Blending DNA binding dyes to improve detection in real-time PCR

Linda Jansson; Marianne Koliana; Maja Sidstedt; Johannes Hedman

doi:10.1016/j.btre.2017.02.002

Blending DNA binding dyes to improve detection in real-time PCR

Linda Jansson, Marianne Koliana, Maja Sidstedt, Johannes Hedman

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

Abstract

The success of real-time PCR (qPCR) analysis is partly limited by the presence of inhibitory compounds in the nucleic acid samples. For example, humic acid (HA) from soil and aqueous sediment interferes with amplification and also quenches the fluorescence of double-stranded (ds) DNA binding dyes, thus hindering amplicon detection. We aimed to counteract the HA fluorescence quenching effect by blending complementary dsDNA binding dyes, thereby elevating the dye saturation levels and increasing the fluorescence signals. A blend of the four dyes EvaGreen, ResoLight, SYBR Green and SYTO9 gave significantly higher fluorescence intensities in the presence and absence of HA, compared with the dyes applied separately and two-dye blends. We propose blending of dyes as a generally applicable means for elevating qPCR fluorescence signals and thus enabling detection in the presence of quenching substances.

Original language	English
Pages (from-to)	34-37
Number of pages	4
Journal	Biotechnology Reports
Volume	14
DOIs	https://doi.org/10.1016/j.btre.2017.02.002
Publication status	Published - 2017 Mar 1

Subject classification (UKÄ)

Medical Laboratory and Measurements Technologies

Free keywords

Fluorescence quenching
Humic acid
PCR inhibition
qPCR
Soil

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10.1016/j.btre.2017.02.002

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title = "Blending DNA binding dyes to improve detection in real-time PCR",

abstract = "The success of real-time PCR (qPCR) analysis is partly limited by the presence of inhibitory compounds in the nucleic acid samples. For example, humic acid (HA) from soil and aqueous sediment interferes with amplification and also quenches the fluorescence of double-stranded (ds) DNA binding dyes, thus hindering amplicon detection. We aimed to counteract the HA fluorescence quenching effect by blending complementary dsDNA binding dyes, thereby elevating the dye saturation levels and increasing the fluorescence signals. A blend of the four dyes EvaGreen, ResoLight, SYBR Green and SYTO9 gave significantly higher fluorescence intensities in the presence and absence of HA, compared with the dyes applied separately and two-dye blends. We propose blending of dyes as a generally applicable means for elevating qPCR fluorescence signals and thus enabling detection in the presence of quenching substances.",

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author = "Linda Jansson and Marianne Koliana and Maja Sidstedt and Johannes Hedman",

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T1 - Blending DNA binding dyes to improve detection in real-time PCR

AU - Jansson, Linda

AU - Koliana, Marianne

AU - Sidstedt, Maja

AU - Hedman, Johannes

PY - 2017/3/1

Y1 - 2017/3/1

N2 - The success of real-time PCR (qPCR) analysis is partly limited by the presence of inhibitory compounds in the nucleic acid samples. For example, humic acid (HA) from soil and aqueous sediment interferes with amplification and also quenches the fluorescence of double-stranded (ds) DNA binding dyes, thus hindering amplicon detection. We aimed to counteract the HA fluorescence quenching effect by blending complementary dsDNA binding dyes, thereby elevating the dye saturation levels and increasing the fluorescence signals. A blend of the four dyes EvaGreen, ResoLight, SYBR Green and SYTO9 gave significantly higher fluorescence intensities in the presence and absence of HA, compared with the dyes applied separately and two-dye blends. We propose blending of dyes as a generally applicable means for elevating qPCR fluorescence signals and thus enabling detection in the presence of quenching substances.

AB - The success of real-time PCR (qPCR) analysis is partly limited by the presence of inhibitory compounds in the nucleic acid samples. For example, humic acid (HA) from soil and aqueous sediment interferes with amplification and also quenches the fluorescence of double-stranded (ds) DNA binding dyes, thus hindering amplicon detection. We aimed to counteract the HA fluorescence quenching effect by blending complementary dsDNA binding dyes, thereby elevating the dye saturation levels and increasing the fluorescence signals. A blend of the four dyes EvaGreen, ResoLight, SYBR Green and SYTO9 gave significantly higher fluorescence intensities in the presence and absence of HA, compared with the dyes applied separately and two-dye blends. We propose blending of dyes as a generally applicable means for elevating qPCR fluorescence signals and thus enabling detection in the presence of quenching substances.

KW - Fluorescence quenching

KW - Humic acid

KW - PCR inhibition

KW - qPCR

KW - Soil

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DO - 10.1016/j.btre.2017.02.002

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SN - 2215-017X

VL - 14

SP - 34

EP - 37

JO - Biotechnology Reports

JF - Biotechnology Reports

ER -

Blending DNA binding dyes to improve detection in real-time PCR

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