RNA interference microarrays: High-throughput loss-of-function genetics in mammalian cells
AUTOR(ES)
Silva, Jose M.
FONTE
National Academy of Sciences
RESUMO
RNA interference (RNAi) is a biological process in which a doubles-tranded RNA directs the silencing of target genes in a sequence-specific manner. Exogenously delivered or endogenously encoded double-stranded RNAs can enter the RNAi pathway and guide the suppression of transgenes and cellular genes. This technique has emerged as a powerful tool for reverse genetic studies aimed toward the elucidation of gene function in numerous biological models. Two approaches, the use of small interfering RNAs and short hairpin RNAs (shRNAs), have been developed to permit the application of RNAi technology in mammalian cells. Here we describe the use of a shRNA-based live-cell microarray that allows simple, low-cost, high-throughput screening of phenotypes caused by the silencing of specific endogenous genes. This approach is a variation of “reverse transfection” in which mammalian cells are cultured on a microarray slide spotted with different shRNAs in a transfection carrier. Individual cell clusters become transfected with a defined shRNA that directs the inhibition of a particular gene of interest, potentially producing a specific phenotype. We have validated this approach by targeting genes involved in cytokinesis and proteasome-mediated proteolysis.
ACESSO AO ARTIGO
http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=404082Documentos Relacionados
- Loss-of-function genetics in mammalian cells: the p53 tumor suppressor model
- Phenotype MicroArrays for High-Throughput Phenotypic Testing and Assay of Gene Function
- High-Throughput Variation Detection and Genotyping Using Microarrays
- Profiling the humoral immune response to infection by using proteome microarrays: High-throughput vaccine and diagnostic antigen discovery
- A High-Throughput Arabidopsis Reverse Genetics System
