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Infection Dissemination and Transmission of a West Nile Virus Green Fluorescent Protein Infectious Clone by Culex pipiens quinquefasciatus Mosquitoes

机译:西尼罗河病毒绿色荧光蛋白感染性克隆的感染传播和传播的蚊子库克蚊。

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摘要

We report the construction and comparative characterization of a full-length West Nile virus (WNV) cDNA infectious clone (ic) that contains a green fluorescent protein (GFP) expression cassette fused within the viral open reading frame. Virus derived from WNV-GFP ic stably infected Culex pipiens quinquefasciatus mosquitoes at comparable rates to virus derived from the parental (non-GFP) ic. However, insertion of this GFP cassette resulted in a temporal delay in in vivo replication kinetics and significantly decreased dissemination to head tissue. Consistent with previous reports of WNV-infected mosquito midguts, focal GFP expression was observed at 3 days post-infection (dpi), with the majority of posterior midgut epithelial cells being positive by 7 dpi. GFP foci were observed in one pair of salivary glands (1/15) dissected 14 dpi. Mice exposed to WNV-GFP–infected mosquitoes developed viremia, and GFP was detected in lymph node homogenates. These data demonstrate the effectiveness of our strategy to generate a replication competent construct with increased reporter gene stability that may be used to study early events in infection.
机译:我们报告的全长西尼罗河病毒(WNV)cDNA感染性克隆(ic)的建设和比较特征,其中包含融合在病毒开放阅读框中的绿色荧光蛋白(GFP)表达盒。源自WNV-GFP ic的病毒以与源自亲本(非GFP)ic的病毒相当的速率稳定感染了库蚊(Culex pipiens quinquefasciatus)蚊子。但是,插入此GFP盒会导致体内复制动力学的时间延迟,并显着降低向头部组织的传播。与以前报道的WNV感染的蚊子中肠一致,在感染后3天(dpi)观察到了局灶性GFP表达,大多数中肠后部上皮细胞在7 dpi时呈阳性。在一对14 dpi的唾液腺(1/15)中观察到GFP病灶。暴露于WNV-GFP感染的蚊子的小鼠发生病毒血症,并且在淋巴结匀浆中检测到GFP。这些数据证明了我们的策略产生具有增加的报告基因稳定性的复制能力构建体的有效性,该构建体可用于研究感染的早期事件。

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