Array-based nuclear run-on analysis

Jinshui Fan; Yu Chi Chen; Tonya Watkins; Chi V. Dang; Myriam Gorospe; Chris Cheadle

doi:10.1007/978-1-61779-376-9_33

Array-based nuclear run-on analysis

Jinshui Fan, Yu Chi Chen, Tonya Watkins, Chi V. Dang, Myriam Gorospe, Chris Cheadle

School of Medicine

Research output: Chapter in Book/Report/Conference proceeding › Chapter

4 Scopus citations

Abstract

There is extensive evidence that posttranscriptional mechanisms of gene regulation, such as mRNA turnover, critically affect the patterns of expressed mRNAs. Conventional microarray analysis measures steady-state messenger RNA (mRNA) levels, which represents the dynamic balance between new transcription and mRNA degradation. Accordingly, only de novo transcription can accurately reflect the temporal and spatial events of transcriptional regulation. In this chapter, we describe a recently reported method to study transcription systematically. It involves the genome-wide labeling of nascent transcripts using nonradioactive modified nucleotides, their isolation for amplification, and their hybridization and analysis using commercial microarrays.

Original language	English (US)
Title of host publication	Transcriptional Regulation
Subtitle of host publication	Methods and Protocols
Editors	Ales Vancura
Pages	505-517
Number of pages	13
DOIs	https://doi.org/10.1007/978-1-61779-376-9_33
State	Published - 2012

Publication series

Name	Methods in Molecular Biology
Volume	809
ISSN (Print)	1064-3745

Keywords

Biotin
Microarray
Nascent RNA
Nuclear run-on
Posttranscriptional regulation

ASJC Scopus subject areas

Molecular Biology
Genetics

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10.1007/978-1-61779-376-9_33

Cite this

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AU - Fan, Jinshui

AU - Chen, Yu Chi

AU - Watkins, Tonya

AU - Dang, Chi V.

AU - Gorospe, Myriam

AU - Cheadle, Chris

PY - 2012

Y1 - 2012

N2 - There is extensive evidence that posttranscriptional mechanisms of gene regulation, such as mRNA turnover, critically affect the patterns of expressed mRNAs. Conventional microarray analysis measures steady-state messenger RNA (mRNA) levels, which represents the dynamic balance between new transcription and mRNA degradation. Accordingly, only de novo transcription can accurately reflect the temporal and spatial events of transcriptional regulation. In this chapter, we describe a recently reported method to study transcription systematically. It involves the genome-wide labeling of nascent transcripts using nonradioactive modified nucleotides, their isolation for amplification, and their hybridization and analysis using commercial microarrays.

AB - There is extensive evidence that posttranscriptional mechanisms of gene regulation, such as mRNA turnover, critically affect the patterns of expressed mRNAs. Conventional microarray analysis measures steady-state messenger RNA (mRNA) levels, which represents the dynamic balance between new transcription and mRNA degradation. Accordingly, only de novo transcription can accurately reflect the temporal and spatial events of transcriptional regulation. In this chapter, we describe a recently reported method to study transcription systematically. It involves the genome-wide labeling of nascent transcripts using nonradioactive modified nucleotides, their isolation for amplification, and their hybridization and analysis using commercial microarrays.

KW - Biotin

KW - Microarray

KW - Nascent RNA

KW - Nuclear run-on

KW - Posttranscriptional regulation

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Array-based nuclear run-on analysis

Abstract

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Keywords

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