 | Acta Crystallographica Section F Acta Crystallographica Section F STRUCTURAL BIOLOGY COMMUNICATIONS |
journal menu
research communications
| STRUCTURAL BIOLOGY COMMUNICATIONS |
accessStructural characterization of the principal mRNA-export factor Mex67–Mtr2 from Chaetomium thermophilum
aMRC Laboratory of Molecular Biology, Francis Crick Avenue, Cambridge Biomedical Campus, Cambridge CB2 0QH, England, and bBiochemie-Zentrum der Universität Heidelberg, Im Neuenheimer Feld 328, 69120 Heidelberg, Germany
*Correspondence e-mail: ms@mrc-lmb.cam.ac.uk
Members of the Mex67–Mtr2/NXF–NXT1 family are the principal mediators of the nuclear export of Mex67/NXF1 has a modular structure based on four domains (RRM, LRR, NTF2-like and UBA) that are thought to be present across species, although the level of sequence conservation between organisms, especially in lower eukaryotes, is low. Here, the crystal structures of these domains from the thermophilic fungus Chaetomium thermophilum are presented together with small-angle X-ray scattering (SAXS) and in vitro RNA-binding data that indicate that, not withstanding the limited sequence conservation between different NXF family members, the molecules retain similar structural and RNA-binding properties. Moreover, the resolution of crystal structures obtained with the C. thermophilum domains was often higher than that obtained previously and, when combined with solution and biochemical studies, provided insight into the structural organization, self-association and RNA-binding properties of Mex67–Mtr2 that facilitate nuclear export.
Keywords: nuclear transport; Mex67; Chaetomium thermophilum; RNA binding.
PDB references: Mex67 RRM, 4wpm; Mex67 UBA, 4wp2; Mex67 NTF2L, 4wp5; Mex67 LRR, 4wp6; Mtr2, 4x2m; Mex67 LRR+NTF2L, 4xm4
1. Introduction
The Mex67–Mtr2 complex (NXF1–NXT1 in metazoans and small bristles in Drosophila melanogastor) is the principal mRNA-export factor in Sacccharomyces cerevisiae (Segref et al., 1997![[Segref, A., Sharma, K., Doye, V., Hellwig, A., Huber, J., Lührmann, R. & Hurt, E. (1997). EMBO J. 16, 3256-3271.]](../../../../../../logos/arrows/f_arr.gif "Segref, A., Sharma, K., Doye, V., Hellwig, A., Huber, J., Lührmann, R. & Hurt, E. (1997). EMBO J. 16, 3256-3271.")
; Herold et al., 2000; Wilkie et al., 2001). Mex67/NXF1 is a modular protein constructed from four domains (Fig. 1): an RNA-recognition motif (RRM) domain, a leucine-rich repeat (LRR) domain, a nuclear transport factor 2-like (NTF2L) domain and an ubiquitin-associated (UBA) domain (reviewed by Valkov et al., 2012). Mtr2 is a ∼15–20 kDa protein that also has an NTF2-like fold and forms a tight heterodimeric complex with the Mex67 NTF2L domain. Mex67–Mtr2 forms direct contacts with cargoes as well as multiple transient low-affinity interactions with phenylalanine–glycine-rich nuclear pore proteins (FG nucleoporins). Translocation of the Mex67–Mtr2+mRNA cargo–carrier complex from the nucleus to the cytoplasm through nuclear pores (NPCs) is thought to rely on rectified whereby a series of low-affinity interaction with FG nucleoporins enables Mex67–Mtr2 and its associated cargo to move back and forth within the pore-transport channel, whereas disassembly of the cargo–carrier complex by DEAD-box helicases on the cytoplasmic NPC face is thought to provide the directionality (reviewed by Stewart, 2010; Valkov et al., 2012). Classically, binding of the RNA cargo has been attributed to the RRM and LRR domains because together these domains are sufficient for Homo sapiens NXF1 to bind the viral RNA CTE (constitutive transport element) sequence motif (Pasquinelli et al., 1997; Grüter et al., 1998; Braun et al., 1999; Wiegand et al., 2002; Teplova et al., 2011). Both the NTF2L domain complexed with Mtr2/NXT1 and the UBA domain interact with a range of FG nucleoporins (Fribourg et al., 2001; Grant et al., 2003). More recently, the NTF2L domain and Mtr2 have also been implicated in binding ribosomal subunits and whereby in S. cerevisiae specific long internal loops may be involved in direct RNA binding as well as domain organization to form a continuous RNA-binding platform with the RRM and LRR domains (Yao et al., 2007; Aibara, Valkov et al., 2015).
![[Figure 1]](mn5088fig1thm.gif) | Figure 1 Schematic illustration of the domain structure of Mex67/NXF1 from H. sapiens, C. thermophilum and S. cerevisiae. Although all three organisms retained the four structural domains (RRM, LRR, NTF2L and UBA), H. sapiens and C. thermophilum had an extended N-terminal region that has been implicated in an auto-regulatory role for NXF1 (Viphakone et al., 2012 ). |
Extensive studies with archaea have demonstrated that proteins obtained from thermophiles often facilitate the determination of high-resolution crystal structures, and this has stimulated interest in eukaryotic thermophiles such as the filamentous fungus Chaetomium thermophilum (Bock et al., 2014). Because the proteins involved in export tend to have multiple roles and conformational states, often associated with the formation of a series of different complexes during the generation of an export-competent mRNP, high-resolution structures of the components of the pathway are a prerequisite for deciphering the structures of the complexes involved. Moreover, the thermostability of proteins from C. thermophilum often facilitates experiments that have proven difficult with their mesophilic counterparts (Leidig et al., 2013; Monecke et al., 2013; Thierbach et al., 2013).
Here, we present the crystal structures of the individual domains of C. thermophilum Mex67–Mtr2 (ctMex67–Mtr2) to provide a complete repertoire of high-resolution structures from a single species to facilitate structural studies of the complexes formed during the formation of export-competent mRNPs. In vitro SAXS and RNA-binding studies have also demonstrated that ctMex67–Mtr2 has similar biochemical properties as H. sapiens NXF1–NXT1 (hsNXF1–NXT1) and, in particular, have shown that the ctMex67 NTF2L domain contributes to binding.
2. Methods
2.1. Cloning and protein purification
Genes corresponding to ctMex67 and ctMtr2 were PCR-amplified from C. thermophilum cDNA using standard procedures. Fragments corresponding to the RRM (ctMex67RRM; residues 93–200) and LRR (ctMex67LRR; residues 191–360) domains were cloned into the first multiple cloning site (MCS) of pETDuet-1 to generate His6-tagged constructs. Fragments corresponding to the NTF2L domain (ctMex67NTF2L; residues 365–564) and ctMtr2 were cloned into the first and second MCS sites of pETDuet-1, respectively, to generate His6-tagged ctMex67NTF2L–Mtr2. A fragment corresponding to the UBA domain (ctMex67UBA; residues 600–657) was cloned into pMCSG10 to generate a TEV-cleavable GST-tagged construct. Longer constructs containing multiple domains of ctMex67 [LRR-NTF2L (residues 180–556), ΔNΔUBA (residues 93–556) and ΔN (residues 70–657)] and Mtr2 were also cloned into the first and second MCS sites of pETDuet-1, respectively, to generate TEV-cleavable His6-tagged constructs. All protein constructs were expressed in Escherichia coli BL21-CodonPlus(DE3)-RIL cells by IPTG induction at 291 K over 16 h and all purification steps and manipulations were conducted at 277 K unless stated otherwise. Harvested cell pellets were resuspended at 5 ml per gram of wet cell pellet in 50 mM Tris–HCl pH 7.4, 500 mM NaCl, 20 mM imidazole pH 8.0 (His6-tagged constructs) or 50 mM Tris–HCl pH 7.4, 500 mM NaCl, 5 mM DTT (GST-tagged constructs) and lysed by high-pressure cavitation using two passes through an EmulsiFlex C3 (Avestin). Lysates were clarified by centrifugation and the supernatant was incubated with Ni–NTA agarose beads or glutathione Sepharose 4B beads for 1 h. Nonspecifically bound proteins were removed by washing with the buffer used for lysis, after which the His6-tagged proteins were eluted with 50 mM Tris–HCl pH 7.4, 500 mM NaCl, 250 mM imidazole and GST-tagged proteins were eluted with 50 mM Tris–HCl pH 7.4, 500 mM NaCl, 5 mM DTT, 2 mM reduced glutathione. TEV-cleavable tags were then removed by incubation with TEV protease overnight. Constructs with more than one domain were purified further using heparin as described in Aibara, Valkov et al. (2015). All proteins were finally purified to by using a HiLoad 26/60 Superdex 75 or 200 column equilibrated in 20 mM Na HEPES pH 8.0, 200 mM NaCl (for all multi-domain constructs), 20 mM Na HEPES pH 8.0, 750 mM NaCl, 5 mM DTT (for ctMex67UBA) or 20 mM Tris–HCl pH 7.4, 50 mM NaCl (for all other single-domain constructs). Small aliquots of purified proteins were flash-frozen in liquid nitrogen and stored at 193 K until required.
2.2. X-ray crystallography
Protein crystals were grown at 291 K by sitting-drop vapour diffusion in which 200 nl purified protein solution was mixed with 200 nl well buffer (see Table 1) and cryocooled in mother liquor supplemented with 20% glycerol. X-ray diffraction data were collected on beamlines I04, I04-1 and I24 at Diamond Light Source, Didcot, England. Reflections were indexed and integrated using XDS (Kabsch, 2010) and then scaled and merged in AIMLESS, ensuring a completeness of >98% in the outermost shell while maintaining CC1/2 > 0.3 (Evans & Murshudov, 2013). The ctMex67RRM, ctMex67LRR and ctMtr2 structures were obtained by using the MR-Rosetta pipeline (DiMaio et al., 2011) with human RRM and LRR domains (Teplova et al., 2011; PDB entry 3rw7) and scMtr2 (Fribourg & Conti, 2003; PDB entry 1of5) as search models, whereas ctMex67NTF2L–Mtr2 was solved by using Phaser (McCoy et al., 2007) with the S. cerevisiae homologue (Fribourg & Conti, 2003; PDB entry 1of5) and ctMtr2 (PDB entry 4x2m) as search models. The structure of ctMex67UBA was solved by SAD phasing in Phaser (McCoy et al., 2007) using from S-(dimethylarsenic)cysteine that was derived from cysteines modified by the cacodylate buffer (Maignan et al., 1998; Liu et al., 2011). Iterative cycles of rebuilding using Coot (Emsley et al., 2010) and using PHENIX (Adams et al., 2010) with weightings chosen to minimize Rfree were used to generate the final models (Table 1).
![[\textstyle \sum_{hkl}\sum_{i}|I_{i}(hkl)- \langle I(hkl)\rangle|/]](teximages/mn5088fi1.gif) ![[\textstyle \sum_{hkl}\sum_{i}I_{i}(hkl)]](teximages/mn5088fi2.gif) , where Ii(hkl) is an individual intensity measurement and 〈I(hkl)〉 is the average intensity for all i observations of reflection hkl. ‡Rmeas = ![[\textstyle \sum_{hkl}\{N(hkl)/[N(hkl)-1]\}^{1/2}\sum_{i}|I_{i}(hkl)- \langle I(hkl)\rangle|/]](teximages/mn5088fi3.gif) , where Ii(hkl) is an individual intensity measurement and 〈I(hkl)〉 is the average intensity for all i observations of reflection hkl. §Rp.i.m. = ![[\textstyle \sum_{hkl}\{1/[N(hkl)-1]\}^{1/2}\sum_{i}|I_{i}(hkl)- \langle I(hkl)\rangle|/]](teximages/mn5088fi5.gif) , where Ii(hkl) is an individual intensity measurement and 〈I(hkl)〉 is the average intensity for all i observations of reflection hkl. ¶Rwork = ![[\textstyle \sum_{hkl}\big ||F_{\rm obs}|-|F_{\rm calc}|\big |/]](teximages/mn5088fi7.gif) ![[ \textstyle \sum_{hkl}|F_{\rm obs}|]](teximages/mn5088fi8.gif) , where Fobs and Fcalc are the observed and calculated structure-factor amplitudes, respectively. Rfree is defined as Rwork for a randomly selected 5% of reflections. ††The all-atom clashcore is the number of unfavourable all-atom steric overlaps of ≥0.4 Å per 1000 atoms (Word et al., 1999 ) and the MolProbity score (MPscore) is calculated as follows (Keedy et al., 2009): MPScore = 0.426ln(1 + clashscore) + 0.33ln[1 + max(0, rota_out − 1)] + 0.25ln[1 + max(0, rama_iffy − 2)] + 0.5. | |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
2.3. Small-angle X-ray scattering
Small-angle X-ray scattering (SAXS) data were collected on beamline BM29 at the European Synchrotron Radiation Facility, Grenoble, France using an online HPLC system (Viscotek) equipped with a Superdex 200 Increase 3.2/300 column (GE Healthcare) with a sample flow rate of 0.1 ml min−1. Data were collected at 293 K using a wavelength of 0.995 Å and a sample-to-detector distance of 1 m, and were processed automatically using the online AUTOSUB pipeline (Konarev et al., 2003). All gave linear Guinier plots for s*Rg < 1.3. Pair distance distribution functions of the particles P(r) and their maximum sizes Dmax were computed using GNOM (Svergun, 1992) and molecular weights were estimated by comparing the extrapolated of the samples obtained from Guinier analysis using AUTORG (Konarev et al., 2003) with that of a bovine serum albumin standard (Sigma–Aldrich). Theoretical SAXS profiles based on atomic models and comparisons with experimental SAXS profiles were obtained using the FoXS server (Schneidman-Duhovny et al., 2010, 2013).
2.4. In vitro RNA-binding assays
The interaction of RNA with a range of ctMex67 domain-based constructs was assessed using fluorescence anisotropy, in which 10 nM DY-547-labelled homopolymeric RNA (polyA15, polyU15, polyC15, polyG15) was mixed with serially diluted protein in 20 mM Tris–HCl pH 8.0, 50 mM NaCl as described previously (Aibara, Valkov et al., 2015).
3. Results and discussion
3.1. Structural conservation of domains in C. thermophilum Mex67
Although ctMex67 shared only 23.0% sequence identity with scMex67 and 23.5% identity with hsNXF1, the crystal structures obtained for the RRM domain (2.4 Å resolution), the LRR domain (1.7 Å resolution), ctMtr2 alone (2.0 Å resolution), NTF2L–Mtr2 (2.9 Å resolution) and the UBA domain (1.7 Å resolution) of ctMex67–Mtr2 (Table 1) generally retained the key features of their yeast and metazoan counterparts, albeit with several differences.
The 2.4 Å resolution of ctMex67RRM resembled that of hsNXF1RRM (Liker et al., 2000; Teplova et al., 2011; PDB entries 1fo1 and 3rw6) and was based on the characteristic RRM βαββαβ fold (Figs. 2a, 2b and 2c). Like other NXF family members, ctMex67RRM did not contain a typical RRM consensus sequence that is based on two motifs: RNP1, (K/R)o-G-(F/Y)o-(G/A)i-Fo-Vi-Xo-(F/Y)i, and RNP2, (L/I)i-(Y/F)o-(V/I)i-(G/N)o-(G/N)o-(L/M)i, where the subscript `o' or `i' signifies whether the side chain is surface-exposed or facing the core of the RRM fold (Liker et al., 2000; Maris et al., 2005). In ctMex67RRM the RNP1 (residues 143–150) and RNP2 (residues 101–106) sequences were G-Do-Yo-Vi-Wo-Li-Ko-Vi and Ii-Ko-Ii-Lo-G-Li, respectively. The RNP2 motif appeared to be more conserved than RNP1, although the characteristic aromatic group at position 2 that typically forms ring-stacking interactions with RNA was instead lysine in ctMex67RRM. The large deviations from the RNP1 and RNP2 sequences found in different members of the NXF1/Mex67 family may reflect that they bind RNA in a more general, non-base-specific way, as appeared to be the case in the of hsNXF1RRM-LRR–CTE-B, in which the hsNXF1 RRM domain formed mainly phosphate–backbone interactions with the CTE-B RNA (Teplova et al., 2011). The 1.7 Å resolution of ctMex67LRR showed the characteristic pattern of alternating α-helices and β-strands arranged to form a gently curving structure similar to that seen in this domain in homologous structures (Figs. 2d, 2e and 2f; Liker et al., 2000; Teplova et al., 2011), although ctMex67LRR had an additional α-helix inserted between the first α-helix and β-strand of the domain core (Fig. 2e; denoted α2c).
![[Figure 2]](mn5088fig2thm.gif) | Figure 2 (a) Overview of the 2.4 Å resolution of ctMex67RRM. (b) A schematic illustration of the secondary-structural elements present in the RRM domain, which showed the characteristic βαββαβ fold. The RRM domain from ctMex67 had a short β-strand prior to β4 that was not found in other organisms (denoted β4′). (c) Three representative views of the final 2Fo − Fc maps for the ctMex67RRM structure contoured at the 1σ level. (d) Overview of the 1.7 Å resolution of ctMex67LRR. (e) Schematic illustration of the secondary-structural elements present in the LRR domain whereby tandem repeating α-helices and β-sheets generate a curved structure. Disordered regions are shown as red dotted lines. The LRR domain from ctMex67 includes an extra helix insertion between α2b and β2 when compared with the H. sapiens homologue. (f) Three representative views of the final 2Fo − Fc maps for the ctMex67LRR structure contoured at the 1σ level. |
The ctMex67NTF2L and ctMtr2 chains interacted through their highly curved β-sheets in a pseudo-twofold-symmetric manner in the 2.9 Å resolution similar to that observed in the analogous complexes from H. sapiens and S. cerevisiae (Fribourg et al., 2001; Fribourg & Conti, 2003). In the complex, ctMtr2 was not altered when compared with the isolated structure, with a Cα r.m.s.d. of 0.38 Å over 148 residues. Although the folds of the NTF2-like domains in both Mex67 and Mtr2 were similar across species, those in ctMex67NTF2L–Mtr2 had more extensive and longer loops and β-sheets than those observed in H. sapiens and S. cerevisiae (Fig. 3a). Neither ctMex67NTF2L nor ctMtr2 had the larger internal loops between strands β4 and β5 present in S. cerevisiae but which were disordered in previous structures (Fribourg & Conti, 2003; Fig. 3b). These loops have been implicated in pre-60S ribosomal export, where a surface flanked by these loops is formed on the NTF2L–Mtr2 region that is separate from that used for bulk export (Yao et al., 2007, 2008) and also contribute to the ordered arrangement of domains in S. cerevisiae Mex67 (Aibara, Valkov et al., 2015). There was clear density for these loops in the ctMex67NTF2L–Mtr2 but as in hsNXF1NTF2L–NXT1 they did not form an extended surface, suggesting that ctMex67–Mtr2 may not be involved in ribosomal export in C. thermophilum in the quite same way as in S. cerevisiae. A crystal contact in which the C-terminal region (residues 557–564) of the ctMex67NTF2L chain made contact with the cavity formed between α2′ and β1′ from a symmetry-related ctMex67NTF2L chain resulted in ctMex67NTF2L having an additional β-strand (β1′ in Fig. 3b) compared with H. sapiens NXF1NTF2L, although the biological significance of this interaction remains to be established. There was clear density for the N-terminal region of ctMex67NTF2L (the pre-α1 loop, residues 365–376) that placed this region in a position in which it spanned across the surface of ctMtr2 (Fig. 4a). In particular, Leu368 was buried in a hydrophobic pocket present in ctMtr2. This arrangement of the Mex67NTF2L pre-α1 loop is also present in the H. sapiens homologue as well as in the multi-domain structure of S. cerevisiae Mex67ΔUBA–Mtr2 (Fribourg et al., 2001; Aibara, Valkov et al., 2015). In S. cerevisiae, the pre-α1 loop formed a rich network of interactions that appeared to make a major contribution to the spatial arrangement of Mex67 domains (Fig. 4b) and thus the observation that this interaction is conserved between S. cerevisiae, C. thermophilum and H. sapiens indicates that it represents a conserved structural feature within these complexes.
![[Figure 3]](mn5088fig3thm.gif) | Figure 3 (a) Overview of the 2.9 Å resolution of ctMex67NTF2L–Mtr2. The two chains are related in a twofold-symmetric manner, where the highly curved β-sheets form a tight heterodimeric complex. (b) Schematic illustration of the secondary-structural elements in the NTF2L domain and Mtr2. Disordered regions are shown as red dotted lines. The internal loop present between β4 and β5 in both the NTF2L domain and Mtr2 were ordered, but not extended as shown to be the case in S. cerevisiae (circled with a dotted green line). The pre-α1 loop region of the NTF2L domain was also ordered in ctMex67 and was bound across Mtr2 in an analogous way to that seen in hsNXF1NTF2L–NXT1 (PDB entry 1jkg; Fribourg et al., 2001 ). An extra β-strand was present in the NTF2L domain when compared with the hsNXF1 NTF2L domain and was probably owing to a lattice contact involving the extreme C-terminus of the NTF2L domain (denoted β1′ and circled with a dotted purple line). (c) Three representative views of the final 2Fo − Fc maps for the ctMex67NTF2L–Mtr2 structure contoured at the 1σ level (the ctMex67NTF2L domain is shown in yellow and ctMtr2 is shown in green). |
![[Figure 4]](mn5088fig4thm.gif) | Figure 4 (a) Detailed view of the pre-α1 loop region (represented as sticks) spanning the surface of Mtr2 (yellow). Hydrophobic contacts between Mex67 and Mtr2 centring on Leu368 of Mex67 were found outside the NTF2-like core. (b) Schematic representation of the interactions between the pre-α1 loop (yellow) and Mtr2 (grey) found outside the NTF2-like core. Solid lines represent hydrophobic interactions and dotted lines represent putative hydrogen bonds. |
The 2.95 Å resolution ctMex67LRR-NTF2L had two copies of the protein in the that generated a pseudo-homodimer through extensive interactions between the highly curved β-sheets of each Mex67 NTF2L domain (Fig. 5a) that were analogous to those seen in the S. cerevisiae Mex67–Mtr2 heterodimer or NTF2 homodimer (Bayliss et al., 2002). Two copies of the LRR domain were also present in the but the LRR-NTF2L linker was disordered. However, both LRR domains had the same orientation with respect to ctMex67NTF2L, and when aligned the two copies had a Cα r.m.s.d. of 1.03 Å (Fig. 5b). Comparison of the fold of ctMex67NTF2L in this structure with that observed when it was complexed with Mtr2 indicated that the major secondary-structural elements of the NTF2-like core were not perturbed, although there were several rearrangements in the loop regions (Fig. 5c). However, the previously ordered pre-α1 loop that gave rise to the asymmetry in the NTF2L–Mtr2 region was now disordered, perhaps thereby allowing the symmetric homodimeric Mex67 to be generated. Although it has been proposed that a motif known as the `NXF plug' formed by residues present in the core of the NTF2L domain would inhibit Mex67 homodimerization (Kerkow et al., 2012), this motif was still present in the current structure (Fig. 5d). Moreover, ctMex67LRR-NTF2L appeared to form a homodimer in solution, and in coupled with multi-angle the protein migrated as a single peak with a molecular mass of 82 g mol−1 (Supplementary Fig. S2), consistent with a dimer (each chain has a theoretical mass of 42 g mol−1).
![[Figure 5]](mn5088fig5thm.gif) | Figure 5 (a) Overview of the 2.95 Å resolution of ctMex67LRR-NTF2L. Two copies of the protein in the were assumed in a homodimeric configuration analogous to that of S. cerevisiae NTF2 (Bayliss et al., 2002 ; PDB entry 1gyb). Residues corresponding to the LRR-NTF2L linker (residues 362–378) were disordered as depicted in the schematic representation using dotted lines. (b) Structural alignment of the two copies of ctMex67LRR-NTF2L in the the LRR domain was placed in the same position with respect to the NTF2L domain in both copies. A Cα r.m.s.d. of 1.03 Å was observed over 294 residues. (c) Schematic of the secondary-structure elements present in the NTF2L domain for the structure of ctMex67LRR-NTF2L. No major changes in the NTF2-like core were observed, although rearrangements in the loop regions were detected. The pre-α1 loop which was previously ordered in the structure of ctMex67NTF2L–Mtr2 was disordered in this structure (depicted as a dotted red line). (d) View of the electrostatic of the β-sheet interface between the two NTF2L domains. The `NXF plug' previously identified to confer specificity for the Mex67–Mtr2 interaction (Kerkow et al., 2012) was still present in this structure of homodimeric Mex67. (e) Three representative views of the final 2Fo − Fc maps for the ctMex67LRR-NTF2L structure contoured at the 1σ level (one copy of ctMex67LRR-NTF2L is shown in yellow and the other is shown in green). |
The 1.7 Å resolution of ctMex67UBA showed a clear As anomalous signal from a dimethylarsenic group on Cys623 that was derived from the cacodylate buffer (Figs. 6a, 6b and 6c). The ctMex67UBA fold was based on three α-helices similar to those seen in H. sapiens and S. cerevisiae (Grant et al., 2003; Hobeika et al., 2009) and there was a hydrophobic pocket in an equivalent position to where a FG nucleoporin peptide binds in the H. sapiens homologue (Grant et al., 2003), indicating that ctMex67UBA probably also interacts with FG nucleoporins in a similar fashion. Cys623 was also located in this solvent-accessible pocket (Fig. 6d). The ctMex67 UBA domain contained a four-residue C-terminal extension compared with the H. sapiens homologue that formed interactions with the end of α1 in seven copies of the eight in the and which might contribute to thermostability.
![[Figure 6]](mn5088fig6thm.gif) | Figure 6 (a) Overview of the 1.7 Å resolution of ctMex67UBA. Like other UBA domains of Mex67/NXF1 from H. sapiens and S. cerevisiae, the domain was based on three principal α-helices together with the extreme C-terminal region that formed contacts with the first α-helix (α1). (b) Schematic illustration of the secondary-structural elements in the UBA domain. (c) Detailed view of the dimethylarsenic group conjugated to Cys623 of ctMex67. An anomalous difference Fourier contoured at 6σ (represented in blue) showed clear density around the As atom. (d) Surface representation of the FG nucleoporin binding site present in the UBA domains of ctMex67 (left) and hsNXF1 (right). The UBA domain from ctMex67 clearly has the same binding pocket as present in hsNXF1, although the dimethylarsenic group described in (c) was found to be bound there. (e) Three representative views of the final 2Fo − Fc map for the ctMex67UBA structure contoured at the 1σ level. |
In summary, the fold of all four domains of C. thermophilum Mex67 and Mtr2 was conserved when compared with the H. sapiens homologue and displayed a low Cα r.m.s.d. values when aligned structurally across species (Table 2). The UBA domains and Mtr2/NXT1 showed a high level of structural conservation (Cα r.m.s.d. < 0.8 Å), whereas the NTF2L domain showed the greatest variation (Cα r.m.s.d. = 1.9 Å). However, despite the conservation of the fold, even after structure-based alignment the number of identical equivalent residues remained remarkably low. The UBA domain showed the greatest conservation (29% sequence identity over 55 residues), whereas the RRM domain had the lowest (15% identity over 73 residues). An unexpected homodimeric form of ctMex67 was also observed in which the two copies of ctMex67NTF2L formed a dimer analogous to that in S. cerevisiae NTF2.
| ||||||||||||||||||||||||||
3.2. SAXS indicates that C. thermophilum and S. cerevisiae Mex67–Mtr2 have a similar spatial arrangement of domains
Previous studies indicated that there is a defined spatial relationship between the Mex67 RRM, LRR and NTF2L domains (Aibara, Valkov et al., 2015). Despite extensive crystallization trials, crystals of constructs containing multiple domains of ctMex67 complexed with ctMtr2 could not be obtained, and therefore small-angle X-ray scattering (SAXS) was used to investigate the solution state of ctMex67–Mtr2 using systematic truncations of domains (Table 3). Because the scMex67–Mtr2 RRM-LRR linker showed some flexibility (Aibara, Valkov et al., 2015), a ctMex67LRR-NTF2L–Mtr2 complex was initially examined. The theoretical SAXS profile generated from an atomic model of scMex67LRR-NTF2L–Mtr2 showed an excellent fit to the C. thermophilum data (χFoXS = 1.0), consistent with this domain arrangement probably being conserved. The scMex67ΔUBA–Mtr2 (Aibara, Valkov et al., 2015) showed two different RRM-LRR domain arrangements that were tested separately, but whereas configuration 1 (Fig. 7b, blue) fitted the SAXS profile of ctMex67ΔNΔUBA–Mtr2 well (χFoXS = 1.03), configuration 2 (Fig. 7b, red) fitted less well (χFoXS = 2.5). Models of ctMex67ΔN–Mtr2 were generated by in BILBOMD (Pelikan et al., 2009) to investigate the position of the UBA domain relative to the rest of Mex67–Mtr2. The individual Mex67 domains were joined by polyalanine linkers and then allowed to move as rigid bodies while scoring the fit against the measured SAXS profile of ctMex67ΔN–Mtr2. The three best models all had excellent fits [χFoXS = 1.04, 1.02 and 1.09 for configurations 1 (orange), 2 (green) and 3 (blue), respectively; Fig. 7c]. Aligning the three best models based on the NTF2L–Mtr2 region showed that consistent with the SAXS data obtained with Mex67LRR-NTF2L–Mtr2, the RRM domain showed flexibility whereas the LRR domain position remained constant. Strikingly, the UBA domain in these models was placed in three very different positions, consistent with the spatial positions of the NTF2L and UBA domains not being strongly constrained.
‡Determined using GNOM. | ||||||||||||||||||||||||||||||||
![[Figure 7]](mn5088fig7thm.gif) | Figure 7 (a) The theoretical scattering of scMex67LRR-NTF2L–Mtr2 matched the observed SAXS profile for the equivalent ctMex67–Mtr2 construct. (b) The theoretical scattering of the two configurations of the RRM domain present in the of scMex67ΔUBA–Mtr2 fitted to varying degrees: configuration 1 (blue) fitted the SAX data well, whereas configuration 2 (red) fitted less well. (c) A range of atomic models of the ctMex67ΔN–Mtr2 were generated by BILBOMD and the three best models had excellent fits to the experimental SAXS profile. The spatial arrangement of the LRR domain relative to the NTF2L domain was conserved between models, whereas the position of the UBA domain was variable. |
3.3. RNA binding of ctMex67–Mtr2
Fluorescence anisotropy assays (Fig. 8) showed that ctMex67–Mtr2 bound all four RNA tested (A15/U15/C15/G15) in vitro but with different affinities. Similar to that from S. cerevisiae, ctMex67–Mtr2 bound polyA15 and polyG15 (Kd of 350 and 310 nM, respectively) more strongly than polyU15 and polyC15 (Kd of 930 and 6.0 µM, respectively). Removal of the UBA domain did not reduce the affinity significantly and the observed Kd for ctMex67ΔUBA–Mtr2 (370 nM) was indistinguishable from that for the complete complex (350 nM). However, deletion of either the RRM domain or the NTF2L–Mtr2 region reduced the affinity more than 15-fold. Thus, the Kd for the ctMex67LRR-NTF2L–Mtr2 (RRM domain deletion) was 6.8 µM, whereas that for ctMex67RRM-LRR (NTF2L–Mtr2 region deletion) was 5.5 µM. These data indicated that as in S. cerevisiae (Aibara, Valkov et al., 2015) the RRM, LRR and NTF2L–Mtr2 regions all contribute to RNA binding by ctMex67–Mtr2. Indeed, the RRM domain and the NTF2L–Mtr2 region appeared to contribute roughly equally, since removal of either reduced the affinity for polyA15 RNA by ∼15-fold. This result contrasts with scMex67–Mtr2, where removal of the RRM domain had a smaller impact on the binding than removal of the NTF2L–Mtr2 region (Aibara, Valkov et al., 2015). The apparent differences in the contributions of the RRM and NTF2L domains may reflect differences between organisms, since Liker et al. (2000) showed that although hsNXF1RRM-LRR bound RNA in vitro the equivalent scMex67 construct did not. Similarly, the NTF2L–Mtr2 region of scMex67–Mtr2 has been proposed to have extended loops that contribute to binding (Yao et al., 2008) but which are absent in hsNXF1–NXT1. The observation that ctMex67RRM-LRR showed a stronger affinity for RNA than that observed with scMex67RRM-LRR, whereas the NTF2L–Mtr2 region appeared to make a smaller contribution, suggests that from the perspective of RNA binding ctMex67–Mtr2 may be more similar to hsNXF1–NXT1. The structure of scMex67ΔUBA–Mtr2 (Aibara, Valkov et al., 2015; PDB entry 4wwu) indicated that a continuous RNA-binding interface could be generated from the way in which the LRR and NTF2L domains of Mex67 assumed a defined three-dimensional arrangement through interactions with Mtr2. Although this arrangement has not directly been observed for ctMex67–Mtr2 using X-ray crystallography, binding assays identifying interactions between RNA and the NTF2L–Mtr2 region in addition to the RRM and LRR domains are consistent with ctMex67–Mtr2 adopting a similar conformation to generate an extended positively charged region to mediate RNA binding.
![[Figure 8]](mn5088fig8thm.gif) | Figure 8 (a) Fluorescence anisotropy assays using ctMex67ΔN–Mtr2. Data were fitted to the standard quadratic binding equation to obtain Kd values. All four RNA tested were bound, albeit with different affinities. Similar to scMex67–Mtr2, ctMex67ΔN–Mtr2 bound polyA15 and polyG15 more tightly than polyU15 and polyG15. (b) Deletion of either the RRM or NTF2L–Mtr2 domains reduced the affinity of ctMex67 by >15-fold. On the other hand, deletion of the UBA domain from ctMex67ΔN–Mtr2 did not reduce the affinity towards polyA15 RNA significantly. Curves reproduced from (a) are shown as dotted lines without data points. |
In summary, the crystal structures of all four domains of C. thermophilum Mex67–Mtr2 provide atomic resolution information on the Mex67–Mtr2 complex from a single species and indicate that although there is only low sequence identity in some regions within this family of nuclear-export proteins, the folds of the four domains are conserved, demonstrating the highly structurally conserved nature of the NXF family. C. thermophilum Mex67–Mtr2 retained features found in both S. cerevisiae and H. sapiens and conserved the hydrophobic pocket identified as the nucleoporin-binding site found in NTF2L domains from other organisms. The position of the pre-α1 loop, which has been implicated in the spatial arrangement of the Mex67 domains in S. cerevisiae, occupied a similar position in ctMex67NTF2L to that observed in S. cerevisiae and H. sapiens. Notably, Leu368 was positioned in a structurally equivalent position to scMex67Leu263 and hsNXF1Leu370, indicating that the NTF2L pre-α1 loop position may be conserved across species (Fribourg et al., 2001; Aibara, Katahira et al., 2015; Aibara, Valkov et al., 2015). The homodimeric complex of NTF2L domains in the ctMex67LRR-NTF2L crystals was unanticipated because it had been thought that complex formation between Mex67 and Mtr2 was a prerequisite for efficient nuclear export of (Santos-Rosa et al., 1998). Although SEC-MALS indicated that ctMex67LRR-NTF2L is homodimeric in solution, whether Mex67 is ever not complexed to Mtr2 in vivo is currently unclear and whether the configuration observed simply represents an inactive form of the Mex67–Mtr2 complex or whether homodimeric Mex67 has another role in the cell has yet to be established.
Supporting information
PDB references: Mex67 RRM, 4wpm; Mex67 UBA, 4wp2; Mex67 NTF2L, 4wp5; Mex67 LRR, 4wp6; Mtr2, 4x2m; Mex67 LRR+NTF2L, 4xm4
Supplementary figures. DOI: https://doi.org/10.1107/S2053230X15008766/mn5088sup1.pdf
Footnotes
‡Present address: Department of Biochemistry, Max Planck Institute for Developmental Biology, Spemannstrasse 35, 72076 Tübingen, Germany.
Acknowledgements
This work was supported by the Medical Research Council (U105178939 to MS) and a Wellcome Trust Programme grant (MS). Conflict of interest statement: none declared. We are most grateful to Stephen McLaughlin and Chris Johnson for assistance with biophysical measurements, Rafael Leiro for SAXS data collection and to our colleagues for their assistance and advice.
References
Adams, P. D. et al. (2010). Acta Cryst. D66, 213–221. Web of Science CrossRef CAS IUCr Journals Google Scholar
Aibara, S., Katahira, J., Valkov, E. & Stewart, M. (2015). Nucleic Acids Res. 43, 1883–1893. CrossRef PubMed Google Scholar
Aibara, S., Valkov, E., Lamers, M. & Stewart, M. (2015). Nucleic Acids Res. 43, 1927–1936. CrossRef PubMed Google Scholar
Bayliss, R., Leung, S. W., Baker, R. P., Quimby, B. B., Corbett, A. H. & Stewart, M. (2002). EMBO J. 21, 2843–2853. Web of Science CrossRef PubMed CAS Google Scholar
Bock, T. et al. (2014). Nucleic Acids Res. 42, 13525–13533. Web of Science CrossRef CAS PubMed Google Scholar
Braun, I. C., Rohrbach, E., Schmitt, C. & Izaurralde, E. (1999). EMBO J. 18, 1953–1965. CrossRef PubMed CAS Google Scholar
DiMaio, F., Terwilliger, T. C., Read, R. J., Wlodawer, A., Oberdorfer, G., Wagner, U., Valkov, E., Alon, A., Fass, D., Axelrod, H. L., Das, D., Vorobiev, S. M., Iwaï, H., Pokkuluri, P. R. & Baker, D. (2011). Nature (London), 473, 540–543. Web of Science CrossRef CAS PubMed Google Scholar
Emsley, P., Lohkamp, B., Scott, W. G. & Cowtan, K. (2010). Acta Cryst. D66, 486–501. Web of Science CrossRef CAS IUCr Journals Google Scholar
Evans, P. R. & Murshudov, G. N. (2013). Acta Cryst. D69, 1204–1214. Web of Science CrossRef CAS IUCr Journals Google Scholar
Fribourg, S., Braun, I. C., Izaurralde, E. & Conti, E. (2001). Mol. Cell, 8, 645–656. Web of Science CrossRef PubMed CAS Google Scholar
Fribourg, S. & Conti, E. (2003). EMBO Rep. 4, 699–703. CrossRef PubMed CAS Google Scholar
Grant, R. P., Neuhaus, D. & Stewart, M. (2003). J. Mol. Biol. 326, 849–858. Web of Science CrossRef PubMed CAS Google Scholar
Grüter, P., Tabernero, C., von Kobbe, C., Schmitt, C., Saavedra, C., Bachi, A., Wilm, M., Felber, B. K. & Izaurralde, E. (1998). Mol. Cell, 1, 649–659. PubMed Google Scholar
Herold, A., Suyama, M., Rodrigues, J. P., Braun, I. C., Kutay, U., Carmo-Fonseca, M., Bork, P. & Izaurralde, E. (2000). Mol. Cell. Biol. 20, 8996–9008. CrossRef PubMed CAS Google Scholar
Hobeika, M., Brockmann, C., Gruessing, F., Neuhaus, D., Divita, G., Stewart, M. & Dargemont, C. (2009). J. Biol. Chem. 284, 17575–17583. CrossRef PubMed CAS Google Scholar
Kabsch, W. (2010). Acta Cryst. D66, 125–132. Web of Science CrossRef CAS IUCr Journals Google Scholar
Keedy, D. A., Williams, C. J., Headd, J. J., Arendall, W. B., Chen, V. B., Kapral, G. J., Gillespie, R. A., Block, J. N., Zemla, A., Richardson, D. C. & Richardson, J. S. (2009). Proteins, 77, 29–49. CrossRef PubMed CAS Google Scholar
Kerkow, D. E., Carmel, A. B., Menichelli, E., Ambrus, G., Hills, R. D. Jr, Gerace, L. & Williamson, J. R. (2012). J. Mol. Biol. 415, 649–665. CrossRef CAS PubMed Google Scholar
Konarev, P. V., Volkov, V. V., Sokolova, A. V., Koch, M. H. J. & Svergun, D. I. (2003). J. Appl. Cryst. 36, 1277–1282. Web of Science CrossRef CAS IUCr Journals Google Scholar
Leidig, C., Bange, G., Kopp, J., Amlacher, S., Aravind, A., Wickles, S., Witte, G., Hurt, E., Beckmann, R. & Sinning, I. (2013). Nature Struct. Mol. Biol. 20, 23–28. CrossRef CAS Google Scholar
Liker, E., Fernandez, E., Izaurralde, E. & Conti, E. (2000). EMBO J. 19, 5587–5598. CrossRef PubMed CAS Google Scholar
Liu, X., Zhang, H., Wang, X.-J., Li, L.-F. & Su, X.-D. (2011). PLoS One, 6, e24227. CrossRef PubMed Google Scholar
Maignan, S., Guilloteau, J.-P., Zhou-Liu, Q., Clément-Mella, C. & Mikol, V. (1998). J. Mol. Biol. 282, 359–368. CrossRef CAS PubMed Google Scholar
Maris, C., Dominguez, C. & Allain, F. H.-T. (2005). FEBS J. 272, 2118–2131. CrossRef PubMed CAS Google Scholar
McCoy, A. J., Grosse-Kunstleve, R. W., Adams, P. D., Winn, M. D., Storoni, L. C. & Read, R. J. (2007). J. Appl. Cryst. 40, 658–674. Web of Science CrossRef CAS IUCr Journals Google Scholar
Monecke, T., Haselbach, D., Voss, B., Russek, A., Neumann, P., Thomson, E., Hurt, E., Zachariae, U., Stark, H., Grubmüller, H., Dickmanns, A. & Ficner, R. (2013). Proc. Natl Acad. Sci. USA, 110, 960–965. Web of Science CrossRef CAS PubMed Google Scholar
Pasquinelli, A. E., Ernst, R. K., Lund, E., Grimm, C., Zapp, M. L., Rekosh, D., Hammarskjöld, M. L. & Dahlberg, J. E. (1997). EMBO J. 16, 7500–7510. CrossRef CAS PubMed Google Scholar
Pelikan, M., Hura, G. L. & Hammel, M. (2009). Gen. Physiol. Biophys. 28, 174–189. Web of Science CrossRef PubMed CAS Google Scholar
Santos-Rosa, H., Moreno, H., Simos, G., Segref, A., Fahrenkrog, B., Panté, N. & Hurt, E. (1998). Mol. Cell. Biol. 18, 6826–6838. CAS PubMed Google Scholar
Schneidman-Duhovny, D., Hammel, M. & Sali, A. (2010). Nucleic Acids Res. 38, W540–W544. Web of Science CAS PubMed Google Scholar
Schneidman-Duhovny, D., Hammel, M., Tainer, J. A. & Sali, A. (2013). Biophys. J. 105, 962–974. Web of Science CAS PubMed Google Scholar
Segref, A., Sharma, K., Doye, V., Hellwig, A., Huber, J., Lührmann, R. & Hurt, E. (1997). EMBO J. 16, 3256–3271. CrossRef CAS PubMed Google Scholar
Stewart, M. (2010). Trends Biochem. Sci. 35, 609–617. CrossRef CAS PubMed Google Scholar
Svergun, D. I. (1992). J. Appl. Cryst. 25, 495–503. CrossRef Web of Science IUCr Journals Google Scholar
Teplova, M., Wohlbold, L., Khin, N. W., Izaurralde, E. & Patel, D. J. (2011). Nature Struct. Mol. Biol. 18, 990–998. Web of Science CrossRef CAS Google Scholar
Thierbach, K., von Appen, A., Thoms, M., Beck, M., Flemming, D. & Hurt, E. (2013). Structure, 21, 1672–1682. CrossRef CAS PubMed Google Scholar
Valkov, E., Dean, J. C., Jani, D., Kuhlmann, S. I. & Stewart, M. (2012). Biochim. Biophys. Acta, 1819, 578–592. CrossRef CAS PubMed Google Scholar
Viphakone, N., Hautbergue, G. M., Walsh, M., Chang, C.-T., Holland, A., Folco, E. G., Reed, R. & Wilson, S. A. (2012). Nature Commun. 3, 1006. CrossRef Google Scholar
Wiegand, H. L., Coburn, G. A., Zeng, Y., Kang, Y., Bogerd, H. P. & Cullen, B. R. (2002). Mol. Cell. Biol. 22, 245–256. CrossRef PubMed CAS Google Scholar
Wilkie, G. S., Zimyanin, V., Kirby, R., Korey, C., Francis-Lang, H., Van Vactor, D. & Davis, I. (2001). RNA, 7, 1781–1792. PubMed CAS Google Scholar
Word, J. M., Lovell, S. C., LaBean, T. H., Taylor, H. C., Zalis, M. E., Presley, B. K., Richardson, J. S. & Richardson, D. C. (1999). J. Mol. Biol. 285, 1711–1733. Web of Science CrossRef CAS PubMed Google Scholar
Yao, W., Lutzmann, M. & Hurt, E. (2008). EMBO J. 27, 6–16. CrossRef PubMed CAS Google Scholar
Yao, W., Roser, D., Köhler, A., Bradatsch, B., Bassler, J. & Hurt, E. (2007). Mol. Cell, 26, 51–62. CrossRef PubMed CAS Google Scholar
This is an open-access article distributed under the terms of the Creative Commons Attribution (CC-BY) Licence, which permits unrestricted use, distribution, and reproduction in any medium, provided the original authors and source are cited.
| STRUCTURAL BIOLOGY COMMUNICATIONS |
