Nuclear run-on assay using biotin labeling, magnetic bead capture and analysis by fluorescence-based RT-PCR

G. Patrone; F. Puppo; R. Cusano; M. Scaranari; I. Ceccherini; A. Puliti; R. Ravazzolo

Nuclear run-on assay using biotin labeling, magnetic bead capture and analysis by fluorescence-based RT-PCR

G. Patrone, F. Puppo, R. Cusano, M. Scaranari, I. Ceccherini, A. Puliti, R. Ravazzolo

Istituto "Giannina Gaslini"

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

Abstract

In this report, we present a fluorescence-based approach to the assessment of cellular gene expression and transcription rates. Nuclear run-on was performed by supplying biotin-16-UTP to nuclei, and labeled transcripts were bound to streptavidin-coated magnetic beads. Total cDNA was then synthesized by means of random hexamer primed reverse transcription of captured molecules. To monitor transcript abundance in cDNA, both from nuclear run-on and total RNA, we propose a semiquantitative PCR approach based on the use of fluorescent primers.

Original language	English
Pages (from-to)	1012-1017
Number of pages	6
Journal	BioTechniques
Volume	29
Issue number	5
Publication status	Published - 2000

ASJC Scopus subject areas

Biochemistry, Genetics and Molecular Biology(all)
Clinical Biochemistry

Cite this

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T1 - Nuclear run-on assay using biotin labeling, magnetic bead capture and analysis by fluorescence-based RT-PCR

AU - Patrone, G.

AU - Puppo, F.

AU - Cusano, R.

AU - Scaranari, M.

AU - Ceccherini, I.

AU - Puliti, A.

AU - Ravazzolo, R.

PY - 2000

Y1 - 2000

N2 - In this report, we present a fluorescence-based approach to the assessment of cellular gene expression and transcription rates. Nuclear run-on was performed by supplying biotin-16-UTP to nuclei, and labeled transcripts were bound to streptavidin-coated magnetic beads. Total cDNA was then synthesized by means of random hexamer primed reverse transcription of captured molecules. To monitor transcript abundance in cDNA, both from nuclear run-on and total RNA, we propose a semiquantitative PCR approach based on the use of fluorescent primers.

AB - In this report, we present a fluorescence-based approach to the assessment of cellular gene expression and transcription rates. Nuclear run-on was performed by supplying biotin-16-UTP to nuclei, and labeled transcripts were bound to streptavidin-coated magnetic beads. Total cDNA was then synthesized by means of random hexamer primed reverse transcription of captured molecules. To monitor transcript abundance in cDNA, both from nuclear run-on and total RNA, we propose a semiquantitative PCR approach based on the use of fluorescent primers.

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JO - BioTechniques

JF - BioTechniques

IS - 5

ER -

Nuclear run-on assay using biotin labeling, magnetic bead capture and analysis by fluorescence-based RT-PCR

Abstract

ASJC Scopus subject areas

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