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A lentiviral system for efficient knockdown of proteins in neuronal cultures version 1; referees: 2 approved

机译:用于有效敲除神经元培养物中蛋白质的慢病毒系统版本1;裁判员:2批准

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摘要

We have devised a protocol for highly efficient and specific knockdown of proteins in neuronal cultures. Small hairpin RNAs (shRNAs) are embedded into a microRNA (miRNA) context by oligo annealing to create shRNAmiRs, which are expressed from within the 3′-UTR of a reporter protein. This reporter protein/synthetic miRNA cassette is transferred to a targeting vector and lentivirus is produced in HEK-293-T cells following co-transfection of the targeting vector with three additional vectors encoding essential lentiviral proteins. Mature virus is harvested by collecting culture medium from transfected HEK-293-T cells, the virus is purified by centrifugation, and virus titers are determined prior to addition to neuronal cultures. Near 100% transduction efficiency of cultured hippocampal neurons is routinely observed and allows for the population-wide inhibition of target protein expression and the simultaneous knockdown of multiple proteins with little or no toxicity. The lentivirus generated can be used for protein knockdown in multiple neuronal culture models and at a variety of developmental stages. The steps from shRNAmiR design to ready-to-use virus stocks can be completed in as little as two weeks.
机译:我们设计了一种协议,可以高效,特异性地敲除神经元培养物中的蛋白质。小发夹式RNA(shRNA)通过寡核苷酸退火嵌入到microRNA(miRNA)上下文中,以生成shRNAmiR,该shRNAmiR在报道蛋白的3'-UTR中表达。将该报道蛋白/合成的miRNA盒转移至靶向载体,并在将HEK-293-T细胞与编码必需慢病毒蛋白的三种其他载体共转染后,在HEK-293-T细胞中产生慢病毒。通过从转染的HEK-293-T细胞中收集培养基来收获成熟病毒,通过离心纯化病毒,并在加入神经元培养物之前确定病毒滴度。常规观察到培养的海马神经元的转导效率接近100%,并能在整个人群范围内抑制靶蛋白的表达,并同时敲除多种蛋白而几乎没有毒性。产生的慢病毒可用于多种神经元培养模型和各种发育阶段的蛋白敲低。从shRNAmiR设计到即用型病毒库的步骤仅需两周即可完成。

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