Active DNA unwinding and transport by a membrane-adapted helicase nanopore

Nanoscale transport through nanopores and live-cell membranes plays a vital role in both key biological processes as well as biosensing and DNA sequencing. Active translocation of DNA through these nanopores usually needs enzyme assistance. Here we present a nanopore derived from truncated helicase E1 of bovine papillomavirus (BPV) with a lumen diameter of c.a. 1.3 nm. Cryogenic electron microscopy (cryo-EM) imaging and single channel recording confirm its insertion into planar lipid bilayer (BLM). The helicase nanopore in BLM allows the passive single-stranded DNA (ssDNA) transport and retains the helicase activity in vitro. Furthermore, we incorporate this helicase nanopore into the live cell membrane of HEK293T cells, and monitor the ssDNA delivery into the cell real-time at single molecule level. This type of nanopore is expected to provide an interesting tool to study the biophysics of biomotors in vitro, with potential applications in biosensing, drug delivery and real-time single cell analysis.

Helicases play a vital role for all living organisms to unpackage their genes fueled by ATP hydrolysis 23,24 . The BPV E1 protein is a hexamer helicase from bovine papillomavirus (BPV). It has a central pore with lumen diameter of 1.1-1.5 nm 25 . The wild-type BPV E1 contains N-terminal domain (residues 1-141), DNA binding domain (DBD) (residues 142-307), helicase domain (residues 308-577), and C-terminal domain (residues 578-605) 26,27 . BPV E1 helicase plays an important role in the virus genome replication, during the unwinding process, the helicase moves along the one strand of the dsDNA in the direction of 3′-5′ powered by ATP hydrolysis. BPV E1 helicase with DBD can bind to the specific sequence of the viral genome DNA (origin of DNA replication) with the assistance of E2 transcription factor and start the unwinding of genomic DNA in vivo. While in vitro, the truncated BPV E1 (without DBD) has no sequence specificity and needs single strand arm of dsDNA for the binding and unwinding 28 . The 28-aa peptide C-terminal is important for the E1 complex formation 27 .
Single-molecule studies provide a powerful tool revealing the detailed dynamics of biomotors, including DNA unwinding process by helicases, such as optical tweezers 29 , fluorescence resonance energy transfer (FRET) microscopy 30,31 , nanopore 32 , and DNA curtains 33 . The real-time study on kinetics of enzyme at high spatial resolution and time resolution have been reported on motor proteins, including helicase 21,34 , polymerase 20 , and other proteins such as exonuclease I 35 , and single-base resolution at the single-molecule level could be realized 20 .
Inspired by the structural similarity of helicase E1 from BPV and other hexametric transmembrane channels, here we report that BPV E1 can be truncated into a helicase nanopore and inserted into a planar lipid bilayer. Its membrane compatibility has been studied with liposome vesicles using cryo-EM, reconstitution into planar lipid bilayer by single channel recording. In high-salt conditions ssDNA could be transported based on an external applied voltage, while in physiological conditions dsDNA containing a single-stranded arm could be unwound and transported through the helicase nanopore in a way that is comparable with helicase activity in vitro. And meanwhile, this helicase nanopore is introduced to cell electrophysiology realizing realtime ssDNA transfection into a HEK293T cell as well as macromolecule extraction from inside the cell. The helicase nanopore enables potential applications in single-molecule enzyme kinetics, biosensing, and live cell analysis in situ.

Results
Construction of the helicase nanopore and membrane fusion. The hexametric BPV E1 possesses a nanoscale lumen and shares structural similarities with commonly used protein nanopores such as MspA and α-hemolysin, except that there is no transmembrane domain in BPV E1. To evaluate the possibility of reconstructing a membrane-adapted helicase nanopore based on BPV E1, the electrostatic surface was shown in Fig. 1a, b and the hydrophobic residues were shown in green in Supplementary  Fig. 1. It could be observed that more hydrophobic residues spread over the middle of the facing the N-terminal (panel b left), which may facilitate the adhesion and insertion of the protein into the lipid bilayer membrane. In order to increase its solubility in aqueous solution, a glutathione S-transferase (GST)-tag was added to the N-terminal. In this study, two kinds of truncated BPV E1 protein containing 306-577 fragment (BPV E1 helicase domain) and 306-605 fragment (BPV E1 helicase domain and C-terminal tail) were reconstructed with N-terminal GST fusion protein into pGEX-6P-1 plasmid and expressed in Escherichia coli (E. coli), respectively (Supplementary Table 1, Fig. 2a, b). Both expressed proteins were purified by size exclusion chromatography ( Supplementary Fig. 2c, d) and then identified by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) (Fig. 1c). Compared with E1 306-577 (with GST-tag) and E1 306-605 (with GST-tag cleaved) which tended to precipitate, E1 306-605 with GST-tag was more stable. Hence, we chose truncated E1 306-605 protein with GST-tag as helicase nanopore in the following studies unless otherwise specified.
To verify whether the helicase nanopore could be inserted into the lipid bilayer membrane or not (as shown in Fig. 1d), we prepared proteoliposome vesicles containing the helicase nanopore for cryo-EM characterization (Fig. 1e, Supplementary Fig. 3). Synthetic lipid diphytanoyl phosphatidylcholine (DPhPC) was used in this study for vesicle and planar lipid bilayer preparation unless otherwise specified. High resolution images of 67 helicase nanopores from 45 independent images were collected and analyzed, and red solid lines and blue dashed lines highlighting the bilayer membrane and helicase nanopore, respectively were provided in the insets. Compared with the control sample of blank liposome (Fig. 1e left), those proteoliposome vesicle images provided direct evidences of helicase nanopore insertion into lipid bilayer membrane (Fig. 1e right). Further detailed analysis was performed on the 67 membrane-embedded helicase nanopores. The perpendicular orientation of the helicase nanopore to the membrane plane was strongly preferred, with majority of the helicase nanopore tilting close to vertical from the membrane ( Supplementary Fig. 4a). As shown in Supplementary  Fig. 4b, the numbers of inserted/attached helicase nanopore from outside the vesicles and from inside the vesicles were close. It can be concluded that about half of the helicase nanopores were attached on the bilayer surface (similar to the truncated α-hemolysin pores 36 ), and another half were inserted into the bilayer with varying depths (Supplementary Fig. 4c). Statistical analysis revealed a relatively wide distribution of inserted lengths of the helicase nanopores into vesicle membrane (4.7 ± 0.6 nm, the error bars indicated standard deviation in this work unless otherwise specified, Supplementary Fig. 4d), and 83.5% of the insertion were N-terminal incorporation ( Supplementary Fig. 4e). These observations and analysis provided interesting information of the interaction of helicase nanopore with bilayer membranes in proteoliposome vesicles.
ssDNA translocation through the helicase nanopore in BLM. The conductivity of the helicase nanopore in the lipid bilayer was performed using a single channel conductance assay setup 11 (Fig. 2a). Solution containing the helicase nanopore (final concentration of 2-10 ng/mL) was added to the buffer solution in the cis-side of the BLM chambers, which was connected to the ground electrode. When a single helicase nanopore was inserted into the membrane, an instantaneous current increase can be observed as shown in a current trace under either a positive or negative bias voltage (Fig. 2b, 0.5 M KCl, 5 mM HEPES, pH 7.5). Occasionally, larger current increase was observed as shown in a current recording of 760 s with three pores inserted simultaneously in Supplementary Fig. 5 (bias voltage of +70 mV in the buffer solution of 1 M KCl, 5 mM HEPES, pH 7.5), which could be attributed to the simultaneous insertion of helicase nanopores. The Gaussian fit to the conductance histogram for Fig. 2c gave the peak value of 1.34 ± 0.03 nS in the buffer solution of 1 M KCl, 5 mM HEPES, pH 7.5 under a bias voltage of +70 mV, and was 0.23 ± 0.01 nS in phosphate buffered saline (PBS) (n = 34 from 19 trials). The conductance measurements were also performed under a ramping voltage. The slope from the fitted curve was c.a. 1.3 nS for a single pore in buffer solution of 1 M KCl, 5 mM HEPES, pH 7.5 (Fig. 2d).
We also compared the measured conductance with the value calculated using the equation from Hall 37 . The equation was used on the alpha-hederin 38 nanopore sharing similar lumen characteristics with the helicase nanopore. The variation of the conductance as a function of the diameter can be described as below where σ KCl (11.1 S/m) is the molar conductivity of the electrolyte (1 M KCl), h is the effective thickness of the nanopore, and d is the diameter of the nanopore. Effective mean thicknesses of 6.7 nm and the diameter range from 1.1 to 1.5 nm for helicase nanopore were obtained from its crystal structure 25,28,39 . The calculated conductance for the helicase nanopore in 1 M KCl solution (electrolyte conductivity 11.1 S/m) was 1.39-2.49 nS. This is comparable to the measured conductance value (1.34 ± 0.03 nS). The pore conductance was compared to that of α-hemolysin under the same condition. The membrane insertion efficiency of the helicase nanopores with and without the GST-tag into planar lipid bilayer were tested, where the insertion efficiency was defined as the ratio of number of trials with helicase nanopore inserted into lipid bilayer to the total number of trials. From the statistics of 672 independent trials of single channel recording experiments, the efficiency of insertion was c.a. 44.8% ( Supplementary Fig. 6). The results showed that the helicase nanopore with GST-tag (253 out of 494 trials, 51.2%) was more membrane-compatible than that without GST-tag (48 out of 178 trials, 27.0%). Supplementary  Fig. 7 showed the scatter diagrams of the time consumption of the helicase nanopore insertion and the duration time of helicase nanopore embedded in BLM. We also investigated the helicase nanopore insertion using E. coli total lipid extract besides DPhPC. Under similar experiment conditions, two types of lipid component showed similar insertion efficiency and membrane stability.
To verify the capability of ssDNA translocation through the helicase nanopore, we added ssDNA (sequence A of 48 nt, Supplementary Table 2) into the buffer solution to cis-chamber  Table 2) could induce a large number of current blockages after a single pore insertion (Fig. 2e). The residual current of the blockage events could be obtained by I r = I o − I b , where I r represented the residual current when the pore was blocked, I b was the blocked current, and I o was the open pore current. Analysis of the current blockage events indicated that the ssDNA caused both distinct blockage events, and nonspecific spikes due to occasional background noise or ssDNA random collision with the helicase nanopore. Under +50 mV in 0.5 M KCl buffer solution, Gaussian fitting of these current blockage events gave the peak value of (I b /I o ) 81.850 ± 0.001% (Fig. 2f) and a mean dwell time of 1.1 ± 0.2 ms (Fig. 2g). After changing the bias voltage to +100 mV, the events frequency increased with a mean dwell time of 0.64 ± 0.02 ms (Fig. 2h) and a peak value of 80.5 ± 0.5% (Fig. 2i). This is comparable to the report that oligo-ssDNA immobilized inside the lumen of α-hemolysin induced current blockages ranging from 50% to 90% due to the different compositions of nucleotides 40 .
In order to verify that the resistance pulse-like blockage events appearing in the current traces were indeed caused by ssDNA, a nuclease degradation experiment was implemented. Interestingly, when DNase I was added into the cis-chamber (0.25 µg/mL) following the addition of ssDNA (Sequence B of 80 nt, 200 nM), the large number of transient blockages decreased after 20 min, and hardly signals could be observed after 50 min (0.5 M KCl, 5 mM HEPES, pH 7.5, under +50 mV, Supplementary Fig. 8). This result confirmed that the blockage signals was induced by ssDNA. To rule out the impact of nonspecific event signals brought by transient binding and dissociation, we carried out additional concentration-dependent ssDNA translocation experiments ( Supplementary Fig. 9, 0.5 M KCl, 5 mM HEPES, pH 7.5). As shown in panel a and b, with ssDNA concentration increased from 25 pM to 25 nM, the translocation events frequency showed linear increase. Moreover, with the bias voltage increased from +50 to +100 mV, the dwell time of blockage events and interevent gap time reduced significantly while the events frequency increased (panels c-e). The frequency of DNA translocation through protein nanopore could be increased by augmenting the internal positive charge of the nanopore 41 , and it was interesting to found that the frequency of ssDNA translocation events through the helicase nanopore was higher compared with α-hemolysin even with internal positive charge augment under similar condition 41 . The reason for faster DNA capture rates could be attributed to the nature of the virus-derived helicase motor to process and unwind dsDNA in host cell during infection, in contrast to the bacteria derived pore-forming toxin nanopores. These data demonstrated that the blockage signals were attributed to ssDNA translocation rather than random collisions.
The above results confirmed that the helicase nanopore could be inserted into the lipid bilayer membrane similar to other reported protein nanopores with the ability of passive translocation of ssDNA driven by electric field force.
Unwinding of dsDNA by the helicase nanopore in vitro. It is reported that BPV E1 belongs to the super family 3 (SF3) class of helicases, and DNA enter the BPV E1 helicase in the direction of 3′-5′ 28 . We measured the unwinding activity of the helicase nanopores by in vitro helicase assay 42 . A dsDNA substrate was designed, with quencher BHQ2 and fluorophore Cy3 at each end of one of its strands (sequence C of 22 bp, structure shown in Supplementary Fig. 10). Totally, 5 nM DNA substrate was incubated with 50 nM helicase nanopore in the reaction buffer at 37°C for 30 min. During the first 10 min, the baseline fluorescence was measured as a background signal. After the addition of 2 mM ATP, the fluorescence gradually decreased due to fluorescence quenching (Fig. 3a). This result can be explained that the helicase motor first bound to the poly-T region of the oligonucleotide followed by ATP hydrolysis-driven unwinding of the duplex region from 3′ to 5′. Once the dsDNA substrate was separated by helicase nanopore, a hairpin formed and the fluorescence of Cy3 was quenched by BHQ2, inducing a fluorescence decrease. This result demonstrated that the helicase nanopore from BPV E1 (306-605, with GST-tag) maintained the capability of unwinding, whereas the BPV E1 (306-605, without GST-tag) and BPV E1 (306-577, with GST-tag) showed no activity ( Supplementary  Fig. 11). Thus, helicase nanopore from BPV E1 (306-605, with GST-tag) was used in the following studies.
Using linear dsDNA with partially complementary sequence possessing a single strand arm (24-bp dsDNA sequence D, structure shown in Supplementary Fig. 10), we investigated whether the helicase nanopore in BLM retains helicase activity or not. In the presence of dsDNA, blockage signals with a current change of c.a. 25 pA can be observed at the voltage of +120 mV (Fig. 3b, buffer condition: PBS, 1.5 mM ATP, 3 mM MgCl 2 , pH 7.0). Interesting patterned steps in an individual signal was observed (Fig. 3c-e). They were fundamentally different from the passive ssDNA translocation events driven by voltage, but similar to the single-channel recording signals induced by the topological variations of DNA complex through a solid-state nanopore 43 . A schematic drawing (top right panel in Fig. 3) was proposed according to the structure of the dsDNA and the function of the helicase nanopore, showing the three stages of dsDNA unwinding and translocation through the helicase nanopore corresponding to the three steps in the current recording events: (1) The capture of the 3′ end of the single strand arm by the helicase nanopore; (2) the unwinding process of dsDNA; and (3) the release of ssDNA. In addition, the number of blockage steps could vary from 1 to 3. A faster velocity of dsDNA unwinding was observed at a higher bias voltage for the 24-bp dsDNA as substrates (Fig. 3f), as well as an increased translocation events frequency (Fig. 3g). To investigate the relationship between dsDNA length and unwinding time, the unwinding of dsDNA of different lengths (Sequence E of 44 bp, Sequence F of 80 bp) by the helicase nanopore inserted in BLM under the same voltage of +120 mV were studied (buffer condition: PBS, 1.5 mM ATP, 3 mM MgCl 2 , pH 7.0). The results demonstrated that longer unwinding time was required for longer dsDNA (Fig. 3h). The calculated unwinding speed for dsDNA was 7 ± 5 bp per 100 ms under +120 mV. The unidirectionality of dsDNA transport through the helicase nanopore was observed. Whenever dsDNA was added to both cis-and trans-side of the chamber, the translocation events could only be observed at one voltage direction ( Supplementary  Fig. 12). Some pores would appear to be inactive while dsDNA was added to one side of chamber. Furthermore, no obvious translocation signals could be observed when the single strand arm was located in 5′ (sequence G of 38-bp dsDNA), thus only the dsDNA with 3′ single strand arm could be transported through the helicase nanopore ( Supplementary Fig. 13).
We performed additional experiments to investigate the role of key factors involved in enzyme kinetics, including Mg 2+ concentration, ATP, and temperature, for dsDNA unwinding through the helicase nanopore. dsDNA (Sequence D of 24 bp, 15 nM) was premixed into the chamber before the helicase nanopore embedded in the BLM (buffer condition: PBS, 1.5 mM ATP, 3 mM MgCl 2 , pH 7.0). The blockage signal was hardly observed while the ATP was absent. After addition of EDTA into the buffer solution, the frequency of dsDNA translocation through the helicase nanopore decreased by 90 ± 9% after a short period of time (Fig. 3i, j), which indicated that Mg 2+ was also required for dsDNA unwinding by the helicase nanopore. For the influence of temperature, dsDNA unwinding frequency decreased by 83 ± 3% at the temperature of 11-14°C compared with the unwinding frequency at the temperature of 30-34°C (Fig. 3k, l). Those results were consistent with the enzyme kinetics of BPV E1 in vivo. In our 52 dsDNA unwinding experiments by the helicase nanopore, 25 of them only showed the occurrence of DNA translocation at a positive voltage, while other 27 experiments only showed DNA translocation/unwinding signal at negative voltage. The result indicated there was no directional preference of the helicase nanopore insertion into the BLM in single channel recording (buffer solution: PBS, pH 7.0) (Supplementary Fig. 14).
Incorporation into live cell membrane and membrane transport. Based on the results of helicase nanopore fusion with vesicle membrane and planar lipid bilayer, we further used patch-clamp technique to study the ability of the helicase nanopore incorporation into live cell membranes 17 . The human embryonic kidney (HEK293T) cell line was chosen for the patch-clamp experiments since the cell line had low endogenous channel activity and was widely used in cell electrophysiology research. A patch pipette containing the intracellular solution and the helicase nanopores was used to approach a single live cell (Fig. 4a). After gigaseal was formed, resistance current pulses and the resulting changes in electrical conductance of the patch were monitored. In successfully patched HEK293T cells, the cell membrane exhibited channel-like activities a few minutes after the helicase nanopore addition through the pipette under −60 mV (18 out of 176 cells, Fig. 4a and Supplementary Fig. 15). The mean conductance of the helicase nanopore was 76 ± 4 pS (Fig. 4b). Meanwhile, control experiments without helicase nanopore in the patch pipette were performed and showed no apparent channel activity under the same voltage (16 out of 16 cells). Those results confirmed the ability that the helicase nanopore could be spontaneously inserted into live cell membranes. The occurrence of successful incorporation of the helicase nanopore into the cell membrane was c.a.  Supplementary  Fig. 16). Analysis of the insertion was shown in Supplementary  Table 3, and the median residence time of the nanopore incorporation on cell membrane was 1.75 s, which was far less than that observed in BLM experiments. These could be attributed to the dynamics of live cell membrane and fusion interaction of the helicase nanopore with the cell. The translocation of ssDNA through the helicase nanopore in live cell membrane was also studied (Fig. 4c). A glass pipette with premixed helicase nanopore (0.9 µM) and ssDNA (Sequence B of 80 nt, 200 nM) was used for cell patch. After current step corresponding to a pore insertion into the membrane was observed under −60 mV (12 out of 98 trials), large amounts of blockage-like events were observed (5 out of 12 cells, Fig. 4c and Supplementary Fig. 17). The mean blockage was 64 ± 8%, and the mean dwell time of the events was 0.9 ± 0.2 ms (Fig. 4d). As a comparison, no obvious changes in conductance were observed in the control experiment (ssDNA was added into the pipette while the helicase nanopore was not added, 20 out of 20 cells). This confirmed the pipette-assisted real-time, single-molecule voltagedriven delivery of ssDNA into an individual live cell through the helicase nanopore.
The helicase nanopore can also be inserted into the cell membrane under positive voltages (8 out of 79 cells, Fig. 4e and Supplementary Fig. 18) and blockage events were also observed (6 out of 8 cells). The mean current blockage of the events from patched cells was 76 ± 3%, and the mean dwell time for most of the translocation events was 0.5 ± 0.3 ms (Fig. 4f). In contrast to the HEK293T cells control which showed no specific blockage events (top trace in Fig. 4e), transient blockage signals were observed in the same experiment condition for a helicase nanopore embedded in the cell membrane (bottom trace in Fig. 4e). Those control experiments revealed that the signals were associated with the cytoplasm in which water, ion and macromolecules were the major content in cytosol. In the setup of a positive charge applied to the electrode outside the cell membrane, negatively charged macromolecules was expected to transport toward the helicase nanopore from inside the cytoplasm, which could be peptides, RNA, or other small biomolecules, etc. Analysis and statistics of the signals showed a dwell time and blockage percentage comparable to that of ssDNA (Panel d and f in Fig. 4). These results indicated the molecular transport toward the artificial membrane channel formed by helicase nanopore on live cell membrane.
We also carried out the study of spontaneous interaction of the helicase nanopore with live cells. Fluorescein isothiocyanate (FITC)-conjugated helicase nanopore was co-incubated with LN-229 cells for 4 h. FITC-conjugated albumin (ALB) was used as a positive control, as it has been reported that ALB can enter into cells using gp60 44 mediation. The nuclei were dyed with 4′,6diamidino-2-phenylindole (DAPI) with blue fluorescence, and the cell membranes were colored by 1,1′-dioctadecyl-3,3,3′,3′tetramethylindocarbocyanine perchlorate (Dil) with red fluorescence. As shown in Fig. 4g (see Supplementary Fig. 19 for complete view), the green fluorescence emitted under the FITC excitation light 45 demonstrated that the labeled helicase nanopore could be inserted into LN-229 cell membranes and entered the cytoplasm (21 out of 29 cells). To assay the cytotoxicity of the helicase nanopore to cells, the Cell Counting Kit-8 (CCK-8) method was used 46 . During the 72 h observation of the cells coincubated with helicase nanopore (0.5 mg/mL), the helicase nanopore did not show noticeable cytotoxicity toward LN-229 cells (Supplementary Fig. 20).
In addition to ssDNA translocating through the membraneadapted helicase nanopore described above, helicase nanopore assisted exogenous ssDNA translocation into live cells in vitro was studied. After incubated with HEK293T cells with both purified helicase nanopore (0.5 mg/mL) and exogenous ssDNA (Sequence B of 80 nt, 110 nM) for 3 h in a cell culture medium which contained extra 2 mM ATP and 5 mM MgCl 2 27 , total DNA from the HEK293T cells was extracted for quantitative polymerase chain reaction (Q-PCR). For control groups of DMEM, ALB, and helicase nanopore only, no amplification of ssDNA was observed. When incubated with ssDNA and ATP, helicase nanopore showed higher amplification level of ssDNA compared with DMEM and ALB. (Fig. 4h). Error bars represented the standard error of mean between three independent experiments. In the case of incubation with ssDNA and without ATP, the amplification of ssDNA was much lower and showed no significant difference with DMEM, ALB, and the helicase nanopore (lower panel of Fig. 4h). Those results proved that the ATP was necessary for ssDNA translocation into cells by the helicase nanopore.

Discussion
Compared with other native membrane channels, the helicase nanopore showed relatively low efficiency of ssDNA internalization into a cell and short residence time at the cell membrane. In order to improve the membrane affinity, further protein engineering is necessary. On the other hand, short residence time on membrane would significantly reduce its toxicity to the cell. Depending on the purpose of application, for example drug delivery, single cell analysis and target therapy to tumor cells, specific interaction could be designed.
In summary, we constructed a helicase nanopore from BPV E1 helicase, and it was reconstituted into lipid bilayer and live cell membranes. It exhibited the ability for passive transport similar to the well-studied protein nanopore, while retaining interesting helicase activity when embedded in BLM. The dynamics and kinetics of the active transport driven by ATP-hydrolysis was revealed by the current trace recording during individual dsDNA unwinding, providing a powerful tool for single-molecule study of biomotors. The helicase nanopore also formed dynamic channels in live cell membrane, and ssDNA could be delivered into the cell and observed in single-cell level. With the low toxicity to cells, it exhibited potential applications in nanopore sensing, drug delivery and single-cell analysis.

Methods
Expression and purification of the helicase nanopore. The construction of BPV E1 genes with residues 306-577 and 306-605 were designed into pEGX-6P-1 vectors and synthetized by GENEWIZ, Inc. China. Briefly, the E1 306-577 and E1 306-605 plasmids were achieved by PCR. Firstly, E1 306-577 was cloned with primer pair F1 and R1 (Supplementary Table 1) at BamH-I and Xho-I sites, and E1 306-605 fragment was obtained by addition of E1 578-605 fragment to E1 306-577 fragment by primer pair F2 and R2 (Supplementary Table 1) at Nsi-I and Xho-I sites. Both two proteins were finally expressed in E. coli as N-terminal GST fusion proteins ( Supplementary Fig. 2). Using the buffer containing 20 mM Tris and 150 mM NaCl (pH 8.0), the GST fusion proteins were purified by glutathione agarose affinity chromatography (20 mM glutathione added to the buffer) and Superdex ™ 200 Increase 10/300 GL column (GE Healthcare). For removal of GSTtag, Prescission Protease (PSP) was added. The uncropped and unprocessed scan of the gel in Fig. 1c is provided as a Source Data file.
Preparation of helicase nanopore proteoliposome vesicles. To prepare the giant lipid vesicles, 0.8 mL of 25 mg/mL 1,2-diphytanoyl-sn glycerol-3-phosphocholine (DPhPC) (Avanti, USA) was added to a 2-mL vial. Chloroform was evaporated using a rotatory evaporator. To rehydrate the lipid film, 2 mL of 200-300 mM sucrose was used to bud the vesicles off the glass and into the solution. The vial was then covered with parafilm and stored overnight. Incorporation helicase nanopore into giant vesicles was accomplished as described above, and a volume of 100 μL of helicase nanopore protein were added to the aforementioned dehydrated lipid.
Cryo-EM specimen preparation and imaging. The preparation of cryo-EM specimens followed a previous study 47 . In brief, an aliquot (~4 mL) of vesical and the helicase nanopore mixture sample at a concentration of~2.5 mg/mL was placed on a glow-discharged holey carbon film-coated copper grid (QUANTIFOIL ® R 2/2, Electron Microscopy Sciences). The samples were blotted with filter paper on both sides at~100% humidity and 4°C with a FEI Vitrobot rapid-plunging device and then flash-frozen in liquid ethane. The flash-frozen grids were transferred into liquid nitrogen for storage. Cryo-EM samples were examined using a FEI Talos F200C TEM operating at 200 kV high tension at −178°C in low-dose mode. A Gatan 626 cryo-holder was used. The micrographs were acquired with a highsensitivity 4 K × K pixel FEI CETA CMOS camera under a magnification of 22-120 kx (each pixel of micrographs corresponded to~0.54-0.10 nm of specimen) under a dose of~10-40 e −1 /Å 2 and a defocus of 1-5 μm. The uncropped and unprocessed of the original cryo-EM images is provided as a Source Data file.
Incorporation into BLM and electrophysiological assay. A bilayer of DPhPC was formed on an aperture (200 μm) in a Teflon partition (25 μm thick) (Eastern Scientific LLC, USA) that divided a planar bilayer chamber into cis and trans compartments (Warner, USA). Planar lipid bilayer was formed using the methods as reported 13 . The aperture (both surfaces) was pre-painted with 0.5 μL 0.5 mg/mL DPhPC n-decane solution twice before loading the buffer, and then painted with 1 μL of 20 mg/mL DPhPC solution in n-decane for bilayer formation. The experiments were performed using a series of symmetrical buffer conditions containing a 2.0-mL solution of various KCl concentrations and 5 mM HEPES (pH 7.5) at 25°C. The helicase nanopore was added to the cis compartment, which was connected to ground electrode and transmembrane voltage was +100 mV. The final concentration of the helicase nanopore was 2-10 ng/mL. Discrete current increase steps could be observed, indicating the incorporation of helicase nanopore into the planar lipid bilayer. Currents were recorded with a patch clamp amplifier (HEKA 10USB, Wiesenstraβe 71 D-67466 Lambrecht/Pfalz. Germany, and Axon 200 B, Molecular Devices, USA). They were low-pass filtered with a Bessel filter at 5 kHz and sampled at 100 kHz by a computer equipped with a Patchmaster 2.65.
ssDNA translocation. During the ssDNA translocation experiments, ssDNA (Sequence A of 48 nt, TaKaRa, Japan) was added to the cis-side or both two chambers, including 5 mM HEPES (pH7.5)/1 M KCl or 0.5 M KCl buffer solution. Two methods were used to add DNA to the chamber for the translocation experiments: (1) DNA was added under a voltage of 0 mV after the nanopore insertion. When the voltage was switched back, the ssDNA moved towards the nanopore via free diffusion of DNA and was driven by bias voltage; (2) DNA was premixed with buffer completely in the chamber before the nanopore insertion.
The DNA movement relied mainly on bias voltage. All ssDNA translocation experiments were performed using the first method.
Nuclease degradation experiments. During the ssDNA translocation experiments through the helicase nanopore, 200 nM (final concentration) ssDNA (Sequence B of 80 nt, TakaRa, Japan) was added into the cis-chamber, which containing symmetric 5 mM HEPES (pH 7.5)/0.5 M KCl buffer solution. When a large number of blockages signals appeared, adding extra 0.25 μg/mL (final concentration) DNase I into the cis-chamber. The experiment was performed at +50 mV at room temperature.
dsDNA unwinding. During the dsDNA unwinding experiment, PBS (pH 7.0) with 3 mM Mg 2+ and 1.5 mM ATP was used as the dsDNA translocation buffer. All the dsDNA (Sequence D of 24 bp; Sequence E of 44 bp; Sequence F of 80 bp; Sequence G of 38 bp) were synthesized by Sangon Biotech (Shanghai) Co., Ltd. The dsDNA was prepared by an annealing process: 95°C for 3 min and the sample was cooled to room temperature slowly for 2 h. Annealed dsDNA was premixed and added into the trans-chamber to a final concentration of 15 nM.
Helicase inhibition assay. Ethylenediaminetetraacetic acid (EDTA) was used in the inhibition assay of the helicase nanopore. EDTA was added into the chamber while the dsDNA was unwinding through the helicase nanopore. The working concentration of EDTA in the chamber was 1 mM.
Cell culture. HEK293T cells (Cell Bank of the Typical Culture Preservation Committee, Chinese Academy of Sciences, Cat. No: SCSP-502) were cultured in high glucose Dulbecco's modified Eagle's medium (DMEM) (Hyclone, USA) with 10% fetal bovine serum (FBS) (Gibco, USA) in a 35-mm culture dish with a 0.8 mm glass slide. The total area of cells could not exceed 30% area of culture dish for follow-up patch clamp experiment. LN-229 cells (ATCC ® CRL-2611 ™ ) were cultured in DMEM containing 5% FBS 50 in culture flask. All the cells were cultured under 37°C with 5% CO 2 (v/v).
Cell electrophysiology. The glass slide containing the cells was set into cellrecording track filled with the following extracellular solution: 145 mM NaCl, 10 mM HEPES, 10 mM glucose, 4 mM KCl, 2 mM CaCl 2 , 1 mM MgCl 2 , pH 7.4. The pipettes were produced by a Sutter P-1000 puller from borosilicate glass (Science Products, GB150-10) and filled with intracellular solution: 150 mM KCl, 1 mM EDTA, 10 mM HEPES, pH 7.4; the resistance of the pipette was 6-9 MΩ. The solution containing helicase nanopores was added into the pipette before each experiment, (dilute to 0.054 mg/mL). The concentration of ssDNA (Sequence B of 80 nt) added in the pipette was 200 nM. The data were obtained and preprocessed by the Axon patch-clamp 700B, V hold , −60 mV and +20 mV, with a 5-kHz sampling rate, and filtered at 2 kHz.
Confocal microscopy imaging. The helicase nanopore was labeled with FITC (FluoroTag™ FITC Conjugation Kit) (Sigma, USA) and the effective tagged helicase nanopore was obtained according to the manufacturer's protocols. The helicase nanopore (0.2 mg/mL) were added into LN-229 cells seeded on Lab-Tek ™ II chamber slides (NUNC, USA) and incubated for 4 h. DAPI (Sigma, USA) and Dil (Sigma, USA) were used to label the nuclei and membranes. After sealing the slides with coverslips and antifade agent (ProLong ® Diamond Antifade Mountants) (Life, USA), the slides were observed under confocal microscopy (Zeiss, Germany).
Exogenous ssDNA translocation into cell in cell culture. For quantitatively analyzing DNA translocation into cells, the Q-PCR method was used. HEK293T cells were incubated with both purified helicase nanopore (0.5 mg/mL) and exogenous ssDNA (Sequence B of 80 nt, 110 nM, Tsingke, China) in DMEM with extra MgCl 2 (5 mM) (Sigma, USA) and ATP (2 mM) (Sigma, USA) for 3 h. Total DNA of HEK293T cells was extracted according to the protocols of the manufacturer (PureLink ® Genomic DNA Kits) (Life, USA). Q-PCR was carried out in the CFX Connect Real-Time System (Bio-Rad, USA) and the samples were prepared according to the protocols of the manufacturer (SYBR ® Premix Ex Taq™ II) (TaKaRa, Japan). The primers were 5′-CTTCC AGGCA TTAGA GAAAA AGGC-3′ (forward) and 5′-TGTTT TGCGA ACTCC CCAAT ACTT-3′ (reverse).
Reporting summary. Further information on research design is available in the Nature Research Reporting Summary linked to this article.