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首页> 外文期刊>The Journal of biological chemistry >Rabies Virus Envelope Glycoprotein Targets Lentiviral Vectors to the Axonal Retrograde Pathway in Motor Neurons
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Rabies Virus Envelope Glycoprotein Targets Lentiviral Vectors to the Axonal Retrograde Pathway in Motor Neurons

机译:Rabies病毒包膜糖蛋白靶向慢病毒载体到电机神经元的轴突逆行途径

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Rabies pseudotyped lentiviral vectors have great potential in gene therapy, not least because of their ability to transduce neurons following their distal axonal application. However, very little is known about the molecular processes that underlie their retrograde transport and cell transduction. Using multiple labeling techniques and confocal microscopy, we demonstrated that pseudotyping with rabies virus envelope glycoprotein (RV-G) enabled the axonal retrograde transport of two distinct subtypes of lentiviral vector in motor neuron cultures. Analysis of this process revealed that these vectors trafficked through Rab5-positive endosomes and accumulated within a non-acidic Rab7 compartment. RV-G pseudotyped vectors were co-transported with both the tetanus neurotoxin-binding fragment and the membrane proteins thought to mediate rabies virus endocytosis (neural cell adhesion molecule, nicotinic acetylcholine receptor, and p75 neurotrophin receptor), thus demonstrating that pseudotyping with RV-G targets lentiviral vectors for transport along the same pathway exploited by several toxins and viruses. Using motor neurons cultured in compartmentalized chambers, we demonstrated that axonal retrograde transport of these vectors was rapid and efficient; however, it was not able to transduce the targeted neurons efficiently, suggesting that impairment in processes occurring after arrival of the viral vector in the soma is responsible for the low transduction efficiency seen in vivo, which suggests a novel area for improvement of gene therapy vectors.
机译:狂犬病假型慢病毒载体在基因治疗中具有很大的潜力,并非最不重要的是因为它们在远端轴突施用之后转移神经元的能力。然而,关于其逆行传输和细胞转导的分子过程是非常熟知的。使用多种标记技术和共聚焦显微镜,我们证明了具有狂犬病病毒包膜糖蛋白(RV-G)的假型化使得在运动神经元培养物中的两个不同亚副血管载体的轴突逆行传输。对该过程的分析表明,这些载体通过Rab5阳性内体贩运并累积在非酸性Rab7隔间内。 RV-G伪型载体与破伤风神经毒素结合片段和膜蛋白思想介导狂犬病病毒内吞作用(神经细胞粘附分子,烟碱乙酰胆碱受体和P75神经营养蛋白受体)共同运输,从而证明了与RV-的假型g针对慢病毒载体进行沿着几种毒素和病毒利用的相同途径运输。使用在划分室中培养的电动神经元,我们证明了这些载体的轴突逆行传输迅速有效;然而,它不能有效地转染目,表明病毒病毒载体到达后发生的过程的损伤是对体内观察到的低转导效率,这表明了一种改善基因治疗载体的新区域。

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