CRISPR interference-based specific and efficient gene inactivation in the brain.
Yi ZhengWei ShenJian ZhangBo YangYao-Nan LiuHuihui QiXia YuSi-Yao LuYun ChenYu-Zhou XuYun LiFred H GageShuangli MiJun YaoPublished in: Nature neuroscience (2018)
CRISPR-Cas9 has been demonstrated to delete genes in postmitotic neurons. Compared to the establishment of proliferative cell lines or animal strains, it is more challenging to acquire a highly homogeneous consequence of gene editing in a stable neural network. Here we show that dCas9-based CRISPR interference (CRISPRi) can efficiently silence genes in neurons. Using a pseudotarget fishing strategy, we demonstrate that CRISPRi shows superior targeting specificity without detectable off-target activity. Furthermore, CRISPRi can achieve multiplex inactivation of genes fundamental for neurotransmitter release with high efficiency. By developing conditional CRISPRi tools targeting synaptotagmin I (Syt1), we modified the excitatory to inhibitory balance in the dentate gyrus of the mouse hippocampus and found that the dentate gyrus has distinct regulatory roles in learning and affective processes in mice. We therefore recommend CRISPRi as a useful tool for more rapid investigation of gene function in the mammalian brain.
Keyphrases
- genome wide
- crispr cas
- genome wide identification
- genome editing
- dna methylation
- high efficiency
- neural network
- copy number
- transcription factor
- genome wide analysis
- resting state
- white matter
- spinal cord
- cerebral ischemia
- cancer therapy
- bioinformatics analysis
- escherichia coli
- bipolar disorder
- gene expression
- functional connectivity
- high throughput
- type diabetes
- cognitive impairment
- drug delivery
- high fat diet induced
- insulin resistance
- spinal cord injury
- adipose tissue
- skeletal muscle
- loop mediated isothermal amplification
- blood brain barrier
- subarachnoid hemorrhage
- brain injury
- sensitive detection