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Expression of Factor X in BHK-21 Cells Promotes Low Pathogenic Influenza Viruses Replication

机译:BHK-21细胞中X因子的表达促进低致病性流感病毒复制

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摘要

A cDNA clone for factor 10 (FX) isolated from chicken embryo inserted into the mammalian cell expression vector pCDNA3.1 was transfected into the baby hamster kidney (BHK-21) cell line. The generated BHK-21 cells with inducible expression of FX were used to investigate the efficacy of the serine transmembrane protease to proteolytic activation of influenza virus hemagglutinin (HA) with monobasic cleavage site. Data showed that the BHK-21/FX stably expressed FX after ten serial passages. The cells could proteolytically cleave the HA of low pathogenic avian influenza virus at multiplicity of infection 0.01. Growth kinetics of the virus on BHK-21/FX, BHK-21, and MDCK cells were evaluated by titrations of virus particles in each culture supernatant. Efficient multicycle viral replication was markedly detected in the cell at subsequent passages. Virus titration demonstrated that BHK-21/FX cell supported high-titer growth of the virus in which the viral titer is comparable to the virus grown in BHK-21 or MDCK cells with TPCK-trypsin. The results indicate potential application for the BHK-21/FX in influenza virus replication procedure and related studies.
机译:从插入到哺乳动物细胞表达载体pCDNA3.1的鸡胚中分离的10因子(FX)cDNA克隆被转染到仓鼠肾(BHK-21)细胞系中。产生的具有可诱导的FX表达的BHK-21细胞用于研究丝氨酸跨膜蛋白酶对具有一元切割位点的流感病毒血凝素(HA)的蛋白水解激活的功效。数据显示,BHK-21 / FX经过十次连续传代后稳定表达了FX。这些细胞可以通过蛋白水解切割低致病性禽流感病毒在感染复数为0.01时的HA。通过滴定每种培养物上清液中的病毒颗粒来评估病毒在BHK-21 / FX,BHK-21和MDCK细胞上的生长动力学。在随后的传代中,在细胞中明显检测到有效的多周期病毒复制。病毒滴定表明BHK-21 / FX细胞支持病毒的高滴度生长,其中病毒滴度可与在带有TPCK-胰蛋白酶的BHK-21或MDCK细胞中生长的病毒相比。结果表明BHK-21 / FX在流感病毒复制程序和相关研究中的潜在应用。

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