Single-cell RNA sequencing of glioblastoma cells treated with CRISPR/Cas13a gene editing system

Barcoded signal-cell GEMs were created by 10x Genomics® ChromiumTM. GEMs were then reverse transcript to generate single cell RNA-seq libraries. cDNAs in single-cell RNA sequencing libraries were then amplified and sequenced. The analyses of single-cell transcriptome were conducted using LOUPETM cell browser.