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undergraduate course at Davidson College.
Song, et
al's"Deep RNA Sequencing Reveals Novel Cardiac Transcriptomic
Signatures for Physiological and Pathological Hypertrophy"
Figure 2
This figure begin to explore the general
interaction patterns of DEGs in PAH and PHH models,
attempting to identify key players in the
differentiation of the hypertrophy models.
Part A of this figure
represents a network of interactions of the genes up-regulated in PAH
heart tissue relative to the normal or PHH heart tissue. The network was
derived through Ingenuity
Pathway Analysis (IPA), a software approach which generates
plausible interactions of genes/proteins, based on interactions described in
scientific literature. Each red node represents a gene upregulated in PAH
relative to controls or PHH heart cells. White nodes thus represent genes
expressed in PAH but also control heart cells.
This approach showed that the transcription
regulator genes Foxm1 (Forkhead
box M1),
Plk1
(polo-like kinase 1) and
E2F1
(E2F transcription factor 1) – or more directly their corresponding
proteins – are implicated in the regulation of a number of other proteins
involved in PAH suggesting a strong role of these proteins in PAH
pathogenesis.
Part B of this figure elaborates on
figures 1B and 2A, providing histograms illustrating the degree of
expression of the three specific genes which, as portrayed above, are
strongly implicated as upstream regulators of many factors involved in
PAH. The y axes, though unlabeled, represent the relative
degree of gene expression in each experimental group at each point along the
gene, based on the number of reads collected from each of the four mouse
types' that could be mapped to the UCSC Genome Browser database. Each
of these three genes is seen to be over-expressed in the PAH models (TAC)
relative to PHH models (Exercise) or controls (Sham and Sedentary),
further implicating these proteins in PAH pathogenesis. Positions
along each gene are designated by the blue lines below the TAC read from
each gene category, where thicker segments correspond to exons.
Part C of this
figure shows variations in sequences (illustrated in the sequence logos;
the four diagrams with variable T, A, G and C heights) 1000 base pairs
upstream of 417 genes up-regulated in PAH. This was done to inspect
whether these sequences matched the binding sites of the transcription
factors FOXM1 and PU.1, to substantiate these transcription factors'
influence over expression of these genes.
The first and third sequence logos from the top show the consensus
sequences (binding sites) of FOXM1 and PU.1 respectively (whose expression
across experimental groups are represented in the horizontal heatmaps; both
are particularly enhanced in PAH models), and the patterns observed in the
PAH up-regulated genes are shown in the second and fourth letter diagrams
from the top. Letter height relative to a given position in a motif
corresponds to the frequency at whcih a given nucleotide occurs at that
position. Overall height at a position corresponds to "information
content," corresponding to the probability at which the given
nucleotide ratio labeled at a given position will be identified.
Given the similarity between these genes' upstream
promoter regions and the consensus sequences of FOXM1 and PU.1, this
figure suggests that the expression of many of the genes upregulated in
PAH is influenced by activity of FOXM1 or PU.1, with FOXM1 being more
selectively involved in the process as it is the only of the two
proteins selectively up-regulated in PAH.
Sh = sham; T = TAC; Se = sedentary; Ex =
exercise.
Figure 2D provides another
heatmap representing the degree of expression of the
genes targeted by FOXM1. Strong expression of FOXM1 as
reported in figure 2C is more notable due to the accompanying increased
expression of the protein's downstream targets, further implying that this
protein exerts a key role in PAH pathogenesis.
PMID = PubMed Identifier (a number associated with PubMed
databases with the corresponding gene.
Overall, figure 2 suggests FOXM1 as a likely
transcription factor involved in PAH pathogenesis due to its and its
targets up-regulation in PAH relative to PHH models and controls.
Table 1 and subsequent figures elaborate further on some of the gene
expression differences between PAH and PHH, focusing on alternative
splicing, a more specific aspect of genomic alterations that may occur
between PAH and PHH models.
References
Song,
H. K., Hong, S. E., Kim, T., Kim D. H., et al. (2012). Deep
RNA sequencing reveals novel cardiac transcriptomic signatures for
physiological and pathological hypertrophy. PLoS One, 7,
e35552.
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