Tuesday, August 20, 2019
Ebola Virus Mechanism of Infection
Ebola Virus Mechanism of Infection The Ebola virus (EBOV) is an enveloped, non-segmented, negative-strand RNA virus, whichà together with Marburg virus, makes up the filoviridae family. The virus causes severeà hemorrhagic fever associated with 50-90% human mortality1. Four species of the virus (Zaire,à Sudan, Cà ´te dââ¬â¢Ivoire, and Reston ebolavirus) have thus far been identified, with Zaire typicallyà associated with the highest human lethality2. A fifth EBOV species is confirmed in a 2007à outbreak in Bundibugyo, Uganda3,4. Infection with EBOV results in uncontrolled viralà replication and multiple organ failure with death occurring 6-9 days after onset ofà symptoms5. Fatal cases are associated with high viremia and defective immune responses,à while survival is associated with early and vigorous humoral and cellular immuneà responses6-9. Although preliminary vaccine trials in primates have been highlyà successful10-13, no vaccines, specific immunotherapeutics, or post-exposure treatments areà currently approved for human use. Since 1994, EBOV outbreaks have increased more thanà four-fold, thus necessitating the urgent development of vaccines and therapeutics for use in theà event of an intentional, accidental or natural EBOV release. The EBOV genome contains seven genes, which direct the synthesis of eight proteins. Transcriptional editing of the fourth gene (GP) results in expression of a 676-residue transmembrane-linked glycoprotein termed GP, as well as a 364-residue secreted glycoproteinà termed sGP14,15. EBOV GP is the main target for the design of vaccines and entry inhibitors. GP is post-translationally cleaved by furin16 to yield disulfide-linked GP1 and GP2à subunits17. GP1 effects attachment to host cells, while GP2 mediates fusion of viral and hostà membranes16,18-20. EBOV is thought to enter host cells through receptor-mediatedà endocytosis via clathrin-coated pits and caveolae21, followed by actin and microtubuledependentà transport to the endosome21, where GP is further processed by endosomalà cathepsins22-24. Essential cellular receptor(s) have not yet been identified, but DC-SIGN/LSIGN25,à hMGL26, à ²-integrins27, folate receptor-à ±28 and Tyro3 family receptors29 have allà been implicated as cellular factors in entry. Here, we report the crystal structure of EBOV GP,à at 3.4 Ã⦠resolution, in its trimeric, pre-fusion conformation in complex with neutralizingà antibody Fab KZ52. GP1 is responsible for cell surface attachment, which is probably mediated by a regionà including residues 54-20132. GP1 is composed of a single d omain (Ã¢Ë ¼65 Ã⦠Ãâ" 30 Ã⦠Ãâ" 30 Ãâ¦),arranged in the topology shown in Fig. 2a, and can be further subdivided into the (I) base, (II)à head and (III) glycan cap regions (Fig. 2a and Supplemental Fig. S3). The base (I) subdomainà is composed of two sets of à ² sheets, forming a semi-circular surface which clamps the internalà fusion loop and a helix of GP2 through hydrophobic interactions (Fig. 2b). Moreover, thisà subdomain contains Cys53, which is proposed to form an intermolecular disulfide bridge toà Cys609 of the GP2 subunit17. Cys53 resides near GP2 in the à ²2-à ²3 loop at the viral membraneproximalà end of the base subdomain (Fig. 2a-b). Our EBOV GP contains an intact GP1-GP2à disulfide bridge, based on reducing and non-reducing SDS-PAGE analysis. However, the region containing the counterpart GP2 cysteine is disordered, which may reflect functionallyà important mobility in the region. The head (II) is located between the base and glycan cap à regions towards the host membrane surface. Two intramolecular disulfide bonds stabilize theà head subdomain and confirm the biochemically determined disulfide bridge assignments17.à Cys108-Cys135 connects a surface-exposed loop (à ²8-à ²9 loop) to strand à ²7, while Cys121-Cys147 bridges the à ²8-à ²9 and à ²9-à ²10 loops (Fig. 2a). The glycan cap (III) contains fourà predicted N-linked glycans (at N228, N238, N257 and N268) in an à ±/à ² dome over the GP1à head subdomain (Fig. 1b and 2a). This subdomain does not form any monomer-monomerà contacts and is fully exposed on the upper and outer surface of the chalice. The central à ² sheetsà from the head and glycan cap together form a fairly flat surface and, in the context of the GPà trimer, form the three inner sides of the chalice bowl. Ebola virus GP2 GP2 is responsible for fusion of viral and host cell membranes and contains the internal fusionà loop and the heptad repeat regions, HR1 and HR2. Many viral glycoproteins have fusionà peptides, located at the N terminus of their fusion subunit, which are released upon cleavageà of the precursor glycoprotein. By contrast, class II and class III fusion proteins, as well as classà I glycoproteins from Ebola, Marburg, Lassa and avian sarcoma leukosis viruses, containà internal fusion loops lacking a free N terminus. The crystal structure reveals that the EBOVà GP internal fusion loop, which encompasses residues 511-556, utilizes an antiparallel à ²Ã stranded scaffold to display a partially helical hydrophobic fusion peptide (L529, W531, I532,à P533, Y534 and F535) (Fig. 2c). The side chains of these hydrophobic residues pack into aà region on the GP1 head of a neighboring subunit in the trimer, reminiscent of the fusion peptideà packing in the pre-fusion parainfluenz a virus 5 F structure33. A disulfide bond between Cys511à at the base of à ²19 and Cys556 in the HR1 helix covalently links the antiparallel à ² sheet. Thisà disulfide bond between the internal fusion loop and HR1 is conserved among all filoviruses,à and is analogous to a pair of critical cysteines flanking the internal fusion loop in avian sarcomaà leukosis virus34,35. Interestingly, the EBOV internal fusion loop has features more similar toà those observed in class II and III viral glycoproteins (in particular to flaviviruses) than thoseà previously observed for class I glycoproteins (Supplemental Fig. S4). It thus appears thatà regardless of viral protein class, internal fusion loops share a common architecture for theirà fusion function. EBOV GP2 contains two heptad repeat regions (HR1 and HR2), connected by a 25-residueà linker containing a CX6CC motif and the internal fusion loop. The crystal structures of postfusionà GP2 fragments30,31 have revealed that the two heptad repeat regions form antiparallelà à ± helices and that a CX6CC motif forms an intrasubunit disulfide bond between Cys601 andà Cys608 (Supplemental Fig. S5). In the pre-fusion EBOV GP, HR2 and the CX6CC motif areà disordered. By contrast, the HR1 region is well ordered and can be divided into four segments:à HR1A, HR1B, HR1C and HR1D (Fig. 2c), which together assemble the cradle encircling GP1. Similarly, heptad repeat regions in influenza and parainfluenza viruses also contain multipleà segments in their pre-fusion helices that substantially rearrange in their post-fusionà conformations33,36,37. The first two segments, HR1A and HR1B (residues 554-575), together form an à ± helix with anÃ Ã¢Ë ¼40à ° kink at T565, which delineates HR1A from HR1B. Interestingly, the bend betweenà HR1A and HR1B contains an unusual 3-4-4-3 stutter, which may act as a conformationalà switch31, rather than the typical 3-4 periodicity of heptad repeats (Supplemental Fig. S6). Aà similar stutter has also been noted in parainfluenza virus 5 F33. The Ebola virus HR1C (residuesà 576-582) forms an extended coil linking HR1B to the 14-residue à ± helix of HR1D (residuesà 583-598). HR1D forms an amphipathic helix and the hydrophobic faces of each HR1D join toà form a three-helix bundle at the trimer interface. Although the breakpoint maps directly to aà Lee et al. Page 3 Nature. Author manuscript; available in PMC 2009 June 22. NIH-PA Author Manuscript NIH-PA Author Manuscript NIH-PA Author Manuscriptà chloride ion binding site in the post-fusion conformation of GP230,31 and at least two otherà viruses38,39, no chloride ion is observed here as HR1 and HR2 do not come together to formà the six-helix bundle. Instead, the pre-fusion GP2 adopts a novel conformation, intimatelyà curled around GP1 (Fig. 1c). Ebola virus GP-KZ52 interface KZ52 is an antibody isolated from a human survivor of a 1995 outbreak in Kikwit, Democraticà Republic of the Congo (formerly Zaire)40. This antibody neutralizes Zaire ebolavirus inà vitro40 and offers protection from lethal EBOV challenge in rodent models41, but has minimalà effects on viral pathogenicity in non-human primates42. KZ52 is directed towards a vulnerable,à non-glycosylated epitope at the base of the GP chalice, where it engages three discontinuousà segments of EBOV GP: residues 42-43 at the N terminus of GP1, and 505-514 and 549-556à at the N terminus of GP2 (Fig. 3 and Supplemental Fig. S7). Although the majority of the GPà surface buried by KZ52 belongs to GP2, the presence of both GP1 and GP2 are critical forà KZ52 recognition43. It is likely that GP1 is required to maintain the proper pre-fusionà conformation of GP2 for KZ52 binding. Indeed, KZ52 is the only antibody known to bridgeà both attachment (GP1) and fusion (GP2) subunits of any viral gly coprotein. Given that KZ52à requires a conformational epitope seen only in the GP2 pre-fusion conformation and that theà KZ52 epitope is distant from the putative receptor-binding site (RBS), KZ52 likely neutralizesà by preventing rearrangement of the GP2 HR1A/HR1B segments and blocking host membraneà insertion of the internal fusion loop. Alternatively, IgG KZ52 may sterically hinder access toà the RBS or to a separate binding site of another cellular factor, especially if multiple attachmentà events are required for entry. The KZ52 epitope of GP is convex and does not have a high shape complementarity to theà antibody (Sc index of 0.63), although Ã¢Ë ¼1600 Ãâ¦2 of each GP monomer are occluded upon KZ52à binding. The antibody contacts a total of 15 GP residues by van der Waals interactions and 8à direct hydrogen bonds (Supplemental Fig. S7). Ten out of 15 residues in the structurally definedà KZ52 epitope are unique to Zaire ebolavirus (Supplemental Fig. S6), thus explaining the Zaireà specificity of KZ52. Ebola virus GP glycosylation We generated a fully glycosylated molecular model of EBOV GP to illustrate the native GPà trimer as it exists on the viral surface (Fig. 4). The majority of N-linked glycosylation sites areà concentrated in the mucin-like domain and glycan cap of GP1. Given that the mucin-likeà domain is Ã¢Ë ¼75 kDa in mass (protein and oligosaccharide), the volume of this domain isà predicted to be similar to each GP monomer observed here. The crystal structure suggests thatà the mucin-like domain is linked to the side of each monomer and may further build up the wallsà of the chalice, forming a deeper bowl (Fig. 4). Although a mixture of complex, oligomannoseà and hybrid-type glycans are found on intact, mucin-containing GP144, those glycans outsideà the mucin-like domain are likely to be complex in nature: the mucin-deleted GP used forà crystallization is sensitive to PNGaseF, but not to EndoH treatment (Supplemental Fig. S8).à Modeling of complex-type oligosaccharides on the EBOV GP indicates that the majority ofà the GP trimer is cloaked by a thick layer of oligosaccharide, even without the mucin-likeà domain (Fig. 4). The Ã¢Ë ¼19 additional oligosaccharides on the full-length GP (17 on the mucinlikeà domain and 2 more on GP1, disordered here) further conceal the sides and top of theà chalice. The KZ52 binding site and, presumably, the flexible regions of HR2 and theà membrane-proximal external region (MPER) remain exposed and perhaps vulnerable toà binding of antibodies and inhibitors. Lee The development of neutralizing antibodies is limited in natural Ebola virus infection. Manyà survivors have low or insignificant titres1,7, and those antibodies that are elicited preferentiallyà recognize a secreted version of the viral glycoprotein that features an alternate quaternaryà structure and lacks the mucin-like domain43. The glycocalyx surrounding EBOV GP likelyà forms a shield that protects it from humoral immune responses and/or confers stability insideor outside a host. The mucin-like domain and glycan cap sit together as an external domain toà the viral attachment and fusion subunits, reminiscent of the glycan shields of HIV-1à gp12045,46à and Epstein-Barr virus gp35047, perhaps pointing to a common theme for immuneà evasion. Alignment of filoviral sequences indicate that regions involved in immune evasionà have a low degree of sequence conservation [i.e. GP1 glycan cap (Ã¢Ë ¼5%) and mucin-like domainà (0%)], but the N-glycosylation sites in the glycan cap are mostly conserved among all EBOVà subtypes (Supplemental Fig. S6), indicating the functional importance of these posttranslationalà modifications. Sites of receptor binding and cathepsin cleavage Although a definitive receptor for EBOV remains to be identified, previous studies32,48,49à have determined that residues 54-201, which map to the base and head subdomains of GP1,à form a putative receptor-binding site (RBS) for attachment to host cells. Additionalà experimental studies have identified at least 19 GP1 residues, assigned into four groups basedà on the location in the structure, that are critical for viral entry48-50 (Fig. 5). Many of theseà residues are apolar or aromatic and are involved in maintaining the structural integrity of GP1à for receptor binding or fusion. However, six residues (K114, K115, K140, G143, P146 andà C147) cluster within a Ã¢Ë ¼20 Ãâ" 15 Ã⦠surface in the inner bowl of the chalice and may thusà represent important receptor contact sites. All residues in the putative RBS are highly conservedà among Ebola virus species (Supplemental Fig. S6). Importantly, this putative RBS is recessed beneath the glycan cap and perhaps further maskedà by the mucin-like domain (Fig. 4), suggesting that additional conformational change or removalof the mucin-like domain could reveal additional surfaces required for receptor or cofactorà binding. It has been demonstrated that endosomal proteolysis of EBOV GP by cathepsin Là and/or B removes the mucin-like domain to produce a stable Ã¢Ë ¼18 kDa GP1 intermediate whichà has enhanced viral binding and infectivity22-24. The precise site of cathepsin cleavage isà unknown and the role of cathepsins in natural infection is as yet unclear. However, formationà of an Ã¢Ë ¼18 kDa GP1 fragment implies that cathepsin may cleave near the GP1 à ²13-à ²14 loopà (residues 190-213). Indeed, this loop is unresolved in the pre-fusion structure, suggestingà enhanced mobility and accessibility to enzymatic cleavage. Cleavage within this loop wouldà remove the entire mucin-like domain and glyc an cap region (Fig. 5). As a result, à ²7 to à ²9à strands and their associated loops would become exposed. These regions of GP are in proximityà to the previously identified residues critical for viral entry. The fold, location andà physicochemical properties of this site should now provide new leads in the search for theà elusive filoviral receptor(s). A summary of the Ebola virus mechanism of infection, including the events of cathepsinà cleavage and conformational changes to GP2 during fusion, is presented.
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