Magnetically guided non-invasive CRISPR-Cas9/gRNA delivery across blood-brain barrier to eradicate latent HIV-1 infection

CRISPR-Cas9/gRNA exhibits therapeutic efficacy against latent human immunodeficiency virus (HIV) genome but the delivery of this therapeutic cargo to the brain remains as a challenge. In this research, for the first time, we demonstrated magnetically guided non-invasive delivery of a nano-formulation (NF), composed of Cas9/gRNA bound with magneto-electric nanoparticles (MENPs), across the blood-brain barrier (BBB) to inhibit latent HIV-1 infection in microglial (hμglia)/HIV (HC69) cells. An optimized ac-magnetic field of 60 Oe was applied on NF to release Cas9/gRNA from MENPs surface and to facilitate NF cell uptake resulting in intracellular release and inhibition of HIV. The outcomes suggested that developed NF reduced HIV-LTR expression significantly in comparison to unbound Cas9/gRNA in HIV latent hμglia/HIV (HC69) cells. These findings were also validated qualitatively using fluorescence microscopy to assess NF efficacy against latent HIV in the microglia cells. We believe that CNS delivery of NF (CRISPR/Cas9-gRNA-MENPs) across the BBB certainly will have clinical utility as future personalized nanomedicine to manage neuroHIV/AIDS.

target by complementary base pairing. Target DNA sequence recognition by Cas9/gRNA requires protospacer adjacent motif (PAM) trinucleotide sequence, which enables targeting and successive endonuclease disruption. Cas9/gRNA together bind to the target DNA sequence, and Cas9 makes a double stranded break (DSB) upstream PAM. These breaks are then repaired by NHEJ (non-homologous end joining) DNA repair mechanism, which is error prone and results in insertions or deletions (InDels) leading to frameshifts or stop codons resulting in disrupted Open Reading Frames (ORFs). Recently, CRISPR/Cas9 is being used to target and eliminate the HIV in latently infected CD4+ T lymphocytic cells, macrophages, and microglia in cell culture, without causing genotoxicity or off-targeting, confirmed by whole-genome sequencing and SURVEYOR assays 17,18 . Yarn like DNA nanoparticles known as DNA nanoclews are the recently discovered vehicle synthesized via rolling circle amplification, and reported as a nanocarrier (NCs) to deliver Cas9/gRNA to the target 24 . Nanoparticle assisted delivery of CRISPR to the brain has recently been demonstrated in mice using intracranial administration to manage fragile X syndrome from exaggerated repetitive behavior 25 . Unfortunately, the non-invasive delivery of Cas9/ gRNA across the BBB is not fully explored yet. Site-specific delivery of Cas9/gRNA is extremely promising against retroviruses and more studies in context to HIV are urgently required. Therefore, an effective strategy for controlled delivery of NFs containing Cas9/gRNA across the BBB to activate and eradicate the latent HIV reservoir in the brain is worth exploring.
The one-long-terminal-repeat (1-LTR) circle, the 2-LTR circle, and linear DNA are 3 forms where nonintegrated DNA of HIV exists. In HIV-1, Trans-Activator of Transcription (Tat) activates viral transcription by stimulating elongation from LTR. Therefore, LTR will be a target gene for the eradication of latent HIV infection from the body. In this manuscript, we demonstrate a magnetically guided non-invasive delivery and on-demand controlled release of Cas9/gRNA targeting HIV-1 LTR across the BBB using magneto-electric nanoparticles (MENPs) as a drug NCs. The MENPs are ferromagnetic, non-toxic (up to 50 µg), 25 ± 5 nm in size and able to across the BBB under a static magnetic field. The MENPs also exhibited a feature of on-demand release of drug upon external ac-magnetic field stimulation which causes polarization changes on MENPs surface leading to the desired breakdown of bonds between particle and drug. A magnetic NF consisting of Cas9/gRNA bound with MENPs was developed for non-invasive delivery across the BBB under a static magnetic field of 0.8 T. Further, the on-demand release of Cas9/gRNA was achieved on applying ac-magnetic field stimulation via customized electromagnetic coil. The obtained reduced viral LTR expression levels in the Cas9/gRNA treated latent HIV infected hμglia/HIV cells 26 confirms the successful delivery of NF across the BBB for targeting of latent virus. Such developed therapeutic NF i.e., MENPs-Cas9/gRNA can be used as a potential therapy to target and eradicate latently HIV-1 infection in the brain.

Results
NF (MENPs-Cas9/gRNA) preparation. The MENPs utilized in this research as a Cas9/gRNA carriers are well characterized using a vibrating-sample magnetometer (VSM) for magnetization assessment, transmission electron microscopy (TEM) for particles size estimation, X-ray diffraction (XRD) pattern for phase purity evaluation. The outcomes of these studies have been described in our previous manuscript 16,27 . In brief, MENPs [BaTiO 3 (BTO) @CoFe 2 O 4 (CFO)] of particle size ranging from 20 to 30 nm (Fig. 1Aa) exhibited diffraction peaks associated with crystallographic planes of CFO (JCPDS 00-022-1086) and BTO (JCPDS 04-001-7269) confirming the phase purity and crystalline characteristics of MENPs composed of BTO and CFO phases 16,27 . This arrangement of magnetic core and piezoelectric shell showed a ferromagnetic magnetism (34 emu/g), a desired property of an electro-active material to achieve on-demand release of a drug from the MENPs surface system through an externally applied ac-magnetic field stimulation 27 .
The MENPs are monodispersed (PDI value of 0.24) positively surface charged (zeta potential −30 mV) nanoparticles and can easily bind with negatively charged Cas9/gRNA system via electrostatic interaction. This low value of PDI reveals mono-dispersive characteristics of MENPs useful for good binding with water soluble drugs like Cas9/gRNA and systemic administration in targeted animal model 16 . The strategy of MENPs-Cas9/gRNA NF preparation and Cas9/gRNA release on ac-magnetic field stimulation is illustrated in Fig. 1A and described with scientific reasoning in respective sections. Time kinetics of Cas9/gRNA binding with MENPs and further release profile of cas9/gRNA from NF as a function of ac-magnetic field stimulation were studied using optical density (OD) method (Fig. 1B). The bound Cas9/gRNA concentration was estimated via measuring OD (at 260 nm) of unbound fraction of plasmid (supernatant). Based on findings of OD study, a calibration curve was established as a function of absorption intensity at 260 nm and Cas9/gRNA concentrations ranging from 1 to 20 µg (Fig. 1Ba). This linear (r 2 = 0.989) calibration curve was used to estimate % binding of Cas9/gRNA over the time and % release of Cas9/gRNA as a function of applied magnetic field. The results of OD density showed that 60% of 10 µg Cas9/gRNA binds with 50 µg of MENPs within 30 minutes of incubation time (Inset, Fig. 1Ba). Since, only 60% cas9/gRNA bind with MENPs, we selected only 6 µg of Cas9/gRNA to prepare NF to conduct further experiments.
The NF i.e. MENPs-Cas9/gRNA was exposed to an ac-magnetic field generated from an indigenously customized electromagnetic coils. Externally applied ac-magnetic fields stimulation (40 and 60 Oe at 100 kHz) exposed to NF alter polarization in MENPs and cause expansion and contraction in ionic bonds available on MENPs surface. This phenomena occurs repeatedly and break electrostatic bonding and releases Cas9/gRNA system from MENPs surface. After applying ac-magnetic field, the mixture was centrifuged to conduct OD study for the estimation of % release Cas9/gRNA system. The results of OD suggested that the release of Cas9/gRNA system is a function of applied field and stimulation time. At a constant exposure time for 30 minutes, applied filed of 40 Oe field exhibited 70% release of Cas9/gRNA, while approximately 98% Cas9/gRNA release was obtained on applying magnetic field of 60 Oe (Fig. 1Bb). These findings suggest that a magnetic field of 60 Oe applied for 30 minutes would be enough to release maximum % of plasmid in in-vitro BBB models also. tion and deformation of binding during preparation of MENPs-Cas9/gRNA NF and on-demand release of Cas9/ gRNA from NF were evaluated using Raman spectroscopy (Fig. 2). Nucleic acids exhibits strong Raman bands in mid-frequency region (600 to 1800 cm −1 ) corresponds to intramolecular modes of nucleic acid bases such as adenosine (A), guanine (G), cytosine (C), thymidine (T), d-deoxyribose of sugar phosphate scaffold. We also selected this region to evaluate NF preparation and release of Cas9/gRNA. The Raman spectra of Cas9/gRNA The MENPs exhibited Raman active modes (curve c) associated with BTO 31 and CFO 32 to confirm the presence of MENPs i.e., BTO@CFO. Raman mode at 500 cm −1 and 670 cm −1 are attributed to tetragonal phase of BTO and cubical inverse-spinel structure, respectively. Raman observed below 300 cm −1 is attributed to E www.nature.com/scientificreports www.nature.com/scientificreports/ (transversal (TO) and longitudinal (LO) components TO + LO) mixed mode. Raman band at 515 cm −1 corresponds to transversal modes i.e., E (TO) and A 1 (TO) of BTO 31 . Further Raman peak around 800 cm −1 corresponds to stacking-fault density of BTO phase, and appears due to high temperature calcination of MENPs at 780 °C. The cubic spinal active Raman modes, mainly due to E g , and three of F 2g symmetries were observed at 300 cm −1 . The peak observed at 670 cm −1 is attributed to the F 2g symmetry of CFO which is a characteristic Co-O displacement.
The NF was stimulated through ac-magnetic field and as explained above, it detached Cas9/gRNA from MENPs surface. Raman spectra of NF after ac-magnetic field stimulation was measured (curve d) to prove the release of Cas9/gRNA through breaking of ionic bonds on ac-magnetic field stimulation. It was observed that Raman modes associated with Cas9/gRNA disappeared, which confirm the release of Cas/gRNA. Though 100% drug release in general is not possible, this is the reason that some bands of low intensities are still visible in curve. However, the Raman modes observed in NF after ac-magnetic field stimulation seem corresponds to MENPs only. This confirmed the release of Cas9/gRNA from NF due to breakdown of bonding through ac-magnetic field stimulation via electromagnetic coil.

Toxicity assessment of MENPs and NFs (MENPs-Cas9/gRNA). The in-vitro cytotoxicity of MENPs
(10-100 µg), Cas9/gRNA (6 µg) and NF [MENPs (50 µg)-Cas9/gRNA (6 µg)] was assessed by performing XTT assay (Fig. 3). Cells associated with in-vitro BBB model; Human Astrocytes (HA), Human Pericytes (HP), Human Brain Microvascular Endothelial Cells (HBMEC), and CHME5 cell lines upon treatment with MENPs concentrations ranging from 10 to 50 µg exhibited approximately 90% cell viability compared to control (Fig. 3A). However, cell viability reduced to 70% upon treatment with high dose of MENPs (100 µg). Therefore 50 µg of MENPs was found to be an optimized dose for preparing a NF using Cas9/gRNA system (6 µg). The MENP concentrations we have used in this cytotoxicity experiment are very high considering the number of cells we have used, the surface  www.nature.com/scientificreports www.nature.com/scientificreports/ area and amount of the media. We have chosen to use these broad ranges of MENP concentrations to determine the biosafety of our nanoformulations even at high concentrations. We have observed no cytotoxicity up to 50 µg of MENP which indicate the biosafety of our nanoparticles even at high concentrations.

Evaluation of in-vitro BBB integrity and NF transmigration across the BBB.
Various parameters such as nanoparticle at interface of cells, HIV infection, and magnetic field stimulation may affect the tight junction of BBB and facilitate the transmigration of unwanted element to the brain. Thus exploring BBB junction integrity becomes crucial in this study. An in-vitro BBB model was placed on a static magnet (0.8 T) for 3 hours to facilitate navigation of NF across the BBB as illustrated in Fig. 4A. The upper chambers of the both normal (Fig. 4A) and HIV infected (Fig. 4B) BBB models, were treated with MENPs (50 µg), Cas9/gRNA (6 µg) and NF. www.nature.com/scientificreports www.nature.com/scientificreports/ The integrity of BBB model was evaluated via measuring transepithelial electrical resistance (TEER) values and Fluorescein isothiocyanate (FITC) intensity of control and each treated wells. The findings from TEER values and FITC experiments explained that each treatments does not affect BBB integration in the both models.
Ammonium thiocyanate-based photometric assay (490 nm) was performed to estimate concentration of MENPs which was able to cross the BBB. The assay results suggested that 26% MENPs crossed the BBB in-vitro. Upon estimation of OD, from media collected from the lower chamber of the BBB model after ac-magnetic field stimulation, we observed that that 2 µg Cas9/gRNA was released in the lower chamber subsequent to the BBB transmigration.
On-demand release and functionality evaluation of Cas9/gRNA system. To release Cas9/gRNA from NF, HIV-infected BBB model was placed in an electromagnetic coil for ac-magnetic stimulation, as illustrated in Fig. 5A. An optimized ac-magnetic field of 60 Oe was applied for 30 minutes to achieve Cas9/gRNA release in the lower chamber of the BBB model. To compare the functionality of released Cas9/gRNA, an identical experiment was performed wherein, the BBB was treated using only Cas9/gRNA. The media from lower chamber of treated BBB model (with HIV alone, Cas9/gRNA-HIV, and NF-HIV) was collected and amount of released Cas9/gRNA was estimated, by deciphering it ability to reduce HIV long terminal repeat (LTR) expression level (Fig. 5B) in HC69 cells grown in basal chamber of the in vitro BBB model.
The LTR level in HIV infected sample was estimated as 65, compared to uninfected control. In case of only Cas9/gRNA treated the BBB, the treatment reduced LTR level to 48 confirming that Cas9/gRNA remains functional and does not lose its activity on applying ac-magnetic field. The LTR expression levels reduced remarkably to 40 on treatment with released Cas9/gRNA from NF on ac-magnetic field stimulation. This significant reduction in LTR expression, compared to HIV infected cells, may be attributed to intracellular eradicating mechanism due to significantly high cell uptake. This is due to easy and high cell uptake of NF via electroporation on applying ac-magnetic field. Electroporation in cells on applying ac-magnetic field of 60 Oe has been demonstrated in our previous publication 12 . In brief, CFO core of MENPs went through a strain change on applying ac-magnetic field stimulation. This deformation was further absorbed by BTO piezoelectric shell of MENPs to cause pressure waves. This generated pressure wave is capable to misaligned phospholipid later of cell member to cause poration when MENPs is at µm distance from the cell. This ac-magnetic field induced nano-electro-poration caused NF delivery inside the cell resulted in higher efficacy.
Due to electroporation, there is a high uptake of NF by H-MG cells followed up by intracellular release of Cas9/gRNA on stimulation, as schematically illustrated in Fig. 5C. This phenomena cause HIV-infection eradication intracellularly resulting in more reduction in HIV-LTR expression level than using pure Cas9/gRNA. In the quantitative analysis of the efficacy of Cas9/gRNA and its MENP based NF using florescent microscopy (Fig. 6A), we have observed significantly reduced GFP fluorescence in Cas9/gRNA treated cells when compared to the untreated control cells indicating significantly reduced latent infection in HIV-GFP cells. Furthermore, using MENP based NF of Cas9/gRNA, we have observed further reduction of latent infection when compared to the Cas9/gRNA alone treatment. Intensity of the florescence is directly proportional to the HIV-1 LTR levels which www.nature.com/scientificreports www.nature.com/scientificreports/ is an indicative of HIV infection levels in those cells. Quantitative assessment of fluorescent intensity analysis of images indicates that NF is more efficient in reducing the latent infection levels when compared to the Cas9/ gRNA alone (Fig. 6B).

Discussion
We propose positively surface charged mono-dispersed ferromagnetic MENPs as potential NCs to navigate Cas9/ gRNA across the BBB under the influence of static magnetic field, which is safe and non-invasive. Additionally, we demonstrated an on-demand release of Cas9/gRNA from NF on applying ac-magnetic field externally through electromagnetic coil. The Cas9/gRNA binds to MENPs via electrostatic binding due to opposite surface charges, as demonstrated by Raman analysis. The results of OD studies values demonstrated that within 30 minutes of incubation time, 60% Cas9/gRNA of 10 µg with 50 µg of MENPs and ~98% Cas9/gRNA released on applying 60 Oe ac-magnetic field. The cytotoxicity studies and TEER value measurement studies confirmed that MENPs (50 µg), Cas9/gRNA system (6 µg) and NF do not adversely affect cell viability and also the BBB integrity on each respective treatment. Our developed NF has the ability to cross the BBB, in-vitro model, under the influence of a static magnetic field due to the magnetic nature of NF. Thus demonstrated magnetically guided non-invasive BBB transmigration technique may be effective and practicable over the conventional techniques such as focused ultrasound methods, electric field, photosensitization etc. These methods are not well adopted due to transient BBB opening which can allow entrance of other foreign moieties 8,33 which induce cell damage and slow recovery. We estimated that 26% MENPs navigated across the BBB which is significant in comparison of TAT-mediated 34 and liposome 35 encapsulated delivery of organic and inorganic nanostructures for drug delivery application. Development of an efficient NF which can be guided externally across the BBB without any side effects becomes extremely important. Thus our proposed delivery method seems to be one of the potential solution to overcome challenges 8 .
Cas9/gRNA was released across the BBB, in controlled manner via applying an optimized ac-magnetic field of 60 Oe for 30 min. The released Cas9/gRNA was biologically active and reduced HIV-LTR expression levels in latent HIV-1 infected cells. The results of presented studies showed that the Cas9/gRNA released form NF exhibit superior therapeutic efficacy in comparison of treatment using Cas9/gRNA only. This is attributed to higher uptake of NF due to electroporation and its ability to target latent HIV-1 genome suggesting as a promising therapeutic approach. Our investigated on-demand and controlled intracellular HIV-1 infection eradication approach using nanotechnology is unique and has never been demonstrated before. The other available approaches are multicomponent therapeutics to activate latent virus and further to eradicate HIV infection. The integration of all these agents results in a large size (>150) which exhibit poor efficacy because of size constraints due to intact integrity of the BBB 36,37 . The development of effective therapeutic NFs based on minimal sized therapeutic agent system which can cross the BBB and activate and eradicate HIV in brain reservoirs are urgently required. We demonstrate that designed Cas9/gRNA recognize and eliminate HIV-1 infection, confirmed by reduction in LTR expression level, in CNS cells upon successful delivery across the BBB using nanotechnology with the feature of on-demand release and no noticeable side-effects. This technology is of crucial significance against HIV reservoirs in the brain. Earlier studies by Dr. Khalili's group recently reported that Cas9/gRNA specifically targeting U3 region of HIV-1 LTR, inactivates viral gene transcription and thereby the viral replication in latently infected cells 38 . Our results suggest that MENP guided delivery of Cas9/gRNA across the BBB will have a translational significance in eradicating HIV latency in the brain. www.nature.com/scientificreports www.nature.com/scientificreports/ In conclusion, we demonstrated non-invasive magnetically guided delivery of Cas9/gRNA across the BBB using MENPs as a drug NC. High cell-uptake of NF via nano-electroporation and on-demand release of Cas9/ gRNA (98%) through ac-magnetic field stimulation resulting in significant HIV-LTR reduction than control Cas9/gRNA. Due to salient features such as bio-compatibility, non-invasive CNS delivery, and on-demand Cas9/ gRNA release our developed NF has potential to manage neuroHIV. As a viewpoint, aiming to develop a Cas9/ gRNA nanomedicine as therapy for neuroHIV, this such developed NF delivery need to be demonstrated in appropriate animal model. Authors are in process to optimized/develop an appropriate animal to demonstrate herein proposed technology to eradicate neuroHIV. We have previously demonstrated non-invasive and safe delivery of MENPs to the mice brain and observed uniform distribution of MENPs in all brain cell types without agglomeration and without altering motor coordination function of mice 16 . As future direction, in combination with our established magnetically guided delivery to the brain technology, Cas9/gRNA can successfully be delivered to the brain for the eradication of neuroHIV/AIDS. Online methods. Cas9/gRNA selection. A complete procedure, bio-informatics screening, genetic sequences, functionality and capability to reduce HIV-LTR of CRISPR designed Cas9/gRNA employed in this work has been discussed by Khalili et al. 38 . Bio-informatics screening and efficiency/off target prediction identified four gRNA targets within the HIV-1 LTR, named A, B, C and D that avoid conserved transcription factor binding sites, minimizing the likelihood of altering host gene expression. Expression of these gRNAs by a vector that also expresses the Cas9 protein in the CHME5 cells, a microglial cell line that harbors integrated copies of a single round HIV-1 reporter (pNL4-3-ΔGag-d2EGFP), drastically suppressed LTR promoter-driven expression as measured by the fraction of EGFP positive cells, reported in previous publication 38 . The gRNA specific to LTR-B in CHME-5 cells exhibited maximum reduction in LTR promoter-driven expression shown by p24 and LTR fold change. We have used Cas9/gRNA specific to LTR-B for navigation across the BBB using MENPs as NCs non-invasively. Dr. Khalili's group has reported at the multiplex expression of LTR A/B gRNAs in CHME5 cells caused deletion of 190 bp fragment between the A & B target sites and led to junction site mutations to various degrees as detected by PCR and Sanger sequencing 38 . This treatment completely suppressed the appearance of EGFP positive cells, due to inhibition of LTR transcription in the cells. This group has estimated viral load using p24 ELISA and real time PCR analysis. The results of these studies showed a substantial decrease in viral replication. The low, but detectable, residual viral presence is almost certainly due to the background of transfected cells. www.nature.com/scientificreports www.nature.com/scientificreports/ Preparation of in-vitro BBB model and navigation of NF across the BBB. An established procedure as described earlier was used to prepare a BBB model 39 . The model consisted of two-compartment wells in a culture plate, with the upper compartment separated from the lower by a cyclopore polyethylene terephthalate membrane (Collaborative Biochemical Products, Becton Dickinson, San Jose, CA) with a pore diameter of 3 μm. In a 24 well cell culture insert, 2 × 10 5 primary HBMECs were grown to confluency on the upper side whereas a confluent layer of primary HA and HP (1 × 10 5 cells/insert) were grown on the underside. A 0.5 × 10 5 CHME-5 cells population was added to the 24 well plate surfaces. Intactness of the BBB was determined by measuring the transendothelial electrical resistance (TEER) using Millicell ERS microelectrodes (Millipore, Billerica, MA). To prepare a HIV infected the BBB model, CHME-5 HIV infected cells (5dpi) were added to the lower surface of the 24 well plate after checking the intactness of the BBB. The BBB model was used for experiments at least 5 days after cell seeding.
The upper chamber of such constructed BBB was treated with 100 µL of MENPs (50 µg), Cas9/gRNA (10 µg), and MENPs-Cas9/gRNA (50 µg: 6 µg) NF. BBB containing 24 well plate was placed on top of a static magnet (0.8 T) for 3 hour. The applied static magnetic field facilitates transmigration of MENPs containing NF across the BBB 10 . TEER measurements were performed after 3 hrs and 24 hrs of treatments. The electrical resistance of blank inserts with medium alone was subtracted from TEER readings obtained from inserts with confluent monolayers. The resulting TEER values represent the resistance of the endothelial cell monolayers. The results are presented as percent of control. In parallel, the effects of the treatment on the paracellular transport of flourescein isothiocyanate-labeled (FITC) dextran (molecular weight 40000) were measured according to the procedure described earlier 40,41 . FITC-dextran (Sigma Aldrich) of 100 mg/mL was added to the upper chamber of the inserts and further incubated for 4 h. Samples were collected from the bottom chamber after 4 h and fluorescence intensity was measured using a excitation wavelength of 485 nm and emission wavelength of 520 nm using Biotek Synergy HT multimode microplate reader instrument. FITC-dextran transport was expressed as fluorescence units of FITC-dextran transported across the BBB into the lower compartment. All data are presented as the mean ± the standard deviation of the mean (S.D). The results were analyzed using ANOVA (Kruskal-Wallis test) followed by Dunn's Multiple Comparison post-test to determine statistical significance (Graph Pad 5 Software, Inc., La Jolla, CA, USA).
The navigation of MENPs across the BBB to the lower chamber was quantitatively confirmed via estimating Fe ion concentration using ammonium thiocyanate-based photometry assay as described in our previous paper 10 . The qualitative confirmation of MENPs was also performed using TEM imaging of lower chamber media.
On-demand release of Cas9/gRNA and functional assessment. A 24 well-plate containing MENPs-Cas9/gRNA NF navigated across the BBB was placed in an indigenously designed electromagnetic coil (dimension 4 × 6 inches) for field control release of Cas9/gRNA system. The Cas9/gRNA release procedure was performed using ac-magnetic field of 40 and 60 Oe at a constant frequency of 1 KHz and time of 30 minutes to optimize maximum drug release (around 98%). These H-MG and HIV latent H-MG cells were provided by the research group of Dr. Jonathan Karn, Department of Molecular Biology and Microbiology, Case Western Reserve University, Cleveland, OH.
HC69.5 (HIV/GFP) and HIV-GFP cells were treated with LTR-B plasmid (Cas9/gRNA) and related MENPs based NF. Cells were incubated for 2 hrs followed by applying ac-magnetic field (60 Oe for 30 minutes) to release the plasmid. The functionality assessment of release plasmid was performed via LTR expression (quantitative) and immunofluorescence imaging (qualitative) as a function of GFP fluorescence. For LTR expression, cells were cultured under 1% of FBS. The C20 clone, the parenteral cells were used as a negative control. RNA was extracted using RNeasy Mini kit (QIAGEN) and reverse transcribed (High-Capacity cDNA Reverse Transcription Kit; Life technologies) followed by quantitative real time analysis using PCR for LTR gene. For fluorescence microscopic analysis, clone HC69.5 (HIV/GFP) cells treated with LTR-B (Cas9/gRNA) plasmid and related NF was cultured under 1% of FBS and incubated for 2hrs followed by applying release conditions identically. After this procedure, the cells were fixed using PFA 4% to perform fluorescence imaging using a Keyence ALL in one microscope (10X) Statistical analysis. Experiments conducted in this study were performed at least three times in duplicate and values were expressed as means ± standard deviation (SD). An unpaired student t-test was performed and a p values ≤ 0:05 were regarded as significant. For more than 2 groups, the data were analyzed using GraphPad Prism software. Comparisons between groups were performed using one-way ANOVA and Turkey's Multiple Comparison Post Test. Differences were considered significant at p ≤ 0.05.