Virology tidbits

Virology tidbits

Friday 8 August 2014

Coronavirus structural proteins and ER stress

The accumulation of viral proteins at the ER during an infection can induce ER stress as outlined before via three main pathways, PERK, ATF6, and IRE1, which are commonly refereed to as the unfolded Protein Response (UPR) or ER stress response. This response results in the transcriptional activation of genes encoding for ER chaperones, increasing autophagy, or regulating apoptosis.
Coronaviruses are no exception. Both structural and non-structural proteins localise to the ER - followed by the formation of Replication Transcription Centers in the case of non-structural proteins or the co-localisation in ER-Golgi Intermediate Compartments (ERGIC), the sites of viral genome replication and assembly respectively.

Prototype Coronavirus particle


                                                    S (Spike) protein

The Coronavirus S protein plays a pivotal role in the entry of the Coronavirus particle, by mediating receptor binding, membrane fusion as well as eliciting the formation of neutralising antibodies. newly synthesised S protein co-localises with the other structural proteins in the ERGIC where viral assembly takes place. Although the viral assembly site is distinct from the ER, newly synthesised S protein localises to the ER where the protein is slowly folded and glycosylated prior release into the cytoplasm of the cell where it is retained in the ERGIC by a dilysine signal (in the case of IBV S) or a dibasic signal (KXHXX) (SARS-CoV S, TGEV S); interestingly, the S proteins of BCV and MHV-A59 both do not contain similar localisation signals. These signals not only localise S to the ERGIC, but also retain S protein in the cytoplasm instead of being localised to the plasma membrane.
Since the S is glycosylated and localises to the ER, the viral S protein modulates the ER stress response. As it the case with the viral E, HCOV-Nl63 orf3, and SARS-CoV orf3a proteins, S activates PERK, but not ATF6 and IRE1. Similar to these proteins, the expression of S results in PERK and phosphorylated eIF2α induced transcriptional activation of intraluminal ER chaperones GRP94/78, thus facilitating the correct folding and processing of viral proteins inside the ER. Indeed, the expression of S does not induce CHOP, nor ATF4 or splicing of XBP1, although in SARS-CoV slightly elevated levels of sXBP1 can be detected (independent of S). If the latter is required for viral replication since sXBP1 has also chaperone activity or not is not clear.

                                              M (Membrane protein)

The Coronavirus M is the main structural component of the virion, its function associated not only with incorporating the nascent nucleocapsid via interaction with the viral N protein into the viral particle but also recruiting other viral  structural components to the site of viral assembly. Although the precise topology of the M protein is still disputed, the consensus is that the three putative transmembrane domains predominantly localise in the Golgi, as well as in trafficking vesicles, with the N and C termini are either in a Nexo//Cexo  or Nexo/Cendo orientation (exo referring to ectodomain, endo to endodomain). In the case of SARS-CoV M, the protein is N-Glycosylated on the N-terminal ectodomain prior to insertion into the ERGIC at the ER, with the glycosylation site facing the ER lumen and thus favoring a Nexo-Cendo orientation. Consequently, the highly immunogenic C terminus is located inside the mature virus particle with the less immunogenic N terminus protruding from the viral surface. This is different from Transmissible Gastroenteritis Virus (TGEV) and the feline Coronavirus (FCoV),  where the M protein adopts not only a Nexo-Cendo orientation but also a Nexo - Cexo configuration with the N- and C-terminus both protruding the viral particle and thus exposing the C-terminus; indeed, TGEV and FCoV infection induces the formation of highly specific antibodies targeting the viral M protein. The Nexo-Cendo orientation not only prevents the formation of antibodies against M but also is also required for the interaction with the N protein and subsequent recruitment of the viral positive sense ssRNA to sites of viral assembly. Indeed, in TGEV virions we find both conformations of M, with the Nexo-Cendo conformation being predominant. 


Membrane topology of M proteins derived from SARS-CoV and TGEV



Although the N-glycosylation of SARS-CoV M and the O-glycosylation of MHV M are dispensable for viral assembly -glycosylation mutants do recruit both the viral S and N proteins to the ERGIC-, budding, and infectivity, the N-glycosylation of M might be required to induce antiviral signaling, specifically the induction of Interferon-α and -β.
Since the Coronaviral M protein is localised to the ER prior to be transported to the ERGIC and glycosylated by ER resident enzymes, it might be conceivable to assume that the expression of M induces the ER stress response by lipid depletion. So far, however the induction of the UPR has not been reported.


                                              E (Envelope)

In addition to the M protein, the coronaviral E protein is also involved in the formation of viral and virus-like particles and as such localises to the ERGIC, the viral assembly site located in close proximity to the ER and Golgi. Indeed if transfected into cells,  the SARS-CoV and PEDV E protein E can be detected both in the ER and the Golgi, although not in a reticulate pattern but in membrane clusters. In contrast to the viral M or the SARS-CoV orf3a protein, both the N- and C-Termini of SARS-CoV E are located on the cytoplasmic side with no lumenal domain, although tin the case for IBV E a different topology has been reported. In the case of SARS-CoV E protein, this transmembrane helical hairpin domain might not only be responsible for the membrane curvature of the viral particle but is also palmitoylated. In contrast to the M protein, the E protein from both SARS-CoV and PEDV have been shown to interfere with the ER stress response, albeit the results are contradictory. In the case of SARS-CoV, the expression of the E protein inhibits the IRE1 pathway but PERK or ATF6 mediated signalling and thus inhibits apoptosis induced by IRE1 activation in cells infected with a recombinant SARS-CoVΔE virus or RSV, as well as in cells treated with thapsigargin or tunicamycin.  On the other hand, both the expression of SARS-CoV and PDEV E activates PERK and PERK mediated expression of pro inflammatory cytokines such as Interleukin-8 by activating NF-κB as well as inducing the expression of Bcl2 and thus preventing apoptosis. Indeed cells infected with rSARS-CoVΔE not only have an increased stress response but also exhibit a decreased inflammatory response - yet rSARS-CoVΔE is attenuated.


Membrane topology of Coronavirus E proteins derived from SARS-CoV, MHV, and IBV



                          SARS-CoV orf3a/HCoV-NL63 orf3

The SARS-CoV open reading frame (orf) 3a protein is encoded by one of the so called “group specific genes” and has no known structural nor sequence homology to any of the known proteins of other coronaviruses, although it bears some similarities to the Coronavirus M protein. Similar to the M protein, orf3a has three transmembrane domains with the same topology as SARS-CoV M, it localizes predominately to the Golgi and ERGIC, both are structural proteins, both are glycosylated, and both interact with the viral S and E proteins. In contrast to M, the three transmembrane domains have been postulated to form an ion channel with the domain 2 and 3 forming the pore via a cysteine rich domain (AA 81-60) and the central region (AA 125-200) be required for binding the 5’-UTR of the SARS-CoV genome. Although both orf3a and M are glycosylated, orf3a is O-glycosylated postranslationally similar to MHV M whereas SARS-CoV M is N-Glycosylated cotranslationally.
The C-terminus contains both the Yxx𝛟 (with x representing any AA and 𝚽 is a hydrophobic amino acid residue) and the diacidic motifs (ExD, where x represents any AA). Whilst the Yxx𝛟 domain is required for the localisation of the viral particle to the endosome during viral entry, the diacidic motif is required for the export from the ER to the ERGIC/Golgi as well as preventing the retrograde Rab6GTPase dependent transport from the Golgi to the ER, thus facilitating the accumulation of orf3a at the plasma membrane. As mentioned in a previous post, the expression of orf3a has been associated with the induction of the ER stress response through the activation of the PERK pathway but does not trigger the activation of IRE1 or ATF6 nor the Endoplasmic Reticulum Associated Degradation (ERAD) pathway. Constitutive activation of PERK by orf3a induces apoptosis through the expression of ATF4 and CHOP as described before as well as activating p38 MAPK mediated release of mitochondrial Cytochrome c.


SARS-CoV orf3a and HCoV-NL63 orf3



In a similar way to SARS-CoV orf3a, the HCoV-NL63 orf 3 protein co-localises with the viral S, M, E, and N proteins within the ERGIC compartment in Huh7 cells transfected with the respective expression plasmids. In addition, HCoV-NL63 is N-glycosylated at the ER luminal side. If the expression of HCoV-NL63 induces the ER stress response however is not known, but the author of these lines would predict that akin to SARS-CoV orf 3a, HCoV-NL63 orf3 induces the PERK pathway.


                                        N (Nucleocapsid)
In contrast to the aforementioned proteins, the Nucleocapsid protein does not integrate into the membrane of either the virion, the ER, or the ERGIC due to the absence of a transmembrane domain but binds both the M and E protein (in addition to nsp3) and  in cells infected with CoV or co-transfected with either M and E respectively, although N is not required for the formation of virus like particles. Mass spectrometric characterisation of the SARS-CoV revealed 12 potential glycosylation sites were identified, suggesting that N is N-glycosylated within the ER co- or postranslationally. Based on these findings is seems possible that the expression of N induces a ER stress response although the N protein itself does not predominantly localise to the ER but both within the cytoplasm and as well as the nucleolus in infected cells and cells transfected with IBV, MHV, SARS-CoV, and TGEV N. An exception might be however the PEDV (Porcine Epidemic Diarrhoea Virus) N protein, which seems to localise to the ER (according to the authors at least) -I should note that I however  profoundly disagree with the authors of the paper in question about since from the published figures seems to be absent from the region labeled with ER tracker. In any case, the published data suggest that PEDV N might activate NF-κB signalling in a similar way to HCoV-OC43 via binding to microRNA9 instead. In my opinion, it is the glycosylation of N, which might induce the ER stress pathway instead as indicated by unregulated expression of GRP78, a ER chaperone - a hypothesis that could and should have been tested by mutating the putative glycosylation sites. In infected cells, the viral nsp-3 protein binds N and thus localises N to the replication complex, as does binding of N to non-glycosylated M. In these cases however, it is not N itself which would cause ER stress, but the respective binding partner, although it might be possible that N excaberates ER stress. The SARS-CoV N protein itself however localises to stress granules upon arsenite treatment which can be inhibited by phosphorylation of a Serine residue via SR protein kinase 1in the C-terminal domain, maybe similar to PEDV N. Indeed, mutating this Serine residue to Alanine stabilises the formation of N containing stress granules. So in the end, it is not clear if the glycosylation of N induces the ER stress response  but there is strong evidence that the C-terminal domain is involved in inducing the ER stress response via the formation of protein aggregates in HeLa cells treated with arsenite.

Interestingly, the author of this post did some research in the past where preliminary data suggested that B23 remains nucleolar in the presence of IBV N in contrast to a nucleolar and perinuclear distribution in mock-transfected cells. If this is the case indeed, this could explain how IBV N might interfere with the ER stress response.

B23 in Vero cells transfected with backbone vector (top) or IBV-N (bottom)




So what is final conclusion? The expression of coronaviral structural proteins certainly interferes with the ER stress, but the general pattern is, that this interference is limited to the PERK pathway and does not involve the ATF6 or IRE1 response, thus preventing CHOP mediated apoptosis. If genes related to autophagy are induced remains to be seen; if so, then this might provide a mechanism to evade apoptosis.



Activation of PERK during Coronavirus infection by the structural proteins



ResearchBlogging.org






Further reading

Fung TS, & Liu DX (2014). Coronavirus infection, ER stress, apoptosis and innate immunity. Frontiers in microbiology, 5 PMID: 24987391


Liu DX, Fung TS, Chong KK, Shukla A, & Hilgenfeld R (2014). Accessory proteins of SARS-CoV and other coronaviruses. Antiviral research, 109C, 97-109 PMID: 24995382


Nal B, Chan C, Kien F, Siu L, Tse J, Chu K, Kam J, Staropoli I, Crescenzo-Chaigne B, Escriou N, van der Werf S, Yuen KY, & Altmeyer R (2005). Differential maturation and subcellular localization of severe acute respiratory syndrome coronavirus surface proteins S, M and E. The Journal of general virology, 86 (Pt 5), 1423-34 PMID: 15831954


Lontok E, Corse E, & Machamer CE (2004). Intracellular targeting signals contribute to localization of coronavirus spike proteins near the virus assembly site. Journal of virology, 78 (11), 5913-22 PMID: 15140989


Chan CP, Siu KL, Chin KT, Yuen KY, Zheng B, & Jin DY (2006). Modulation of the unfolded protein response by the severe acute respiratory syndrome coronavirus spike protein. Journal of virology, 80 (18), 9279-87 PMID: 16940539


Versteeg GA, van de Nes PS, Bredenbeek PJ, & Spaan WJ (2007). The coronavirus spike protein induces endoplasmic reticulum stress and upregulation of intracellular chemokine mRNA concentrations. Journal of virology, 81 (20), 10981-90 PMID: 17670839


Chang YJ, Liu CY, Chiang BL, Chao YC, & Chen CC (2004). Induction of IL-8 release in lung cells via activator protein-1 by recombinant baculovirus displaying severe acute respiratory syndrome-coronavirus spike proteins: identification of two functional regions. Journal of immunology (Baltimore, Md. : 1950), 173 (12), 7602-14 PMID: 15585888


de Haan CA, de Wit M, Kuo L, Montalto-Morrison C, Haagmans BL, Weiss SR, Masters PS, & Rottier PJ (2003). The glycosylation status of the murine hepatitis coronavirus M protein affects the interferogenic capacity of the virus in vitro and its ability to replicate in the liver but not the brain. Virology, 312 (2), 395-406 PMID: 12919744


 Risco C, Antón IM, Suñé C, Pedregosa AM, Martín-Alonso JM, Parra F, Carrascosa JL, & Enjuanes L (1995). Membrane protein molecules of transmissible gastroenteritis coronavirus also expose the carboxy-terminal region on the external surface of the virion. Journal of virology, 69 (9), 5269-77 PMID: 7636969


Voss D, Pfefferle S, Drosten C, Stevermann L, Traggiai E, Lanzavecchia A, & Becker S (2009). Studies on membrane topology, N-glycosylation and functionality of SARS-CoV membrane protein. Virology journal, 6 PMID: 19534833


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Minakshi R, Padhan K, Rani M, Khan N, Ahmad F, & Jameel S (2009). The SARS Coronavirus 3a protein causes endoplasmic reticulum stress and induces ligand-independent downregulation of the type 1 interferon receptor. PloS one, 4 (12) PMID: 20020050


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Nishimura N, & Balch WE (1997). A di-acidic signal required for selective export from the endoplasmic reticulum. Science (New York, N.Y.), 277 (5325), 556-8 PMID: 9228004


Müller MA, van der Hoek L, Voss D, Bader O, Lehmann D, Schulz AR, Kallies S, Suliman T, Fielding BC, Drosten C, & Niedrig M (2010). Human coronavirus NL63 open reading frame 3 encodes a virion-incorporated N-glycosylated membrane protein. Virology journal, 7 PMID: 20078868


Yang Y, Zhang L, Geng H, Deng Y, Huang B, Guo Y, Zhao Z, & Tan W (2013). The structural and accessory proteins M, ORF 4a, ORF 4b, and ORF 5 of Middle East respiratory syndrome coronavirus (MERS-CoV) are potent interferon antagonists. Protein & cell, 4 (12), 951-61 PMID: 24318862


Yuan Q, Liao Y, Torres J, Tam JP, & Liu DX (2006). Biochemical evidence for the presence of mixed membrane topologies of the severe acute respiratory syndrome coronavirus envelope protein expressed in mammalian cells. FEBS letters, 580 (13), 3192-200 PMID: 16684538


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DeDiego ML, Nieto-Torres JL, Jiménez-Guardeño JM, Regla-Nava JA, Alvarez E, Oliveros JC, Zhao J, Fett C, Perlman S, & Enjuanes L (2011). Severe acute respiratory syndrome coronavirus envelope protein regulates cell stress response and apoptosis. PLoS pathogens, 7 (10) PMID: 22028656


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