Genome delivery to the proper cellular compartment for transcription and replication is a primary goal of viruses. However, methods for analyzing viral genome localization and differentiating genomes with high identity are lacking, making it difficult to investigate entry-related processes and co-examine heterogeneous RNA viral populations. Here, we present an RNA labeling approach for single-cell analysis of RNA viral replication and co-infection dynamics in situ, which uses the versatility of padlock probes. We applied this method to identify influenza A virus (IAV) infections in cells and lung tissue with single-nucleotide specificity and to classify entry and replication stages by gene segment localization. Extending the classification strategy to co-infections of IAVs with single-nucleotide variations, we found that the dependence on intracellular trafficking places a time restriction on secondary co-infections necessary for genome reassortment. Altogether, these data demonstrate how RNA viral genome labeling can help dissect entry and co-infections.

Influenza neuraminidase (NA) is a sialidase that contributes to viral mobility by removing the extracellular receptors for the haemagglutinin (HA) glycoprotein. However, it remains unclear why influenza NAs evolved to function as Ca2+-dependent tetramers that display variable stability. Here, we show that the Ca2+ ion located at the centre of the NA tetramer is a major stability determinant, as this Ca2+ ion is required for catalysis and its binding affinity varies between NAs. By examining NAs from 2009 pandemic-like H1N1 viruses, we traced the affinity variation to local substitutions that cause residues in the central Ca2+-binding pocket to reposition. A temporal analysis revealed that these local substitutions predictably alter the stability of the 2009 pandemic-like NAs and contribute to the tendency for the stability to vary up and down over time. In addition to the changes in stability, the structural plasticity of NA was also shown to support the formation of heterotetramers, which creates a mechanism for NA to obtain hybrid properties and propagate suboptimal mutants. Together, these results demonstrate how the structural restrictions for activity provide influenza NA with several mechanisms for adaptation and diversification.

N-linked glycans commonly contribute to secretory protein folding, sorting, and signaling. For enveloped viruses, such as the influenza A virus (IAV), large N-linked glycans can also be added to prevent access to epitopes on the surface antigens hemagglutinin (HA or H) and neuraminidase (NA or N). Sequence analysis showed that in the NA head domain of H1N1 IAVs, three N-linked glycosylation sites are conserved and that a fourth site is conserved in H3N2 IAVs. Variable sites are almost exclusive to H1N1 IAVs of human origin, where the number of head glycosylation sites first increased over time and then decreased with and after the introduction of the 2009 pandemic H1N1 IAV of Eurasian swine origin. In contrast, variable sites exist in H3N2 IAVs of human and swine origin, where the number of head glycosylation sites has mainly increased over time. Analysis of IAVs carrying N1 and N2 mutants demonstrated that the N-linked glycosylation sites on the NA head domain are required for efficient virion incorporation and replication in cells and eggs. It also revealed that N1 stability is more affected by the head domain glycans, suggesting N2 is more amenable to glycan additions. Together, these results indicate that in addition to antigenicity, N-linked glycosylation sites can alter NA enzymatic stability and the NA amount in virions.

Seasonal mass-vaccinations currently provide the best available defense against influenza. However, it currently takes a long time to prepare these vaccines and they have low efficacy. The vaccines are solely quantified by and mainly elicit an immune defense against hemagglutinin (HA). Several studies show that antibodies against neuraminidase (NA) provide additional protection against infection. Therefore, addition of NA has been proposed to improve the influenza vaccines. 

Unfortunately, the tetrameric NA easily disassociate during vaccine production. It is largely unknown which the main stabilizing factors are. Stabilized NA could be utilized to provide a better vaccine, and molecules able to destabilize NA could be potent antivirals.

Known stabilizing factors of proteins include N-linked glycosylation and disulfide bridges. In this work, using a knowledge-based bioinformatical approach, we observe that N-linked glycosylation is mainly conserved within but not between subtypes. Also, we see that the monomeric cysteine network is conserved, but with one additional disulfide bridge found in group 2 NAs. Finally, it’s noted that several residues are entirely conserved within subtypes and some even across several subtypes. These often uncategorized residues are assumed to be essential for viral fitness. Of extra interest is W296, a surface accessible tryptophan entirely conserved in most influenza serotypes.

This article identifies several essential conserved and/or stabilizing NA factors and residues, with the hope that this knowledge can provide a platform to produce more efficient vaccines and antivirals in the future.