Catalytically inactive, purified RNase H1: A specific and sensitive probe for RNA-DNA hybrid imaging

被引:48
作者
Crossley, Magdalena P. [1 ]
Brickner, Joshua R. [1 ]
Song, Chenlin [1 ]
Zar, Su Mon Thin [2 ]
Maw, Su S. [2 ]
Chedin, Frederic [3 ,4 ]
Tsai, Miaw-Sheue [2 ]
Cimprich, Karlene A. [1 ]
机构
[1] Stanford Univ, Dept Chem & Syst Biol, Sch Med, Stanford, CA 94305 USA
[2] Lawrence Berkeley Natl Lab, Biol Syst & Engn, Berkeley, CA USA
[3] Univ Calif Davis, Dept Mol & Cellular Biol, Davis, CA USA
[4] Univ Calif Davis, Genome Ctr, Davis, CA USA
基金
美国国家卫生研究院;
关键词
TRANSCRIPTIONAL PAUSE SITES; R-LOOPS; MONOCLONAL-ANTIBODY; RNA/DNA HYBRID; STRANDED-RNA; SENATAXIN; BRCA1;
D O I
10.1083/jcb.202101092
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
R-loops are three-stranded nucleic acid structures with both physiological and pathological roles in cells. R-loop imaging generally relies on detection of the RNA-DNA hybrid component of these structures using the S9.6 antibody. We show that the use of this antibody for imaging can be problematic because it readily binds to double-stranded RNA (dsRNA) in vitro and in vivo, giving rise to nonspecific signal. In contrast, purified, catalytically inactive human RNase H1 tagged with GFP (GFP-dRNH1) is a more specific reagent for imaging RNA-DNA hybrids. GFP-dRNH1 binds strongly to RNA-DNA hybrids but not to dsRNA oligonucleotides in fixed human cells and is not susceptible to binding endogenous RNA. Furthermore, we demonstrate that purified GFP-dRNH1 can be applied to fixed cells to detect hybrids after their induction, thereby bypassing the need for cell line engineering. GFP-dRNH1 therefore promises to be a versatile tool for imaging and quantifying RNA-DNA hybrids under a wide range of conditions.
引用
收藏
页数:19
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