Mercurial > repos > mingchen0919 > rmarkdown_wgcna
annotate wgcna_eigengene_visualization.Rmd @ 5:a1a34771304e draft
remove unnecessary r package
author | mingchen0919 |
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date | Sun, 26 Nov 2017 11:00:55 -0500 |
parents | 4275479ada3a |
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rev | line source |
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planemo upload for repository https://github.com/statonlab/docker-GRReport/tree/master/my_tools/rmarkdown_wgcna commit d91f269e8bc09a488ed2e005122bbb4a521f44a0-dirty
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1 --- |
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2 title: 'WGCNA: eigengene visualization' |
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3 output: |
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4 html_document: |
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5 number_sections: true |
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6 toc: true |
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7 theme: cosmo |
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8 highlight: tango |
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9 --- |
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10 |
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11 ```{r setup, include=FALSE, warning=FALSE, message=FALSE} |
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12 knitr::opts_chunk$set( |
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13 echo = ECHO |
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14 ) |
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15 ``` |
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16 |
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17 # Import workspace |
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18 |
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19 This step imports workspace from the **WGCNA: construct network** step. |
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20 |
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21 ```{r} |
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22 fcp = file.copy("CONSTRUCT_NETWORK_WORKSPACE", "deseq.RData") |
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23 load("deseq.RData") |
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24 ``` |
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25 |
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26 |
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27 # Gene modules {.tabset} |
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28 |
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29 ```{r} |
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30 if(!is.na(SOFT_THRESHOLD_POWER)) soft_threshold_power = SOFT_THRESHOLD_POWER |
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31 ``` |
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32 |
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33 ## Identify gene modules |
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34 |
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35 The gene network is constructed based on **soft threshold power = `r soft_threshold_power`** |
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36 |
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37 ```{r} |
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38 gene_network = blockwiseModules(expression_data, power = soft_threshold_power, |
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39 TOMType = "unsigned", minModuleSize = 30, |
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40 reassignThreshold = 0, mergeCutHeight = 0.25, |
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41 numericLabels = TRUE, pamRespectsDendro = FALSE, |
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42 verbose = 3) |
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43 ``` |
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44 |
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45 |
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46 ```{r} |
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47 modules = table(gene_network$colors) |
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48 n_modules = length(modules) - 1 |
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49 module_size_upper = modules[2] |
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50 module_size_lower = modules[length(modules)] |
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51 |
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52 module_table = data.frame(model_label = c(0, 1:n_modules), |
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53 gene_size = as.vector(modules)) |
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54 datatable(t(module_table)) |
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55 ``` |
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56 |
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57 The results above indicates that there are **`r n_modules` gene modules**, labeled 1 through `r length(n_modules)` in order of descending size. The largest module has **`r module_size_upper` genes**, and the smallest module has **`r module_size_lower` genes**. The label 0 is reserved for genes outside of all modules. |
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58 |
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59 |
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60 ## Dendrogram and module plot |
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61 |
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62 ```{r} |
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63 # Convert labels to colors for plotting |
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64 module_colors = labels2colors(gene_network$colors) |
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65 # Plot the dendrogram and the module colors underneath |
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66 plotDendroAndColors(gene_network$dendrograms[[1]], module_colors[gene_network$blockGenes[[1]]], |
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67 "Module colors", |
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68 dendroLabels = FALSE, hang = 0.03, |
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69 addGuide = TRUE, guideHang = 0.05) |
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70 ``` |
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71 |
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72 |
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73 # Gene module correlation |
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74 |
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75 We can calculate eigengenes and use them as representative profiles to quantify similarity of found gene modules. |
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76 |
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77 ```{r} |
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78 n_genes = ncol(expression_data) |
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79 n_samples = nrow(expression_data) |
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80 ``` |
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81 |
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82 ```{r} |
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83 diss_tom = 1-TOMsimilarityFromExpr(expression_data, power = soft_threshold_power) |
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84 set.seed(123) |
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85 select_genes = sample(n_genes, size = PLOT_GENES) |
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86 select_diss_tom = diss_tom[select_genes, select_genes] |
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87 |
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88 # calculate gene tree on selected genes |
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89 select_gene_tree = hclust(as.dist(select_diss_tom), method = 'average') |
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90 select_module_colors = module_colors[select_genes] |
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91 |
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92 # transform diss_tom with a power to make moderately strong connections more visiable in the heatmap. |
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93 plot_diss_tom = select_diss_tom^7 |
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94 # set diagonal to NA for a nicer plot |
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95 diag(plot_diss_tom) = NA |
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96 ``` |
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97 |
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98 |
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99 ```{r fig.align='center'} |
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100 TOMplot(plot_diss_tom, select_gene_tree, select_module_colors, main = "Network heatmap") |
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101 ``` |
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102 |
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103 |
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104 # Eigengene visualization {.tabset} |
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105 |
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106 ## Eigengene dendrogram |
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107 |
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108 ```{r fig.align='center'} |
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109 module_eigengenes = moduleEigengenes(expression_data, module_colors)$eigengenes |
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110 plotEigengeneNetworks(module_eigengenes, "Eigengene dendrogram", |
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111 plotHeatmaps = FALSE) |
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112 ``` |
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113 |
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114 ## Eigengene adjacency heatmap |
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115 |
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116 ```{r fig.align='center'} |
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117 plotEigengeneNetworks(module_eigengenes, "Eigengene adjacency heatmap", |
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118 marHeatmap = c(2, 3, 2, 2), |
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119 plotDendrograms = FALSE, xLabelsAngle = 90) |
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120 ``` |
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121 |