Combinatory use of distinct single-cell RNA-seq analytical platforms reveals the heterogeneous transcriptome response.
Yukie KashimaAyako SuzukiYing LiuMasahito HosokawaHiroko MatsunagaMasataka ShiraiKohji ArikawaSumio SuganoTakashi KohnoHaruko TakeyamaKatsuya TsuchiharaYutaka SuzukiPublished in: Scientific reports (2018)
Single-cell RNA-seq is a powerful tool for revealing heterogeneity in cancer cells. However, each of the current single-cell RNA-seq platforms has inherent advantages and disadvantages. Here, we show that combining the different single-cell RNA-seq platforms can be an effective approach to obtaining complete information about expression differences and a sufficient cellular population to understand transcriptional heterogeneity in cancers. We demonstrate that it is possible to estimate missing expression information. We further demonstrate that even in the cases where precise information for an individual gene cannot be inferred, the activity of given transcriptional modules can be analyzed. Interestingly, we found that two distinct transcriptional modules, one associated with the Aurora kinase gene and the other with the DUSP gene, are aberrantly regulated in a minor population of cells and may thus contribute to the possible emergence of dormancy or eventual drug resistance within the population.
Keyphrases
- rna seq
- single cell
- high throughput
- transcription factor
- poor prognosis
- genome wide
- copy number
- gene expression
- genome wide identification
- health information
- induced apoptosis
- heat shock
- healthcare
- long non coding rna
- dna methylation
- cell cycle arrest
- cell death
- social media
- cell proliferation
- mass spectrometry
- young adults
- pi k akt