Human Coronavirus 229E Papain-Like Proteases Have Overlapping Specificities but Distinct Functions in Viral Replication

Abstract

Expression of the exceptionally large RNA genomes of CoVs involves multiple regulatory mechanisms, including extensive proteolytic processing of the large replicase polyproteins, pp1a and pp1ab, by two types of cysteine proteases: the chymotrypsin-like main protease and papain-like accessory proteases (PL ^pro s). Here, we characterized the proteolytic processing of the human coronavirus 229E (HCoV-229E) amino-proximal pp1a/pp1ab region by two paralogous PL ^pro activities. Reverse-genetics data revealed that replacement of the PL2 ^pro active-site cysteine was lethal. By contrast, the PL1 ^pro activity proved to be dispensable for HCoV-229E virus replication, although reversion of the PL1 ^pro active-site substitution to the wild-type sequence after several passages in cell culture indicated that there was selection pressure to restore the PL1 ^pro activity. Further experiments showed that both PL1 ^pro and PL2 ^pro were able to cleave the nsp1-nsp2 cleavage site, with PL2 ^pro cleaving the site less efficiently. The PL1 ^pro -negative mutant genotype could be stably maintained in cell culture when the nsp1-nsp2 site was replaced by a short autoproteolytic sequence, suggesting that the major driving force for the observed reversion of the PL1 ^pro mutation was the requirement for efficient nsp1-nsp2 cleavage. The data suggest that the two HCoV-229E PL ^pro paralogs have overlapping substrate specificities but different functions in viral replication. Within the tightly controlled interplay of the two protease activities, PL2 ^pro plays a universal and essential proteolytic role that appears to be assisted by the PL1 ^pro paralog at specific sites. Functional and evolutionary implications of the differential amino-terminal polyprotein-processing pathways among the main CoV lineages are discussed.