Nat Med.作者提供全文的绘图代码,对于学习作图很有帮助(一)

本期教程

获得本期教程全文代码:在订阅号后台回复关键词:20240923

2022年教程总汇

https://mp.weixin.qq.com/s/Lnl258WhbK2a8pRZFuIyVg

2023年教程总汇

https://mp.weixin.qq.com/s/wCTswNP8iHMNvu5GQauHdg

引言

今天分享的文章是2024发表在Nat Med.期刊中,来自上海交通大学医学院的文章,作者提供了全文的绘图代码,确实,对于学习绘图提供充分的素材。也是一个学习作图具重大意义的文章。但是,依旧是基于你有一定基础技能之上。

文中并未给你提供作图原数据,因此,这些都是需要自己去摸索。

文章

Prospective observational study on biomarkers of response in pancreatic ductal adenocarcinoma

文章图形亮点:

1. 全文的图形并不复杂,因此,我们在制图中,并不需要追求那些很复杂的图形,除非,你很牛X,可以自己绘制。
2. 图形中网络图。这个是一个相对值得我们学习的图形之一,WGNCA和DEG都可以做网路图。
3. 提供你全部的绘图代码。

文章图形

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Figure 1

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Figure 2
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Figure 3
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Figure 4

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Figure 5
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Code

1. Figure 1

1.1 PCA

library(scatterplot3d)
library(tidyverse)
library(openxlsx)
library(factoextra) # Extract and Visualize the Results of Multivariate Data Analyses
color.bin <- c("#00599F","#D01910")
dir.create("./results/Figure1",recursive = T)
#----------------------------------------------------------------------------------
#  Step 1: Load Proteomics data
#----------------------------------------------------------------------------------
pro  <- readRDS("./data/proteomics/20230412_PDAC_PRO_exp.rds") # 4787 protein * 281 samples
meta <- readRDS("./data/proteomics/20230412_PDAC_PRO_meta.rds")
identical(rownames(meta),colnames(pro)) # check names
#----------------------------------------------------------------------------------
#  Step 2: PCA
#----------------------------------------------------------------------------------
res.pca.comp <- prcomp(pro, scale = F)
#----------------------------------------------------------------------------------
#  Step 3: Plot
#----------------------------------------------------------------------------------
plot.data <- as.data.frame(res.pca.comp$rotation[, 1:10])
plot.data <- plot.data %>% 
              mutate(ID=rownames(plot.data),
                     Type=meta$Type,
                     TypeColor=color.bin[as.numeric(as.factor(Type))])
pdf("./results/Figure1/1B.PRO_PCA3d.pdf", width = 7, height = 7)
scatterplot3d(x = plot.data$PC2, 
              y = plot.data$PC1, 
              z = plot.data$PC3,
              color = plot.data$TypeColor,
              pch = 16, cex.symbols = 1,
              scale.y = 0.7, angle = 45,
              xlab = "PC2", ylab = "PC1", zlab = "PC3",
              main="3D Scatter Plot of proteomics",
              col.axis = "#444444", col.grid = "#CCCCCC")
legend("bottom", legend = levels(as.factor(meta$Type)),
      col =  color.bin,  pch = 16,
      inset = -0.15, xpd = TRUE, horiz = TRUE)
dev.off()
write.xlsx(plot.data, "./results/Figure1/1B.PRO_PCA3d.xlsx", overwrite = T)
# variance percent of each PC
p <- fviz_eig(res.pca.comp)
var_explained <- get_eig(res.pca.comp)
# var_explained <- res.pca.comp$sdev^2 / sum(res.pca.comp$sdev^2)
ggsave("./results/Figure1/1B.PRO_PCA_percent.pdf",p,width = 5, height = 5)
write.xlsx(var_explained, "./results/Figure1/1B.PRO_PCA_percant.xlsx",rowNames=T, overwrite = T)

1.2 Volcano plot

library(limma)
library(tidyverse)
library(openxlsx)
library(ggpubr)
library(ggthemes)
#----------------------------------------------------------------------------------
#  Step 1: Load Proteomics data
#----------------------------------------------------------------------------------
exp  <- readRDS("./data/proteomics/20230412_PDAC_PRO_exp.rds") # 4787 protein * 281 samples
meta <- readRDS("./data/proteomics/20230412_PDAC_PRO_meta.rds")
identical(rownames(meta),colnames(exp)) # check names
#----------------------------------------------------------------------------------
#  Step 2: limma
#----------------------------------------------------------------------------------
meta      <- meta %>% mutate(contrast=as.factor(Type)) 
design    <- model.matrix(~ 0 + contrast , data = meta) # un-paired
fit       <- lmFit(exp, design)
contrast  <- makeContrasts( Tumor_Normal = contrastT - contrastN , levels = design)
fits      <- contrasts.fit(fit, contrast)
ebFit     <- eBayes(fits)
limma.res <- topTable(ebFit, coef = "Tumor_Normal", adjust.method = 'fdr', number = Inf)
## result
limma.res <- limma.res %>% filter(!is.na(adj.P.Val)) %>% 
              mutate( logP = -log10(adj.P.Val) ) %>%
              mutate( tag = "Tumor -vs- Normal")%>%
              mutate( Gene = ID)
# cutoff:  FC:1.5   adj.p:0.05
limma.res <- limma.res %>% mutate(group=case_when(
                                  (adj.P.Val < 0.05 & logFC > 0.58) ~ "up",
                                  (adj.P.Val < 0.05 & logFC < -0.58) ~ "down",
                                  .default = "not sig"))
table(limma.res$group) # UP:1213 ; DOWN:864 ; not:2710
## output
write.xlsx( limma.res, "./results/Figure1/1C.PRO_Limma_fc1.5.xlsx", overwrite = T, rowNames = F) 
#----------------------------------------------------------------------------------
#  Step 3: Vasualization 
#----------------------------------------------------------------------------------
## volcano
limma.res <- limma.res %>% mutate(group=factor(group,levels = c("up","down","not sig")))
my_label <- paste0( "FC:1.5 ; AdjP:0.05 ; ",
                    "Up:",table(limma.res$group)[1]," ; ",
                    "Down:",table(limma.res$group)[2])
p <- ggscatter(limma.res,
               x = "logFC", y = "logP",
               color = "group", size = 2,
               main = paste0("Tumor -vs- TAC"), # ***
               xlab = "log2FoldChange", ylab = "-log10(adjusted P.value)",
               palette = c("#D01910","#00599F","#CCCCCC"),
               ylim = c(-1, 70),xlim=c(-8,8))+
  theme_base()+
  geom_hline(yintercept = -log10(0.05), linetype="dashed", color = "#222222") +
  geom_vline(xintercept = 0.58 , linetype="dashed", color = "#222222") +
  geom_vline(xintercept = -0.58, linetype="dashed", color = "#222222") +
  labs(subtitle = my_label)+
  theme(plot.background = element_blank())
ggsave("./results/Figure1/1C.PRO_Limma_fc1.5.pdf", p, width = 10, height = 10)

1.3 (d) Enrichment plot

# data : enriched pathways table
plot.data <- read.xlsx("./data/Extended Data Table 3.xlsx", sheet = 2, startRow = 2)
plot.pathway <- c("GO:0006730~one-carbon metabolic process","GO:0006888~ER to Golgi vesicle-mediated transport","hsa00020:Citrate cycle (TCA cycle)","hsa00071:Fatty acid degradation","hsa00190:Oxidative phosphorylation","hsa00250:Alanine, aspartate and glutamate metabolism","hsa00260:Glycine, serine and threonine metabolism","hsa00280:Valine, leucine and isoleucine degradation","hsa00480:Glutathione metabolism","hsa00520:Amino sugar and nucleotide sugar metabolism","hsa00620:Pyruvate metabolism","hsa00630:Glyoxylate and dicarboxylate metabolism","hsa00640:Propanoate metabolism","hsa01100:Metabolic pathways","hsa01200:Carbon metabolism","hsa01212:Fatty acid metabolism","hsa01240:Biosynthesis of cofactors","hsa03010:Ribosome","hsa03060:Protein export","hsa04141:Protein processing in endoplasmic reticulum","hsa04972:Pancreatic secretion","GO:0001916~positive regulation of T cell mediated cytotoxicity","GO:0006096~glycolytic process","GO:0007165~signal transduction","GO:0007266~Rho protein signal transduction","GO:0045087~innate immune response","GO:0050778~positive regulation of immune response","GO:0050853~B cell receptor signaling pathway","GO:0050870~positive regulation of T cell activation","GO:0071346~cellular response to interferon-gamma","hsa04015:Rap1 signaling pathway","hsa04062:Chemokine signaling pathway","hsa04066:HIF-1 signaling pathway","hsa04151:PI3K-Akt signaling pathway","hsa04512:ECM-receptor interaction","hsa04610:Complement and coagulation cascades","hsa04621:NOD-like receptor signaling pathway","hsa04666:Fc gamma R-mediated phagocytosis")
plot.data <- plot.data %>% filter(Term %in% plot.pathway) %>% 
                    mutate(LogFDR= -log10(FDR))
# plot
color.bin <- c("#00599F","#D01910")
p <- ggscatter(plot.data, x = "LogFDR", y = "Fold.Enrichment", color = "Type",
               main = "Enrichment of tumor/TAC protein",
               size = "Ratio", shape = 16,
               label = plot.data$Term, palette = color.bin) + theme_base()
p <- p + scale_size(range = c(4,20)) + 
         scale_x_continuous(limit = c(-10, 40)) + 
         theme(plot.background = element_blank())
ggsave(paste0("./results/Figure1/1D.PRO_deg.tn_enrich.pdf"), p, width = 11, height = 10)

2. Figure 2

2.1 (a) WGCNA

library(WGCNA)
dir.create("./results/Figure2/WGCNA",recursive = T)
#----------------------------------------------------------------------------------
#  Step 1: Loading expression data and set parameters
#----------------------------------------------------------------------------------
protein.nona.tumor <- readRDS("./data/proteomics/wgcna/20230412_PDAC_PRO_Tumor_exp.rds")
corType = "pearson"
corFnc = ifelse(corType=="spearman", cor, bicor)
maxPOutliers = ifelse(corType=="pearson",1, 0.05)
# input data normalization
plot.mat <- t(protein.nona.tumor - rowMeans(protein.nona.tumor)) # row: samples | col: genes
#----------------------------------------------------------------------------------
#  Step 2: identification of outlier samples
#----------------------------------------------------------------------------------
sampleTree = hclust(dist(plot.mat), method = "ward.D")
pdf(paste0("./results/Figure2/WGCNA/1.tree.pdf"), width = 20, height = 9)
plot(sampleTree, main = "Sample clustering to detect outliers", sub="", xlab="")
dev.off()
#----------------------------------------------------------------------------------
#  Step 3: analysis of network topology
#----------------------------------------------------------------------------------
# Choose a set of soft-thresholding powers
powers = c(c(1:10), seq(from = 12, to = 30, by = 2))
# Call the network topology analysis function
sft = pickSoftThreshold(plot.mat, powerVector=powers, 
                        networkType="unsigned", verbose=5)
# Plot the results:
pdf(paste0("./results/Figure2/WGCNA/2.power.pdf"), width = 12, height = 8)
par(mfrow = c(1,2))
cex1 = 0.9
plot(sft$fitIndices[,1], -sign(sft$fitIndices[,3])*sft$fitIndices[,2],
     xlab="Soft Threshold (power)",
     ylab="Scale Free Topology Model Fit, signed R^2",type="n",
     main = paste("Scale independence"))
text(sft$fitIndices[,1], -sign(sft$fitIndices[,3])*sft$fitIndices[,2],
     labels=powers,cex=cex1,col="red")
abline(h=0.85,col="red")
plot(sft$fitIndices[,1], sft$fitIndices[,5],
     xlab="Soft Threshold (power)",ylab="Mean Connectivity", type="n",
     main = paste("Mean connectivity"))
text(sft$fitIndices[,1], sft$fitIndices[,5], labels=powers, 
     cex=cex1, col="red")
dev.off()
#----------------------------------------------------------------------------------
#  Step 4: soft threshold : power
#----------------------------------------------------------------------------------
power = sft$powerEstimate
power
#----------------------------------------------------------------------------------
#  Step 5: One-step network construction and module detection
#----------------------------------------------------------------------------------
net = blockwiseModules(plot.mat, power = power, maxBlockSize = ncol(plot.mat),
                       TOMType = "signed", minModuleSize = 20, 
                       reassignThreshold = 0, mergeCutHeight = 0.0001,
                       numericLabels = TRUE, pamRespectsDendro = FALSE,
                       saveTOMs=TRUE, corType = corType, 
                       maxPOutliers = 1, loadTOMs=TRUE,
                       randomSeed = 931, # seed
                       saveTOMFileBase = paste0("./results/Figure2/WGCNA/WGCNA.tom"),
                       verbose = 3, pearsonFallback = "none", deepSplit = 3 )
# module:
table(net$colors) # 0 corresponds to unclassified genes
# Convert [number] labels to [colors] for plotting
moduleLabels = net$colors
moduleColors = labels2colors(moduleLabels)
# plot
pdf(paste0( "./results/Figure2/WGCNA/3.module.pdf"), width = 8, height = 6)
plotDendroAndColors(net$dendrograms[[1]], moduleColors[net$blockGenes[[1]]],
                    "Module colors",
                    dendroLabels = FALSE, hang = 0.03,
                    addGuide = TRUE, guideHang = 0.05)
dev.off()
#----------------------------------------------------------------------------------
#  Step 6: Vasualization
#----------------------------------------------------------------------------------
## data
node.data <- readRDS("./data/proteomics/wgcna/2D-node.data.rds")
edge.data <- readRDS("./data/proteomics/wgcna/2D-edge.data.rds")
color.module <- c("#CCCCCC","#ecb888","#af88bb","#a032cb","#efbed6","#fc496a","#b6d37f","#589336","#7fd68e","#52c465","#3372e0","#84d7f6","#5394c3","#6376b3","#7f6cd7","#c4ceff","#fc9d40","#5c95e0","#cd7560","#ff70e4", "#ff8738", "#ffcead","#1cbf8b", "#b76d38", "#1584ff", "#7f006d", "#ffd35f","#E66F73","#F57F20","#1DBB95","#9CB79F","#F0B8D2","#A0485E","#A0688E","#C7E1DF","#51B1DF","#6D97D7","#5D6193","#CEC3E0","#A9917E","#7C7D80","#F4E192","#ADD666")
names(color.module) <- paste0("ME", seq(0,length(color.module)-1) %>% str_pad(width = 2,side = "left",pad = "0"))
## plot network 
gg <- ggplot()
gg <- gg + geom_segment(mapping = aes(x = from.x, y = from.y, xend = to.x, yend = to.y),
                        color = "#CCCCCC", size = 0.01, data = edge.data) # draw a straight line
gg <- gg + geom_point(mapping = aes(x = pos.x, y = pos.y, color = Module), 
                      size = 2, data = node.data) # add point
gg <- gg + scale_size(range = c(0, 6) * 2) # specifies the minimum and maximum size 
gg <- gg + theme_void()
gg <- gg + labs(x = "", y = "", title = paste0("PPI"))
gg <- gg + scale_colour_manual(values = color.module)
ggsave(paste0("./results/Figure2/2A-PRO-modules.png"), gg, width = 10, height = 8)

2.2 (b) Significantly up/down-regulated proteins

#----------------------------------------------------------------------------------------------
#  Overlay the log2 fold change between tumor and TAC on PRO in the WGCNA network
#----------------------------------------------------------------------------------------------
## data 
node.data <- readRDS("./data/proteomics/wgcna/2D-node.data.rds") # DEG & module genes
edge.data <- readRDS("./data/proteomics/wgcna/2D-edge.data.rds")
## plot
gg <- ggplot()
gg <- gg + geom_segment(mapping = aes(x = from.x, y = from.y, xend = to.x, yend = to.y),
                        color = "#CCCCCC", size = 0.01, data = edge.data)
gg <- gg + geom_point(mapping = aes(x = pos.x, y = pos.y, color = proSig), size = 1,
                      data = node.data[which(node.data$proSig == "zz"), ])
gg <- gg + geom_point(mapping = aes(x = pos.x, y = pos.y, color = proSig), size = 2.5,
                      data = node.data[which(node.data$proSig != "zz"), ])
gg <- gg + scale_size(range = c(0, 6) * 2)
gg <- gg + theme_void()
gg <- gg + labs(x = "", y = "", title = paste0("color by proSig"))
gg <- gg + scale_colour_manual(values = c("#00599F","#D01910","#AAAAAA"))
ggsave(paste0("./results/Figure2/2B-proSig.png"), gg, width = 8.5, height = 8)

2.3 (c) Modules enrichment score

color.bin <- c("#00599F","#d80700")
#----------------------------------------------------------------------------------
#  Step 1: Load the RJ-cohort 1 Data
#----------------------------------------------------------------------------------
# Scores of the 32 modules in TACs and PDACs of RJ-cohort 1
plot.data <- read.xlsx("./data/Extended Data Table 4.xlsx", sheet = 2, startRow = 2, rowNames = T)
#                       ME01         ME02        ME03       ME04
# RJ-01-0143-N_PRO 0.3474261 -0.114677437 -0.04291552 0.06708347
# RJ-01-0768-N_PRO 0.2532539  0.009051615 -0.03585508 0.03486392
# RJ-01-0697-N_PRO 0.2839048 -0.032966990 -0.02943711 0.05803330
# RJ-01-0609-N_PRO 0.3206755 -0.087559353 -0.05749618 0.10310726
plot.info <- NULL
module.name <- colnames(plot.data)
plot.stat <- data.frame(Module = module.name,
                        Wilcox.P = NA,
                        Wilcox.Padj = NA)
#----------------------------------------------------------------------------------
#  Step 2: wilcox.test
#----------------------------------------------------------------------------------
for (i in 1:ncol(plot.data)) {
  sub <- data.frame(Sample = rownames(plot.data),
                    Score = as.numeric(plot.data[, i]), 
                    ScoreScale = scale(as.numeric(plot.data[, i])),
                    Module = colnames(plot.data)[i],
                    Type = substr(rownames(plot.data), 12, 16))
  plot.stat$Wilcox.P[i] <- wilcox.test(sub$ScoreScale ~ sub$Type)$p.value
  plot.info <- rbind(plot.info, sub)
}
plot.info <- plot.info %>% mutate(Type=factor(as.character(Type), levels = c("N_PRO","T_PRO"))) 
plot.stat <- plot.stat %>% mutate(Wilcox.Padj=p.adjust(Wilcox.P, method = "fdr"))
#----------------------------------------------------------------------------------
#  Step 3: plot
#----------------------------------------------------------------------------------
p <- ggbarplot(plot.info, x = "Module", y = "ScoreScale",
               color = "Type", fill = "Type",
               palette = color.bin, width = 0.5, size = 0,
               add = c("mean_se"), add.params = list(width = 0.5),
               order = module.name,
               position = position_dodge(0.6),
               xlab = "", ylab = "Module Score of Protein")
p <- p + theme_base() 
p <- p + geom_hline(yintercept = 0, color = "black")
p <- p + theme(axis.text.x = element_text(angle = 90, hjust = 1, vjust = 0.5))
p <- p + stat_compare_means(aes(group = Type, label = ..p.format..), size = 1, method = "wilcox.test", label.y = 1.2)  + theme(plot.background = element_blank())
#----------------------------------------------------------------------------------
#  Step 4: output
#----------------------------------------------------------------------------------
ggsave(paste0("./results/Figure2/Figure2c-1.pdf"), p, width = 12, height = 4)
write.xlsx(plot.stat, paste0("./results/Figure2/Figure2c.padj-1.xlsx"))

3. Figure 3

3.1 (a) LASSO model for PDAC

library(glmnet)
library(openxlsx)
library(survminer)
library(survival)
library(tidyverse)
library(RColorBrewer)
library(ComplexHeatmap)
library(forestmodel)
library(ROCR)
dir.create("./results/Figure3/lasso",recursive = T)
#----------------------------------------------------------------------------------
#  Step 1: load data
#----------------------------------------------------------------------------------
## PDAC Tumor proteomics
pdac.pro  <- readRDS('./data/proteomics/20230412_PDAC_PRO_exp.rds') 
pdac.pro  <- pdac.pro [,grep('_T_',colnames(pdac.pro))]   %>% t() %>% as.data.frame() # 191 tumor samples * 4787 protein
## WGCNA protein
wgcna <- readRDS("./data/proteomics/wgcna/2D-node.data.rds")
pdac.pro <- pdac.pro [,intersect(wgcna$Gene,colnames(pdac.pro))] #  191 samples * 3906 protein
## PDAC clinical data
cli.pdac <- readRDS('./data/clinical/20230412_PDAC_191_patients_clinical.rds')
rownames(cli.pdac) <- cli.pdac$ID
## Lasso data
y.train <- data.frame(time=cli.pdac$Time_OS,
                      status=cli.pdac$Censoring_OS,
                      row.names = row.names(cli.pdac)) %>% 
           na.omit(y.train) %>% 
           as.matrix() 
x.train <- pdac.pro[row.names(y.train),] %>% as.matrix() %>% na.omit()
y.train <- y.train[row.names(x.train),]
#----------------------------------------------------------------------------------
#  Step 2: Fit the Lasso Regression Model
#----------------------------------------------------------------------------------
set.seed(1000) 
fit <-glmnet(x=x.train,
             y=y.train, 
             family = "cox",  # cox : cox , binomial : logistic
             alpha  = 1)      # 1 : lasso penalty, 0 : ridge penalty.
pdf('./results/Figure3/lasso/0.Coefficients.pdf',width = 5,height = 4)
plot(fit,xvar="lambda",label=F) 
dev.off()
# Cross-validation
cvfit <- cv.glmnet(x=x.train,
                   y=y.train,
                   family = "cox",
                   type.measure="deviance",  
                   alpha  = 1,
                   nfolds = 10)
png(paste0('./results/Figure3/lasso/S5A-Coeff.png'), width = 5,height = 5,res=1200,units="in")
plot(fit,xvar="lambda",label=F) 
abline(v = log(cvfit$lambda.min), col = "black",lty=2)
text(-4,-4, labels = paste0("lambda.min:  ", round(cvfit$lambda.min,4)),col = "black",cex = 0.75)
dev.off()
png(paste0('./results/Figure3/lasso/S5B-cvfit.png'), width = 5,height = 5,res=1200,units="in")
plot(cvfit)
text(-3,250, labels = paste0("lambda.min:  ", round(cvfit$lambda.min,4)),col = "red",cex = 0.75)
text(-3,200, labels = paste0("lambda.1se:  ", round(cvfit$lambda.1se,4)),col = "black",cex = 0.75)
dev.off()
#----------------------------------------------------------------------------------
#  Step 3: Best Lasso model
#----------------------------------------------------------------------------------
lasso_best <- glmnet(x = x.train, 
                     y = y.train, 
                     alpha = 1,                    
                     lambda = cvfit$lambda.min,   
                     nfolds = 10, 
                     family = "cox")
gene.coef  <- as.matrix(round(coef(lasso_best), 4))
coef.lasso <- gene.coef[which(gene.coef[, 1] != 0), ]
coef.lasso <- data.frame(genes=names(coef.lasso),
                   coefficient=as.numeric(coef.lasso)) %>% arrange(-coefficient)
write.xlsx(coef.lasso, "./results/Figure3/lasso/2.coef_PDAC.Pro.xlsx", rowNames = F,colNames = T,overwrite = T)
## Lasso score 
y <- as.data.frame(y.train) %>%
        mutate(LassoScore=predict(lasso_best,s=cvfit$lambda.min,newx=x.train)) %>% 
        mutate(LassoScore=as.numeric(LassoScore), ID=rownames(y.train))
y <- y %>% mutate(LASSO.level=ifelse(LassoScore>median(LassoScore),"High" ,"Low")) %>%
           mutate(LASSO.level=factor(LASSO.level,levels = c( "Low","High"))) ## cutoff : median
write.xlsx(y,paste0('./results/Figure3/lasso/3.Lasso_Score.xlsx'),rowNames = T,colNames = T,overwrite = T)
#----------------------------------------------------------------------------------
#  Step 4: Visualization
#----------------------------------------------------------------------------------
## bar plot : gene cofficient 
df.coef <- coef.lasso
rownames(df.coef) <- df.coef$genes
df.coef <- df.coef %>% transmute(gene=genes,cor=coefficient) %>% 
                mutate(gene=paste0(gene," (",cor,")")) %>% 
                arrange(cor) %>%  
                mutate(gene=factor(gene,levels = gene)) %>% 
                mutate(group=ifelse(cor>0,"A","B"))
p1 <- ggplot(df.coef, aes(gene, cor, fill = group)) + 
  geom_bar(stat = 'identity') +
  ylab('coefficient') +
  xlab('') +
  guides(colour=F,fill=F) + 
  theme_bw(base_size = 12) + 
  scale_fill_manual(values = brewer.pal(9,'Set1')) +
  theme(panel.grid =element_blank(),
        axis.text = element_text(colour = 'black'),
        axis.text.x = element_text(size = 8)) +
  coord_flip()
ggsave("./results/Figure3/5A-Lasso_cofficient_barplot.png",p1,width = 3,height = 4)
## dot plot : lasso score
df.score <- y
df.score <- df.score %>% mutate(samples=rownames(df.score))  %>% 
                arrange(LassoScore) %>% 
                mutate(samples=factor(samples,levels = samples))
p2 <- ggscatter(df.score, x="samples", y="LassoScore", color = "LASSO.level",
                palette = c("#0ac9c9","#ea358d"))+
  geom_hline(yintercept=median(df.score$LassoScore), linetype=2,color='black') +
  geom_vline(xintercept=median(1:nrow(df.score))+0.5, linetype=2,color='black') +
  annotate('text', 
           x=median(1:nrow(df.score))+15, 
           y=median(df.score$LassoScore)+0.5, 
           label=paste0('cutoff: ', round(median(df.score$LassoScore),4)),size=5, color='black') +
  ylab('PDAC Score') +
  xlab('') 
ggsave("./results/Figure3/5A-Lasso_score_dotplot.png",p2,width = 8,height = 4)
## Heatmap : protein abundance
heat.data <- t(x.train)
heat.data <- heat.data[rev(rownames(df.coef)),row.names(df.score)]
heat.data <- t(scale(t(heat.data)))
png("./results/Figure3/5A-Lasso_gene_heatmap.png",width = 8,height = 4,res=1200,units="in")
p3 <- Heatmap(heat.data, name = "Z-score",
              col = colorRampPalette(c("#00599F","#1c7ec9","#FFFFFF",
                                        "#e53f39","#D01910"))(100),
              cluster_rows = F,cluster_columns = F,show_column_names = F)
draw(p3)
dev.off()
#----------------------------------------------------------------------------------
#  Step 5: receiver operating characteristic (ROC)
#----------------------------------------------------------------------------------
# performance of model
lasso.prob <- predict(cvfit, newx=x.train , family = "cox",
                      s=c(cvfit$lambda.min, cvfit$lambda.1se) )
re <- cbind(as.data.frame(y.train),lasso.prob)  %>% as.data.frame()
colnames(re) <- c('time','status','prob_min','prob_1se')
# model: lambda.min
pred_min <- prediction(predictions=re$prob_min, labels=re$status) # predictions: containing the prediction. labels: true class labels
perf_min <- performance(pred_min,"tpr","fpr")
auc_min  <- performance(pred_min,"auc")@y.values[[1]]
# mocel: lambda.1se
pred_1se <- prediction(re$prob_1se, re$status)
perf_1se <- performance(pred_1se,"tpr","fpr")
auc_1se  <- performance(pred_1se,"auc")@y.values[[1]]
## plot
png(paste0('./results/Figure3/lasso/S5C-ROC.png'), width = 5,height = 5,res=1200,units="in")
plot(perf_min,colorize=F, col="red") 
plot(perf_1se,colorize=F, col="blue",add = T)
lines(c(0,1),c(0,1), col = "gray", lty = 4 )
text(0.7,0.3, labels = paste0("lambda.min: AUC=", round(auc_min,2)),col = "red")
dev.off()
#----------------------------------------------------------------------------------
#  Step 6: Multivariate analysis
#----------------------------------------------------------------------------------
# data
y_forest <- y %>% left_join(cli.pdac , by =c('ID'='ID'))
y_forest <- y_forest %>% select(  c('time','status','LASSO.level',
                        'age','gender','CA125',
                        'CA19_9','CEA','Smoking',"Drinking",'AJCC_V8',
                        'Censoring_chemo'))
y_forest <- y_forest %>% rename(LassoLevel=LASSO.level,
                                Age=age,Gender=gender,
                                CA199=CA19_9,
                                Adjuvant_therapy=Censoring_chemo,
                                AJCC_stage=AJCC_V8)
y_forest <- y_forest %>% mutate(Gender=factor(Gender,levels = c("Female","Male")))
# AJCC_stage
table(y_forest$AJCC_stage)
a <- y_forest$AJCC_stage
b <- recode(a, Ia = "I", Ib = "I",IIa= "II", IIb= "II",III="III",IV="IV")
y_forest$AJCC_stage <- factor(b,levels = c("I","II","III"))
# coxph
cfit <- coxph(Surv(time,status)~LassoLevel+Age+Gender+CA125+CA199+
                CEA+Smoking+Drinking+AJCC_stage+Adjuvant_therapy,
              data = y_forest)
# Forest plots
p <- forest_model(cfit,
      format_options = forest_model_format_options(colour = brewer.pal(9,'Set1')[2],                 shape = 16,text_size =  15,point_size = 2.5, banded = T),
      factor_separate_line = F )
ggsave(paste0("./results/Figure3/S5D-multivariate_forest.png"), p,  width = 8, height = 6)

3.2 (b) Kaplan-Meier curves in OS/DFS

#----------------------------------------------------------------------------------
#  Step 1: Loading data 
#----------------------------------------------------------------------------------
# (1) Sample information and clinical characteristics of the 191 PDAC patients (the RJ-cohort 1)
rj1.cohort <- read.xlsx("./data/Extended Data Table 2.xlsx", startRow = 2)
#           ID     Proteomic_ID        RNAseq_ID Age Gender      BMI DM Smoking
# 1 RJ-01-0020 RJ-01-0020-T_PRO RJ-01-0020-T_RNA  61 Female 19.63000  1       0
# 2 RJ-01-0038 RJ-01-0038-T_PRO RJ-01-0038-T_RNA  73   Male 22.46003  0       0
# 3 RJ-01-0050 RJ-01-0050-T_PRO RJ-01-0050-T_RNA  69 Female 17.63085  0       0
# 4 RJ-01-0069 RJ-01-0069-T_PRO RJ-01-0069-T_RNA  69 Female 17.48179  1       0
# 5 RJ-01-0070 RJ-01-0070-T_PRO RJ-01-0070-T_RNA  65   Male 23.43750  0       0
# 6 RJ-01-0074 RJ-01-0074-T_PRO RJ-01-0074-T_RNA  61   Male 23.66144  0       0
rj1.cohort <- rj1.cohort %>%  mutate(LassoLevel=factor(as.character(LassoLevel), levels = c("Low","High")))
color.bin.lasso <- c("#00599F","#d80700")
#----------------------------------------------------------------------------------
#  Step 2: OS survival stratified by lasso level
#----------------------------------------------------------------------------------
info <- summary(coxph(Surv(OS_month, OS_status) ~ LassoLevel, data = rj1.cohort))
anno.text <- ""
for (i in 1:nrow(info$conf.int)) {
  anno.text <- paste0(anno.text, "\n", paste0(rownames(info$conf.int)[i], " HR=", round(info$conf.int[i, 1], 3), " CI=", round(info$conf.int[i, 3], 3), "-", round(info$conf.int[i, 4], 3), " P=", signif(info$coefficients[i, 5], 4) ))
}
anno.text <- paste0(anno.text, "\nKaplan-Meier P=", signif(survdiff(Surv(OS_month, OS_status) ~ LassoLevel, data = rj1.cohort)$pvalue, 4) )
anno.text <- str_replace_all(anno.text, "LassoLevel", "")
fit <- survfit(Surv(OS_month, OS_status) ~ LassoLevel, data = rj1.cohort)
p1 <- ggsurvplot(fit, 
                 data = rj1.cohort,
                 xlab = 'Time (Months)',
                 pval = TRUE,
                 risk.table = TRUE, 
                 risk.table.height = 0.28,
                 conf.int.alpha = 0.05,
                 conf.int = TRUE, 
                 palette = color.bin.lasso,
                 axes.offset = TRUE,
                 break.time.by = 12,  xlim = c(0, 48),
                 title= paste0("OS LassoLevel \n", anno.text))
#----------------------------------------------------------------------------------
#  Step 2: DFS survival stratified by lasso level
#----------------------------------------------------------------------------------
info <- summary(coxph(Surv(DFS_month, DFS_status) ~ LassoLevel, data = rj1.cohort))
anno.text <- ""
for (i in 1:nrow(info$conf.int)) {
  anno.text <- paste0(anno.text, "\n", paste0(rownames(info$conf.int)[i], " HR=", round(info$conf.int[i, 1], 3), " CI=", round(info$conf.int[i, 3], 3), "-", round(info$conf.int[i, 4], 3), " P=", signif(info$coefficients[i, 5], 4) ))
}
anno.text <- paste0(anno.text, "\nKaplan-Meier P=", signif(survdiff(Surv(DFS_month, DFS_status) ~ LassoLevel, data = rj1.cohort)$pvalue, 4) )
anno.text <- str_replace_all(anno.text, "LassoLevel", "")
fit <- survfit(Surv(DFS_month, DFS_status) ~ LassoLevel, data = rj1.cohort)
p2 <- ggsurvplot(fit, 
                 data = rj1.cohort,
                 xlab = 'Time (Months)',
                 pval = TRUE,
                 risk.table = TRUE, 
                 risk.table.height = 0.28,
                 conf.int.alpha = 0.05,
                 conf.int = TRUE, 
                 palette = color.bin.lasso,
                 axes.offset = TRUE,
                 break.time.by = 12,  xlim = c(0, 48),
                 title= paste0("DFS LassoLevel \n", anno.text))
## output
p <- arrange_ggsurvplots(list(p1, p2), ncol = 2, nrow = 1, print = FALSE)
ggsave(paste0("./results/Figure3/Figure3b.pdf"), p, width = 16, height = 10)

3.3 (c) Lasso proteins in module

## data
node.data <- readRDS("./data/proteomics/wgcna/2D-node.data.rds")
edge.data <- readRDS("./data/proteomics/wgcna/2D-edge.data.rds")
## lasso gene plot
color.module <- c("#ecb888","#af88bb","#a032cb","#efbed6","#fc496a","#b6d37f","#589336","#7fd68e","#52c465","#3372e0","#84d7f6","#5394c3","#6376b3","#7f6cd7","#c4ceff","#fc9d40","#5c95e0","#cd7560","#ff70e4", "#ff8738", "#ffcead","#1cbf8b", "#b76d38", "#1584ff", "#7f006d", "#ffd35f","#E66F73","#F57F20","#1DBB95","#9CB79F","#F0B8D2","#A0485E","#A0688E","#C7E1DF","#51B1DF","#6D97D7","#5D6193","#CEC3E0","#A9917E","#7C7D80","#F4E192","#ADD666")
gg <- ggplot()
gg <- gg + geom_segment(mapping = aes(x = from.x, y = from.y, xend = to.x, yend = to.y), color = "#CCCCCC", size = 0.01, data = edge.data)
gg <- gg + geom_point(mapping = aes(x = pos.x, y = pos.y, color = Module), size = 1, data = node.data)
gg <- gg + geom_point(mapping = aes(x = pos.x, y = pos.y, color = Module), fill = "red", size = 5, shape = 21, data = node.data[which(node.data$ISlassoGene == "yes"), ])
gg <- gg + geom_text(mapping = aes(x = pos.x, y = pos.y, label = Gene), size = 5, color = "black", data = node.data[which(node.data$ISlassoGene == "yes"), ])
gg <- gg + scale_size(range = c(0, 6) * 2)
gg <- gg + theme_void()
gg <- gg + labs(x = "", y = "", title = paste0("color by ISlassoGene"))
gg <- gg + scale_colour_manual(values = color.module)
gg <- gg + theme(legend.position = "none")
ggsave(paste0("./results/Figure3/3c-Lasso_gene_in_module.png"), gg, width = 8, height = 8.2)

3.4 (d) LassoScore~ModuleScore

library(ggcorrplot)
#----------------------------------------------------------------------------------
#  Step 1: Load the Data
#----------------------------------------------------------------------------------
# (1) Sample information and clinical characteristics of the 191 PDAC patients (the RJ-cohort 1)
rj1.cohort <- read.xlsx("./data/Extended Data Table 2.xlsx", startRow = 2)
#           ID     Proteomic_ID        RNAseq_ID Age Gender      BMI DM Smoking
# 1 RJ-01-0020 RJ-01-0020-T_PRO RJ-01-0020-T_RNA  61 Female 19.63000  1       0
# 2 RJ-01-0038 RJ-01-0038-T_PRO RJ-01-0038-T_RNA  73   Male 22.46003  0       0
# 3 RJ-01-0050 RJ-01-0050-T_PRO RJ-01-0050-T_RNA  69 Female 17.63085  0       0
# 4 RJ-01-0069 RJ-01-0069-T_PRO RJ-01-0069-T_RNA  69 Female 17.48179  1       0
# 5 RJ-01-0070 RJ-01-0070-T_PRO RJ-01-0070-T_RNA  65   Male 23.43750  0       0
# 6 RJ-01-0074 RJ-01-0074-T_PRO RJ-01-0074-T_RNA  61   Male 23.66144  0       0

# (2) Scores of the 32 modules in TACs and PDACs of RJ-cohort 1. 
module.ssgsea.pro.all <- read.xlsx("./data/Extended Data Table 4.xlsx", sheet = 2, startRow = 2, rowNames = T)
module.ssgsea.pro.all <- t(module.ssgsea.pro.all)
#      RJ-01-0143-N_PRO RJ-01-0768-N_PRO RJ-01-0697-N_PRO RJ-01-0609-N_PRO RJ-01-1055-N_PRO
# ME01       0.34742611      0.253253916       0.28390477       0.32067554      0.325797851
# ME02      -0.11467744      0.009051615      -0.03296699      -0.08755935     -0.096947986
# ME03      -0.04291552     -0.035855079      -0.02943711      -0.05749618      0.016639009
# ME04       0.06708347      0.034863920       0.05803330       0.10310726      0.007498371
# ME05       0.19099018      0.100153070       0.14246697       0.16675071      0.127932887
# ME06       0.03893163      0.240865770       0.14178269       0.07618613      0.038306853
#----------------------------------------------------------------------------------
#  Step 2:  Spearman correlation : lasso score ~ module score
#----------------------------------------------------------------------------------
plot.mat <- data.frame(t(module.ssgsea.pro.all[, rj1.cohort$Proteomic_ID]), LassoScore = rj1.cohort[, c("LassoScore")] )
corr <- cor(plot.mat, use = "complete.obs", method = "spearman")
p.mat <- cor_pmat(plot.mat, use = "complete.obs", method = "spearman")
p.adj <- p.mat
for (i in 1:ncol(p.adj)) {
  p.adj[, i] <- p.adjust(p.adj[, i], method = "fdr")
}
write.xlsx(list(Corr = corr, p.mat = p.mat, p.adj = p.adj), "./results/Figure3/Figure3d-1.xlsx", overwrite = T, rowNames = T)
# plot
pdf(paste0("./results/Figure3/Figure3d-1.pdf"), width = 10, height = 10)
corrplot::corrplot(corr[, ], method = "ellipse",
                   col = colorRampPalette(c("#1B3361","#76C7FF","#FFFFFF","#FF987A","#6A0D28"))(200)) 
dev.off()
#----------------------------------------------------------------------------------
#  Step 3:  Spearman correlation : lasso score ~ module score in Cao et al cohort
#----------------------------------------------------------------------------------
module.ssgsea.pro.cell <- readRDS("./data/Figure2/cao.module.ssgsea.pro.rds")
cell.meta.data <- read.xlsx("./data/Figure2/cao.meta.data.xlsx")
cell.meta.data$LassoLevel <- factor(as.character(cell.meta.data$LassoLevel), levels = c("Low","High"))
plot.mat <- data.frame(t(module.ssgsea.pro.cell[, cell.meta.data$Proteomic_ID]), LassoScore = cell.meta.data[, c("LassoScore")] )
# Spearman correlation
corr <- cor(plot.mat, use = "complete.obs", method = "spearman")
p.mat <- cor_pmat(plot.mat, use = "complete.obs", method = "spearman")
p.adj <- p.mat
for (i in 1:ncol(p.adj)) {
  p.adj[, i] <- p.adjust(p.adj[, i], method = "fdr")
}
write.xlsx(list(Corr = corr, p.mat = p.mat, p.adj = p.adj), "./results/Figure3/Figure3d-2.xlsx", overwrite = T, rowNames = T)
# plot 
pdf(paste0("./results/Figure3/Figure3d-2.pdf"),  width = 10, height = 10)
corrplot::corrplot(corr[, ], method = "ellipse",
                   col = colorRampPalette(c("#1B3361","#76C7FF","#FFFFFF","#FF987A","#6A0D28"))(200)) 
dev.off()

3.5 (e) Cao et al validation

## data
cell.meta.data <- read.xlsx("./data/Figure2/cao.meta.data.xlsx")
color.bin.lasso <- c("#00599F","#d80700")
cell.meta.data <- cell.meta.data %>% mutate(LassoLevel=factor(LassoLevel,level=c("Low","High")))
## coxph
info <- summary(coxph(Surv(OS_month, OS_status) ~ LassoLevel, data = cell.meta.data))
anno.text <- ""
for (i in 1:nrow(info$conf.int)) {
  anno.text <- paste0(anno.text, "\n", paste0(rownames(info$conf.int)[i], " HR=", round(info$conf.int[i, 1], 3), " CI=", round(info$conf.int[i, 3], 3), "-", round(info$conf.int[i, 4], 3), " P=", signif(info$coefficients[i, 5], 4) ))
}
anno.text <- paste0(anno.text, "\nKaplan-Meier P=", signif(survdiff(Surv(OS_month, OS_status) ~ LassoLevel, data = cell.meta.data)$pvalue, 4) )
anno.text <- str_replace_all(anno.text, "LassoLevel", "")
fit <- survfit(Surv(OS_month, OS_status) ~ LassoLevel, data = cell.meta.data)
p1 <- ggsurvplot(fit, 
                 data = cell.meta.data,
                 xlab = 'Time (Months)',
                 pval = TRUE,
                 risk.table = TRUE, 
                 risk.table.height = 0.28,
                 conf.int.alpha = 0.05,
                 conf.int = TRUE, 
                 palette = color.bin.lasso,
                 axes.offset = TRUE,
                 break.time.by = 12,  xlim = c(0, 48),
                 title= paste0("OS LassoLevel \n", anno.text))
p <- arrange_ggsurvplots(list(p1), ncol = 1, nrow = 1, print = FALSE)
ggsave(paste0("./results/Figure3/Figure3e.pdf"), p, width = 8, height = 10)

3.6 (f) RJ-cohort 2 validation

#----------------------------------------------------------------------------------
#  Step 1: Load the Data
#----------------------------------------------------------------------------------
# The LASSO score in RJ-cohort 2
rj2.cohort <- read.xlsx("./data/Extended Data Table 5.xlsx", sheet = 3, startRow = 2)
rj2.cohort <- rj2.cohort %>% mutate(LassoLevel=factor(as.character(LassoLevel), levels = c("Low","High")))
color.bin.lasso <- c("#00599F","#d80700")
#----------------------------------------------------------------------------------
#  Step 2: OS survival stratified by lasso level
#----------------------------------------------------------------------------------
info <- summary(coxph(Surv(OS_month, OS_status) ~ LassoLevel, data = rj2.cohort))
anno.text <- ""
for (i in 1:nrow(info$conf.int)) {
  anno.text <- paste0(anno.text, "\n", paste0(rownames(info$conf.int)[i], " HR=", round(info$conf.int[i, 1], 3), " CI=", round(info$conf.int[i, 3], 3), "-", round(info$conf.int[i, 4], 3), " P=", signif(info$coefficients[i, 5], 4) ))
}
anno.text <- paste0(anno.text, "\nKaplan-Meier P=", signif(survdiff(Surv(OS_month, OS_status) ~ LassoLevel, data = rj2.cohort)$pvalue, 4) )
anno.text <- str_replace_all(anno.text, "LassoLevel", "")
fit <- survfit(Surv(OS_month, OS_status) ~ LassoLevel, data = rj2.cohort)
p1 <- ggsurvplot(fit, 
                 data = rj2.cohort,
                 xlab = 'Time (Months)',
                 pval = TRUE,
                 risk.table = TRUE, 
                 risk.table.height = 0.28,
                 conf.int.alpha = 0.05,
                 conf.int = TRUE, 
                 palette = color.bin.lasso,
                 axes.offset = TRUE,
                 break.time.by = 12,  xlim = c(0, 48),
                 title= paste0("OS LassoLevel \n", anno.text))
#----------------------------------------------------------------------------------
#  Step 3: DFS survival stratified by lasso level
#----------------------------------------------------------------------------------
info <- summary(coxph(Surv(DFS_month, DFS_status) ~ LassoLevel, data = rj2.cohort))
anno.text <- ""
for (i in 1:nrow(info$conf.int)) {
  anno.text <- paste0(anno.text, "\n", paste0(rownames(info$conf.int)[i], " HR=", round(info$conf.int[i, 1], 3), " CI=", round(info$conf.int[i, 3], 3), "-", round(info$conf.int[i, 4], 3), " P=", signif(info$coefficients[i, 5], 4) ))
}
anno.text <- paste0(anno.text, "\nKaplan-Meier P=", signif(survdiff(Surv(DFS_month, DFS_status) ~ LassoLevel, data = rj2.cohort)$pvalue, 4) )
anno.text <- str_replace_all(anno.text, "LassoLevel", "")
fit <- survfit(Surv(DFS_month, DFS_status) ~ LassoLevel, data = rj2.cohort)
p2 <- ggsurvplot(fit, 
                 data = rj2.cohort,
                 xlab = 'Time (Months)',
                 pval = TRUE,
                 risk.table = TRUE, 
                 risk.table.height = 0.28,
                 conf.int.alpha = 0.05,
                 conf.int = TRUE, 
                 palette = color.bin.lasso,
                 axes.offset = TRUE,
                 break.time.by = 12,  xlim = c(0, 48),
                 title= paste0("DFS LassoLevelRNA \n", anno.text))
# output
p <- arrange_ggsurvplots(list(p1, p2), ncol = 2, nrow = 1, print = FALSE)
ggsave(paste0("./results/Figure3/Figure3f.pdf"), p, width = 16, height = 10)
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