Cost and time-efficient construction of a 3′-end mRNA library from unpurified bulk RNA in a single tube

Jungwon Choi; Jungheun Hyun; Jieun Hyun; Jae Hee Kim; Ji Hyun Lee; Duhee Bang

doi:10.1038/s12276-024-01164-8

Cost and time-efficient construction of a 3′-end mRNA library from unpurified bulk RNA in a single tube

Jungwon Choi, Jungheun Hyun, Jieun Hyun, Jae Hee Kim, Ji Hyun Lee, Duhee Bang

Department of Chemistry

Research output: Contribution to journal › Article › peer-review

2 Citations (Scopus)

Abstract

The major drawbacks of RNA sequencing (RNA-seq), a remarkably accurate transcriptome profiling method, is its high cost and poor scalability. Here, we report a highly scalable and cost-effective method for transcriptomics profiling called Bulk transcriptOme profiling of cell Lysate in a single poT (BOLT-seq), which is performed using unpurified bulk 3′-end mRNA in crude cell lysates. During BOLT-seq, RNA/DNA hybrids are directly subjected to tagmentation, and second-strand cDNA synthesis and RNA purification are omitted, allowing libraries to be constructed in 2 h of hands-on time. BOLT-seq was successfully used to cluster small molecule drugs based on their mechanisms of action and intended targets. BOLT-seq competes effectively with alternative library construction and transcriptome profiling methods.

Original language	English
Pages (from-to)	453-460
Number of pages	8
Journal	Experimental and Molecular Medicine
Volume	56
Issue number	2
DOIs	https://doi.org/10.1038/s12276-024-01164-8
Publication status	Published - 2024 Feb

Bibliographical note

Publisher Copyright:
© The Author(s) 2024.

All Science Journal Classification (ASJC) codes

Biochemistry
Molecular Medicine
Molecular Biology
Clinical Biochemistry

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10.1038/s12276-024-01164-8

Cite this

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abstract = "The major drawbacks of RNA sequencing (RNA-seq), a remarkably accurate transcriptome profiling method, is its high cost and poor scalability. Here, we report a highly scalable and cost-effective method for transcriptomics profiling called Bulk transcriptOme profiling of cell Lysate in a single poT (BOLT-seq), which is performed using unpurified bulk 3′-end mRNA in crude cell lysates. During BOLT-seq, RNA/DNA hybrids are directly subjected to tagmentation, and second-strand cDNA synthesis and RNA purification are omitted, allowing libraries to be constructed in 2 h of hands-on time. BOLT-seq was successfully used to cluster small molecule drugs based on their mechanisms of action and intended targets. BOLT-seq competes effectively with alternative library construction and transcriptome profiling methods.",

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AU - Lee, Ji Hyun

AU - Bang, Duhee

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Cost and time-efficient construction of a 3′-end mRNA library from unpurified bulk RNA in a single tube

Abstract

Bibliographical note

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