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Evaluation of Genetically Engineered Derivatives of a Chinese Strain of Foot-and-Mouth Disease Virus Reveals a Novel Cell-Binding Site Which Functions in Cell Culture and in Animals

机译:中国口蹄疫病毒株的基因工程衍生物的评估揭示了一种新型的细胞结合位点,在细胞培养和动物中发挥作用。

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摘要

Adaptation of field isolates of foot-and-mouth disease virus (FMDV) to grow in cells in culture can result in changes in viral properties that include acquisition of the ability to bind to cell surface heparan sulfate (HS). After 13 passages on BHK cells to produce a vaccine, a Cathay topotype isolate of FMDV serotype O from China (O/CHA/90) extended its cell culture host range and bound to heparin-Sepharose, although it did not require cell surface HS as a receptor molecule. To understand these phenomena, we constructed chimeric viruses by using a type A12 infectious cDNA and the capsid protein-coding regions of O/CHA/90 and its cell culture-adapted derivative (vac-O/CHA/90). Using a set of viruses derived from these chimeras by exchanging portions of the capsid-coding regions, we discovered that a group of amino acid residues that surround the fivefold axis of the icosahedral virion determine host range in cell culture and influence pathogenicity in pigs. These residues included aromatic amino acids at positions 108 and 174 and positively charged residues at positions 83 and 172 in protein 1D. To test if these residues participated in non-integrin-dependent cell binding, the integrin-binding RGD sequence in protein 1D was changed to KGE in two different chimeras. Evaluation of these KGE viruses indicated that growth in cell culture was not dependent on HS. One of these viruses was tested in pigs, where it produced a mild disease and maintained its KGE sequence. These results are discussed in terms of receptor utilization and pathogenesis of this important pathogen.
机译:口蹄疫病毒(FMDV)野外分离株适应培养中的细胞生长会导致病毒特性发生变化,包括获得与细胞表面硫酸乙酰肝素(HS)结合的能力。在BHK细胞上传代13次以生产疫苗后,来自中国的FMDV O型血清型国泰拓扑分离株(O / CHA / 90)扩展了其细胞培养宿主范围并与肝素-琼脂糖结合,尽管它不需要细胞表面HS作为受体分子。为了了解这些现象,我们通过使用A12型感染性cDNA和O / CHA / 90衣壳蛋白编码区及其适应细胞培养的衍生物(vac-O / CHA / 90)构建了嵌合病毒。使用通过交换衣壳编码区的部分衍生自这些嵌合体的病毒,我们发现围绕二十面体病毒体五倍轴的一组氨基酸残基决定了细胞培养中的宿主范围并影响猪的致病性。这些残基包括蛋白质1D中第108和174位的芳香族氨基酸和第83和172位带正电荷的残基。为了测试这些残基是否参与非整合素依赖性细胞结合,在两种不同的嵌合体中将蛋白质1D中的整合素结合RGD序列更改为KGE。对这些KGE病毒的评估表明,细胞培养物中的生长不依赖于HS。在猪中测试了其中一种病毒,在猪中产生了轻度疾病并保持了其KGE序列。根据该重要病原体的受体利用和发病机理讨论了这些结果。

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