Article ID Journal Published Year Pages File Type
2823159 Infection, Genetics and Evolution 2011 9 Pages PDF
Abstract

The present study describes the in silico prediction of the regulatory network of Leishmania infected human macrophages. The construction of the gene regulatory network requires the identification of Transcription Factor Binding Sites (TFBSs) in the regulatory regions (promoters, enhancers) of genes that are regulated upon Leishmania infection. The promoters of human, mouse, rat, dog and chimpanzee genes were first identified in the whole genomes using available experimental data on full length cDNA sequences or deep CAGE tag data (DBTSS, FANTOM3, FANTOM4), mRNA models (ENSEMBL), or using hand annotated data (EPD, TRANSFAC). A phylogenetic footprinting analysis and a MATCH analysis of the promoter sequences were then performed to predict TFBS. Then, an SQL database that integrates all results of promoter analysis as well as other genome annotation information obtained from ENSEMBL, TRANSFAC, TRED (Transcription Regulatory Element Database), ORegAnno and the ENCODE project, was established. Finally publicly available expression data from human Leishmania infected macrophages were analyzed using the genome-wide information on predicted TFBS with the computer system ExPlain™. The gene regulatory network was constructed and activated signal transduction pathways were revealed. The Irak1 pathway was identified as a key pathway regulating gene expression changes in Leishmania infected macrophages.

Research highlights▶ We built a comprehensive promoter database of human, mouse, rat, dog and chimpanzee. ▶ We found all TF bindings sites using PWMs, phylogenetic footprinting and ChIP-seq. ▶ We applied Match and ExPlain to study differentially expressed genes upon infection. ▶ We analyzed signal transduction pathways regulating transcription of such genes. ▶ We found Irak-1 as a key pathway in human macrophage infection by Leishmania major.

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