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Pathway sensor-based functional genomics screening identifies modulators of neuronal activity

机译:基于通路传感器的功能基因组学筛选可确定神经元活动的调节剂

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Neuronal signal transduction shapes brain function and malfunction may cause mental disorders. Despite the existence of functional genomics screens for proliferation and toxicity, neuronal signalling has been difficult to address so far. To overcome this limitation, we developed a pooled screening assay which combines barcoded activity reporters with pooled genetic perturbation in a dual-expression adeno-associated virus (AAV) library. With this approach, termed pathScreener, we comprehensively dissect signalling pathways in postmitotic neurons. This overcomes several limitations of lentiviral-based screens. By applying first a barcoded and multiplexed reporter assay, termed cisProfiler, we identified the synaptic-activity responsive element (SARE) as top performance sensor of neuronal activity. Next, we targeted more than 4,400 genes and screened for modulatory effects on SARE activity in primary cortical neurons. We identified with high replicability many known genes involved in glutamatergic synapse-to-nucleus signalling of which a subset was validated in orthogonal assays. Several others have not yet been associated with the regulation of neuronal activity such as the hedgehog signalling members Ptch2 and Ift57. This assay thus enhances the toolbox for analysing regulatory processes during neuronal signalling and may help identifying novel targets for brain disorders.
机译:神经元信号转导会影响大脑功能,而机能障碍可能会导致精神障碍。尽管存在针对增殖和毒性的功能基因组学筛选,但迄今为止,神经元信号一直难以解决。为克服此限制,我们开发了一种合并筛选检测方法,该方法将条形码活性报告子与双重表达腺相关病毒(AAV)文库中的合并遗传扰动相结合。通过这种称为pathScreener的方法,我们可以全面剖析有丝分裂后神经元中的信号通路。这克服了基于慢病毒的筛选的一些限制。通过首先应用条形码和多重报告基因测定法,称为cisProfiler,我们确定了突触活性反应元件(SARE)作为神经元活动的顶级性能传感器。接下来,我们靶向了4,400多个基因,并筛选了对原代皮层神经元SARE活性的调节作用。我们以高可复制性鉴定出许多涉及谷氨酸能突触至细胞核信号传导的已知基因,其中一部分在正交试验中得到了验证。尚未将其他几个与神经元活动的调节相关联,例如刺猬信号传导成员Ptch2和Ift57。因此,该测定法增强了用于分析神经元信号传导过程中调节过程的工具箱,并可能有助于确定脑部疾病的新靶标。

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