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Complete guide RNA design for CRISPR-mediated regulation of human long noncoding RNA transcription

Complete guide RNA design for CRISPR-mediated regulation of human long noncoding RNA transcription

来源:bioRxiv_logobioRxiv
英文摘要

Abstract Transcription inhibition and activation of long noncoding RNAs (lncRNAs) mediated by clustered regularly interspaced short palindromic repeat (CRISPR)/Cas9 technology provides potential advantages in high-throughput functional genomics studies over RNA interference or overexpression platforms. In this work, we identify over 90,000 lncRNA transcription start sites (TSSs) based on the MiTranscriptome human genome annotation and design single guide RNA (sgRNA) libraries with strong predicted activities and low off-target effects for CRISPR-mediated inhibition and activation (CRISPRi/a) of their transcription. A large fraction of these TSSs correspond to putative genes that are not annotated in common reference genome annotations and have never been functionally studied. Our CRISPRi/a libraries, or their context-dependent subsets, are potentially useful in genome-scale functional studies of human lncRNAs.

Saberi Amir、Zhu Renjun、Kwon Chulan

10.1101/290338

基础医学生物科学研究方法、生物科学研究技术分子生物学

Saberi Amir,Zhu Renjun,Kwon Chulan.Complete guide RNA design for CRISPR-mediated regulation of human long noncoding RNA transcription[EB/OL].(2025-03-28)[2025-05-01].https://www.biorxiv.org/content/10.1101/290338.点此复制

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