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Furin cleavage of the SARS coronavirus spike glycoprotein enhances cell–cell fusion but does not affect virion entry

机译:SARS冠状病毒刺突糖蛋白的弗林蛋白酶切割增强细胞间融合但不影响病毒体进入

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摘要

The fusogenic potential of Class I viral envelope glycoproteins is activated by proteloytic cleavage of the precursor glycoprotein to generate the mature receptor-binding and transmembrane fusion subunits. Although the coronavirus (CoV) S glycoproteins share membership in this class of envelope glycoproteins, cleavage to generate the respective S1 and S2 subunits appears absent in a subset of CoV species, including that responsible for the severe acute respiratory syndrome (SARS). To determine whether proteolytic cleavage of the S glycoprotein might be important for the newly emerged SARS-CoV, we introduced a furin recognition site at single basic residues within the putative S1–S2 junctional region. We show that furin cleavage at the modified R667 position generates discrete S1 and S2 subunits and potentiates membrane fusion activity. This effect on the cell–cell fusion activity by the S glycoprotein is not, however, reflected in the infectivity of pseudotyped lentiviruses bearing the cleaved glycoprotein. The lack of effect of furin cleavage on virion infectivity mirrors that observed in the normally cleaved S glycoprotein of the murine coronavirus and highlights an additional level of complexity in coronavirus entry.
机译:I类病毒包膜糖蛋白的融合潜力可通过前体糖蛋白的蛋白质裂解来激活,以生成成熟的受体结合和跨膜融合亚基。尽管冠状病毒(CoV)S糖蛋白在此类包膜糖蛋白中共享成员身份,但在一部分CoV物种(包括造成严重急性呼吸系统综合症(SARS)的物种)中似乎没有产生相应的S1和S2亚基的裂解。为了确定S糖蛋白的蛋白水解切割对于新出现的SARS-CoV是否重要,我们在假定的S1-S2连接区域内的单个基本残基处引入了弗林蛋白酶识别位点。我们表明,在修饰的R667位置进行弗林蛋白酶切割可产生离散的S1和S2亚基,并增强膜融合活性。 S糖蛋白对细胞-细胞融合活性的这种影响并未反映在携带切割的糖蛋白的假型慢病毒的感染性上。弗林蛋白酶裂解对病毒体感染力缺乏影响,这在正常情况下在鼠冠状病毒中裂解的S糖蛋白中观察到,并突出了在冠状病毒进入过程中的复杂程度。

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