Potential pitfalls in the accuracy of analysis of natural sense-antisense RNA pairs by reverse transcription-PCR

Potential pitfalls in the accuracy of analysis of natural sense-antisense RNA pairs by reverse transcription-PCR

<p>Abstract</p> <p>Background</p> <p>The ability to accurately measure patterns of gene expression is essential in studying gene function. The reverse transcription polymerase chain reaction (RT-PCR) has become the method of choice for the detection and measurement of R...

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Main Authors: Guo Hongyan, Giger Julie M, Qin Anqi X, Haddad Fadia, Baldwin Kenneth M
Format: Article
Language:English
Published: BMC 2007-05-01
Series:BMC Biotechnology
Online Access:http://www.biomedcentral.com/1472-6750/7/21
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spelling doaj-53205ef3d83041fda90f7eb319d2b7d62020-11-25T03:42:29ZengBMCBMC Biotechnology1472-67502007-05-01712110.1186/1472-6750-7-21Potential pitfalls in the accuracy of analysis of natural sense-antisense RNA pairs by reverse transcription-PCRGuo HongyanGiger Julie MQin Anqi XHaddad FadiaBaldwin Kenneth M<p>Abstract</p> <p>Background</p> <p>The ability to accurately measure patterns of gene expression is essential in studying gene function. The reverse transcription polymerase chain reaction (RT-PCR) has become the method of choice for the detection and measurement of RNA expression patterns in both cells and small quantities of tissue. Our previous results show that there is a significant production of primer-independent cDNA synthesis using a popular RNase H<sup>- </sup>RT enzyme. A PCR product was amplified from RT reactions that were carried out without addition of RT-primer. This finding jeopardizes the accuracy of RT-PCR when analyzing RNA that is expressed in both orientations. Current literature findings suggest that naturally occurring antisense expression is widespread in the mammalian transcriptome and consists of both coding and non-coding regulatory RNA. The primary purpose of this present study was to investigate the occurrence of primer-independent cDNA synthesis and how it may influence the accuracy of detection of sense-antisense RNA pairs.</p> <p>Results</p> <p>Our findings on cellular RNA and <it>in vitro </it>synthesized RNA suggest that these products are likely the results of RNA self-priming to generate random cDNA products, which contributes to the loss of strand specificity. The use of RNase H<sup>+ </sup>RT enzyme and carrying the RT reaction at high temperature (50°C) greatly improved the strand specificity of the RT-PCR detection.</p> <p>Conclusion</p> <p>While RT PCR is a basic method used for the detection and quantification of RNA expression in cells, primer-independent cDNA synthesis can interfere with RT specificity, and may lead to misinterpretation of the results, especially when both sense and antisense RNA are expressed. For accurate interpretation of the results, it is essential to carry out the appropriate negative controls.</p> http://www.biomedcentral.com/1472-6750/7/21
collection DOAJ
language English
format Article
sources DOAJ
author Guo Hongyan
Giger Julie M
Qin Anqi X
Haddad Fadia
Baldwin Kenneth M
spellingShingle Guo Hongyan
Giger Julie M
Qin Anqi X
Haddad Fadia
Baldwin Kenneth M
Potential pitfalls in the accuracy of analysis of natural sense-antisense RNA pairs by reverse transcription-PCR
BMC Biotechnology
author_facet Guo Hongyan
Giger Julie M
Qin Anqi X
Haddad Fadia
Baldwin Kenneth M
author_sort Guo Hongyan
title Potential pitfalls in the accuracy of analysis of natural sense-antisense RNA pairs by reverse transcription-PCR
title_short Potential pitfalls in the accuracy of analysis of natural sense-antisense RNA pairs by reverse transcription-PCR
title_full Potential pitfalls in the accuracy of analysis of natural sense-antisense RNA pairs by reverse transcription-PCR
title_fullStr Potential pitfalls in the accuracy of analysis of natural sense-antisense RNA pairs by reverse transcription-PCR
title_full_unstemmed Potential pitfalls in the accuracy of analysis of natural sense-antisense RNA pairs by reverse transcription-PCR
title_sort potential pitfalls in the accuracy of analysis of natural sense-antisense rna pairs by reverse transcription-pcr
publisher BMC
series BMC Biotechnology
issn 1472-6750
publishDate 2007-05-01
description <p>Abstract</p> <p>Background</p> <p>The ability to accurately measure patterns of gene expression is essential in studying gene function. The reverse transcription polymerase chain reaction (RT-PCR) has become the method of choice for the detection and measurement of RNA expression patterns in both cells and small quantities of tissue. Our previous results show that there is a significant production of primer-independent cDNA synthesis using a popular RNase H<sup>- </sup>RT enzyme. A PCR product was amplified from RT reactions that were carried out without addition of RT-primer. This finding jeopardizes the accuracy of RT-PCR when analyzing RNA that is expressed in both orientations. Current literature findings suggest that naturally occurring antisense expression is widespread in the mammalian transcriptome and consists of both coding and non-coding regulatory RNA. The primary purpose of this present study was to investigate the occurrence of primer-independent cDNA synthesis and how it may influence the accuracy of detection of sense-antisense RNA pairs.</p> <p>Results</p> <p>Our findings on cellular RNA and <it>in vitro </it>synthesized RNA suggest that these products are likely the results of RNA self-priming to generate random cDNA products, which contributes to the loss of strand specificity. The use of RNase H<sup>+ </sup>RT enzyme and carrying the RT reaction at high temperature (50°C) greatly improved the strand specificity of the RT-PCR detection.</p> <p>Conclusion</p> <p>While RT PCR is a basic method used for the detection and quantification of RNA expression in cells, primer-independent cDNA synthesis can interfere with RT specificity, and may lead to misinterpretation of the results, especially when both sense and antisense RNA are expressed. For accurate interpretation of the results, it is essential to carry out the appropriate negative controls.</p>
url http://www.biomedcentral.com/1472-6750/7/21
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