Anthony Philippakis scite author profile

Recent advances in sequencing technology make it possible to comprehensively catalogue genetic variation in population samples, creating a foundation for understanding human disease, ancestry and evolution. The amounts of raw data produced are prodigious and many computational steps are required to translate this output into high-quality variant calls. We present a unified analytic framework to discover and genotype variation among multiple samples simultaneously that achieves sensitive and specific results across five sequencing technologies and three distinct, canonical experimental designs. Our process includes (1) initial read mapping; (2) local realignment around indels; (3) base quality score recalibration; (4) SNP discovery and genotyping to find all potential variants; and (5) machine learning to separate true segregating variation from machine artifacts common to next-generation sequencing technologies. We discuss the application of these tools, instantiated in the Genome Analysis Toolkit (GATK), to deep whole-genome, whole-exome capture, and multi-sample low-pass (~4×) 1000 Genomes Project datasets.

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Diversity and Complexity in DNA Recognition by Transcription Factors

Badis

Berger

Philippakis

et al. 2009

Science

907

1,124

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Sequence preferences of DNA-binding proteins are a primary mechanism by which cells interpret the genome. Despite these proteins' central importance in physiology, development, and evolution, comprehensive DNA-binding specificities have been determined experimentally for few proteins. Here, we used microarrays containing all 10-base-pair sequences to examine the binding specificities of 104 distinct mouse DNA-binding proteins representing 22 structural classes. Our results reveal a complex landscape of binding, with virtually every protein analyzed possessing unique preferences. Roughly half of the proteins each recognized multiple distinctly different sequence motifs, challenging our molecular understanding of how proteins interact with their DNA binding sites. This complexity in DNA recognition may be important in gene regulation and in evolution of transcriptional regulatory networks.The interactions between transcription factors (TFs) and their DNA binding sites are an integral part of the gene regulatory networks that control development, core cellular processes, and responses to environmental perturbations. However, only a handful of sequence-specific TFs have been characterized well enough to identify all the sequences that they can and, just as importantly, can not bind. Computational analysis of microarray readout of chromatin immunoprecipitation experiments (ChIP-chip) suggests extensive use of low affinity binding sites in yeast (1), and computational models of gene expression during fly embryonic development suggest that low affinity binding sites contribute as much as high affinity sites (2).The availability of TF binding data spanning the full affinity range would improve our understanding of the biophysical phenomena underlying protein-DNA recognition, and would improve accuracy in analyzing cis regulatory elements. Here we report the comprehensive determination of the DNA binding specificities of 104 known and predicted mouse TFs using the universal protein binding microarray (PBM) technology (3). These TFs represent 22 different DNA binding domain (DBD) structural classes that are the major DBD classes found in metazoan TFs.We created (4) N-terminal GST fusion constructs of the DBDs of 104 known and predicted mouse TFs (Fig. S1 and Table S1). Five of these proteins -Max, Bhlhb2, Gata3, Rfx3, and Sox7 -were also represented as full-length fusions to N-terminal GST, yielding a total set of 109 non-redundant proteins represented by 115 samples (5). Each protein was used in two PBM experiments (6,7) (Figs. S2, S3, S4 and Table S2). DNA binding site motifs initially were derived using the Seed-and-Wobble algorithm (3,8); Seed-and-Wobble first identifies the single 8-mer (ungapped or gapped) with the greatest PBM enrichment score (E-score) (3), and then systematically tests the relative preference of each nucleotide variant at each position both within and outside the seed (5). Later analyses incorporated additional motif finding algorithms, including RankMotif++ (9) and Kafal (5).Beyond simpl...

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Anthony Philippakis

A framework for variation discovery and genotyping using next-generation DNA sequencing data

Diversity and Complexity in DNA Recognition by Transcription Factors

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