The HIV capsid mimics karyopherin engagement of FG-nucleoporins

HIV can infect non-dividing cells because the viral capsid can overcome the selective barrier of the nuclear pore complex and deliver the genome directly into the nucleus1,2. Remarkably, the intact HIV capsid is more than 1,000 times larger than the size limit prescribed by the diffusion barrier of the nuclear pore3. This barrier in the central channel of the nuclear pore is composed of intrinsically disordered nucleoporin domains enriched in phenylalanine–glycine (FG) dipeptides. Through multivalent FG interactions, cellular karyopherins and their bound cargoes solubilize in this phase to drive nucleocytoplasmic transport4. By performing an in vitro dissection of the nuclear pore complex, we show that a pocket on the surface of the HIV capsid similarly interacts with FG motifs from multiple nucleoporins and that this interaction licences capsids to penetrate FG-nucleoporin condensates. This karyopherin mimicry model addresses a key conceptual challenge for the role of the HIV capsid in nuclear entry and offers an explanation as to how an exogenous entity much larger than any known cellular cargo may be able to non-destructively breach the nuclear envelope.

All retroviruses establish infection by converting their single-stranded RNA into double-stranded DNA and integrating it into host chromatin in the nucleus.For most retroviruses, mitosis provides the opportunity to interact with chromosomal DNA during nuclear envelope breakdown.However, lentiviruses, which include HIVs, have evolved to infect non-dividing cells.To do so, these viruses must navigate the gatekeeper of nuclear entry, the nuclear pore complex (NPC).
The human NPC is a 110 MDa complex composed of 30 different nucleoporin proteins (Nups), which occur in stoichiometries ranging from eight to 48 copies per NPC 5 .Movement through the NPC central transport channel is restricted by size.The vast majority of proteins larger than around 40 kDa must recruit karyopherins to facilitate their nuclear transport 3 .The selectivity barrier in the central channel gating nuclear entry is formed from intrinsically disordered Nup domains that are enriched in phenylalanine-glycine (FG) motifs.These FG-repeat domains are found in around one third of Nups (FG-Nups) and contribute in excess of 5,800 individual FG motifs to a single NPC.
The ability of HIV to infect non-dividing cells maps to the capsid protein (CA) 1 .CA self-assembles into a metastable lattice to form a closed 'shell' of around 40 MDa that contains the genomic RNA and viral enzymes.Although the CA lattice was originally thought to disassemble shortly after entry into the host cell, it is now broadly accepted that its integrity is vital for cellular trafficking and reverse transcription, and for protecting the viral genome from cytoplasmic nucleic acid sensors and nucleases [6][7][8] .Furthermore, recent imaging studies have captured intact capsids as they transit the NPC 2 and have demonstrated intact capsids in the nucleus [9][10][11][12][13] .
Critically, it has been unclear how the HIV capsid can overcome the selectivity barrier of the NPC when it is more than 1,000 times greater in size than the passive diffusion limit.Transporters in the karyopherin family can carry large cargoes through the NPC by specifically interacting with the FG motifs of the diffusion barrier.The efficiency of this cargo transport relies on the presence of multiple FG-binding sites on the karyopherin.The interactions are highly specific but weak and with rapid exchange kinetics, enabling the karyopherin and its bound cargo to partition into the selectivity barrier and rapidly diffuse through the NPC 4 .Cocrystal structures have shown that the HIV capsid exterior also possesses an FG-binding pocket, which recruits the cellular cofactors Sec24C 14 , Nup153 (ref.15), and cleavage and polyadenylation specificity factor subunit 6 (CPSF6) 16 .Although these proteins are structurally distinct and found in different cellular compartments, each of their interactions with the HIV capsid depends on an FG motif that buries itself into a pocket in the CA amino-terminal domain.
between the HIV capsid and cellular proteins 17 .In brief, putative binders are expressed as GFP fusions in a cell-free system.After the addition of fluorescent capsid-like particles (CLPs; CA A204C cross-linked assemblies labelled with Alexa Fluor 568), binding is determined by two-colour coincidence detection as individual CLPs pass through a confocal volume generating fluorescence fluctuations (for gel electrophoresis images of cell-free and recombinant proteins, see Supplementary Figs. 1 and 2; for sequences of all proteins used, see Supplementary Table 2; and for cryo-electron tomography (cryo-ET) images of all CLPs used, see Extended Data Fig. 1).Observations are made directly in the cell-free extract, which we have found to be a powerful approach for screening difficult-to-purify putative capsid binders such as the highly disordered FG-Nups.Furthermore, the use of CLPs as the binding platform has three critical advantages: (1) CLPs show a mix of cone, tube and sphere morphologies bearing both CA hexamers and pentamers, and therefore they present all possible CA interfaces; (2) the presence of a CA lattice gives high sensitivity to the measurement by physically concentrating binders on the CLP, thereby enabling detection of interactions well below the dissociation constant (K d ); and (3) the CLP lattice can engage binders that rely on multivalent CA contacts to make detectable capsid interactions.This assay therefore provides a platform for systematic investigation of potentially weak but specific CA:Nup interactions for all FG-Nups across the NPC.
To 'dissect' the NPC, we individually expressed GFP fusions of the ten FG-repeat NPC components (Nup42, Nup50, Nup54, Nup58, Nup62, Nup98, Nup153, Nup214, Nup358 and Pom121; each with 5-42 FG motifs), along with Nup35, Nup88 and Nup133, which do not have FG-repeat domains (for details, see Extended Data Table 1 and Supplementary Information).We also included known CA binders CPSF6, CypA and the cyclophilin domain of Nup358 (Nup358 3044-3224 ).For Nups that did not express as full-length proteins, we either truncated the transmembrane domain (Pom121 266-1249 ) or expressed only the FG-repeat domain (Nup98 1-499 , Nup214 1210-2090 ).Nups either remained as monomeric protein (as exemplified by POM121, Fig. 1a, flat blue trace) or spontaneously oligomerized (as exemplified by Nup98, Fig. 1b, fluctuating blue trace).This latter behaviour was not unexpected, given that FG-repeat proteins are known to phase separate in vitro 18 .Binding was identified by the recording of 'mirror plots' after the addition of CLP (Fig. 1a,b and Extended Data Fig. 2, orange traces, represented as negative values for clarity), showing that capsid and Nup were colocated.The degree of coincidence is reported as the 'Nup/CLP intensity ratio' 17 .The positive controls (CPSF6, CypA and Nup358 3044-3224 ) were recruited to the CA lattice as expected (Extended Data Fig. 2), whereas the non-FG-repeat Nups (Nup35, Nup88 and Nup133) showed no detectable binding (Fig. 1c,d and Extended Data Fig. 2).Of the monomeric Nups, those with the most FG motifs in unstructured FG domains, Nup58 (14 FGs), Pom121 (24 FGs) and Nup214 (42 FGs), showed the clearest CLP binding (Fig. 1c and Extended Data Fig. 2), whereas Nup62 (six FGs) also bound.A similar trend was observed for the oligomeric Nups, with Nup42 (12 FGs), Nup153 (29 FGs) and Nup98 (40 FGs) all binding (Fig. 1d and Extended Data Fig. 2).When we accounted for stoichiometry, the seven Nups that showed CLP binding were found to contribute 83% of the total FG-repeat motifs in the NPC (Fig. 1e).Furthermore, these Nups were found to be distributed throughout the NPC, including in the cytoplasmic filaments (Nup42, Nup62, Nup98 and Nup214), the central transport channel (Nup58, Nup62, Nup98 and Pom121) and the nuclear basket (Nup153) (Fig. 1f).The clear coincidence between CLPs and Nup98 was particularly striking, as this Nup is present at 48 copies per NPC, making it the most significant contributor of FGs to the diffusion barrier.

FG repeats bind a specific pocket on CA
FG-containing peptides are known to have different capsid-binding modes.Previous crystal structures have shown that the short peptides Nup153 1407-1423 and CPSF6 313-327 bury their respective FG motifs in the CA N-terminal domain.Although these FG motifs are conformationally identical, the peripheral interactions differ.Nup153 1407-1423 adopts a linear conformation that bridges two CA monomers, whereas CPSF6 313-327 forms a more compact structure that packs predominantly against a single CA protomer (Fig. 2a).Notably, in both cases, CA residue N57 forms two critical hydrogen bonds with the main-chain NH and O of the buried phenylalanine.Mutation of CA N57 therefore disrupts binding of both cofactors.However, mutation of residue N74 or A77 only disrupts CPSF6 binding, leaving Nup153 unaffected 16 .CLP mutants (N57D, N74D or A77V) reproduced these binding specificities in our FFS assay (Fig. 2b,c and Extended Data Fig. 3), whereas binding of a CypA control was unaffected by these mutations, demonstrating these CLPs to be otherwise competent for assembly and binding (Extended Data Fig. 3).
To investigate how the capsid recognizes FG repeats, we examined interactions of CA mutants with our identified binders (Nup-42 full-length , Nup58 full-length , Nup62 full-length , Nup98 1-499 , Pom121 266-1249 and Nup214 1210-2090 ).These FG-Nups demonstrated similar profiles to the Nup153-peptide (Fig. 2d-i and Extended Data Fig. 4).In each case, binding was significantly reduced by N57D but unaffected (and possibly even  1).*Due to its size, the FG domain of Nup358 was expressed as two fragments, as denoted by the dotted line.f, HIV capsid interacts with Nups distributed throughout the NPC.Nups identified to bind to CLPs are highlighted in bold.n, number of scans per sample.

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enhanced) by N74D or A77V.The results obtained with these CLP mutations indicate that the FG-Nups interact with CA N57 in the FG-binding pocket, and that the binding footprints more closely resemble that of Nup153 1407-1423 than that of CPSF6 313-327 .These observations may explain why capsid N74D and A77V (CPSF6-binding mutants) retain the ability to infect non-dividing cells 8,15,[19][20][21] , as they maintain FG interaction and use of the NPC, whereas N57 mutants (FG-binding mutants) are dependent on cell division for maximal infectivity 15,20 .
Nup98, Pom121 and Nup214 have distinct domain architectures, each possessing a clearly defined FG-repeat domain with 44, 24 and 40 FG motifs, respectively (Fig. 2j).To determine whether the FG domains were solely responsible for CA binding, we performed side-by-side FFS measurements comparing the FG and non-FG domains.Strikingly, binding was observed for all three FG domains, whereas there was no detectable interaction for any non-FG domain (Fig. 2k and Extended Data Fig. 5).To probe whether binding was driven predominantly by specific FG-containing motifs (as is the case for Nup153 (refs.15,16)), we chose the strongest binder, Nup98, and further dissected the FG domain into three regions, each containing 13 FGs.Each of the three FG-repeat fragments bound robustly to the wild-type capsid but not N57D (Fig. 2l and Extended Data Fig. 5).CLP interaction with representative Nup98 peptides containing only a single FG motif (representing both GLFG and FGFG types) was below the detection limit for FFS (Fig. 2l), indicating that capsid binding to Nup98 may be driven by weak but FG-specific interactions enhanced by multivalency.

CA exhibits karyopherin-like properties
Direct interaction between CA and the FG-Nups indicates that the HIV capsid may engage with the diffusion barrier of the NPC.Furthermore, these interactions are reminiscent of the low-affinity multivalent FG binding exhibited by karyopherins, which are uniquely capable of crossing the FG-rich diffusion barrier along with their bound cargoes.
A key advance in the understanding of karyopherin-mediated transport came with the observation that isolated FG-Nups spontaneously form liquid-liquid phase-separated condensates that retain the selective properties of the diffusion barrier of the NPC 18,22 .Although seminal for a mechanistic understanding of nucleocytoplasmic transport, these FG-Nup condensates have not previously been used to study viral nuclear entry.We therefore sought to produce them to explore the interplay between the HIV capsid and the NPC diffusion barrier.Nup98 was chosen as our model system, as it plays a vital part in maintenance of the integrity of the NPC 23 and contributes the most FGs (Fig. 1e), and, among the phase-separating FG-Nups, it produces condensates that most accurately recapitulate the selectivity properties of the diffusion barrier in vitro 18,24,25 .Notably, of the Nups, Nup98 was also the clearest CA binder in our FFS assay (Fig. 1b,d).
We produced the unstructured FG domain of Nup98 (residues 1-499) under denaturing conditions and observed spontaneous formation of spherical, phase-separated condensates (average diameter 1.3 µm) after shock dilution into aqueous buffer (see Methods for details).We tested these condensates for their selective properties by mixing them immediately after formation (when they still maintained liquid-like characteristics) with mCherry fused to the importin-β-binding domain of importin-α (IBB-mCherry).IBB-mCherry (33 kDa) was excluded from the Nup98 phases (Fig. 3a and Extended Data Fig. 6) but was transported into the condensates within minutes of addition of importin-β (Fig. 3b and Extended Data Fig. 6).These results demonstrate that our Nup98 condensates exhibit two essential functions of the NPC permeability barrier, passive exclusion and karyopherin-facilitated transport.Furthermore, the addition of importin-β did not result in uptake of wild-type mCherry (27 kDa; Extended Data Fig. 6), showing that the presence of importin-β does not affect the size-selective properties of the Nup98 condensates.To test whether CA could also enter the FG-Nup phase, we fused mCherry to the carboxyl terminus of CA (CA-mCherry, 52 kDa).At the concentrations used in our assay (45 µM), we expected CA-mCherry to exist in equal amounts as monomer and dimer (K d approximately 40 µM) 26 , with the latter carrying two

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FG-binding sites.Strikingly, CA-mCherry rapidly partitioned into the Nup98 condensates (Fig. 3c and Extended Data Fig. 6), whereas diffusion into the condensate was almost entirely abolished after N57A mutation (Fig. 3d,g and Extended Data Fig. 6).Next, we produced a cysteine cross-linked hexamer (CA hexamer -mCherry) 27 carrying an average of one CA-mCherry per hexamer.At 182 kDa, this construct is well beyond the size limit for passive diffusion across the NPC but presents six FG-binding sites appropriately positioned relative to their neighbouring CA protomers.Again, we observed CA hexamer -mCherry partitioning into the condensates (Fig. 3e and Extended Data Fig. 6), an effect that was again significantly reduced by N57A (Fig. 3f,g and Extended Data Fig. 6).
To further probe the functional relevance of the FG-binding pocket, we sought to test whether known cofactors could compete for CA binding and therefore influence Nup penetration.The recently developed drug lenacapavir binds the FG pocket but was not amenable to study in our systems as it resulted in CA clustering, consistent with its known overassembly effect 28 .As an alternative, we used the host cofactor CPSF6, which had no such confounding effects.CPSF6 313-327 peptide preferentially binds to CA hexamer (K d = 50 µM) over unassembled CA (K d approximately 700 µM) 16 .As expected, pretreatment with 500 µM CPSF6 313-327 had no observable effect on CA-mCherry (Extended Data Fig. 7), whereas it abolished the ability of CA hexamer -mCherry to partition into the Nup98 condensates (Fig. 3h,j and Extended Data Fig. 7).This effect was specific to the interaction with the FG pocket, because CPSF6 313-327 had no effect on CA(N74D) hexamer -mCherry, which does not bind CPSF6 313-327 (Fig. 3i,j and Extended Data Fig. 7).Posttreatment with CPSF6 313-327 also removed CA hexamer -mCherry from the Nup98 condensates.These effects of CPSF6 support the role of the FG-binding pocket in mediating capsid entry into Nup98 condensates; moreover, the pretreatment and posttreatment results indicate that competing cofactors may be able to influence both NPC engagement and disengagement.Indeed, these results are consistent with the proposed 'ratchet' mechanism by which CPSF6 extracts the capsid from the nuclear face of the NPC 9 .
Whereas these results indicate that CA may be able to enter the NPC autonomously, previous studies have suggested that the karyopherins importin-α3 (ref.29), transportin-1 (TNPO1) 30 and transportin-3 (TNPO3) 31 each play a part in HIV-1 nuclear entry through a direct interaction with the capsid.However, we observed no specific binding between capsid and importin-α, TNPO1 or TNPO3 by FFS (Extended Data Fig. 8).Furthermore, rather than enhancing CA entry into Nup98 condensates, these karyopherins reduced entry under our experimental conditions (Extended Data Fig. 8), consistent with the prediction that CA and karyopherins would compete for FG binding and therefore have a similar mechanism of action.Notably, a fully assembled capsid with more than 1,000 FG-binding sites is likely to be a much stronger competitor for the FG motifs than CA hexamers.Thus, we argue that our observation of CA penetrating FG condensates and facilitating the entry of an mCherry pseudo-cargo demonstrates that the HIV capsid protein possesses intrinsic karyopherin-like properties and can function independently of the canonical nucleocytoplasmic transport factors.

HIV capsids enter Nup98 condensates
To chaperone the viral genome and enzymes across the nuclear envelope, the HIV capsid must be capable of entering the NPC intact.To investigate the FG-Nup-penetration properties of complete capsids, we induced coassembly of CA(A204C) with CA(A204C)-mCherry at a ratio of 200:1.These fluorescent CLPs formed the expected heterogeneous mix of lattice structures that model the pleiomorphic capsids found in HIV virions (Extended Data Fig. 1).Confocal microscopy showed that after the addition of CLPs, fluorescent puncta were recruited to the periphery of the Nup98 condensates (Fig. 4a and Extended Data Fig. 9) but could not resolve whether these structures had penetrated the condensates, nor whether the structural integrity of closed CA cones or spheres was maintained after entry.
To examine whether complete HIV-1 capsids can penetrate the Nup98 condensates, we turned to cryo-ET, a technique that (in contrast to previous measurements) also allowed us to study CA-Nup98 condensate interactions in a label-free context.We ensured that the condensates were electron transparent by reducing the Nup98 concentration, resulting in smaller condensates (diameter 400 nm to 1 µm), which we imaged with and without CLPs introduced immediately before freezing.In the absence of CA, Nup98 condensates had a uniform, featureless internal texture, consistent with a phase-separated, intrinsically disordered protein (Fig. 4b and Extended Data Fig. 9).Strikingly, after addition of wild-type CLP to preformed Nup98 condensates, we observed internalized pleomorphic substructures, including conical structures similar to authentic HIV capsids (Fig. 4c,d and Extended Data Fig. 9).These structures carried an electron-dense exterior with evidence of a repetitive lattice structure.Internal negative space confirmed that wild-type CLPs were empty, showing that the integrity of the CLPs was not affected even when they were fully immersed in the FG-motif-dense condensates.Conversely, CLPs carrying the N57D mutation were not internalized and were observed either at the surface of the Nup98 condensates or in the bulk solution (Fig. 4e-g).Furthermore, the median penetration depth of wild-type CLPs was 65 nm (Fig. 4h), which is greater than the 50 nm required to cross the central transport channel of the NPC 32 .These results show that complete HIV capsids have properties that enable them to sufficiently penetrate and enter the key material of the diffusion barrier of the NPC, specifically via the FG-binding pocket, while preventing disordered Nups from infiltrating the capsid interior.

Discussion
There are several reasons the HIV:NPC interaction has remained poorly understood.In cellulo approaches can be confounded by both the essentiality of the Nup genes and the complex interactome of the NPC.Protein depletion approaches may be incomplete and/or result in changes in the abundance and/or mislocalization of other Nups, whereas pulldown assays can yield false positives owing to Nup-Nup interactions 19 .Nevertheless, more than one third of Nups have previously been implicated in various aspects of the HIV lifecycle using these methods 15,19,20,[33][34][35][36][37] (Supplementary Table 1).Despite similar approaches, the consistency with which specific Nups are identified varies considerably.By performing an in vitro screen of the CA:Nup interactions, we have circumvented the cellular challenges to show that the capsid specifically engages with the multitude of FG motifs found within the NPC diffusion barrier.Notably, we observe interactions with Nups located in the cytoplasmic filaments, throughout the central transport channel and in the nuclear basket, implying that capsid:Nup interactions can, in principle, occur at all points along the translocation pathway.FG repeats have been classified into two main types based on the residues immediately upstream, FxFG/FG and GLFG.We observe that the HIV capsid interacts with both.The two types are thought to segregate in the NPC, with FxFG/FG repeats enriched at the cytoplasmic and nuclear peripheries, and GLFG repeats enriched in the central channel where they function as the main component of the diffusion barrier 5 .The only GLFG-containing Nup in the human NPC is Nup98, which is thus a crucial barrier that any foreign entity must overcome to enter the nucleus.It is therefore striking that Nup98 is the clearest CA binder in our assays and that Nup98 condensates readily take up HIV capsids.
Structural studies of karyopherins have shown that they possess multiple surface pockets for binding FG dipeptides, and it is these FG interactions that enable karyopherins and their bound cargoes to selectively cross the diffusion barrier.Several karyopherins have been shown to interact directly with FG motifs of Nup42, Nup62, Nup98, Nup153 and Nup214 (refs.38-42); notably, all of these Nups have been identified as CA binders in our study.The remarkable structural and functional similarities between CA:Nup and karyopherin:Nup interactions imply that rather than engaging with host nuclear transport receptors, the HIV capsid has evolved to become the karyopherin for the protected HIV genome.
The reductionist system of Nup98 condensates allows us to demonstrate the principle of FG-mediated phase partitioning and probe the specific sites on the capsid that permit it to be a client of these phases.We acknowledge that the human NPC is one of the most complex macromolecular assemblies known.The diffusion barrier itself has defied a consensus physicochemical description owing to its intrinsic disorder, multicomponent composition and tethered nano-environment [43][44][45] .Indeed, although it is at present one of the best-known examples of a demixed aqueous environment in the cell, the nuanced complexity means that experimental models are always approximations and limitations should be recognized when extrapolating precise details concerning nuclear entry 25 .In the case of HIV, the concept that the capsid has the ability to partition into FG-containing liquid-liquid phases has several important implications for viral infection.In such a framework, molecular weight does not represent a barrier to nuclear entry.Any assembly should be able to enter the nucleus provided that its dimensions do not exceed those of the central transport channel and that it is not excluded from the FG-Nup phase.Notably, recent cryo-ET images of intact HIV-1 capsids travelling through nuclear pores showed that the central channel can become wider than previously thought to accommodate the width of the complete capsid 2 .On the basis of a combination of these cryo-ET studies with our work presented here, the HIV capsid satisfies both criteria of appropriate size and penetration capability.
Furthermore, the collective effects of FG interactions can be recast in terms of surface energies and, in the simple case of the threefold intersection between capsid-condensate, capsid-cytosol and condensate-cytosol interfaces, a wetting angle.This is important because alongside the geometries of the capsid and the central transport channel, the surface energies determine the capillary forces that act on the capsid 46 , with potential to shed light on how capsids orient relative to the NPC, and possibly explain why, among the retrovirus family, only those that traverse the NPC (that is, the lentiviruses) adopt a conical capsid morphology.
The HIV capsid is also likely to encounter other cellular compartments that could be described as phase separated.One of the bestcharacterized capsid binders, CPSF6, is known to partition into membraneless compartments in the nucleus, where it plays an essential part in targeting HIV integration 6,47,48 .Impairment of the CA:CPSF6 interaction (through A77V, N74D mutations or CPSF6 knockdown 9,11,13,49 ) results in arrest of CA at the nuclear membrane and integration at the nuclear periphery, indicating that the capsid may not be able to properly disengage from the NPC.Furthermore, cytoplasmic mislocalization of CPSF6 (through either ectopic expression of CPSF6 lacking a nuclear localization signal or depletion of the dedicated CPSF6 karyopherin, TNPO3) prevents the HIV capsid from entering the nucleus 6,50 .Our data are consistent with a model in which cytoplasmic CPSF6 competes for FG-Nup binding, thereby preventing nuclear entry, while nuclear CPSF6 helps to extract the capsid out of the NPC into the nucleus and directs it towards the sites of active transcription before integration.It is worth noting that endogenous karyopherins similarly require assistance to disengage from the NPC.Importin-β, for example, is released from the NPC by Ran-GTP 51 .Thus, nuclear CPSF6 probably has an analogous release function in the karyopherin mimicry model of capsid-mediated nuclear entry.We also note that Nups can be found in other compartments of the cell, such as annulate lamellae, and in condensates in the nucleus 52 .Although their relevance to HIV is yet to be established, our data indicate that non-canonical Nup function could potentially influence early infection.
Whether the HIV capsid maintains its structural integrity while embedded in FG-containing phases (the NPC or CPSF6-rich compartments such as speckle-associated domains) remains an open question.Furthermore, it has been proposed that the capsid ultrastructure may remodel after transit of the NPC 2,11,53 .Although we have not explicitly addressed this question with our cross-linked capsid model, the high concentration of FGs in the NPC (more than 100 mM 4 ) indicates that many FG pockets are likely to be occupied simultaneously.High occupancy of the FG pocket with capsid-targeting drug lenacapavir or related compound PF74 affects capsid integrity and CA lattice stability 54 .It is therefore conceivable that effects observed only near saturation (such as changes to the capsid ultrastructure) may indeed take place during NPC transit and/or after arrival in CPSF6-containing nuclear compartments.The role of phase partitioning in HIV uncoating has not previously been considered and will probably provide key insights into this enigmatic process.
In summary, we propose a model in which the HIV capsid mimics the karyopherin mechanism of transiting the NPC by solubilizing in the diffusion barrier through specific, multivalent FG interactions.This mechanism of nuclear entry is likely to be conserved in other medically important viruses, which may prove to be treatable by a strategy analogous to the use of lenacapavir in HIV.Certainly, further study of the HIV capsid will continue to provide a paradigm for viral infection and nuclear transport mechanisms and reveal opportunities for improving lentiviruses as gene delivery vectors, along with new therapeutic approaches that may be extended to unrelated viruses.

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Constructs
Nup42, Nup50, Nup54, Nup62, Nup88, Nup133 and Nup214 in the pDONR221 gateway master vector were purchased from DNASU and cloned into the cell=free expression vector pCellFree_03 (ref.55), using the Gateway method, to produce fusion proteins with an N-terminal GFP tag (see Supplementary Table 2 for details).Nup35, Nup58, Nup98, Nup358 and Pom121 were cloned from complementary DNA (cDNA) prepared from HEK293T cells.Briefly, RNA was extracted using an Isolate II RNA mini kit (Bioline), and cDNA was synthesized using oligo(dT) primers and SuperScript IV (Thermo Fisher Scientific).Target genes were then cloned into pCellFree_03 using the Gibson assembly protocol (New England Biolabs).Nup98 and Pom121 fragments were purchased as gBlocks from IDT and cloned into pCellFree_03.pET28a vectors containing mCherry2-Nup98 fragments, as well as pGEX-6P-3 vectors containing importin-α, TNPO1 and TNPO3 were purchased from GenScript.Cell lines (HEK239T) were only used for cDNA preparation in this study, with gene identity subsequently confirmed by Sanger sequencing.

Protein expression and purification
HIV-1 CA proteins.HIV-1 CA proteins (K158C, A204C, R18G/A204C, N57D/A204C, N74D/A204C, N77V/A204C) were expressed in Escherichia coli C41 or Rosetta2 cells and purified as previously described 56 .HIV-1 CA K158C was labelled with Alexa Fluor 568-C5-maleimide (AF568, Thermo Fisher Scientific, A20341) and mixed in an approximately 1:200 ratio with unlabelled HIV-1 CA A204C before assembly.CA lattice assembly was carried out as described by Lau et al. 17 with the modification of a 15 min incubation at 37 °C and no overnight incubation.CA hexamer , CA hexamer -mCherry and CA-mCherry were purified based on previously described protocols 27 .Briefly, CA hexamer , CA hexamer -mCherry (pOPT) and CA-mCherry (pET21a) were expressed in E. coli C41 cells.Cells were grown at 37 °C, protein expression was induced with 0.5 mM isopropyl β-d-1-thiogalactopyranoside (IPTG) at an optical density of 0.6, and cell growth was continued overnight at 18 °C.Cells were collected (4,000g, 10 min, 4 °C), and the cell pellets were resuspended in lysis buffer (purification buffer 50 mM Tris pH 8, 50 mM NaCl, 2 mM dithiothreitol (DTT); +cOmplete EDTA-free Protease Inhibitor (Roche)) and lysed by sonication.The lysate was cleared by centrifugation (16,000g, 60 min, 4 °C), and an ammonium sulfate (20% w/v) precipitation was carried out on the soluble fraction.After stirring for 30 min at 4 °C, the precipitated material was pelleted (16,000g, 20 min, 4 °C).CA hexamer was further purified by resuspending the pellet in 100 mM citric acid pH 4.5, 2 mM DTT and dialysed against the same buffer three times.The precipitated protein was pelleted (16,000g, 20 min, 4 °C), and the soluble fraction was collected for further purification.CA hexamer -mCherry and CA-mCherry could not be purified with citric acid precipitation owing to a possible loss of mCherry fluorescence.The ammonium-sulfate-precipitated pellets were resuspended in 8 ml purification buffer per litre culture, run over a 20 ml Hi-TRAP Q column in purification buffer and eluted in a 1-100% gradient with buffer B (50 mM Tris pH 8, 500 mM NaCl).Protein-containing fractions were pooled.
CA-mCherry was further purified by gel filtration (Superdex 200 in purification buffer), and fractions containing clean protein were pooled and snap frozen to be stored at −80 °C.
To assemble the final cross-linked hexameric CA hexamer -mCherry, CA hexamer and CA hexamer -mCherry were mixed in a 5:1 ratio and assembled by means of the following dialysis steps: twice against 50 mM Tris pH 8, 1,000 mM NaCl, 2 mM DTT; twice against 50 mM Tris pH 8, 1,000 mM NaCl; and twice against 50 mM Tris pH 8, 40 mM NaCl.The assembled CA hexamer -mCherry was finally purified with gel filtration (S200), and fractions containing hexameric CA hexamer -mCherry carrying one mCherry were pooled and snap frozen to be stored at −80 °C.
Cell-free expression.Cell-free expression of GFP fusion proteins was performed as described by Lau et al. 17 .Briefly Leishmania tarentolae extract was supplemented with RnaseOUT (1:1,000, Invitrogen) on ice.pCellFree_03-Nup plasmids (150 ng µl −1 ) were then added to the expression mix, followed by incubation at 27 °C for 3 h.Following incubation, the undiluted extract was mixed 1:1 with NuPAGE LDS loading buffer (Thermo Fisher Scientific), 10 mM DTT, and the purity and degradation of the expressed Nup were assessed by sodium dodecyl sulfate polyacrylamide gel electrophoresis in-gel fluorescence.
Importin-β, IBB-mCherry, Nup98.The mCherry protein was kindly provided by J. Goyette.Importin-β and IBB-mCherry in pET11a (Gen-Script) were expressed as His-fusion proteins in E. coli Rosetta2 cells.Cells were grown at 37 °C, protein expression was induced with 0.5 mM IPTG at an optical density of 0.6, and cell growth was continued overnight at 18 °C.Cells were collected (4,000g, 10 min, 4 °C), and the cell pellets were resuspended in lysis buffer (purification buffer: 20 mM Tris pH 7.5, 150 mM NaCl, 2 mM DTT; +cOmplete EDTA-free Protease Inhibitor (Roche)) and lysed by sonication.The lysate was cleared by centrifugation (16,000g, 45 min, 4 °C), and the supernatant was bound to Ni-beads (Ni Sepharose High Performance, Cytiva) preincubated in purification buffer; then, imidazole was added to the protein-Ni slurry to a final concentration of 10 mM, and the mixture was incubated for 2 h at 4 °C.The beads were washed with 20 column volumes of wash buffer (purification buffer + 20 mM imidazole) and eluted in 2 ml fractions with elution buffer (purification buffer + 500 mM imidazole).Protein-containing fractions were pooled, and cleavage of the His-tag was achieved with TEV (IBB-mCherry) or SUMO (importin-β) in overnight dialysis against TEV-cleavage buffer (50 mM Tris pH 7.5, 1 mM DTT) or SUMO-cleavage buffer (50 mM Tris pH 7.5, 150 mM NaCl, 1 mM DTT).Cleaved proteins were added to Ni-beads, and the flow-through was collected.Proteins were finally purified by size-exclusion chromatography (SEC; Hi Load16/60 Superdex 200) in purification buffer.Clean protein fractions were pooled and snap frozen to be stored at −80 °C.Nup98 in pET28a was purified as described above with the following changes: the buffers used were purification buffer (6 M GuHCl, 50 mM TrisHCl pH 7.5, 2 mM DTT), wash buffer (6 M GuHCl, 20 mM imidazole pH 8) and elution buffer (500 mM GuHCl, 500 mM imidazole pH 8).After induction with IPTG, cells were grown further for 3 h at 30 °C before being collected.Sufficient purity of the protein was achieved with affinity chromatography; consequently, no SEC was performed.The His-tag was not removed.The protein-Ni slurry was stored at 4 °C for phase-separation assays.

Fluorescence fluctuation spectroscopy
FFS was performed as described by Lau et al. 17 .Briefly, cell-free expressed GFP-Nup proteins (approximately 50 nM; equivalent to approximately 2,500 photon count) or AF488 peptides (100 nM) were mixed with AF568-HIV-1 CA assemblies (12 µM) in 50 mM Tris, pH 8, 150 mM NaCl.Fluorescence traces were recorded for 15 s per trace in 1 ms bins using a scanning stage operated at 1 µm s −1 .Typically, measurements were repeated 10-15 times per sample.
Determining the number of FGs in relative solvent accessibility FG motif accessibility was determined by calculating per-residue relative solvent accessibility (RSA) from AlphaFoldDB structures to determine order and disorder 57 .RSA-based order and disorder for all Nups except Nup358 were accessed through Mobi-DB 58 .
Owing to the length of Nup358, AlphaFold2 predictions were performed as three FG-containing sections (982-2004, 2005-3043 and 3058-3224), with their per-residue RSA-based disorder propensity calculated locally.Binary designations of order and disorder were assigned using a threshold optimized on Critical Assessment of Protein Intrinsic Disorder (CAID) data (0.581) 57 .

Phase separation
For phase-separation assays, the Nup98-saturated Ni slurry ('Protein Expression and Purification'; Nup98 binding capacity Ni-beads 40 mg ml −1 medium) was mixed with Alexa Fluor 488-C5-maleimide (AF488, Thermo Fisher Scientific; final concentration 10 µM), followed by incubation for 5 min.We aimed for as little labelling with AF488 as possible with enough signal to noise to avoid confounding effects from the fluorophore for phase separation.The slurry was washed with 10 column volumes of wash buffer 2 (500 mM GuHCl, 20 mM imidazole pH 8) + 2 mM DTT, followed by a second wash step with wash buffer 2 without DTT to remove the DTT and residual fluorophore.The labelled protein was eluted with elution buffer for a final protein concentration of approximately 4 mg ml −1 (estimated from sodium dodecyl sulfate polyacrylamide gel electrophoresis against a bovine serum albumin standard), and phase separation of Nup98 was induced by 1:10 shock dilution into assay buffer (50 mM Tris pH 7.5, 150 mM NaCl).We observed the most 'fluid' condensates using shock dilution; these condensates 'hardened' within minutes of forming, as tested with an importin-β:IBB-mCherry control.This resulted in limited equilibration of the condensates with some fluorescent substrates (for example, as seen for CA hexamer -mCherry).Fluorescent substrates were added to the phase-separated Nup98 condensates and immediately imaged.
Nup98 condensate-CA experiments were performed with mCherry-labelled CA (CA-mCherry and CA hexamer -mCherry), as it has previously been reported that fluorescent dyes such as Alexa568 can non-specifically interact with Nup condensates 59 .
Experimental details for Fig. 3h,i and Extended Data Figs.8-10: for the CPSF6 P preincubation sample, CA-mCherry, CA hexamer -mCherry and CA N74D hexamer -mCherry (65 µM final) were incubated with CPSF6 (500 µM final) for 10 min, followed by mixing with Nup98 condensates and imaging after around 5 min incubation on the coverslip.The control sample and the CPSF6 postincubation sample were incubated with MQW for 10 min, followed by mixing with Nup98 condensates and imaging after around 5 min incubation on the coverslip.For the CPSF6 postincubation sample, CPSF6 was added to the sample on the coverslip and imaged after 5, 10, 15 and 20 min.
Experimental details for Fig. 4 and Extended Data Fig. 9b-d: CLP-mCherry was assembled with a ratio of 1:100 CA-mCherry (final 0.4 µM) to CA (final 40 µM) by addition of NaCl (final 1 mM) and 15 min incubation at 37 °C.After assembly, the sample was spun down hard (18,000g, 7 min) to separate the assemblies from non-assembled monomer.The pellet was resuspended in assay buffer (50 mM Tris pH 7.5, 150 mM NaCl; resuspension volume the same as the original sample volume), followed by a slow spin of the resuspended pellet (4,000g, 5 min) to remove aggregates.Nup98 condensates were immediately mixed with CA-mCherry assemblies (1 µM monomer concentration) and imaged after around 5 min incubation on the coverslip.

Radial intensity profiles
Averaged radial intensity profiles were obtained using the plugin Radial Profile in ImageJ.Z-slices were chosen at the centres of the phase-separated Nup98 condensates (position with largest diameter).Profiles were background subtracted.The edge of a condensate was defined from the 488 channel as the first intensity value greater than 5.Then, 200 nm was subtracted from this value to account for point spread function of the fluorescent pixel.This point was defined as point 0 µm in the radial averaged intensity graphs (Fig. 3 and Extended Data Figs.6-8).

Cryo-electron microscopy
Nup98 condensates were prepared as for confocal microscopy with the following modifications.To induce the formation of smaller condensates, the unlabelled Nup98 was diluted two-fold in 500 mM GuHCl, 500 mM imidazole pH 8, before a 1:10 shock dilution into assay buffer (50 mM Tris pH 7.5, 150 mM NaCl).
Unlabelled CLPs were prepared as described above.A two-step centrifugation protocol was performed as for confocal microscopy.Equal volumes of CLP suspension were mixed with freshly shock-diluted condensates, immediately before to plunge freezing to minimize sample aggregation.
Frozen-hydrated sample preparation.A mixture (4.5 µl) of freshly mixed Nup98 condensate and capsid with protein A-gold (10 nm) was applied onto a glow-discharged Quantifoil R2/2 copper grid (Quantifoil Micro Tools).The grid was blotted in the front for 2.5 s at 15 °C with 90% relative humidity and then plunged into liquid ethane using a Lecia EM GP device (Lecia Microsystem).The vitrified grids were then stored in liquid nitrogen before cryo-ET imaging.
Cryo-ET imaging and reconstruction.The grids were imaged on a Talos Arctica electron microscope (Thermo Fisher Scientific) operated at 200 kV acceleration voltage.Cryo-ET data were collected with single-axis tilt on a Falcon III direct electron detector (Thermo Fisher Scientific) in linear mode at a magnification of ×28,000 with a pixel size of 5.23 Å. Tilt series were collected using the dose-symmetric scheme 60 from −60 to 60° at 3° intervals using Tomography software (Thermo Fisher Scientific) with the defocus value set to −10 µm.Total dose for each tilt series ranged from 60-70 e/Å 2 .Images of tilt series were binned two-fold before tomograms were reconstructed.Three-dimensional reconstructions from tilt series were generated with the IMOD package 61 .Fiducial tracking was used to align the stack of tilted images.

Statistics and reproducibility
Confocal microscopy images and graphs in Fig. 3 and Extended Data Figs.6-8 show representative data from at least three independent experiments with similar results.Confocal microscopy images in Fig. 4a and Extended Data Fig. 9 are representative of three independent experiments with similar results.Cryo images and graphs in Fig. 4b-h and Extended Data Fig. 9 show representative data from two independent experiments with similar results.

Reporting summary
Further information on research design is available in the Nature Portfolio Reporting Summary linked to this article.f-k, Single z-plane images (cyan, 488-Nup channel; magenta, protein-mCherry channel) of CA hexamer -mCherry (f) or CA (N74D) hexamer -mCherry (l) without CPSF6, with CPSF6 pre-incubated 10 min (g and j), with CPSF6 post-incubated 20 min (h and k).Background subtracted radially averaged fluorescence intensity across condensates for 488-Nup channel (cyan) and protein-mCherry channel (magenta).Mean intensity curves shown in bold.Scale bar 5 µm (main), 1 µm (inset).N = number of condensates analysed per sample.Error bars show standard deviation of the mean.Statistical test for panel e is one-way ANOVA.

Fig. 1 |
Fig. 1 | FG-Nups bind to the HIV-1 capsid.a,b, FFS traces of GFP-Pom121 (a) and GFP-Nup98 (b), alone or mixed with AF568 CLPs (blue, Nup channel; orange, CLP channel).c,d, Nup/CLP fluorescence intensity ratios calculated for monomeric (c) and oligomeric (d) Nups (grey background denotes canonical FG-repeat Nups with the number of FG motifs per Nup in parentheses).Error bars indicate the standard deviation of the mean.e, Relative FG motif contributions to the diffusion barrier based on published Nup stoichiometries (see also Extended Data Table1).*Due to its size, the FG domain of Nup358 was expressed as two fragments, as denoted by the dotted line.f, HIV capsid interacts with Nups distributed throughout the NPC.Nups identified to bind to CLPs are highlighted in bold.n, number of scans per sample.

Fig. 4 |
Fig. 4 | Intact HIV-1 CLPs penetrate Nup98 condensates via FG-binding pocket.a, CLP-mCherry assemblies (punctae) recruited to Nup98 condensates.Single z-plane images for 488 nm (cyan), 568 nm (magenta) and composite.Scale bar, 500 nm.b,c,e, Representative slices from cryo-ET images of Nup98 alone (b), in the presence of CLP WT (c) and or CLP N57D (e).Scale bars, 100 nm.d,f, Zoomed images from c (d) and e (f), showing an average of five slices with a total thickness of 5.2 nm.Scale bars, 100 nm.g, Populations (n) of WT and N57D CLPs excluded from (light grey) or partitioned into (dark grey) condensates.h, Penetration depths of (n) CLP WT, measured from the edge of eight unique condensates.

Extended Data Fig. 2 |Extended Data Fig. 7 |
FFS data for CLPs and interactors.a, FFS trace of AF568-CLP (orange).b, Coincidence heatmaps used to calculate NUP:CLP fluorescence intensity ratios for Pom121 and Nup98 (Fig.1c and d).Representative FFS traces are shown in Fig.1a and b. d, e and f, FFS traces for GFP-binders in the absence and presence of AF568-CLP and heat maps of binder to CLP fluorescence intensity used to calculate fluorescence intensity ratios in c, and Fig. 1c and d.Blue, Nup channel; orange, CLP channel.Error bars show standard deviation of the mean.N=number of scans per sample.Extended Data Fig. 3 | FFS data for known cofactors with wild-type and mutant CLPs.a, FFS traces for GFP-controls in the absence and presence of wild-type and mutant AF568-CLPs.Blue, Nup channel; orange, CLP channel.b, Corresponding coincidence heatmaps used to calculate NUP:CLP fluorescence intensity ratio in c and Fig. 2b, c.Error bars show standard deviation of the mean.N=number of scans per sample.Extended Data Fig. 4 | FFS data for Nup binders with wild-type and mutant CLPs.a, FFS traces for GFP-Nups in the absence and presence of wild-type and mutant AF568-CLPs.Blue, Nup channel; orange, CLP channel.b, Corresponding coincidence heatmaps used to calculate NUP:CLP fluorescence intensity ratio in Fig. 2d, e, f, and g.Extended Data Fig. 5 | FFS data for Nup fragments with wild-type CLP and CLP N57D.a-d, FFS traces and associated coincidence heatmaps for truncation constructs of GFP-Nup214 (a), GFP-Pom121 (b), GFP-Nup98 (c), and AF488-Nup98 peptides in the absence and presence of AF568-CLP (WT or N57D) (d).e as a-d, with mCherry2-Nup98 fragments and AF569-CLP.For all FFS traces: blue, Nup channel; orange, CLP channel.Extended Data Fig. 6 | Confocal fluorescence microscopy (all channels) with Nup98 condensates and mCherry labelled controls or CA-constructs.a-h, Single z-plane images (cyan, 488-Nup channel; magenta, protein-mCherry channel) of control fusion protein IBBmCherry (a), control complex Importinβ:IBBmCherry (b), unassembled CA-mCherry (c), unassembled CA-mCherry carrying FG pocket mutation N57A (d), cross-linked CA hexamer-mCherry (e), cross-linked CA hexamer-mCherry carrying N57A (f), mCherry (g) and control Importin-β and mCherry (h).Background subtracted radially averaged fluorescence intensity across condensates for 488-Nup channel (cyan) and protein-mCherry channel (magenta).Mean intensity curves shown in bold.Scale bar 5 µm (main), 1 µm (inset).N = number of condensates analysed per sample.Confocal fluorescence microscopy (all channels) of Nup98 condensates and CA-mCherry, CA hexamer -mCherry or CA (N74D) hexamer -mCherry in the presence of CPSF6.a-c, Single z-plane images (cyan, 488-Nup channel; magenta, protein-mCherry channel) of CA-mCherry without CPSF6 (a), with CPSF6 pre-incubated for 10 min (b), with CPSF6 postincubated 20 min (c).d, Background subtracted radially averaged fluorescence intensity across condensates for 488-Nup channel (cyan) and protein-mCherry channel (magenta).Mean intensity curves shown in bold.Scale bar 5 µm (main), 1 µm (inset).e, Intensity values (568) at 400 nm from edge of condensates.

Fig. 9 |
Confocal fluorescence microscopy (all channels) and cryo-electron tomography of CLPs bound and partitioned into Nup98 condensates.a, Confocal fluorescence microscopy images of CLPs (puncta) recruited to Nup98 condensates.Single z-plane images for 488 nm (cyan), 568 nm (magenta) and composite.Scale bar 500 nm.b-d, Representative slices from cryo-electron tomograms of Nup98 alone (b), in the presence of CLP WT (c), or CLP N57D (d).Scale bars 100 nm.Tomograms are binned by 2 and displayed as an average of 5 slices with a total thickness of 5.2 nm.