Knowledge based identification of essential signaling from genome-scale siRNA experiments

A Friedman; A Friedman; Armand Bankhead; B Maroto; B Zhang; Carol Rohl; Chester Ni; D Deutscher; DM Levine; E Damoc; E Iorns; G Giaever; IB Weinstein; Iliana Sach; J Harborth; K Oda; M Boutros; M Boutros; Marc Ferrer; Mark Kruger; NL Meur; Nolwenn LeMeur; OM Brunner; R Balasubramanian; R Kittler; R Sacher; RK Curtis; Robert Gentleman; S Draghici; S Li; SA Haney; SE Martin; SR Bartz; X Huang; X Liu

Knowledge based identification of essential signaling from genome-scale siRNA experiments

Authors: A Friedman
A Friedman
Armand Bankhead
B Maroto
B Zhang
Carol Rohl
Chester Ni
D Deutscher
DM Levine
E Damoc
E Iorns
G Giaever
IB Weinstein
Iliana Sach
J Harborth
K Oda
M Boutros
M Boutros
Marc Ferrer
Mark Kruger
NL Meur
Nolwenn LeMeur
OM Brunner
R Balasubramanian
R Kittler
R Sacher
RK Curtis
Robert Gentleman
S Draghici
S Li
SA Haney
SE Martin
SR Bartz
X Huang
X Liu
Publication date: 1 January 2009
Publisher: BioMed Central
Doi

Abstract

Abstract Background A systems biology interpretation of genome-scale RNA interference (RNAi) experiments is complicated by scope, experimental variability and network signaling robustness. Over representation approaches (ORA), such as the Hypergeometric or z-score, are an established statistical framework used to associate RNA interference effectors to biologically annotated gene sets or pathways. These methods, however, do not directly take advantage of our growing understanding of the interactome. Furthermore, these methods can miss partial pathway activation and may be biased by protein complexes. Here we present a novel ORA, protein interaction permutation analysis (PIPA), that takes advantage of canonical pathways and established protein interactions to identify pathways enriched for protein interactions connecting RNAi hits. Results We use PIPA to analyze genome-scale siRNA cell growth screens performed in HeLa and TOV cell lines. First we show that interacting gene pair siRNA hits are more reproducible than single gene hits. Using protein interactions, PIPA identifies enriched pathways not found using the standard Hypergeometric analysis including the FAK <it>cytoskeletal remodeling pathway</it>. Different branches of the <it>FAK </it>pathway are distinctly essential in HeLa versus TOV cell lines while other portions are uneffected by siRNA perturbations. Enriched hits belong to protein interactions associated with cell cycle regulation, anti-apoptosis, and signal transduction. Conclusion PIPA provides an analytical framework to interpret siRNA screen data by merging biologically annotated gene sets with the human interactome. As a result we identify pathways and signaling hypotheses that are statistically enriched to effect cell growth in human cell lines. This method provides a complementary approach to standard gene set enrichment that utilizes the additional knowledge of specific interactions within biological gene sets. </p