRNA construct achieved high level of inhibition of VP2 gene expression in-vitro. PMID: 25153457 [PubMed - in process]

http://www.ncbi.nlm.nih.gov/pubmed/25153457?dopt=Abstract

Source: Animal Biotechnology - August 27, 2014 Category: Biotechnology Authors: Sahare AA, Bedekar MK, Jain SK, Singh A, Singh S, Sarkhel BC Tags: Anim Biotechnol Source Type: research

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