Pitfalls in the normalization of real-time polymerase chain reaction data

被引：65

作者：

Hendriks-Balk, Marielle C. ^{[1
]}

Michel, Martin C. ^{[1
]}

Alewijnse, Astrid E. ^{[1
]}

机构：

[1] Acad Med Ctr, Dept Pharmacol & Pharmacotherapy, NL-1105 AZ Amsterdam, Netherlands

来源：

BASIC RESEARCH IN CARDIOLOGY | 2007年 / 102卷 / 03期

关键词：

real time polymerase chain reaction; normalization; reference gene; housekeeping gene;

D O I：

10.1007/s00395-007-0649-0

中图分类号：

R5 [内科学];

学科分类号：

1002 ; 100201 ;

摘要：

Real-time polymerase chain reaction (PCR) is commonly used for a sensitive and specific quantification of messenger RNA (mRNA). The levels of mRNA are frequently compared between two or more experimental groups. However, such comparisons require normalization procedures, and reference genes are frequently used for this purpose. We discuss pitfalls in normalization and specifically in the choice of reference genes. Reference genes, which prove suitable for some experimental conditions, are not necessarily similarly appropriate for others. Therefore,a proper validation of the suitability of a given reference gene or sets thereof is required for each experimental setting. Several computer programmes are available to aid such validation.

引用

页码：195 / 197

页数：3

共 10 条

[1] Expression of mRNA encoding G protein-coupled receptors involved in congestive heart failure - A quantitative RT-PCR study and the question of normalisation
Brattelid, Trond
Tveit, Kristine
Birkeland, Jon Arne K.
Sjaastad, Ivar
Qvigstad, Eirik
Krobert, Kurt Allen
Hussain, Rizwan I.
Skomedal, Tor
Osnes, Jan-Bjorn
Levy, Finn Olav
[J]. BASIC RESEARCH IN CARDIOLOGY, 2007, 102 (03) : 198 - 208
[2] Bustin Stephen A, 2004, J Biomol Tech, V15, P155
[3] Normalization of gene expression measurements in tumor tissues: comparison of 13 endogenous control genes
de Kok, JB
Roelofs, RW
Giesendorf, BA
Pennings, JL
Waas, ET
Feuth, T
Swinkels, DW
Span, PN
[J]. LABORATORY INVESTIGATION, 2005, 85 (01) : 154 - 159
[4] The implications of using an inappropriate reference gene for real-time reverse transcription PCR data normalization
Dheda, K
Huggett, JF
Chang, JS
Kim, LU
Bustin, SA
Johnson, MA
Rook, GAW
Zumla, A
[J]. ANALYTICAL BIOCHEMISTRY, 2005, 344 (01) : 141 - 143
[5] Real-time RT-PCR normalisation; strategies and considerations
Huggett, J
Dheda, K
Bustin, S
Zumla, A
[J]. GENES AND IMMUNITY, 2005, 6 (04) : 279 - 284
[6] Validation of candidate bovine reference genes for use with real-time PCR
Robinson, T. L.
Sutherland, I. A.
Sutherland, J.
[J]. VETERINARY IMMUNOLOGY AND IMMUNOPATHOLOGY, 2007, 115 (1-2) : 160 - 165
[7] Commonly used reference genes are actively regulated in in vitro stimulated lymphocytes
Roge, R.
Thorsen, J.
Torring, C.
Ozbay, A.
Moller, B. K.
Carstens, J.
[J]. SCANDINAVIAN JOURNAL OF IMMUNOLOGY, 2007, 65 (02) : 202 - 209
[8] Effect of experimental treatment on housekeeping gene expression: validation by real-time, quantitative RT-PCR
Schmittgen, TD
Zakrajsek, BA
[J]. JOURNAL OF BIOCHEMICAL AND BIOPHYSICAL METHODS, 2000, 46 (1-2): : 69 - 81
[9] Unsuitability of using ribosomal RNA as loading control for Northern blot analyses related to the imbalance between messenger and ribosomal RNA content in rat mammary tumors
Solanas, M
Moral, R
Escrich, E
[J]. ANALYTICAL BIOCHEMISTRY, 2001, 288 (01) : 99 - 102
[10] Accurate normalization of real-time quantitative RT-PCR data by geometric averaging of multiple internal control genes
Vandesompele, Jo
De Preter, Katleen
Pattyn, Filip
Poppe, Bruce
Van Roy, Nadine
De Paepe, Anne
Speleman, Frank
[J]. GENOME BIOLOGY, 2002, 3 (07)

← 1 →