CLEAR: Coverage-based Limiting-cell Experiment Analysis for RNA-seq
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Abstract
Direct cDNA preamplification protocols developed for single-cell RNA-seq have enabled transcriptome profiling of precious clinical samples and rare cells without sample pooling or RNA extraction. Currently, there is no algorithm optimized to reveal and remove noisy transcripts in limiting-cell RNA-seq (lcRNA-seq) data for downstream analyses. Herein, we present CLEAR, a workflow that identifies reliably quantifiable transcripts in lcRNA-seq data for differentially expressed gene (DEG) analysis. Libraries at three input amounts of FACS-derived CD5+ and CD5- cells from a chronic lymphocytic leukemia patient were used to develop CLEAR. When using CLEAR transcripts vs. using all transcripts, downstream analyses revealed more shared transcripts across different input RNA amounts, improved Principal Component Analysis (PCA) separation, and yielded more DEGs between cell types. As proof-of-principle, CLEAR was applied to an in-house lcRNA-seq dataset and two public datasets. When imputation is used, CLEAR is also adaptable to large clinical studies and for single cell analyses.