62,829 research outputs found
Wide-Scale Analysis of Human Functional Transcription Factor Binding Reveals a Strong Bias towards the Transcription Start Site
We introduce a novel method to screen the promoters of a set of genes with
shared biological function, against a precompiled library of motifs, and find
those motifs which are statistically over-represented in the gene set. The gene
sets were obtained from the functional Gene Ontology (GO) classification; for
each set and motif we optimized the sequence similarity score threshold,
independently for every location window (measured with respect to the TSS),
taking into account the location dependent nucleotide heterogeneity along the
promoters of the target genes. We performed a high throughput analysis,
searching the promoters (from 200bp downstream to 1000bp upstream the TSS), of
more than 8000 human and 23,000 mouse genes, for 134 functional Gene Ontology
classes and for 412 known DNA motifs. When combined with binding site and
location conservation between human and mouse, the method identifies with high
probability functional binding sites that regulate groups of biologically
related genes. We found many location-sensitive functional binding events and
showed that they clustered close to the TSS. Our method and findings were put
to several experimental tests. By allowing a "flexible" threshold and combining
our functional class and location specific search method with conservation
between human and mouse, we are able to identify reliably functional TF binding
sites. This is an essential step towards constructing regulatory networks and
elucidating the design principles that govern transcriptional regulation of
expression. The promoter region proximal to the TSS appears to be of central
importance for regulation of transcription in human and mouse, just as it is in
bacteria and yeast.Comment: 31 pages, including Supplementary Information and figure
Dynamics of transcription factor binding site evolution
Evolution of gene regulation is crucial for our understanding of the
phenotypic differences between species, populations and individuals.
Sequence-specific binding of transcription factors to the regulatory regions on
the DNA is a key regulatory mechanism that determines gene expression and hence
heritable phenotypic variation. We use a biophysical model for directional
selection on gene expression to estimate the rates of gain and loss of
transcription factor binding sites (TFBS) in finite populations under both
point and insertion/deletion mutations. Our results show that these rates are
typically slow for a single TFBS in an isolated DNA region, unless the
selection is extremely strong. These rates decrease drastically with increasing
TFBS length or increasingly specific protein-DNA interactions, making the
evolution of sites longer than ~10 bp unlikely on typical eukaryotic speciation
timescales. Similarly, evolution converges to the stationary distribution of
binding sequences very slowly, making the equilibrium assumption questionable.
The availability of longer regulatory sequences in which multiple binding sites
can evolve simultaneously, the presence of "pre-sites" or partially decayed old
sites in the initial sequence, and biophysical cooperativity between
transcription factors, can all facilitate gain of TFBS and reconcile
theoretical calculations with timescales inferred from comparative genetics.Comment: 28 pages, 15 figure
Formation of regulatory modules by local sequence duplication
Turnover of regulatory sequence and function is an important part of
molecular evolution. But what are the modes of sequence evolution leading to
rapid formation and loss of regulatory sites? Here, we show that a large
fraction of neighboring transcription factor binding sites in the fly genome
have formed from a common sequence origin by local duplications. This mode of
evolution is found to produce regulatory information: duplications can seed new
sites in the neighborhood of existing sites. Duplicate seeds evolve
subsequently by point mutations, often towards binding a different factor than
their ancestral neighbor sites. These results are based on a statistical
analysis of 346 cis-regulatory modules in the Drosophila melanogaster genome,
and a comparison set of intergenic regulatory sequence in Saccharomyces
cerevisiae. In fly regulatory modules, pairs of binding sites show
significantly enhanced sequence similarity up to distances of about 50 bp. We
analyze these data in terms of an evolutionary model with two distinct modes of
site formation: (i) evolution from independent sequence origin and (ii)
divergent evolution following duplication of a common ancestor sequence. Our
results suggest that pervasive formation of binding sites by local sequence
duplications distinguishes the complex regulatory architecture of higher
eukaryotes from the simpler architecture of unicellular organisms
Adaptive evolution of transcription factor binding sites
The regulation of a gene depends on the binding of transcription factors to
specific sites located in the regulatory region of the gene. The generation of
these binding sites and of cooperativity between them are essential building
blocks in the evolution of complex regulatory networks. We study a theoretical
model for the sequence evolution of binding sites by point mutations. The
approach is based on biophysical models for the binding of transcription
factors to DNA. Hence we derive empirically grounded fitness landscapes, which
enter a population genetics model including mutations, genetic drift, and
selection. We show that the selection for factor binding generically leads to
specific correlations between nucleotide frequencies at different positions of
a binding site. We demonstrate the possibility of rapid adaptive evolution
generating a new binding site for a given transcription factor by point
mutations. The evolutionary time required is estimated in terms of the neutral
(background) mutation rate, the selection coefficient, and the effective
population size. The efficiency of binding site formation is seen to depend on
two joint conditions: the binding site motif must be short enough and the
promoter region must be long enough. These constraints on promoter architecture
are indeed seen in eukaryotic systems. Furthermore, we analyse the adaptive
evolution of genetic switches and of signal integration through binding
cooperativity between different sites. Experimental tests of this picture
involving the statistics of polymorphisms and phylogenies of sites are
discussed.Comment: published versio
The Functional Consequences of Variation in Transcription Factor Binding
One goal of human genetics is to understand how the information for precise
and dynamic gene expression programs is encoded in the genome. The interactions
of transcription factors (TFs) with DNA regulatory elements clearly play an
important role in determining gene expression outputs, yet the regulatory logic
underlying functional transcription factor binding is poorly understood. Many
studies have focused on characterizing the genomic locations of TF binding, yet
it is unclear to what extent TF binding at any specific locus has functional
consequences with respect to gene expression output. To evaluate the context of
functional TF binding we knocked down 59 TFs and chromatin modifiers in one
HapMap lymphoblastoid cell line. We then identified genes whose expression was
affected by the knockdowns. We intersected the gene expression data with
transcription factor binding data (based on ChIP-seq and DNase-seq) within 10
kb of the transcription start sites of expressed genes. This combination of
data allowed us to infer functional TF binding. On average, 14.7% of genes
bound by a factor were differentially expressed following the knockdown of that
factor, suggesting that most interactions between TF and chromatin do not
result in measurable changes in gene expression levels of putative target
genes. We found that functional TF binding is enriched in regulatory elements
that harbor a large number of TF binding sites, at sites with predicted higher
binding affinity, and at sites that are enriched in genomic regions annotated
as active enhancers.Comment: 30 pages, 6 figures (7 supplemental figures and 6 supplemental tables
available upon request to [email protected]). Submitted to PLoS
Genetic
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