Construction of a vector generating both siRNA and a fluorescent reporter: A siRNA study in cultured neurons

Seung Yoon Yoon; Jung Eun Choi; Onyou Hwang; Hea Nam Hong; Heuiran Lee; Yoo Kyum Kim; Sung Woo Cho; Hyun Kim; Dong Hou Kim

doi:10.1016/s1016-8478(23)13091-3

Construction of a vector generating both siRNA and a fluorescent reporter: A siRNA study in cultured neurons

Seung Yoon Yoon, Jung Eun Choi, Onyou Hwang, Hea Nam Hong, Heuiran Lee, Yoo Kyum Kim, Sung Woo Cho, Hyun Kim, Dong Hou Kim

Department of Biomedical Sciences

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

11 Citations (Scopus)

Abstract

RNA interference is an important tool for gene silencing. However, its application to primary cultured cells has been limited by low transfection efficiencies. In this work we developed a vector which encodes both siRNA and red fluorescent protein. Using this vector we could markedly suppress green fluorescent protein (GFP) and bim an endogenous gene. Primary cultured cortical neurons transfected with siRNA against doublecortin showed that doublecortin expression was significantly inhibited in nearly all the transfected neurons. This vector identifies the transfected cells and should be useful for loss-of-gene function studies in neurons.

Original language	English
Pages (from-to)	127-130
Number of pages	4
Journal	Molecules and cells
Volume	18
Issue number	1
DOIs	https://doi.org/10.1016/s1016-8478(23)13091-3
Publication status	Published - 2004 Aug 31

Keywords

Fluorescent reporter
Neuron
siRNA

ASJC Scopus subject areas

Molecular Biology
Cell Biology

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10.1016/s1016-8478(23)13091-3

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abstract = "RNA interference is an important tool for gene silencing. However, its application to primary cultured cells has been limited by low transfection efficiencies. In this work we developed a vector which encodes both siRNA and red fluorescent protein. Using this vector we could markedly suppress green fluorescent protein (GFP) and bim an endogenous gene. Primary cultured cortical neurons transfected with siRNA against doublecortin showed that doublecortin expression was significantly inhibited in nearly all the transfected neurons. This vector identifies the transfected cells and should be useful for loss-of-gene function studies in neurons.",

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T1 - Construction of a vector generating both siRNA and a fluorescent reporter

T2 - A siRNA study in cultured neurons

AU - Yoon, Seung Yoon

AU - Choi, Jung Eun

AU - Hwang, Onyou

AU - Hong, Hea Nam

AU - Lee, Heuiran

AU - Kim, Yoo Kyum

AU - Cho, Sung Woo

AU - Kim, Hyun

AU - Kim, Dong Hou

PY - 2004/8/31

Y1 - 2004/8/31

N2 - RNA interference is an important tool for gene silencing. However, its application to primary cultured cells has been limited by low transfection efficiencies. In this work we developed a vector which encodes both siRNA and red fluorescent protein. Using this vector we could markedly suppress green fluorescent protein (GFP) and bim an endogenous gene. Primary cultured cortical neurons transfected with siRNA against doublecortin showed that doublecortin expression was significantly inhibited in nearly all the transfected neurons. This vector identifies the transfected cells and should be useful for loss-of-gene function studies in neurons.

AB - RNA interference is an important tool for gene silencing. However, its application to primary cultured cells has been limited by low transfection efficiencies. In this work we developed a vector which encodes both siRNA and red fluorescent protein. Using this vector we could markedly suppress green fluorescent protein (GFP) and bim an endogenous gene. Primary cultured cortical neurons transfected with siRNA against doublecortin showed that doublecortin expression was significantly inhibited in nearly all the transfected neurons. This vector identifies the transfected cells and should be useful for loss-of-gene function studies in neurons.

KW - Fluorescent reporter

KW - Neuron

KW - siRNA

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SN - 1016-8478

VL - 18

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JO - Molecules and cells

JF - Molecules and cells

IS - 1

ER -

Construction of a vector generating both siRNA and a fluorescent reporter: A siRNA study in cultured neurons

Abstract

Keywords

ASJC Scopus subject areas

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