TqPCR: A Touchdown qPCR Assay with Significantly Improved Detection Sensitivity and Amplification Efficiency of SYBR Green qPCR

The advent of fluorescence-based quantitative real-time PCR (qPCR) has revolutionized the quantification of gene expression analysis in many fields, including life sciences, agriculture, forensic science, molecular diagnostics, and medicine. While SYBR Green-based qPCR is the most commonly-used plat...

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Autores principales: Zhang, Qian, Wang, Jing, Deng, Fang, Yan, Zhengjian, Xia, Yinglin, Wang, Zhongliang, Ye, Jixing, Deng, Youlin, Zhang, Zhonglin, Qiao, Min, Li, Ruifang, Denduluri, Sahitya K., Wei, Qiang, Zhao, Lianggong, Lu, Shun, Wang, Xin, Tang, Shengli, Liu, Hao, Luu, Hue H., Haydon, Rex C., He, Tong-Chuan, Jiang, Li
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2015
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4501803/
https://www.ncbi.nlm.nih.gov/pubmed/26172450
http://dx.doi.org/10.1371/journal.pone.0132666
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author Zhang, Qian
Wang, Jing
Deng, Fang
Yan, Zhengjian
Xia, Yinglin
Wang, Zhongliang
Ye, Jixing
Deng, Youlin
Zhang, Zhonglin
Qiao, Min
Li, Ruifang
Denduluri, Sahitya K.
Wei, Qiang
Zhao, Lianggong
Lu, Shun
Wang, Xin
Tang, Shengli
Liu, Hao
Luu, Hue H.
Haydon, Rex C.
He, Tong-Chuan
Jiang, Li
author_facet Zhang, Qian
Wang, Jing
Deng, Fang
Yan, Zhengjian
Xia, Yinglin
Wang, Zhongliang
Ye, Jixing
Deng, Youlin
Zhang, Zhonglin
Qiao, Min
Li, Ruifang
Denduluri, Sahitya K.
Wei, Qiang
Zhao, Lianggong
Lu, Shun
Wang, Xin
Tang, Shengli
Liu, Hao
Luu, Hue H.
Haydon, Rex C.
He, Tong-Chuan
Jiang, Li
author_sort Zhang, Qian
collection PubMed
description The advent of fluorescence-based quantitative real-time PCR (qPCR) has revolutionized the quantification of gene expression analysis in many fields, including life sciences, agriculture, forensic science, molecular diagnostics, and medicine. While SYBR Green-based qPCR is the most commonly-used platform due to its inexpensive nature and robust chemistry, quantifying the expression of genes with low abundance or RNA samples extracted from highly restricted or limited sources can be challenging because the detection sensitivity of SYBR Green-based qPCR is limited. Here, we develop a novel and effective touchdown qPCR (TqPCR) protocol by incorporating a 4-cycle touchdown stage prior to the quantification amplification stage. Using the same cDNA templates, we find that TqPCR can reduce the average Cq values for Gapdh, Rps13, and Hprt1 reference genes by 4.45, 5.47, and 4.94 cycles, respectively, when compared with conventional qPCR; the overall average Cq value reduction for the three reference genes together is 4.95. We further find that TqPCR can improve PCR amplification efficiency and thus increase detection sensitivity. When the quantification of Wnt3A-induced target gene expression in mesenchymal stem cells is analyzed, we find that, while both conventional qPCR and TqPCR can detect the up-regulation of the relatively abundant target Axin2, only TqPCR can detect the up-regulation of the lowly-expressed targets Oct4 and Gbx2. Finally, we demonstrate that the MRQ2 and MRQ3 primer pairs derived from mouse reference gene Tbp can be used to validate the RNA/cDNA integrity of qPCR samples. Taken together, our results strongly suggest that TqPCR may increase detection sensitivity and PCR amplification efficiency. Overall, TqPCR should be advantageous over conventional qPCR in expression quantification, especially when the transcripts of interest are lowly expressed, and/or the availability of total RNA is highly restricted or limited.
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spelling pubmed-45018032015-07-17 TqPCR: A Touchdown qPCR Assay with Significantly Improved Detection Sensitivity and Amplification Efficiency of SYBR Green qPCR Zhang, Qian Wang, Jing Deng, Fang Yan, Zhengjian Xia, Yinglin Wang, Zhongliang Ye, Jixing Deng, Youlin Zhang, Zhonglin Qiao, Min Li, Ruifang Denduluri, Sahitya K. Wei, Qiang Zhao, Lianggong Lu, Shun Wang, Xin Tang, Shengli Liu, Hao Luu, Hue H. Haydon, Rex C. He, Tong-Chuan Jiang, Li PLoS One Research Article The advent of fluorescence-based quantitative real-time PCR (qPCR) has revolutionized the quantification of gene expression analysis in many fields, including life sciences, agriculture, forensic science, molecular diagnostics, and medicine. While SYBR Green-based qPCR is the most commonly-used platform due to its inexpensive nature and robust chemistry, quantifying the expression of genes with low abundance or RNA samples extracted from highly restricted or limited sources can be challenging because the detection sensitivity of SYBR Green-based qPCR is limited. Here, we develop a novel and effective touchdown qPCR (TqPCR) protocol by incorporating a 4-cycle touchdown stage prior to the quantification amplification stage. Using the same cDNA templates, we find that TqPCR can reduce the average Cq values for Gapdh, Rps13, and Hprt1 reference genes by 4.45, 5.47, and 4.94 cycles, respectively, when compared with conventional qPCR; the overall average Cq value reduction for the three reference genes together is 4.95. We further find that TqPCR can improve PCR amplification efficiency and thus increase detection sensitivity. When the quantification of Wnt3A-induced target gene expression in mesenchymal stem cells is analyzed, we find that, while both conventional qPCR and TqPCR can detect the up-regulation of the relatively abundant target Axin2, only TqPCR can detect the up-regulation of the lowly-expressed targets Oct4 and Gbx2. Finally, we demonstrate that the MRQ2 and MRQ3 primer pairs derived from mouse reference gene Tbp can be used to validate the RNA/cDNA integrity of qPCR samples. Taken together, our results strongly suggest that TqPCR may increase detection sensitivity and PCR amplification efficiency. Overall, TqPCR should be advantageous over conventional qPCR in expression quantification, especially when the transcripts of interest are lowly expressed, and/or the availability of total RNA is highly restricted or limited. Public Library of Science 2015-07-14 /pmc/articles/PMC4501803/ /pubmed/26172450 http://dx.doi.org/10.1371/journal.pone.0132666 Text en © 2015 Zhang et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Zhang, Qian
Wang, Jing
Deng, Fang
Yan, Zhengjian
Xia, Yinglin
Wang, Zhongliang
Ye, Jixing
Deng, Youlin
Zhang, Zhonglin
Qiao, Min
Li, Ruifang
Denduluri, Sahitya K.
Wei, Qiang
Zhao, Lianggong
Lu, Shun
Wang, Xin
Tang, Shengli
Liu, Hao
Luu, Hue H.
Haydon, Rex C.
He, Tong-Chuan
Jiang, Li
TqPCR: A Touchdown qPCR Assay with Significantly Improved Detection Sensitivity and Amplification Efficiency of SYBR Green qPCR
title TqPCR: A Touchdown qPCR Assay with Significantly Improved Detection Sensitivity and Amplification Efficiency of SYBR Green qPCR
title_full TqPCR: A Touchdown qPCR Assay with Significantly Improved Detection Sensitivity and Amplification Efficiency of SYBR Green qPCR
title_fullStr TqPCR: A Touchdown qPCR Assay with Significantly Improved Detection Sensitivity and Amplification Efficiency of SYBR Green qPCR
title_full_unstemmed TqPCR: A Touchdown qPCR Assay with Significantly Improved Detection Sensitivity and Amplification Efficiency of SYBR Green qPCR
title_short TqPCR: A Touchdown qPCR Assay with Significantly Improved Detection Sensitivity and Amplification Efficiency of SYBR Green qPCR
title_sort tqpcr: a touchdown qpcr assay with significantly improved detection sensitivity and amplification efficiency of sybr green qpcr
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4501803/
https://www.ncbi.nlm.nih.gov/pubmed/26172450
http://dx.doi.org/10.1371/journal.pone.0132666
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