Network condensation - exemplified for stimulations. For each of the panels (a) to (d), in the graphs on the left side a stimulator (S) and a target (T) are connected by a stimulation link. Values in the first (E₁, upper graph) and second experiment (E₂, lower graph) are indicated, where low values are marked green and high values are red (following the heat map metaphor). The coloring scheme is red, pale red, white, pale green and green, in order of decreasing values (see text). The graphs on the right side of each panel show the resulting link after applying our method. For each gene, its values for E₁ and E₂ are now inlineed simultaneously in the circle (value of E₁ on the left, of E₂ on the right side). The link connecting both nodes describes the direction and the amount of change between E₁ and E₂. Links with startup of stimulation are colored in red (a), shutdown links in green (b). If values do not change for both the source and the target, or if they change in a completely inconsistent way, the link is removed, see (c) and (d).

Slider in the ExprEssence user interface. Thresholds may be set independently for both the upper (red arrow) and the lower (green arrow) side of the spectrum of the link scores.

Condensed network resulting from the application of ExprEssence to the network in Fig. 4, using gene expression data from in vivo (left side) and cultured podocytes (right side). Only links with highest and lowest link score were kept (3% quantile on both sides).

A network describing pluripotency-related interaction and regulation data assembled from the literature. The core part describes gene regulation, the upper part signaling pathways, and the part on the left epigenetic phenomena.

Esrrb down-regulation is a later event in the ES-Epiblast transition. Real-time PCR analysis of mouse embryonic stem (ES) cells treated for 12 and 48 hr with a pharmacological inhibitor against JAK to inhibit LIF/JAK/STAT3 signaling, which induces a partial transition to the epiblast state. Note that the known LIF/STAT3 target genes Socs3 and Klf4 are rapidly down-regulated at 12 hr. At this timepoint, Esrrb expression is almost unaffected. As suggested by the model, however, Esrrb inlines down-regulation at 48 hr, whilst Oct4 expression is stable (the FGF/MEK/ERK-inhibitor PD (PD0325901) was applied in all experiments).

Condensed network resulting from the network in Fig. 10. The genes (nodes) contain color-coded (heat map) information about gene expression among young subjects (left side) and old subjects (right side). Expression values for FAS and CASP8 are inlineed to the left and right of the gene (node).

Results of jActiveModules, default parameters, applied to the Pluripotency dataset (case study 2). See also Figs. 7/8.

Network condensation - a gallery of various scenarios. For each gene, its (expression) values are represented by color. For each link, its score is represented by color and thickness. The coloring scheme is red, pale red, white, pale green and green, in order of decreasing values (see text). Links connecting genes with measurement values changing in an inconsistent way are marked by wavy lines. As in Fig. 1, if the interacting genes are linked by a stimulation S → T , the stimulation is assumed to start up, if for both genes, the values go up from E₁ to E₂ ((a), E₁ value: left side of circle, E₂: right side of circle), and it is assumed to be shut down if both values go down (b). An inhibition I ⊣ T is assumed to start up, if the inhibitor value goes up, but the target value goes down (c); it is assumed to shut down if the inhibitor value goes down and the target value goes up (d). In cases (e) and (f) the startup of the stimulation as presented is still a justified hypothesis, even though the target does not go up. For example, in (e) and (f), the stimulation by the source (the stimulator) goes up but it may be counteracted by other inhibiting effects (dashed T-Bar arrow) on the target, as the target does not change (e) or even goes down slightly (f) (source principle, see text). In cases where the amount of the stimulator is constant (g) or goes down slightly (h), the startup of a stimulation is still a justified hypothesis based on the target value. Strictly speaking, we hypothesize the startup of the stimulatory effect on the target gene. For example, in (g), the startup is not concluded from the change in the value of the stimulator, but it may be due to stimulator accumulation in time, and/or due to cooperation of the stimulator with other stimulations of the target which go up at the same time; startup of the stimulating effect is concluded from the behaviour of the target (target principle, see text). Scenario (i) is another example of the source principle: it is a justified hypothesis that the inhibition starts up because the amount of inhibitor increases, even though counteracting stimulations drive the amount of the target. Scenario (k) is another example of the target principle: it is a justified hypothesis that the stimulatory effect goes up, observing the target and assuming other cooperating effects on it. Lastly, if values do not change at all, or if they change in a completely inconsistent way, the amount of change is zero or near to zero, as in (l) and (m) (also see Fig. 1 (c) and (d)). Note that cases (e)-(m) all result in reduced link scores. Hence, inconsistent links tend to be removed from the network, as the link score threshold is made more stringent.

Protein interaction network of the podocyte GBM-interface (STRING-extended expert network).

Podocyte RT-PCR expression analysis of Mag. Mouse kidney and two mouse podocyte cell lines (K5 D and S6) were cultured as reported earlier [63]. Podocyte RNA was isolated using a mixture of guanidine thiocyanate and phenol (TRI Reagent, Sigma) according to the manufacturer's protocol. Reverse transcription was performed on 5 μg denaturated RNA. Real-time PCR was performed with a Light Cycler (Roche Diagnostics, Mannheim, Germany) using the Platinum^® SYBR^® Green qPCR SuperMix-UDG kit (Invitrogen, Heidelberg, Germany) and run at 95°C for 10 min followed by 45 cycles at 95°C for 10 s, 60°C for 5 s, and 72°C for 12 s. Relative expression was normalized using GAPDH. The following primers were used: Mag sense 5'-TGG GCC TAC GAA ACT GTA CC-3', anti-sense: 5'-GCT CCG AGA AGG TGT ACT GG-3', 110 bp expected product size; Gapdh sense 5'-ACC CAG AAG ACT GTG GAT GG-3', antisense 5'-CAC ATT GGG GGT AGG AAC AC-3', 170 bp expected product size. A 50 bp DNA step ladder was loaded in the left lanes.

Network of protein interactions and gene/protein stimulations and inhibitions involved in pluripotency, condensed using ExprEssence and microarray data tracking the transition process from embryonic stem to epiblast-like cell state. Expression values for Trim28, Esrrb, Klf4, Klf2, Klf5 are inlineed to the left (ES state) and to the right (epiblast state) of the gene (node). Esrrb and Trim28 are both found in the upper right corner.

Network adapted from the WikiPathways 'DNA damage response' network in human.

Results of jActiveModules, default parameters, applied to the Podocyte dataset (case study 1). See also Figs. 4/5.

Results of jActiveModules, default parameters, applied to the Ageing dataset (case study 3). See also Figs. 10/11.