2 research outputs found
Not Available
Not AvailableBemisia tabaci (Hemiptera: Aleyrodidae) is a highly efficient vector in the spread of chilli
leaf curl virus (ChiLCV, Begomovirus) which is a major constraint in the production
of chilli in South Asia. Transcriptome analysis of B. tabaci post-6 h acquisition of
ChiLCV showed differential expression of 80 (29 upregulated and 51 downregulated)
genes. The maximum number of DEGs are categorized under the biological processes
category followed by cellular components and molecular functions. KEGG analysis of
DEGs showed that the genes are involved in the functions like metabolism, signaling
pathways, cellular processes, and organismal systems. The expression of highly
expressed 20 genes post-ChiLCV acquisition was validated in RT-qPCR. DEGs such
as cytosolic carboxypeptidase 3, dual-specificity protein phosphatase 10, 15, dynein
axonemal heavy chain 17, fasciclin 2, inhibin beta chain, replication factor A protein
1, and Tob1 were found enriched and favored the virus infection and circulation in
B. tabaci. The present study provides an improved understanding of the networks of
molecular interactions between B. tabaci and ChiLCV. The candidate genes of B. tabaci
involved in ChiLCV transmission would be novel targets for the management of the
B. tabaci-begomovirus complex.Not Availabl
Not Available
Not AvailableBemisia tabaci (Hemiptera: Aleyrodidae) is a highly efficient vector in the spread of chilli leaf curl virus (ChiLCV, Begomovirus) which is a major constraint in the production of chilli in South Asia. Transcriptome analysis of B. tabaci post-6 h acquisition of ChiLCV showed differential expression of 80 (29 upregulated and 51 downregulated) genes. The maximum number of DEGs are categorized under the biological processes category followed by cellular components and molecular functions. KEGG analysis of DEGs showed that the genes are involved in the functions like metabolism, signaling pathways, cellular processes, and organismal systems. The expression of highly expressed 20 genes post-ChiLCV acquisition was validated in RT-qPCR. DEGs such as cytosolic carboxypeptidase 3, dual-specificity protein phosphatase 10, 15, dynein axonemal heavy chain 17, fasciclin 2, inhibin beta chain, replication factor A protein 1, and Tob1 were found enriched and favored the virus infection and circulation in B. tabaci. The present study provides an improved understanding of the networks of molecular interactions between B. tabaci and ChiLCV. The candidate genes of B. tabaci involved in ChiLCV transmission would be novel targets for the management of the B. tabaci-begomovirus complex.Not Availabl