Our cross species analysis approach could also be extended to data from other cell lines, tissues, and human disease, which could be used to establish an ani mal model database instead of cMap. In addition, except for GO, other rules of gene partition such as KEGG were full read also good options. It was our primary goal to build extended references Inhibitors,Modulators,Libraries and additional gene modulation tools in the online service for biomedical research community. Conclusions In the present work, we introduced a new cross species gene expression module comparison method to make the most of animal expression data and analyze the effectiveness of animal models in drug research. Through exploring the relations between drug molecules and mouse disease models, our method was able to assess whether the corresponding model recapitulates the essential features of the human disease.
If so, this model may be suitable for drug molecules screening or even to test novel therapies systematically. Moreover, through data integration, our method could mine some meaningful information for drug research, such as potential drug candidates, possible Inhibitors,Modulators,Libraries drug repositioning, side effects and information about pharmacology. Methods Data source and preprocessing Drug molecule response data was downloaded from Connectivity Map. cMap is a collection of gene expression profiles of cultured human cells treated with bioactive small molecules or drug molecules. The data set was com posed of mRNA expression data for 164 distinct small molecules and corresponding vehicle controls applied to human cell lines.
All the data was generated by means of Affymetrix GeneChip microar rays. We normalized every instance by ranking the gene expressions and stored them in our own database for comparison. The data of animal models were downloaded from GEO. In TSA case, there were 7 microarray data of mouse osteoblastic cells treated by Tri chostatin Inhibitors,Modulators,Libraries A, including three replicates Inhibitors,Modulators,Libraries of TSA treatment and four replicates of control. In hypoxia case, we used 7 microarray assays of bone marrow cells. The response of mouse to hypoxia was derived from a study by Laifen feld in which mice received decreasing oxygen con centrations from 21% to 6% O2 for 30 minutes. Then, the mice remained at 6% O2 for another 120 minutes and the bone marrows were retrieved from the right humerus. In Diabetes drug case, we got microarray assays of mouse 3T3 L1 adipocyte tis sue cultures fed by metformin.
In Alzheimer case, the animal model was transgenic mice expressing human APP695 and bearing the double Inhibitors,Modulators,Libraries Swedish and Indiana amyloid precursor protein mutations. Six microarray assays, a large scale database of orthologs. The orthologs were com puted by the Reciprocal Smallest Distance algo AG014699 rithm, which was developed by Wall et al. For human and mouse, about 13264 genes were selected by RSD algorithm. These genes covered almost all genes in the small molecule database of cMap.