Abstract
BackgroundRNAi screens via pooled short hairpin RNAs (shRNAs) have recently become a powerful tool for the identification of essential genes in mammalian cells. In the past years, several pooled large-scale shRNA screens have identified a variety of genes involved in cancer cell proliferation. All of those studies employed microarray analysis, utilizing either the shRNA's half hairpin sequence or an additional shRNA-associated 60 nt barcode sequence as a molecular tag. Here we describe a novel method to decode pooled RNAi screens, namely barcode tiling array analysis, and demonstrate how this approach can be used to precisely quantify the abundance of individual shRNAs from a pool.ResultsWe synthesized DNA microarrays with six overlapping 25 nt long tiling probes complementary to each unique 60 nt molecular barcode sequence associated with every shRNA expression construct. By analyzing dilution series of expression constructs we show how our approach allows quantification of shRNA abundance from a pool and how it clearly outperforms the commonly used analysis via the shRNA's half hairpin sequences. We further demonstrate how barcode tiling arrays can be used to predict anti-proliferative effects of individual shRNAs from pooled negative selection screens. Out of a pool of 305 shRNAs, we identified 28 candidate shRNAs to fully or partially impair the viability of the breast carcinoma cell line MDA-MB-231. Individual validation of a subset of eleven shRNA expression constructs with potential inhibitory, as well as non-inhibitory, effects on the cell line proliferation provides further evidence for the accuracy of the barcode tiling approach.ConclusionsIn summary, we present an improved method for the rapid, quantitative and statistically robust analysis of pooled RNAi screens. Our experimental approach, coupled with commercially available lentiviral vector shRNA libraries, has the potential to greatly facilitate the discovery of putative targets for cancer therapy as well as sensitizers of drug toxicity.
Highlights
RNA interference (RNAi) screens via pooled short hairpin RNAs have recently become a powerful tool for the identification of essential genes in mammalian cells
From a pooled RNAi screen we identified 28 different short hairpin RNAs (shRNAs) sequences which were depleted from a pool of lentiviral infected cells over a period of four weeks
Half hairpin versus barcode tiling analysis In order to assess sensitivity, reproducibility as well as limitations of the barcode tiling approach, we prepared four different template pools with engineered concentrations of individual pGIPZ shRNA expression plasmids
Summary
RNAi screens via pooled short hairpin RNAs (shRNAs) have recently become a powerful tool for the identification of essential genes in mammalian cells. Several pooled large-scale shRNA screens have identified a variety of genes involved in cancer cell proliferation. All of those studies employed microarray analysis, utilizing either the shRNA’s half hairpin sequence or an additional shRNA-associated 60 nt barcode sequence as a molecular tag. One way to identify such essential genes is the inhibition of their [10,11,13] others used unique barcode sequences to analyze pooled shRNA screens [7,9,12] These 60 nt barcode sequences were cloned adjacent to each shRNA template, allowing the determination of the abundance of individual shRNA templates from a complex pool [7]. This means that the abundance of each shRNA template can be detected from a pool, via hybridization to six different probe sequences rather than just one
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