Revisiting Connectivity Map from a gene co‑expression network analysis
- Authors:
- Published online on: June 8, 2018 https://doi.org/10.3892/etm.2018.6275
- Pages: 493-500
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Copyright: © Liu et al. This is an open access article distributed under the terms of Creative Commons Attribution License.
Abstract
Introduction
With the development of high-throughput drug screening, a tremendous amount of genome-wide drug interaction data has been generated. Although valid, most of this information is of lesser value to drug discovery. Due to the sheer immensity of these results, computational approaches are required to parse this data, and discover underlying patterns and networks of activity. Chemical similarities between drug and ligand sets often predict thousands of unanticipated associations, suggesting that a drug may have more than one target, unintentional side effects, or making it a candidate for drug repositioning (1). Having multiple targets is not uncommon: Numerous approved drugs appear to work by modulating multiple genes, including unknown genes (2). In the clinic, numerous mono-therapies have been demonstrated to have limited effects due to gene function redundancy (3). As such, network pharmacology, the study of drug effects on protein-protein interactions, represents the next paradigm in drug discovery (4).
One of the largest pharmacological databases is provided by the Broad Institute of the Massachusetts Institute of Technology and Harvard-the Connectivity Map (CMap), comprising genome-wide gene expression profiles (from microarrays) for three human cell lines in response to cule treatments (5,6). However, the reductionist methods in pharmacology focus only on the tip of an iceberg. Therefore, there is a requirement to re-analyze genome-wide pharmacological data with approaches from systems or networks (7).
Numerous studies have mined CMap to identify potential drugs with a desired action via ‘signature genes’ (8). For instance, Functional Module CMap used multiple functional gene modules to query the CMap and screen candidate drugs (9). The CMap tool has been used to retrieve candidate drugs via signature genes and a rank-based pattern-matching strategy (10). Iskar et al (11) identified conservative transcriptional modules between human cell lines and rat liver by analyzing CMap and DrugMatrix. Raghavan et al (12) performed a search of the CMap database to identify novel drugs for ovarian cancer based on recurrent gene signatures. Cheng et al (13) compared three CMap-based methods regarding their prediction performance against a curated dataset of 890 true drug-indication pairs and identified that XSum, which is also based on disease signatures, performs best. Thus, the premise of most CMap studies is that disease may be characterized by certain important signature genes. However, many studies have relied on its accuracy and predictive value to an unreasonable extent. First, the parameters for ‘signature genes’ may be influenced by population size, the cell line being studied, disease severity or differential gene expression methods (14). Furthermore, gene expression signatures are defined as an alteration in the expression of a gene (or genes) with validated specificity in terms of diagnosis, prognosis or prediction of therapeutic response, ignoring the possibility of gene interactions (15). The definition just focuses on the quantitative gene expression alteration, but ignores the interconnections between genes. Signature genes may be expressed with high correlation. Finally, gene function is not considered by a ‘signature genes’ approach, due to the possibility of redundant gene activity (16). These issues may be resolved by network biology methods, which consider not only the expression but also the modular function of genes.
To address these issues, the present study applied a method termed Weighted Gene Co-expression Network Analysis (WGCNA) to CMap and identified co-expressed gene sets (modules) with functional annotations. Although the CMap has been extensively analyzed, the common traits among these drugs are often neglected. The present analysis revealed common targets for chemical drugs among transcriptional networks, and is intended to serve as an outline for a module-based method for drug repositioning studies.
Materials and methods
Data acquisition
The microarray dataset was downloaded from the CMap server (https://portals.broadinstitute.org/cmap/cel_file_chunks.jsp). After excluding chips that were not from the Affymetrix HT_HG-U133A platform and disrupted files, 5,195 gene expression profiles from 3 cell lines (MCF7, breast cancer epithelial cells; PC3, human prostate cancer cells; HL60, human promyeloblasts) treated with 1,219 drug-like compounds were analyzed. All of these samples were pooled together for use in WGCNA algorithms to identify common modules (data not shown).
Microarray data analysis
Microarray data analysis was performed by using the Affymetrix Expression Console software (v1.4.1.46; Affymetrix Inc., Santa Clara, CA, USA) and the MAS5 normalization method. WGCNA was performed according to the manual (17). Signed co-expression networks were constructed on the genome-wide 22,215 probes using the WGCNA package (v1.51; R Foundation for Statistical Computing, Vienna, Austria; available from https://cran.r-project.org/src/contrib/WGCNA_1.51.tar.gz) (17) in R (v3.2; R Foundation for Statistical Computing; available from https://www.R-project.org) with the following parameters: Power, 6; minModuleSize, 30; deepSplit, 4; neworkType, ‘signed’. In brief, for each pair of probes, a Pearson correlation coefficient matrix was calculated and the adjacency matrix was then computed by raising the correlation matrix to the power of β, [connection strength=(0.5 + 0.5 × correlation)β] (17). The power of 6 was chosen using the scale-free topology criterion. The weighted network was converted into a network of topological overlap (TO)-an advanced co-expression measurement that considers not only the correlation of two probes with each other, but also the extent of their shared correlations across the weighted network (17). Probes were hierarchically clustered on the basis of their distance as measured by 1-TO. Finally, modules were identified on the dendrogram using the Dynamic Tree Cut algorithm with a height cutoff at 0.995 (18). Highly similar modules were identified by clustering and merged together. Each module was summarized using singular value decomposition so that each module eigengene (ME) represented the first principal component of the module's expression profiles (17). Thus, the ME explains the maximum amount of variation of expression levels within a module, and is considered the most representative gene expression in a module. The ME value was used for downstream analysis.
Functional annotation of the modules
Gene ontology (GO) enrichment analyses for identified modules were performed in the Database for Annotation, Visualization and Integrated Discovery (DAVID) (19).
Clustering of compounds
Based on the ME value, the Euclidean distance was used to cluster compounds. The hierarchical clustering was performed by average linkage clustering. The heatmap was plotted using Genesis software (v1.7.5; Thallinger Lab, Graz, Austria; available from https://genome.tugraz.at/genesisclient/genesisclient_documentation.shtml).
Drug repositioning
The CMap was projected to a nonalcoholic steatohepatitis (NASH) dataset, which was downloaded from the ArrayExpress database (accession no. E-MEXP-3291; available from www.ebi.ac.uk/arrayexpress) and resulted in an ME matrix. The compound ME value was ranked in sequential order. In general, the drug with the highest or lowest ME may be efficient against the selected disease.
Statistical analysis
The correlation between the original module and the sampled module data was calculated by ‘cor’ function in R. In DAVID, the overrepresentation of a term is defined as a modified Fisher's exact P-value with an adjustment for multiple tests using the Benjamini-Hochberg method.
Results
A gene co-expression network for CMap reveals common features of drug pathways
The first task of the present study was to organize and compartmentalize a selection from the CMap database into distinct activity profiles, or modules, which represent widespread gene activation as a result of exposure to drugs. The CMap gene expression profiles were reanalyzed using the WGCNA algorithm. To obtain a scale-free network, a power of 6 was chosen (Fig. 1A). Seven gene co-expression modules were identified (Fig. 1B), and the stability of these modules was verified by sampling a random selection of half of the data in each module 1,000 times and comparing it to the whole module to verify that interconnected gene activities are truly linked-an approach which has been performed previously (20). Each module's stability was expressed as the intra-module connectivity correlation (on a scale from 0 to 1) between the original one and the half-sampled one (Fig. 2A). The module green was the least stable module. The module significance was calculated for each module as the average gene significance of the genes within the module. Four modules had a significant association with drug concentration (Fig. 2B).
To characterize these modules, GO enrichment analysis in the following categories was performed: Biological Process, Cellular Component and Molecular Function. Modules associated with these terms (each assigned a color for simplicity in visual mapping and naming: blue, black, brown, white, green, grey60 and turquoise) were linked to a limited range of molecular functions, which mainly comprised protein, RNA and ATP binding (Table I). Overall, modules that matched these keywords were associated with cell adhesion, extracellular matrix organization, mRNA splicing and translational initiation. Two transcriptionally distinct modules, the blue and black modules, were significantly overrepresentative of cell-cell adhesion genes, although the blue module was highly enriched in nucleoplasm protein-encoding genes and the black module was more enriched with cytosolic genes. Of note, these results suggested that most drugs examined within these modules act through protein binding.
Furthermore, samples were clustered based on ME, and three distinct clusters corresponding to three cell lines used were identified in the CMap, indicating that the cell line contributes more to gene expression than drug treatment (Fig. 3).
Computational drug clustering suggests similar mechanisms of action (MoAs)
In the present study, it was hypothesized that compounds clustered together may trigger similar genes and pathways, which may point to similar MoAs. If correct, a computational approach to determine a drug's MoA based on this premise may provide critical information for determining potential side-effects and repositioning. To further examine the similarity between clustered drugs by ME regarding their MoA, a recently developed computational tool, Drug-Set Enrichment Analysis (21), was used to check for common pathways shared among clustered drugs (Table II). Of note, all 50 drugs that made up Cluster 1 (C1) appeared to operate via upregulation of pathways involved in programmed cell death (data not shown). Another 54-drug cluster (C2), which was the most distant cluster from C1, appeared to be involved in the negative regulation of mesenchymal cell apoptotic processes (P=1.21×10−4). Several drugs from the C2 cluster were antibiotics (data not shown). One of the drugs from the C2 cluster, astemizole, has been reported to be associated with enhanced melanoma growth in mice (22), while another study suggests potential anticancer effects (23). The use of certain antibiotics has already been reported to be associated with increased risk of the incidence and fatality of breast cancer (24), and further studies should therefore be performed to ensure the safety of these drugs.
Table II.The top-ranking Gene Ontology Biological Processes for clusters C1 and C2 determined with the DSEA tool. |
In addition, certain drugs of the C2 module were reported as anticancer agents (data not shown), including estradiol as a treatment for aggressive breast cancer (25) and acetylsalicylic as a preventative cancer treatment (26). However, other studies have provided contradictory reports demonstrating their carcinogenic potential; for instance, astemizole and chloramphenicol have been reported to be anticancer agents and carcinogens (27,28). It is possible that some anti-cancer drugs are DNA alkylating agents and may therefore cause mutations or secondary cancers. These results, while promising, hint at the complexity in the clinically repositioning these drugs, and warrant further investigation.
Module-based analysis for drug repositioning
To provide an example for network-based drug repositioning, a previously reported network of cancer cell lines was used (20). In the present study, a module involved in the cell cycle (red module) was determined to be associated with breast cancer patient survival. The CMap microarray data were projected onto the red module, and the ME was calculated for the 1,219 drug molecules. 8-Azaguanine was identified as the top molecules for cell cycle modulation. In line with these computational predictions, 8-azaguanine has previously been reported to produce marked and reversible growth inhibition, and is clinically used as an anticancer agent (29,30).
This method was also used to screen for genes associated with non-alcoholic fatty liver disease (NAFLD) (Fig. 4). A previous study by our group explored the potential drugs that may be efficient in treating NAFLD using CMap (31). The transcriptome data for NASH were used to construct a network and identify significant gene modules by WGCNA. Modules M4 and M8 were identified as significant modules. They were associated with proteasomal protein degradation (M4) and extracellular matrix (M8). The CMap data were then projected onto the NASH network, and each ME was calculated for the 1,219 chemical molecules. A total of 2 top molecules with the highest MEs were identified for M4 and M8, sulconazole and doxazosin, respectively. Of note, it has been reported that the applications of doxazosin not only include the treatment of hypertension but also the prevention of hepatic steatosis, and even the alleviation of insulin resistance (32). Doxazosin is an antihypertensives drug, but studies on its effects in NASH are currently limited to animal models (32). Sulconazole is an antifungal medication, which is used to treat skin infections (33). Its role in reducing lipid storage (patent no. US9393221; https://google.com/patents/US9393221) and anti-inflammatory (patent no. US5208015 (https://www.google.com/patents/US5208015) has been reported in two US patents. Thus, the promising roles of these drugs in NASH require verification in future clinical studies.
Discussion
CMap is a commonly used database in pharmacology, which has been utilized to identify novel drugs or MoAs. However, most recent studies focus on individual differentially expressed genes or gene signatures, ignoring the gene function redundancy and gene-gene interactions. A disease is thought to rarely be a consequence of an abnormality in a single gene, but is rather reflected by a disruption of a complex gene network (34). The present study re-analyzed the CMap microarray dataset by employing WGCNA, separating drugs and expression profiles into usable modules that may help to predict drug behaviors as well as identify MoAs. In contrast to differential expression analyses, which are based on gene signature methods, the WGCNA method analyzes whole gene clusters involved in similar biological functions. WGCNA ‘modules’ are more stable units than redundant individual signature genes, which may be easily influenced by screening thresholds. In addition, WGCNA may be used to take a deeper look at microarray data, revealing common mechanisms and modes of interaction among drug sets. Of note, this analysis is based upon cellular expression profiles, not the original treatment scope of a drug, meaning that this method also provides a novel opportunity for drug repositioning.
By employing WGCNA methodology, the present study identified 7 biologically meaningful modules associated with cell-cell adhesion, extracellular matrix organization, mRNA splicing, translational initiation and signal transduction. These observed modules demonstrate the activity association of the screened drugs with each other. Clustering based on the ME value may then be performed in order to identify drugs with a similar MoA. Build upon.
Previously, network based techniques have been used for drug repositioning (35). Park et al (36) proposed a network mirroring method, assuming that if two diseases are similar, then a drug for one disease can be effective against the other disease too. Gottlieb et al (37) depended on the observation that similar drugs are indicated for similar diseases to compare multiple drug-drug and disease-disease similarity measures for drug repositioning. Chen et al (38) used bipartite network topology to prioritize the potentially indicated diseases that a drug treats. Luo et al (39) integrated diverse information, including DrugBank database, HPRD database and Comparative Toxicogenomics database, and developed a computational pipeline, called DTINet, to predict novel drug-target interactions from a constructed heterogeneous network. The limitations of these methods include the lack of negative samples and known drug-disease association information. The method in the present study only required the disease and drug gene expression profiles regardless of prior knowledge including protein-protein interactions, drug-disease associations or other sources of information.
Personalized medicine at the molecular level is a useful method to identify drugs tailored to a specific disorder (40). In theory, CMap-based techniques may be used to identify dysfunctional gene expression modules in an affected patient, guiding the clinician to identify drugs that specifically target the dysfunctional gene expression underlying that patient's disorder. Based on this premise, the present study demonstrated how a gene expression phenotype associated with cellular dysregulation may be selected (breast cancer cell cycle), how feature modules of interest associated with that phenotype may be identified and how drugs may be projected onto these modules to identify novel drugs worthy of further investigation and for application to a specific patient's condition.
Based upon this rationale, the present study provided a novel drug discovery/repositioning system. To identify novel treatments for specific diseases or disease subtypes, WGCNA may be used to identify the dysregulated gene expression modules and cross-reference the CMap drug data to the dysregulated modules. The drugs identified may then be ranked according their ME values, and drugs may be screened simply according to their ME.
Acknowledgements
Not applicable.
Funding
This work was supported in part by the National Natural Science Foundation of China (grant nos. 31270454 and 81502091). The authors apologize that not all insightful CMap-associated studies were cited due to lack of space.
Availability of data and materials
The datasets used and/or analyzed during the current study are available from the corresponding author on reasonable request.
Authors' contributions
HH and HT designed the study. SW and LingL collected the data, YL and LiL analyzed the CMap and NAFLD data, WL and WT analyzed the results and drafted the manuscript.
Ethics approval and consent to participate
Not applicable.
Consent for publication
Not applicable.
Competing interests
The authors declare that they have no competing interests.
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