Improving the RNA velocity approach with single-cell RNA lifecycle (nascent, mature and degrading RNAs) sequencing technologies

Author:

Zhang Chen1,Fang Yitong1,Chen Weitian12,Chen Zhichao1,Zhang Ying3,Xie Yeming1,Chen Wenfang1,Xie Zhe1,Guo Mei1,Wang Juan1,Tan Chen1,Wang Hongqi1,Tang Chong1ORCID

Affiliation:

1. BGI ,  Shenzhen 518000 , China

2. BGI Education Center, University of Chinese Academy of Sciences , Shenzhen 518083, China

3. Guangdong Provincial Reproductive Science Institute (Guangdong Provincial Fertility Hospital), Guangzhou, China; NHC Key Laboratory of Male Reproduction and Genetics , Guangzhou , China

Abstract

Abstract We presented an experimental method called FLOUR-seq, which combines BD Rhapsody and nanopore sequencing to detect the RNA lifecycle (including nascent, mature, and degrading RNAs) in cells. Additionally, we updated our HIT-scISOseq V2 to discover a more accurate RNA lifecycle using 10x Chromium and Pacbio sequencing. Most importantly, to explore how single-cell full-length RNA sequencing technologies could help improve the RNA velocity approach, we introduced a new algorithm called ‘Region Velocity’ to more accurately configure cellular RNA velocity. We applied this algorithm to study spermiogenesis and compared the performance of FLOUR-seq with Pacbio-based HIT-scISOseq V2. Our findings demonstrated that ‘Region Velocity’ is more suitable for analyzing single-cell full-length RNA data than traditional RNA velocity approaches. These novel methods could be useful for researchers looking to discover full-length RNAs in single cells and comprehensively monitor RNA lifecycle in cells.

Publisher

Oxford University Press (OUP)

Subject

Genetics

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