Structural Characterization of the Crimean-Congo Hemorrhagic Fever Virus Gn Tail Provides Insight into Virus Assembly*

The RNA virus that causes the Crimean Congo Hemorrhagic Fever (CCHF) is a tick-borne pathogen of the Nairovirus genus, family Bunyaviridae. Unlike many zoonotic viruses that are only passed between animals and humans, the CCHF virus can also be transmitted from human to human with an overall mortality rate approaching 30%. Currently, there are no atomic structures for any CCHF virus proteins or for any Nairovirus proteins. A critical component of the virus is the envelope Gn glycoprotein, which contains a C-terminal cytoplasmic tail. In other Bunyaviridae viruses, the Gn tail has been implicated in host-pathogen interaction and viral assembly. Here we report the NMR structure of the CCHF virus Gn cytoplasmic tail, residues 729–805. The structure contains a pair of tightly arranged dual ββα zinc fingers similar to those found in the Hantavirus genus, with which it shares about 12% sequence identity. Unlike Hantavirus zinc fingers, however, the CCHF virus zinc fingers bind viral RNA and contain contiguous clusters of conserved surface electrostatics. Our results provide insight into a likely role of the CCHF virus Gn zinc fingers in Nairovirus assembly.

Recent outbreaks of the Crimean Congo Hemorrhagic Fever (CCHF) 2 virus along with the reported ability of the virus to transfer between humans have raised concerns of a widespread pandemic (1). The virus is transmitted to humans by tick bite or by direct handling of infected animal meat or blood (1,2). Infection causes a hemorrhagic fever and myalgia resulting in mortality rates approaching 30% (1)(2)(3). The virus contains an antisense RNA genome divided into three segments, and named according to lengths as the S, M, and L (for Small, Medium, and Large) segments (4). The viral proteins are the nucleocapsid protein, two membrane glycoproteins Gn and Gc (also referred to as G1 and G2 in other Bunyaviridae) (5, 6), a nonstructural protein (NSm) (7), and an RNA polymerase (4). In the mature virion, the Gn glycoprotein contains a 176 residue ectodomain followed by a 24 residue transmembrane region and terminates in a long cytoplasmic tail consisting of ϳ100 residues (5,7).
Recent results from other related Bunyaviridae viruses suggest the role of the Gn tail in viral assembly. For example, alanine mutagenesis of the cytoplasmic tails of Uukuniemi virus (genus Phlebovirus) (8) and Bunyamwera virus (genus Orthobunyavirus) (9) affect the ability of virus-like particles (VLPs) to effectively incorporate ribonucleoproteins, thus intimating a role for Gn tails in genome packaging. More recently, the Gn tail of Puumala virus (genus Hantavirus) was shown to co-immunoprecipitate with the Puumala nucleocapsid protein (10). These results suggest that the CCHF virus Gn tail plays an equally important role in viral assembly of genus Nairovirus.
The sequence of the CCHF virus cytoplasmic tail is somewhat variable in Nairoviruses (ϳ24% identity) and even more so when compared with other Bunyaviruses (12% identity with Hantavirus Gn tails). However, one characteristic feature present in four of the five genera of Bunyaviridae is a conserved dual C-X-C-X-H-X-C motifs of cysteine and histidine residues with X representing any amino acid (Fig. 1). Others have suggested that the high cysteine content of the CCHF virus Gn tail could be due to extensive disulfide bonding (5). Recently, we reported that the cysteines in the Andes hantavirus Gn tail fold into a novel arrangement of back-to-back classical ␤␤␣ zinc fingers (11). Despite low sequence identity between the Gn tail of Nairoviruses and Hantaviruses, the spacing of the dual CCHC motif in the CCHF virus most closely resembles that of Hantaviruses, suggesting the presence of a similar dual zinc finger structure. To test this hypothesis, we determined the NMR structure of the CCHF virus Gn cytoplasmic tail from residues 729 -805. We report here the first known atomic structure of any protein component of the CCHF virus and demonstrate that the high cysteine content of the Gn cytoplasmic tail is partly due to the presence of dual, back to back ␤␤␣-type zinc fingers similar to those found in Hantaviruses. Unlike Hantaviral zinc fingers, however, the electrostatic surface of the CCHF virus zinc finger reveals a clear distribution of conserved electrostatic charges. Moreover, we demonstrate using electrophoretic mobility shift assays (EMSA) that these conserved electrostatics may play a role in forming a surface for binding viral RNA. Together, these data provide insight into the role of the Gn tail in Nairovirus assembly.

EXPERIMENTAL PROCEDURES
Protein Expression and Purification-Various constructs of the CCHF virus (strain SPU103/87) Gn cytoplasmic region (spanning residues 719 -819) were subcloned from a synthetic gene (GenScript) into the expression vectors pDZ1 and pDZ3 (12), which expressed His 6 -tagged GB1 fusion proteins with TEV protease cleavage sites. For NMR structure determination, the soluble Gn construct spanning residues 729-805 (Gn 729 -805 ) was expressed and purified under native conditions following the method reported previously for the Andes hantavirus zinc finger domain (11). Briefly, 15 N-and 15 N/ 13 C-labeled proteins were expressed in Escherichia coli BL21(DE3) grown in 1 liter M9 minimal media supplemented with 0.1 mM ZnSO 4 before and after induction. Cells were grown at 37°C, induced with 1 mM isopropyl-␤-D-thiogalactopyranoside at A 600 ϳ0.8, and cell growth was continued in a 15°C shaker incubator overnight (to a final A 600 ϳ2.0). Cells were harvested by centrifugation, resuspended in buffer A (20 mM Tris-HCl pH 8.0, 20 mM NaCl, 1 mM DTT, 0.1 mM ZnSO 4 ), and lysed by sonication. Cellular debris was removed by centrifugation, and to the supernatant was added one-tenth volume of 1% polyethyleneimine (pH 8) to precipitate the nucleic acids. Following centrifugation, the supernatant was bound to a 40 ml of Q column (GE Healthcare) and eluted with a 280 ml linear gradient of buffer B (20 mM Tris-HCl, pH 8.0, 0.5 M NaCl, 1 mM DTT, 1 mM ZnSO 4 ). For TEV protease digestion, fractions containing the fusion pro-tein were pooled and dialyzed at 25°C overnight in buffer (50 mM Tris-HCl pH 8.0, 20 mM NaCl, 1 mM DTT, 1 mM ZnSO 4 ) with 0.16 mg recombinant TEV protease (13) per 10 ml of fusion protein. The TEV digestion mixture was dialyzed back into buffer A and passed again through a 40 ml Q column (GE Healthcare). The GB1 tag (theoretical pI of 5.6) was retained on the column while Gn 729 -805 (theoretical pI of 8.6) was present in the flow-through. The 50 ml flowthrough fraction was concentrated using Ultra-15 centrifugal filters (Amicon) and dialyzed in NMR buffer (10 mM NaPO 4 pH 7.0, 10 mM NaCl, 1 mM DTT, 0.1 mM ZnSO 4 ). The Gn 729 -805 construct retained three residues (Gly-His-Met) cloning artifacts at the N terminus.
Backbone 15 N relaxation parameters were acquired on a 0.5 mM 15 N-labeled sample in NMR buffer. The steady-state heteronuclear { 1 H}-15 N NOE was acquired as a pair of two-dimensional datasets in an interleaved manner (where portions of each two-dimensional spectrum were acquired sequentially until both datasets were completed) (25). The first two-dimensional dataset contained a 3-s proton saturation (achieved with a series of 120°pulses) whereas the second two-dimensional dataset contained a 3-s delay. The heteronuclear { 1 H}-15 N NOE was calculated as the ratio of the intensities for each peak in the two datasets. Each two-dimensional dataset was acquired with 2048 ( 1 H) ϫ 128 ( 15 N) complex points, 32 scans per point, and a 5 s recycle delay. Error bars were estimated using the standard deviation of the background signal of each spectrum. The 15 N backbone relaxation rates R 1 and R 2 were acquired as described (26). The time delays used to determine R 1 were 10, 60, 120, 240*, 400, 900, and 1100 ms, and the time delays used to determine R 2 were 20, 40*, 50, 60, 70, 90, 100, 120, and 150 ms (asterisk denotes spectra acquired in duplicate to estimate reproducibility). Peak intensities were obtained from NMRView (15) and fitted using GNUPLOT (27). Deviations from fitting were reported as error bars. Because of peak overlap, residues 749, 787, 791, and 796 were not used in the analysis.
Structure Calculation-The protocol used for NMR structure calculation has been described previously (11). Briefly, unique NOE distance restraints were classified into upper bounds of 2.7, 3.5, 4.5, and 5.5 Å and lower bound of 1.8 Å based on peak volumes. Backbone dihedral angles in the ␣-helical regions identified by the secondary C␣, C␤, and H␣ chemical shifts (19) were restrained to (Ϫ60 Ϯ 20°) and (Ϫ40 Ϯ 20°). Initial structures were generated using CYANA (28), followed by molecular dynamics and simulated annealing in AMBER7 (29); first in vacuo, then with the generalized Born (GB) potential. Initial structural calculations were performed in CYANA without the Zn 2ϩ restraints to confirm that the zinc finger domain will fold from NOE-derived restraints only. Once the topology of the Zn 2ϩ -coordinated residues were confirmed, subsequent CYANA structure calculations used distance restraints that imposed tetrahedral Zn 2ϩ -coordination to Cys and His residues (22). Iterative cycles of AMBER calculations followed by refinement of NMR-derived restraints were performed until the structures converged with low restraint violations and good statistics in the Ramachandran plot. A family of twenty lowest energy structures were analyzed using PROCHECK (30) and molecular graphics were generated using PYMOL (31). The surface electrostatic potentials were calculated using APBS (32) and visualized in PYMOL (31).
In Vitro Transcription-A DNA oligonucleotide representing the M genomic segment panhandle was assembled by PCR primer extension and used for in vitro transcription. In vitro transcription was carried out following manufacturer's protocol (MAXIscript Kit, Ambion). Briefly, a 20-l reaction was carried out for 1.5 h (37°) and terminated by adding 2 l 0.25 M EDTA and heating to 90°followed by rapid cooling on ice. Reaction mixtures were then treated with DNase I and subjected to ethanol precipitation. The RNA transcripts were resuspended in RNase-free ddH 2 O and analyzed for purity on a native 12% acrylamide gel stained with SYBR Green II dye (Invitrogen).
RNA Binding Assays-To assess protein-RNA binding by gel electrophoresis, RNA transcripts were incubated on ice for 15 min with increasing amounts of either CCHF virus Gn 729 -805 or Andes hantavirus G1 543-599 in binding buffer (30 mM NaPO 4 , 30 mM NaCl, pH 7.4). Samples were mixed with onehalf volume 50% glycerol and loaded onto a native 12% acrylamide Tris borate gel. The gel was run in a cooling water bath at 90 V for 1 h in Tris borate buffer, pH 8.3 and visualized by staining with SYBR Green II dye. For nucleic acid size determination, each gel included a 100 bp DNA ladder (NEB, NO467S).
CD Spectroscopy-CD spectra were collected in triplicate at 25°on a JASCO J-815 Spectro-polarimeter using a scanning speed of 50 nm/min. Protein concentrations were kept at 1 M in buffer (10 M NaPO 4 , 10 M NaCl, 0.1 mM ZnSO 4 ). EDTA and ZnSO 4 titrations were applied to the same sample.

RESULTS
Protein Expression and Purification-Our previous work with Hantavirus glycoprotein cytoplasmic tails indicates expression of the tail is toxic to E. coli (11). Therefore, all constructs of the CCHF virus Gn cytoplasmic tail were expressed as GB1 fusion proteins. The GB1 tag contained His 6 for nickel affinity purification and a TEV protease cleavage site to recover the native Gn zinc finger domain. The fusion protein was expressed in soluble form in E. coli, purified under native conditions, and digested with TEV protease to obtain the Gn zinc finger domain. Longer constructs comprising the entire predicted cytoplasmic tail (Gn 719 -819 ) expressed as insoluble inclusion bodies. Gn 729 -819 , which was missing the first ten residues following the transmembrane region, expressed as soluble protein but with low yield. Gn 729 -805 represented the longest construct containing the conserved C-X 2 -C-X 11-12 -H-X 3 -C (where X is any amino acid) that also expressed in high enough yield to give high resolution NMR data.
Zn 2ϩ Is Required for Proper Folding-To examine the reliance of Zn 2ϩ -coordination on the proper folding of the CCHF virus Gn tail, we recorded the two-dimensional 15 N HSQC of the Gn 729 -805 in the presence of 4 mM EDTA ( Fig. 2A). The spectrum in the presence of EDTA is collapsed between ppm values of 6.5 and 8.6, whereas the folded spectrum in the absence of EDTA is well dispersed between 6.5 and 9.3 ppm. Narrowing of the spectrum suggests a loss of tertiary structure upon removal of Zn 2ϩ , indicating the requirement for Zn 2ϩ binding in folding of the domain. A similar titration using circular dichroism (CD) spectroscopy demonstrates that the presence of EDTA causes a downward spectral shift, indicating a transition toward an unfolded protein (Fig. 2B). Here we also demonstrate that the addition of Zn 2ϩ ion back into the sample recovers the trace of the original native spectrum. Therefore, Zn 2ϩ is required for proper folding of the CCHF virus Gn tail.
NMR Structure Determination-CCHF virus Gn 729 -805 showed a well dispersed two-dimensional 1 H-15 N HSQC (Fig.  3A). Complete backbone assignments were obtained from three-dimensional HNCA, CBCA(CO)NH, HNCACB, and 15 N-edited NOESY-HSQC. The C ␣ , H ␣ , and C ␤ secondary chemical shifts (Fig. 3B) showed the presence of three short ␣-helices with an intervening random coil region between the second and third helix. Two more regions in random coil orientations flanked the central sequence of the domain as indicated by the heteronuclear { 1 H}-15 N NOE (Fig. 4C). Side chain assignments were completed using two-dimensional 1 H-13 C HMQC, three-dimensional HBHA(CO)NH, and three-dimensional 13 C edited HMQC-NOESY. There were six invariant cysteine and two histidine residues (His-752 and His-776) in Gn 729 -805 (Fig. 1) Fig. S1), respectively. Manual analysis of threedimensional 15 N-and 13 C-edited NOESY spectra identified 1193 unambiguous interproton NOE distance restraints. The NOE restraints together with 26 and 26 dihedral angle restraints and zinc coordination restrains (Table 1) were used in structure calculation and refinement in CYANA and  AMBER. The 20 low energy NMR structures of Gn 729 -805 converged into a family of structures (Fig. 5) with low restraint violations and good Ramachandran plot statistics ( Table 1).
Structure of CCHF Virus Zinc Finger-The NMR structure of Gn 729 -805 reveals a rigid, compact three-helix structure with four short ␤-strands (Fig. 5). The structure contains a pair of tightly associated, back to back ␤␤␣ zinc fingers connected by a short four residue linker (Ser 757 -Ile 760 ) (Fig. 5). The first CCHC-zinc finger array (ZF1) consists of a Zn 2ϩ ion coordi-nated to residues Cys-736, Cys-739, His-752, and Cys-756 and forms the classical ␤␤␣ zinc finger fold. Cys-736 and Cys-739 form part of a short ␤-hairpin. Thr-737 and Ile-738 form a loop with Cys-736 and Cys-739 on either side of the hairpin. The structure contains helix ␣1 formed by Ile-747 to Ser-757 that folds back toward the ␤-hairpin, forming the ␤␤␣ zinc finger fold. Cys-756 forms the fourth Zn 2ϩ -coordinating residue and is located on the same surface of helix ␣3 with His-752.
Likewise, the second CCHC-zinc finger array (ZF2) consists of a second Zn 2ϩ ion coordinated to residues Cys-761, Cys-764, His-776, and Cys-780 into a classical ␤␤␣ zinc finger fold. Cys-761 and Cys-764 are positioned on either side of a short ␤-hairpin. Pro-762 and Tyr-763 form a loop between Cys-761 and Cys-764. The structure is followed by a short helix ␣2 formed by Leu773-Cys-780 and folded back toward the ␤-hairpin, forming the ␤␤␣ zinc finger fold. His-776 is located toward the middle of helix ␣3, and the final coordinating cysteine (Cys-780) is located at the end of helix ␣3. Although ZF2 also resembles the classical ␤␤␣ fold, a minor difference exists when compared with ZF1. The helix ␣2 of ZF2 is shorter than helix ␣1 by three residues. This is due to the presence of helix breakers Gly-772 and Pro-781 located at either end of helix ␣2.
In addition to the two classical ␤␤␣ fold zinc fingers, the structure contains an additional helix, helix ␣3, formed by Lys-782 to Glu-791 that packs against the dual zinc finger fold. A hydrophobic interaction between Val-744 of ZF1 and Val-787 keeps helix ␣3 pinned to the core structure. The orientation of helix ␣3 to ZF2 is partially determined by the helix breaker Pro-781, the residue immediately following ZF2. Pro-781 is 100% identical among Nairoviruses (Fig. 1) and serves as a kink between helix ␣2 and ␣3. Strong Cys C␣ to Pro-718 C␦ NOEs indicated a trans proline isomer. The C-terminal 13 residues (Leu-792 to Lys-805) are primarily unstructured. NOEs between Ile-799 C␥2 and Met-751 C␥ indicate the unstructured tail is pinned to the rest of the structure.
The 15 N backbone relaxation rates (R 1 and R 2 ) as well as the heteronuclear { 1 H}-15 N NOE (Fig. 4) showed that the ZF1, linker (residue 757-760), and ZF2 regions behave with nearly similar amide backbone dynamics. The average R 1 values for ZF1, ZF2 and linker regions were well within each other, with values of 1.60 (ϩ 0.15), 1.81 (ϩ 0.40), and 1.65 (ϩ 0.04) s Ϫ1 , respectively (Fig. 4A). ZF1 and the linker had essentially similar R 1 values, however, within ZF2, the R 1 values increased for residues 770 and 771 of the loop connecting ␤4 and ␣2, indicating increased mobility of this region. Likewise, the average R 2 values for ZF1, ZF2, and linker regions were similar to each other, with values of 13.8 (ϩ 1.8), 13.8 (ϩ 1.8), and 15.6 (ϩ 3.1) s Ϫ1 , respectively. Interestingly, the first linker residue, Ser-756, showed increased R 2 without a corresponding increase in R 1 , which suggested chemical exchange on the s-ms timescale for   . 4C), indicating reduced flexibility for the dual zinc finger domain including the linker region. In brief, the NMR amide backbone relaxation parameters ( Fig. 4) confirmed that the two zinc fingers essentially tumble as one entity, that the linker between the two zinc fingers was rigid and tumble at the same rate as the zinc fingers, and that the loops and tails were flexible.

CCHF Virus Zinc Finger Contains Conserved Electrostatic
Surfaces-Analysis of the surface electrostatics of the CCHF virus Gn 729 -805 reveals clustering of positive and negatively charged surfaces on opposite faces of the structure (Fig. 6). Surface residues Glu-740, Glu-750, and Asp-753 of ZF1 converge with surface residues Glu-789 and Glu-791 of helix ␣3 and Glu-797 of the C-terminal unstructured region to form a large, nearly contiguous negatively charged surface. Similarly, Arg-767 and Arg-775 of ZF2 converge with Lys-782, Lys-784, and Lys-786 of helix ␣3 and Arg-798 of the C-terminal unstructured region to form a large contiguous positively charged surface. Of the charged surface residues, only Glu-750, Glu-797, Lys-784, and Arg-798 are not conserved in Nairoviruses. Most of the surface electrostatics, therefore, is a conserved feature of the Nairoviruses zinc finger domain.
CCHF Virus Gn Tail Binds RNA-RNA electrophoretic mobility shift binding assays (EMSA) were carried out using two different proteins: the zinc finger domain of CCHF virus consisting of Gn 729 -805 , and the zinc finger domain G1 534 -599 of the related Andes hantavirus. The RNA sequences used in the EMSA were a 58-mer RNA of the Andes hantavirus and a 51-mer RNA of the CCHF virus (Fig. 7A). Both RNA sequences contain 23-26 nucleotides at the 5Ј and 3Ј termini of the M genomic segments of the Andes and CCHF viruses, and these 5Ј and 3Ј strands are complementary to each other and are expected to form into hairpin-like panhandle structures (Fig.  7A). On a 12% native acrylamide gel, the Andes hantavirus RNA traveled as a single band consistent with a 58-mer hairpin (Fig.  7B), however, the CCHF virus 51-mer RNA migrated as two bands, a higher molecular weight form and a lower band migrating at a size consistent with a 51-mer hairpin (Fig. 7B). Incubation of the Andes hantavirus protein with the 58-mer RNA failed to affect the migration of RNA (Fig. 7B). The RNA bands in the presence of the Andes hantavirus protein were similar to the free RNA band (Fig. 7B). However, incubation of the CCHF virus zinc finger protein notably affected the migration of the CCHF virus RNA, as demonstrated by the appearance of an additional band (marked with asterisk, Fig. 7B) migrating between the hairpin and the higher MW form of the CCHF virus RNA. The protein-RNA complex band was most likely formed between the zinc finger protein and the RNA hairpin. Because the 51-mer CCHFV RNA existed in two forms (the hairpin and the higher MW form), the relative amounts of each form must be in equilibrium and binding of the CCHFV zinc finger protein to the hairpin RNA will also affect the amount of the RNA B form as seen in Fig. 7B. We are designing new RNA sequences that will only form hairpins for future studies of the protein-RNA interaction of the CCHF virus zinc finger. Nevertheless, the main conclusion from the EMSA results demonstrated that the CCHF Nairovirus Gn tail (residues 729 -805) interacted with RNA whereas the Andes hantavirus G1 tail (residues 534 -599) did not.
To test our hypothesis that conserved basic residues in the CCHF virus zinc finger protein may be involved in RNA binding, point mutations were introduced in conserved lysine and arginine residues into aspartic acid and the mutant proteins were used in EMSA. The point mutants K783D, K786D, and R767D retained the ability to bind RNA suggesting these basic residues may not be critical in RNA binding (supplemental Fig.  S2A). However, the K782D mutation disrupted the protein-RNA interaction, as its shift pattern resembles that of RNA alone. Coincidentally, Lys-782 is located at the kink between helix ␣2 and ␣3, and is pointed away from the zinc finger domain (supplemental Fig. S2B), suggesting that the kink between helix ␣2 and ␣3 may be important for RNA binding interaction of the CCHF virus Gn zinc finger.

DISCUSSION
We report here that an envelope glycoprotein of a Nairovirus contains a dual CCHC-type zinc finger (Figs. 2-5) domain that  binds RNA. Although zinc fingers have been known in viruses, in particular, the HIV-1 nucleocapsid protein zinc fingers (33) are critical in RNA packaging and viral assembly, zinc fingers are rarely found in viral envelope glycoproteins. Including the zinc finger in this report, there are currently only three known structures of viral envelope glycoprotein zinc fingers. First is the zinc finger of the Hantavirus G1 envelope glycoprotein (11), and second is the zinc finger of the Junin virus envelope glycoprotein (34) (also an RNA virus, of family Arenaviridae). In all three cases, the cytoplasmic tails of the envelope glycoproteins contain the zinc finger domains. The Junin virus zinc fingers (34) form a unique fold that do not show any structural nor sequence similarity with the Nairovirus and Hantavirus zinc fingers. Although the Nairovirus and the Hantavirus zinc fingers (11), which both belong to family Bunyaviridae (Fig. 1), show an overall similar global fold (supplemental Fig. S3), they also have major structural differences (Fig. 6) and properties (Fig. 7).
Key Differences between Nairovirus and Hantavirus Gn Zinc Fingers-Examination of the surface electrostatics of the CCHF virus Gn tail reveals key differences when compared with the Andes hantavirus structure (Fig. 6). Whereas the CCHF Gn tail displays sharp clustering of conserved charges that form a large contiguous swath on the protein surface, the Andes hantavirus zinc fingers display charges that are predominately negative and apparently randomly dispersed (Fig. 6). The variation in charge conservation is also evident in the sequence analysis (supplemental Fig. S3). Whereas the spacing of CCHC motif is mostly conserved, the spacing between conserved charges is highly variable. The CCHF virus displays conserved negative charges on ZF1 and conserved positive charges on ZF2. The Andes hantavirus sequence, however, displays clustering of conserved positive charges on the sequences flanking the negatively charged core zinc finger structure.
Moreover, the CCHF virus Gn tail contains a structural motif that is absent in the Andes hantavirus structure. Helices ␣2 and ␣3 (Fig. 3B), residues Leu-773 to Leu-792, form a helix-kinkhelix motif due the positioning of the conserved helix breaker Pro-781. While not an uncommon motif, this structural aspect in the CCHF Gn tail forms the core scaffold for a large positively charged surface partly composed of the conserved charges at Arg-775, Lys-782, and Lys-786 (Fig. 6A). By contrast, the Andes hantavirus structure contains neither the corresponding proline nor the charges to support a similar motif (Fig. 1). Instead, it contains the non-conserved helix breaker Gly-598 followed by conserved charges exclusively on the C-terminal end of ZF2 (Fig. 1). In this respect, the surface electrostatics of the CCHF virus Gn tail may more closely resemble that of Orthobunyaviruses, with conserved helix breakers flanked by conserved basic charges (Fig. 1). Perhaps not coincidentally, Nairoviruses and Orthobunyaviruses are both arthropod-borne, whereas Hantaviruses are rodent-borne (3). Overall, the general preservation of the fold indicates that the dual zinc finger motif plays a general but important role in the life cycle of both Nairoviruses and Hantaviruses. However, the major differences in the surface electrostatics of the CCHF virus and Hantavirus cytoplasmic tail structures (Fig. 6) also suggests that while general, the function of the tail may be species specific.
Proposed Role in Viral Assembly-Given the data available regarding the Bunyaviridae Gn role in viral assembly (8 -10), it is likely that the surface electrostatics play an important role in assembly of the CCHF virus, presumably via direct interaction with some component of the ribonucleoprotein. The large positively charged surface of the Gn tail would suggest RNA binding, as is the traditional role for zinc fingers in retroviruses (33,35). Our EMSA results (Fig. 7) suggest that this may in fact be the case. Using increasing amounts of Gn 729 -805 revealed the migration of an additional RNA band (Fig. 7B), which likely represents a protein-RNA complex consisting of Gn 729 -805 and the hairpin-like M segment panhandle. While the observed complex is weakly bound and therefore likely to be nonspecific, these results suggest RNA interaction mediated by some of the conserved residues in the Gn tail. Additionally, these results suggest the possibility of an interaction between the Gn tail and the RNA component of the ribonucleoproteins (Fig. 7C). A reverse genetics system for studying the CCHF virus has only recently been developed (36), thus allowing testing of this model in the future.
In summary, we present the NMR structure of a zinc finger domain in the Gn tail of the CCHF virus. Currently, this is the only available atomic structure for a protein component of the Nairovirus genus. The global fold of this zinc finger is similar to that of the Hantavirus zinc finger, which represents a unique fold of two classical-type ␤␤␣-zinc fingers that are stuck together (in contrast, individual classical ␤␤␣-zinc fingers behave as independent domains, like beads-on-a-string). We also demonstrated that the CCHF virus Gn tail binds RNA in vitro, thus suggesting the possibility of an interaction between the Gn tail with the viral RNA. Taken together, our results contribute novel mechanistic insight toward understanding the CCHF virus life cycle.