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与在非洲绿猴肾细胞中繁殖的登革病毒相比,在人胚肺成纤维细胞中繁殖的登革病毒具有更高的遗传稳定性。

High genetic stability of dengue virus propagated in MRC-5 cells as compared to the virus propagated in vero cells.

作者信息

Liu Chia-Chyi, Lee Shiang-Chi, Butler Michael, Wu Suh-Chin

机构信息

Institute of Biotechnology, Department of Life Science, National Tsing Hua University, Hsinchu, Taiwan.

出版信息

PLoS One. 2008 Mar 19;3(3):e1810. doi: 10.1371/journal.pone.0001810.

Abstract

This work investigated the replication kinetics of the four dengue virus serotypes (DEN-1 to DEN-4), including dengue virus type 4 (DEN-4) recovered from an infectious cDNA clone, in Vero cells and in MRC-5 cells grown on Cytodex 1 microcarriers. DEN-1 strain Hawaii, DEN-2 strain NGC, DEN-3 strain H-87, and DEN-4 strain H-241 , and DEN-4 strain 814669 derived from cloned DNA, were used to infect Vero cells and MRC-5 cells grown in serum-free or serum-containing microcarrier cultures. Serum-free and serum-containing cultures were found to yield comparable titers of these viruses. The cloned DNA-derived DEN-4 started genetically more homogeneous was used to investigate the genetic stability of the virus propagated in Vero cells and MRC-5 cells. Sequence analysis revealed that the DEN-4 propagated in MRC-5 cells maintained a high genetic stability, compared to the virus propagated in Vero cells. Amino acid substitutions of Gly(104)Cys and Phe(108)Ile were detected at 70%, 60%, respectively, in the envelope (E) protein of DEN-4 propagated in Vero cells, whereas a single mutation of Glu(345)Lys was detected at 50% in E of the virus propagated in MRC-5 cells. Sequencing of multiple clones of three separate DNA fragments spanning 40% of the genome also indicated that DEN-4 propagated in Vero cells contained a higher number of mutations than the virus growing in MRC-5 cells. Although Vero cells yielded a peak virus titer approximately 1 to 17 folds higher than MRC-5 cells, cloned DEN-4 from MRC-5 cells maintained a greater stability than the virus from Vero cells. Serum-free microcarrier cultures of MRC-5 cells offer a potentially valuable system for the large-scale production of live-attenuated DEN vaccines.

摘要

本研究调查了四种登革病毒血清型(DEN-1至DEN-4),包括从感染性cDNA克隆中获得的登革病毒4型(DEN-4),在Vero细胞以及在Cytodex 1微载体上生长的MRC-5细胞中的复制动力学。使用DEN-1夏威夷株、DEN-2 NGC株、DEN-3 H-87株、DEN-4 H-241株以及源自克隆DNA的DEN-4 814669株,感染在无血清或含血清微载体培养物中生长的Vero细胞和MRC-5细胞。发现无血清和含血清培养物产生的这些病毒滴度相当。源自克隆DNA的DEN-4起始时基因更均一,被用于研究在Vero细胞和MRC-5细胞中增殖的病毒的遗传稳定性。序列分析显示,与在Vero细胞中增殖的病毒相比,在MRC-5细胞中增殖的DEN-4保持了较高的遗传稳定性。在Vero细胞中增殖的DEN-4包膜(E)蛋白中,分别有70%和60%检测到Gly(104)Cys和Phe(108)Ile的氨基酸替换,而在MRC-5细胞中增殖的病毒的E蛋白中,有50%检测到Glu(345)Lys的单一突变。对跨越基因组40%的三个独立DNA片段的多个克隆进行测序也表明,在Vero细胞中增殖的DEN-4比在MRC-5细胞中生长的病毒含有更多的突变。尽管Vero细胞产生的病毒滴度峰值比MRC-5细胞高约1至17倍,但来自MRC-5细胞的克隆DEN-4比来自Vero细胞的病毒保持了更高的稳定性。MRC-5细胞的无血清微载体培养为减毒活DEN疫苗的大规模生产提供了一个潜在有价值的系统。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2195/2265545/9d7bf9b284ac/pone.0001810.g001.jpg

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