Identification of candidate miRNA biomarkers from miRNA regulatory network with application to prostate cancer

MicroRNAs (miRNAs) are a class of small non-coding RNAs of approximately 22 nucleotides in length with the potential to regulate human genes through translation inhibition or mRNA cleavage [1]. Recent studies have shown that miRNAs are involved in a wide variety of biological processes such as cell proliferation [2], development [3], and apoptosis [4]. Abnormal expression of miRNAs has been implicated in various human cancers and may constitute a potential signature for cancer diagnosis [5‐7]. However, limited data on cancer related miRNAs are available, and their regulatory mechanisms remain largely unknown.

Extensive research efforts have focused on the identification of potential cancer miRNA biomarkers [6‐10]. The preliminary detection of differentially expressed (DE) miRNAs from large-scale miRNA expression profiling data and low-throughput experimental validation for selected outlier miRNAs are the routine methods used in these studies. As the activities of outlier miRNAs are at least partially reflected in the aberrant expression of their target genes [11], systematic computational approaches that integrate miRNA regulatory data and gene expression profiling data were shown to be more effective to infer potential outlier miRNA activities in cancers [11, 12].

MiRNAs are known to function in a multiple-to-multiple relationship with their target genes, and a concept referred to as miRNA regulation module was proposed based on this theory [13]. This idea was further explored in cancer studies, and attempts have been made to identify candidate abnormal miRNAs or miRNA regulatory modules in cancer [12, 14‐17]. The assumption that abnormal miRNAs associated with cancer show increased functional synergism because of their co-regulatory effects on the same genes [18] was the underlying foundation of these computational approaches.

In contrast to these analyses, the miRNA regulatory network was shown to follow power-law distribution in our study. This implies that more miRNAs tend to have fewer target genes and fewer genes have more miRNA regulators. Based on this analysis, we defined a novel out degree (NOD) measure to characterize the independent regulatory power of individual miRNAs, i.e., the number of genes uniquely regulated by one specific miRNA. Our analysis indicated that miRNAs with larger NOD values are statistically more likely to be candidate cancer biomarkers, which implies that abnormal miRNAs in cancer generally have independent regulatory power. Based on this observation, we proposed a novel pipeline to infer candidate cancer miRNA biomarkers, and applied this method to prostate cancer (PCa). The schematic workflow of our pipeline is shown in Figure 1. Paired miRNA and mRNA expression profiling data for PCa, and reliable miRNA-mRNA interaction data were integrated to generate a PCa conditional miRNA regulatory network, and then candidate PCa miRNA biomarkers in the above conditional network were prioritized according to their independent regulatory power. PubMed citation analysis of the known PCa abnormal miRNAs and in vitro q-PCR technology were used to verify the accuracy of our prediction results. Finally, systematic methods were applied to explore the relationship between PCa and the unique target genes of candidate PCa miRNA biomarkers. The results indicated that our method can detect potential miRNA-mRNA target relationships in specific cancers and can be applied for the identification of miRNA biomarkers in cancer.

Previous studies have provided evidence of multiple-to-multiple relationships between miRNAs and their target genes [41, 42, 51]. From the average view of the miRNA-mRNA target network, that conclusion seems reasonable. Indeed, there are on average 51 target genes for each individual miRNA, and 4 co-regulator miRNAs for each gene in the whole miRNA-mRNA targeting network according to our analysis of the reconstructed network, as described in the Methods section. Based on this theory, numerous attempts have been made to predict cancer related miRNA regulatory modules [14], and cancer miRNAs were shown to have more synergism with their co-regulatory effects on the same genes [18].

In the present study, we conducted an in-depth exploration of this matter. Our results revealed the scale-free feature of the miRNA-mRNA target network. We introduced the NOD index to measure the independent regulatory power of an individual miRNA. Contrary to the functional synergism of cancer miRNAs, our data showed that miRNAs with greater independent regulatory power were more likely to be potential biomarkers in human cancers. Based on this evidence, we developed a novel integrative method to infer candidate cancer miRNA biomarkers from the miRNA regulatory network by linking paired miRNA and gene expression data, and highly reliable miRNA-mRNA target data. This pipeline was further applied to PCa. A total of 39 miRNAs were predicted as potential PCa miRNA signatures. Among these miRNAs, 20 have previously been reported to be PCa aberrant miRNAs by low-throughput methods, and 16 miRNAs were shown to be deregulated in other cancers. In vitro q-PCR experiments and functional analysis further verified the accuracy of our predictions and miR-648 was identified as a novel candidate PCa miRNA biomarker. The target genes of miR-648 are listed in Figure 8. With the exception of BCL11A, the other nine genes are exclusively regulated by miR-648. Among these 10 genes, PAK3 and IL15RA were previously shown to be involved in PCa progression [52, 53], and PAK3 was identified as an epigenetic biomarker for the prognostic diagnosis of PCa [52]. Despite the fact that no reports on the association of the remaining genes with PCa were found, these genes were shown to be associated with the progression of other cancers, such as breast cancer [54] pancreatic cancer [55] and leukemia [56]. These evidences support that miR-648 could be involved in PCa and act as a novel molecular biomarker for PCa diagnosis.

The miRNA-mRNA network reconstructed in this study consisted of experimentally validated data and computational predicted data. The data resources of the computational prediction databases used in this study, HOCTAR [25], ExprTargetDB [26], and starBase [27], were derived from the predictions based on gene expression information, such as microarray data and Next-generation sequencing data. Therefore, this predicted data should be more accurate than data predicted by programs merely based on sequence level, such as TargetScan [57] and RNAhybrid [58]. The reliable miRNA-mRNA targeting data could guarantee the accuracy of the predicted activities of outlier miRNAs.

The present results provide a basis for the development of algorithms for cancer miRNA biomarker identification. Indeed, two points require further improvement. Firstly, as the gene transcriptional expression data do not reflect changes in protein expression levels [11], the cancer miRNA activity cannot be predicted by our method for miRNAs that function through translational repression. Secondly, the detailed outlier patterns (up-regulation or down-regulation) for the prediction of outlier miRNAs need to be further explored. The integration of protein expression data, transcription factor (TF) information and other omics data is a potential method to improve the prediction. This information will be incorporated in future studies aimed at further developing and refining our method.

The present analysis revealed novel distinctive features of cancer miRNA biomarkers. A novel bioinformatics framework was proposed to infer candidate cancer miRNA biomarkers from a miRNA regulatory network. The methodology may accelerate the discovery of novel miRNA signatures for cancer diagnosis and treatment, and should also be feasible for the study of other diseases.