Error in conversion of SCE object to Seurat Object.
1
0
Entering edit mode
@rohitsatyam102-24390
Last seen 8 weeks ago
India

Hi Everyone

I was trying to convert my Single Cell Experiment Object into Seurat, but for some reason, it is failing. Can I get some help here? I looked up the source code of Tsparse of Package Matrix and it's breaking somewhere there. But I don't know the workaround!!

Below is the code and session info:

seurat <- as.Seurat(sce_clean,counts = "counts", data = "logcounts",assay = 'RNA',project = 'SingleCellExperiment')
Warning: Non-unique cell names (colnames) present in the input matrix, making unique
Warning: Feature names cannot have underscores ('_'), replacing with dashes ('-')
Warning: Feature names cannot have underscores ('_'), replacing with dashes ('-')
Error in intI(j, n = d[2], dn[[2]], give.dn = FALSE) : 
  invalid character indexing
> sessionInfo()
R version 4.0.3 (2020-10-10)
Platform: x86_64-conda-linux-gnu (64-bit)
Running under: Ubuntu 20.04.2 LTS

Matrix products: default
BLAS/LAPACK: /home/pichkari/miniconda3/envs/R/lib/libopenblasp-r0.3.12.so

locale:
 [1] LC_CTYPE=en_IN.UTF-8       LC_NUMERIC=C              
 [3] LC_TIME=en_IN.UTF-8        LC_COLLATE=en_IN.UTF-8    
 [5] LC_MONETARY=en_IN.UTF-8    LC_MESSAGES=en_IN.UTF-8   
 [7] LC_PAPER=en_IN.UTF-8       LC_NAME=C                 
 [9] LC_ADDRESS=C               LC_TELEPHONE=C            
[11] LC_MEASUREMENT=en_IN.UTF-8 LC_IDENTIFICATION=C       

attached base packages:
[1] parallel  stats4    stats     graphics  grDevices utils    
[7] datasets  methods   base     

other attached packages:
 [1] SeuratObject_4.0.0          Seurat_4.0.1               
 [3] scDblFinder_1.4.0           scran_1.18.7               
 [5] BiocSingular_1.6.0          harmony_1.0                
 [7] Rcpp_1.0.6                  scater_1.18.6              
 [9] ggplot2_3.3.3               DropletUtils_1.10.3        
[11] scales_1.1.1                SingleCellExperiment_1.12.0
[13] SummarizedExperiment_1.20.0 Biobase_2.50.0             
[15] GenomicRanges_1.42.0        GenomeInfoDb_1.26.7        
[17] IRanges_2.24.1              MatrixGenerics_1.2.1       
[19] matrixStats_0.58.0          S4Vectors_0.28.1           
[21] BiocGenerics_0.36.1        

loaded via a namespace (and not attached):
  [1] utf8_1.2.1                reticulate_1.19          
  [3] R.utils_2.10.1            tidyselect_1.1.1         
  [5] htmlwidgets_1.5.3         grid_4.0.3               
  [7] BiocParallel_1.24.1       Rtsne_0.15               
  [9] devtools_2.4.0            munsell_0.5.0            
 [11] codetools_0.2-18          ica_1.0-2                
 [13] statmod_1.4.35            xgboost_1.4.1.1          
 [15] future_1.21.0             miniUI_0.1.1.1           
 [17] withr_2.4.2               colorspace_2.0-0         
 [19] rstudioapi_0.13           ROCR_1.0-11              
 [21] tensor_1.5                listenv_0.8.0            
 [23] labeling_0.4.2            GenomeInfoDbData_1.2.4   
 [25] polyclip_1.10-0           farver_2.1.0             
 [27] rhdf5_2.34.0              rprojroot_2.0.2          
 [29] parallelly_1.24.0         vctrs_0.3.8              
 [31] generics_0.1.0            R6_2.5.0                 
 [33] ggbeeswarm_0.6.0          rsvd_1.0.5               
 [35] locfit_1.5-9.4            bitops_1.0-7             
 [37] rhdf5filters_1.2.0        spatstat.utils_2.1-0     
 [39] cachem_1.0.4              DelayedArray_0.16.3      
 [41] assertthat_0.2.1          promises_1.2.0.1         
 [43] beeswarm_0.3.1            gtable_0.3.0             
 [45] beachmat_2.6.4            globals_0.14.0           
 [47] processx_3.5.1            goftest_1.2-2            
 [49] rlang_0.4.10              splines_4.0.3            
 [51] lazyeval_0.2.2            spatstat.geom_2.1-0      
 [53] BiocManager_1.30.12       yaml_2.2.1               
 [55] reshape2_1.4.4            abind_1.4-5              
 [57] httpuv_1.6.0              usethis_2.0.1            
 [59] tools_4.0.3               ellipsis_0.3.2           
 [61] spatstat.core_2.1-2       RColorBrewer_1.1-2       
 [63] sessioninfo_1.1.1         ggridges_0.5.3           
 [65] plyr_1.8.6                sparseMatrixStats_1.2.1  
 [67] zlibbioc_1.36.0           purrr_0.3.4              
 [69] RCurl_1.98-1.3            ps_1.6.0                 
 [71] prettyunits_1.1.1         rpart_4.1-15             
 [73] deldir_0.2-10             pbapply_1.4-3            
 [75] viridis_0.6.0             cowplot_1.1.1            
 [77] zoo_1.8-9                 ggrepel_0.9.1            
 [79] cluster_2.1.2             fs_1.5.0                 
 [81] magrittr_2.0.1            data.table_1.14.0        
 [83] RSpectra_0.16-0           scattermore_0.7          
 [85] lmtest_0.9-38             RANN_2.6.1               
 [87] fitdistrplus_1.1-3        pkgload_1.2.1            
 [89] patchwork_1.1.1           mime_0.10                
 [91] xtable_1.8-4              gridExtra_2.3            
 [93] testthat_3.0.2            compiler_4.0.3           
 [95] tibble_3.1.1              KernSmooth_2.23-18       
 [97] crayon_1.4.1              R.oo_1.24.0              
 [99] htmltools_0.5.1.1         mgcv_1.8-35              
[101] later_1.2.0               tidyr_1.1.3              
[103] DBI_1.1.1                 MASS_7.3-53.1            
[105] Matrix_1.3-2              cli_2.5.0                
[107] R.methodsS3_1.8.1         igraph_1.2.6             
[109] pkgconfig_2.0.3           plotly_4.9.3             
[111] scuttle_1.0.4             spatstat.sparse_2.0-0    
[113] vipor_0.4.5               dqrng_0.2.1              
[115] XVector_0.30.0            stringr_1.4.0            
[117] callr_3.7.0               digest_0.6.27            
[119] sctransform_0.3.2         RcppAnnoy_0.0.18         
[121] spatstat.data_2.1-0       leiden_0.3.7             
[123] uwot_0.1.10               edgeR_3.32.1             
[125] DelayedMatrixStats_1.12.3 shiny_1.6.0              
[127] lifecycle_1.0.0           nlme_3.1-152             
[129] jsonlite_1.7.2            Rhdf5lib_1.12.1          
[131] BiocNeighbors_1.8.2       desc_1.3.0               
[133] viridisLite_0.4.0         limma_3.46.0             
[135] fansi_0.4.2               pillar_1.6.0             
[137] lattice_0.20-41           fastmap_1.1.0            
[139] httr_1.4.2                pkgbuild_1.2.0           
[141] survival_3.2-11           remotes_2.3.0            
[143] glue_1.4.2                png_0.1-7                
[145] bluster_1.0.0             stringi_1.5.3            
[147] HDF5Array_1.18.1          memoise_2.0.0            
[149] dplyr_1.0.5               irlba_2.3.3              
[151] future.apply_1.7.0
SingleCellExperiment • 5.7k views
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0
Entering edit mode
traceback()
    9: stop("invalid character indexing")
    8: intI(j, n = d[2], dn[[2]], give.dn = FALSE)
    7: subCsp_ij(x, i, j, drop = drop)
    6: new.data[new.features, colnames(x = object), drop = FALSE]
    5: new.data[new.features, colnames(x = object), drop = FALSE]
    4: SetAssayData.Assay(object = a, slot = "data", new.data = mats$data)
    3: SetAssayData(object = a, slot = "data", new.data = mats$data)
    2: as.Seurat.SingleCellExperiment(sce_clean)
    1: as.Seurat(sce_clean)
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2
Entering edit mode

Even if this might not be the correct platform to ask about this I just though I could share that I got exactly the same error and ensuring my cellnames were unique solved the problem for me.

# this did the trick for me
colnames(sce) <- sce$Barcodes
# you could also try something like
colnames(sce) <- make.unique(colnames(sce))

I hope that helps

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0
Entering edit mode

Well !! The seurat function worked after all. Couldn't figure out what was the issue

counts <- assays(sce_clean)[[1]]
seurat <- CreateSeuratObject(counts = counts, project = "Harmony_All", min.cells = 5)
t2 <- seurat@meta.data
t <- data.frame(colData(sce_clean))
t3 <- data.frame(t,t2)
seurat@meta.data <- t3

I tried this code though. I am inquisitive why you used make.unique function and what will happen if I don't use that?

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Entering edit mode

In my case colnames(sce) was NULL and that was causing the error you were getting. Seurat expects colnames to be present so I added them, copying from the metadata under the sce$Barcodes. However, again in my case, these Barcodes were not unique so it was still yielding an error. I did modify the colnames in a sensible way for my experiment, and here I just suggested make.unique() as an easy workaround ( this adds a .1 to the string if the Barcode is duplicated). I will post that issue here, where a similar problem was discussed in the Seurat github page, they might be able to solve it or give better advise.

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Entering edit mode
Peter Hickey ▴ 740
@petehaitch
Last seen 7 weeks ago
WEHI, Melbourne, Australia

This is a Seurat function, right? Although SCE is a Bioconductor data structure, Bioconductor don't control how the Seurat authors attempt to convert from an SCE to a Seurat object.

Have you asked the Seurat authors for support?

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