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Structures of Coxsackievirus A16 Capsids with Native Antigenicity: Implications for Particle Expansion, Receptor Binding, and Immunogenicity

  • Ren J
  • Wang X
  • Zhu L
  • et al.
Journal of Virology (2015) 89(20) 10500-10511
DOI: 10.1128/jvi.01102-15
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Abstract

Enterovirus 71 (EV71) and coxsackievirus A16 (CVA16) are the primary causes of the epidemics of hand-foot-and-mouth disease (HFMD) that affect more than a million children in China each year and lead to hundreds of deaths. Although there has been progress with vaccines for EV71, the development of a CVA16 vaccine has proved more challenging, and the EV71 vaccine does not give useful cross-protection, despite the capsid proteins of the two viruses sharing about 80% sequence identity. The structural details of the expanded forms of the capsids, which possess nonnative antigenicity, are now well understood, but high resolution information for the native antigenic form of CVA16 has been missing. Here, we remedy this with high resolution X-ray structures of both mature and natural empty CVA16 particles and also of empty recombinant viruslike particles of CVA16 produced in insect cells, a potential vaccine antigen. All three structures are unexpanded native particles and antigenically identical. The recombinant particles have recruited a lipid moiety to stabilize the native antigenic state that is different from the one used in a natural virus infection. As expected, the mature CVA16 virus is similar to EV71; however, structural and immunogenic comparisons highlight differences that may have implications for vaccine production. IMPORTANCE Hand-foot-and-mouth disease is a serious public health threat to children in Asian-Pacific countries, resulting in millions of cases. EV71 and CVA16 are the two dominant causative agents of the disease that, while usually mild, can cause severe neurological complications, leading to hundreds of deaths. EV71 vaccines do not provide protection against CVA16. A CVA16 vaccine or bivalent EV71/CVA16 vaccine is therefore urgently needed. We report atomic structures for the mature CVA16 virus, a natural empty particle, and a recombinant CVA16 virus-like particle that does not contain the viral genome. All three particles have similar structures and identical antigenicity. The recombinant particles, produced in insect cells (a system suitable for making vaccine antigen), are stabilized by recruiting from the insect cells a small molecule that is different from that used by the virus in a normal infection. We present structural and immunogenic comparisons with EV71 to facilitate structure-based drug design and vaccine development.

Figures

  • TABLE 1 Data collection and refinement statistics
  • FIG 1 Electron density maps, showing electron density in the pocket factor binding region of VP1 in the full particles (A), natural empty particles (B), and recombinant VLPs (C) after NCS real space averaging.
  • FIG 2 Overall structures. (A to C) Radius-colored surface representations of the mature CVA16, empty CVA16, and mature EV71 particles, respectively, cut away in panel A to highlight an individual protomer with proteins color coded as follows: VP1, blue; VP2, green; VP3, red; and VP4, yellow. (D) An enlarged protomer structure of the mature CVA16 as shown in panel A. The bound pocket factor in VP1 is drawn as magenta sticks. (E and F) Comparisons of the mature CVA16 protomer with those of empty CVA16 (E) and mature EV71 (F). Structural differences are mapped onto the protomer of the mature CVA16 virion; the thickness and color of the worm representation reflects the local deviation between the structures (from blue [ 0.5 Å] through green, to red [ 2.0 Å]). Regions missing in any particle are shown in red. The pocket factors are shown as gray sticks for empty CVA16 and mature EV71.
  • FIG 3 The structure of the particle inner surface. The N termini of VP1 and VP4 (blue and yellow ribbons, respectively) of mature CVA16 are compared with those (black) of empty CVA16 (A), expanded CVA16 (B), mature EV71 (C), and empty EV71 (D). VP1 (excluding the first 75 residues), VP2, and VP3 of mature CVA16 are shown as surface representations in pale blue, green, and red, respectively. Black arrows indicate where the N terminus of VP1 exits the capsid in the expanded 135S CVA16 (B) and the beginning of ordered structure in empty EV71 (D).
  • FIG 4 Comparison of the three CVA16 particle structures. (A to C) Protomer inner surfaces of the full, natural empty, and VLP particles, respectively, colored according to B factors (blue for the most rigid, through green, to red for the most flexible), showing that the internal structure of the VLP is more flexible than those of the full and empty natural particles and that more residues in the VP1 N terminus and VP4 are disordered (boxed area in panel C). (D) Ribbon diagram showing superimposed protomers of CVA16 full particle (colored as described in the legend to Fig. 2D) and VLP (gray). (E) Close-up view of the overlaid pocket factor binding sites in the full, natural empty, and VLP particles. For clarity, only the main chains of the full particle are shown as ribbons; the side chains are colored in blue, cyan, and gray and pocket factors in magenta, cyan, and gray for the full, empty, and VLP particles, respectively.
  • FIG 5 Structural differences around the VP1 pocket among enteroviruses. The structure of the mature CVA16 around the VP1 pocket is compared with those of empty CVA16 (A), EV71 (B), and poliovirus (C). The main chains are shown as ribbons, and the side chains as sticks with atom coloring. The mature CVA16 is colored as described in the legend to Fig. 2D, and the others in gray. Side chains of the mature CVA16 (A), EV71 (B), and poliovirus (C) are labeled. (D) Comparison of the positions of the bound pocket factors relative to residue Trp203 in CVA16 (blue), EV71 (orange), and poliovirus, bovine enterovirus 1, human rhinovirus 16, and swine vesicular disease virus (the latter four are in gray). (E) Sequence alignment of two VP1 regions of five enteroviruses. BEV2, bovine enterovirus 2.
  • FIG 6 Conserved surface areas between CVA16 and EV71. (A) Surface shape variations between CVA16 and EV71 (see Materials and Methods) are colored from blue ( 0.5 Å) to red ( 3.0 Å) on a pentamer of CVA16. (B) Amino acid conservation between CVA16 and EV71 is mapped onto the surface of a CVA16 pentamer by rainbow coloring based on a conservation score (from 0.0 to 4.0). Ten strains of both CVA16 and EV71 from different regions were selected, and a conservation score for each residue was calculated using CONSURF (63). Two large conserved areas are indicated by arrows. (C and D) Ribbon diagrams show a closeup view of the structures of the two conserved areas labeled 1 (C) and 2 (D) in panel B. The color scheme is as described in the legend to Fig. 2D, and the strands of the -sheet and loops are labeled according to convention.
  • FIG 7 Antigenic sites. Electrostatic surfaces of CVA16 (A) and EV71 (B) displayed on pentamers of the respective structures. These were calculated using PYMOL; red represents a negative charge and blue a positive charge ( 5 kT/e, where temperature [T] is equal to 298.15). (C and D) Epitopes of CVA16 (C) and EV71 (D). Surfaces of VP1, VP2, and VP3 are in pale blue, green, and red, respectively; epitopes are in bright colors.

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Ren, J., Wang, X., Zhu, L., Hu, Z., Gao, Q., Yang, P., … Stuart, D. I. (2015). Structures of Coxsackievirus A16 Capsids with Native Antigenicity: Implications for Particle Expansion, Receptor Binding, and Immunogenicity. Journal of Virology, 89(20), 10500–10511. https://doi.org/10.1128/jvi.01102-15

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