An accurate quantitative method for screening effective siRNA probes targeting a Hepatitis B virus transcript in single living cells

Wen ping Tong; Yu Zhou; Xinxin Wang; Fan Yang; Kai Lang Wu; Jianguo Wu; Yi Zhang

doi:10.1016/j.bbrc.2008.01.025

An accurate quantitative method for screening effective siRNA probes targeting a Hepatitis B virus transcript in single living cells

Wen ping Tong
, Yu Zhou
, Xinxin Wang
, Fan Yang
, Kai Lang Wu
, Jianguo Wu
, Yi Zhang

Wuhan University

科研成果: 期刊稿件 › 文章 › 同行评审

6 引用（Scopus）

摘要

A dual fluorescence reporter plasmid expressing EGFP and DsRed-Monomer from separate promoters was constructed for quantitative flow cytometry analysis. Cloning the hepatitis B virus (HBV) X gene into the 3′ UTR region of DsRed-Monomer allowed quantifying the efficacy of ten siRNAs designed according to the accessibility of HBx mRNA measured in vitro. Using EGFP as an internal control, a justified calculation of the changed mean fluorescence intensity of DsRed-Monomer in each transfected cell yielded highly consistent results, and revealed all 10 siRNAs achieved over 50% inhibition among which a super effective siRNA achieved 88% inhibition at a very low concentration (0.33 μg/ml). This provides a quantification method critical for therapeutic application of siRNA.

源语言	英语
页（从-至）	866-873
页数	8
期刊	Biochemical and Biophysical Research Communications
卷	367
期	4
DOI	https://doi.org/10.1016/j.bbrc.2008.01.025
出版状态	已出版 - 21 3月 2008
已对外发布	是

联合国可持续发展目标

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可持续发展目标 3 良好健康与福祉

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10.1016/j.bbrc.2008.01.025

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@article{7e703bf295e94f6793d22e1dbeb6d3ba,

title = "An accurate quantitative method for screening effective siRNA probes targeting a Hepatitis B virus transcript in single living cells",

abstract = "A dual fluorescence reporter plasmid expressing EGFP and DsRed-Monomer from separate promoters was constructed for quantitative flow cytometry analysis. Cloning the hepatitis B virus (HBV) X gene into the 3′ UTR region of DsRed-Monomer allowed quantifying the efficacy of ten siRNAs designed according to the accessibility of HBx mRNA measured in vitro. Using EGFP as an internal control, a justified calculation of the changed mean fluorescence intensity of DsRed-Monomer in each transfected cell yielded highly consistent results, and revealed all 10 siRNAs achieved over 50\% inhibition among which a super effective siRNA achieved 88\% inhibition at a very low concentration (0.33 μg/ml). This provides a quantification method critical for therapeutic application of siRNA.",

keywords = "Dual fluorescence reporter, Hepatitis B virus, Hepatitis B virus X protein, Quantitative flow cytometry, siRNA",

author = "Tong, \{Wen ping\} and Yu Zhou and Xinxin Wang and Fan Yang and Wu, \{Kai Lang\} and Jianguo Wu and Yi Zhang",

year = "2008",

month = mar,

day = "21",

doi = "10.1016/j.bbrc.2008.01.025",

language = "英语",

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pages = "866--873",

journal = "Biochemical and Biophysical Research Communications",

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TY - JOUR

T1 - An accurate quantitative method for screening effective siRNA probes targeting a Hepatitis B virus transcript in single living cells

AU - Tong, Wen ping

AU - Zhou, Yu

AU - Wang, Xinxin

AU - Yang, Fan

AU - Wu, Kai Lang

AU - Wu, Jianguo

AU - Zhang, Yi

PY - 2008/3/21

Y1 - 2008/3/21

N2 - A dual fluorescence reporter plasmid expressing EGFP and DsRed-Monomer from separate promoters was constructed for quantitative flow cytometry analysis. Cloning the hepatitis B virus (HBV) X gene into the 3′ UTR region of DsRed-Monomer allowed quantifying the efficacy of ten siRNAs designed according to the accessibility of HBx mRNA measured in vitro. Using EGFP as an internal control, a justified calculation of the changed mean fluorescence intensity of DsRed-Monomer in each transfected cell yielded highly consistent results, and revealed all 10 siRNAs achieved over 50% inhibition among which a super effective siRNA achieved 88% inhibition at a very low concentration (0.33 μg/ml). This provides a quantification method critical for therapeutic application of siRNA.

AB - A dual fluorescence reporter plasmid expressing EGFP and DsRed-Monomer from separate promoters was constructed for quantitative flow cytometry analysis. Cloning the hepatitis B virus (HBV) X gene into the 3′ UTR region of DsRed-Monomer allowed quantifying the efficacy of ten siRNAs designed according to the accessibility of HBx mRNA measured in vitro. Using EGFP as an internal control, a justified calculation of the changed mean fluorescence intensity of DsRed-Monomer in each transfected cell yielded highly consistent results, and revealed all 10 siRNAs achieved over 50% inhibition among which a super effective siRNA achieved 88% inhibition at a very low concentration (0.33 μg/ml). This provides a quantification method critical for therapeutic application of siRNA.

KW - Dual fluorescence reporter

KW - Hepatitis B virus

KW - Hepatitis B virus X protein

KW - Quantitative flow cytometry

KW - siRNA

UR - https://www.scopus.com/pages/publications/38649095213

U2 - 10.1016/j.bbrc.2008.01.025

DO - 10.1016/j.bbrc.2008.01.025

M3 - 文章

C2 - 18201553

AN - SCOPUS:38649095213

SN - 0006-291X

VL - 367

SP - 866

EP - 873

JO - Biochemical and Biophysical Research Communications

JF - Biochemical and Biophysical Research Communications

IS - 4

ER -

An accurate quantitative method for screening effective siRNA probes targeting a Hepatitis B virus transcript in single living cells

摘要

联合国可持续发展目标

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