Flow cytometric analysis of RNA synthesis by detection of bromouridine incorporation

J K Larsen; Peter Østrup Jensen; J Larsen

doi:10.1002/0471142956.cy0712s12

Flow cytometric analysis of RNA synthesis by detection of bromouridine incorporation

J K Larsen, Peter Østrup Jensen, J Larsen

Ph.d.-studienævnet for Medicin

Publikation: Bidrag til tidsskrift › Tidsskriftartikel › Forskning › peer review

6 Citationer (Scopus)

Abstract

RNA synthesis has traditionally been investigated by a laborious and time-consuming radiographic method involving incorporation of tritiated uridine. Now a faster non-radioactive alternative has emerged, based on immunocytochemical detection. This method utilizes the brominated RNA precursor bromouridine, which is taken into a cell, phosphorylated, and incorporated into nascent RNA. The BrU-substituted RNA is detected by permeabilizing the cells and staining with certain anti-BrdU antibodies. This dynamic approach yields information complementing that provided by cellular RNA content analysis at a given time and may be of value in studies of cellular activation and gene expression.

Originalsprog	Engelsk
Tidsskrift	Current protocols in cytometry / editorial board, J. Paul Robinson, managing editor ... [et al.]
Vol/bind	Chapter 7
Sider (fra-til)	Unit 7.12
DOI	https://doi.org/10.1002/0471142956.cy0712s12
Status	Udgivet - 2001

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Citationsformater

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title = "Flow cytometric analysis of RNA synthesis by detection of bromouridine incorporation",

abstract = "RNA synthesis has traditionally been investigated by a laborious and time-consuming radiographic method involving incorporation of tritiated uridine. Now a faster non-radioactive alternative has emerged, based on immunocytochemical detection. This method utilizes the brominated RNA precursor bromouridine, which is taken into a cell, phosphorylated, and incorporated into nascent RNA. The BrU-substituted RNA is detected by permeabilizing the cells and staining with certain anti-BrdU antibodies. This dynamic approach yields information complementing that provided by cellular RNA content analysis at a given time and may be of value in studies of cellular activation and gene expression.",

keywords = "Animals, Antigens, Cell Membrane, Cell Nucleus, Cell Separation, Flow Cytometry, Gene Expression, Humans, RNA, Time Factors, Uridine",

author = "Larsen, {J K} and Jensen, {Peter {\O}strup} and J Larsen",

year = "2001",

doi = "10.1002/0471142956.cy0712s12",

language = "English",

volume = "Chapter 7",

pages = "Unit 7.12",

journal = "Current protocols in cytometry / editorial board, J. Paul Robinson, managing editor ... [et al.]",

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TY - JOUR

T1 - Flow cytometric analysis of RNA synthesis by detection of bromouridine incorporation

AU - Larsen, J K

AU - Jensen, Peter Østrup

AU - Larsen, J

PY - 2001

Y1 - 2001

N2 - RNA synthesis has traditionally been investigated by a laborious and time-consuming radiographic method involving incorporation of tritiated uridine. Now a faster non-radioactive alternative has emerged, based on immunocytochemical detection. This method utilizes the brominated RNA precursor bromouridine, which is taken into a cell, phosphorylated, and incorporated into nascent RNA. The BrU-substituted RNA is detected by permeabilizing the cells and staining with certain anti-BrdU antibodies. This dynamic approach yields information complementing that provided by cellular RNA content analysis at a given time and may be of value in studies of cellular activation and gene expression.

AB - RNA synthesis has traditionally been investigated by a laborious and time-consuming radiographic method involving incorporation of tritiated uridine. Now a faster non-radioactive alternative has emerged, based on immunocytochemical detection. This method utilizes the brominated RNA precursor bromouridine, which is taken into a cell, phosphorylated, and incorporated into nascent RNA. The BrU-substituted RNA is detected by permeabilizing the cells and staining with certain anti-BrdU antibodies. This dynamic approach yields information complementing that provided by cellular RNA content analysis at a given time and may be of value in studies of cellular activation and gene expression.

KW - Animals

KW - Antigens

KW - Cell Membrane

KW - Cell Nucleus

KW - Cell Separation

KW - Flow Cytometry

KW - Gene Expression

KW - Humans

KW - RNA

KW - Time Factors

KW - Uridine

U2 - 10.1002/0471142956.cy0712s12

DO - 10.1002/0471142956.cy0712s12

M3 - Journal article

C2 - 18770724

SN - 1934-9300

VL - Chapter 7

SP - Unit 7.12

JO - Current protocols in cytometry / editorial board, J. Paul Robinson, managing editor ... [et al.]

JF - Current protocols in cytometry / editorial board, J. Paul Robinson, managing editor ... [et al.]

ER -