Disease Modeling with Human Neurons Reveals LMNB1 Dysregulation Underlying DYT1 Dystonia

Cell lines and culture condition

HEK 293T cells (CRL-11 268) and SH-SY5Y (CRL-11 266) cells were purchased from ATCC. DYT1 fibroblast and healthy controls, GM03211 (DYT1-1, male, 30 years old), NDS00305 (DYT1-2, male, 22 years old), GM02304 (DYT1-3, female, 17 years old), NDS00301 (DYT1-4, female, 53 years old), GM00024 (Control-1, male, 31 years old), GM03652 (Control-2, male, 24 years old), GM04506 (Control-3, female, 20 years old), and AG07473 (Control-4, female, 50 years old) were obtained from the Coriell Institute for Medical Research or NINDS Human Cell and Data Repository (NHCDR). Human age-matched wild-type (WT) iPSC (GM23476) was obtained from Coriell and H9 embryonic stem cell (ESC) line (WA09) was purchased from WiCell Research Institute. Human iPSCs were maintained in complete mTeSR1 medium (STEMCELL Technologies) on Matrigel (Corning) coated dishes at 37°C and 5% CO₂, and the medium was daily replaced.

The medium recipes were as following:

1. HEK medium: DMEM supplemented with 10% fetal bovine serum (FBS) and 1% penicillin/streptomycin (P/S).

2. Fibroblast medium: DMEM supplemented with 15% FBS and 1% P/S.

3. Neuronal induction medium: DMEM:F12:neurobasal (2:2:1), 0.8% N2 (Invitrogen), 0.8% B27 (Invitrogen), 1% P/S, and supplemented with 10 mm Forskolin (FSK, Sigma-Aldrich), 1 mm dorsomorphin (DM; Millipore), and 10 ng/ml basic fibroblast growth factor (bFGF; PeproTech).

4. Neuronal maturation medium: DMEM:F12:neurobasal (2:2:1), 0.8% N2 (Invitrogen), 0.8% B27 (Invitrogen), 1% P/S, and supplemented with 5 mm FSK and 10 ng/ml each of BDNF, GDNF, and NT3 (PeproTech).

5. ESC medium: DMEM/F12 medium with 20% KnockOut Serum Replacement (KOSR; Thermo Fisher Scientific), 1% GlutaMax, 1% non-essential amino acid (NEAA), 50 μm β-mercaptoethanol (β-ME), 1% P/S, and 10 ng/ml bFGF (PeproTech).

6. Neurosphere medium (NSP medium): DMEM/F12 medium containing 1% N2, 1% GlutaMax, 1% NEAA, 50 μm β-ME, 1% P/S, 8 μg/ml Heparin, 20 ng/ml bFGF, and 20 ng/ml epidermal growth factor (EGF; PeproTech).

7. Neural progenitor cell medium: DMEM/F12 and neurobasal medium (1:1) containing 0.5% N2 (Invitrogen), 1% B27 (Invitrogen), 1% GlutaMax, 1% NEAA, 50 μm β-ME, 1% P/S, 10 ng/ml EGF and 10 ng/ml bFGF.

8. SH-SY5Y medium: DMEM supplemented with 15% FBS and 1% P/S.

9. SH-SY5Y differentiation medium: DMEM supplemented with 3% FBS, 10 μm all-trans-retinoic acid (RA; Sigma) and 1% P/S.

Plasmid construction and virus production

A third-generation lentiviral vector (pCSC-SP-PW-IRES-GFP) was used to express NEUROG2-IRES-GFP-T2A-Sox11, NEUROG2-IRES-Sox11, or ISL1-T2A-LHX3. cDNAs for TOR1A and TOR1AΔE were provided by Gonzalo E. Torres (Torres et al., 2004) and were individually subcloned into pCSC-SP-PW-IRES-GFP vector at the BamHI and XhoI restriction sites. Another third-generation lentiviral vector (LV-CAG-mCherry-miRE-Luc) was used to express TOR1A-shRNAs or LMNB1-shRNAs as described in previously report (Pelossof et al., 2017). Briefly, shRNA oligos targeting the gene coding regions were synthesized, PCR amplified with flanking miR-30 sequences, and ligated into the above lentiviral vector at the XhoI and EcoRI restriction sites. The targeting sequences are AACGGTGTTCACCAAGTTAGAT (TOR1A-shRNA-1), CAGCAAGATCATCGCAGAGAATA (TOR1A-shRNA-2), AGCTTCTTGATGTAAAGTTA (LMNB1-shRNA-1), or CAGACTGTCATCAGAGATGAA (LMNB1-shRNA-2). All plasmids were verified by restriction enzyme digestions and DNA sequencing. The dual reporter 2Gi2R was generously provided by Fred H. Gage (Mertens et al., 2015). The Moloney murine leukemia virus-based retroviral vectors (pMXs) carrying OCT4, SOX2, KLF4, or c-MYC were obtained from Addgene (Takahashi et al., 2007). Each of these vectors was co-transfected with packaging plasmids (pCMV-Gag-Pol and pCMV-VSVG) into HEK293T cells for retrovirus production. Replication-incompetent lentiviruses were produced and viral supernatants were collected at 48 and 72 h posttransfection (Ding and Kilpatrick, 2013). The viral supernatants were filtered through 0.45-μm syringe filters and stored at 4°C before cell transduction.

Direct conversion of adult fibroblasts into MNs

Lentiviral delivery of four factors (NEUROG2, Sox11, ISL1, and LHX3) was used as previously described (Liu et al., 2016; Tang et al., 2017; Ding et al., 2020). In brief, fibroblasts were plated at a density of 1 × 10⁴ cells/cm² onto Matrigel-coated dishes. Cells were transduced the next day with lentiviral supernatants supplemented with 6 mg/ml polybrene. Fibroblast medium was refreshed after overnight incubation. One day later, the culture was replaced with neuronal induction medium and half-changed every other day until 14 d postinfection (dpi). A replating procedure (Liu et al., 2013) was used to purify induced neurons. The purified cells were cultured in neuronal maturation medium onto Matrigel-coated coverslips with or without the presentence of astrocytes depending on desired experiments. The medium was half changed twice a week until analysis.

DYT1 iPSC generation

DYT1 fibroblasts were plated into gelatin-coated 10 cm dishes (8 × 10⁵ cells/dish) and transduced with a cocktail of four retroviruses (1:1:1:1) expressing OCT4, SOX2, KLF4, and c-MYC. Two days later, fibroblasts received a second round of virus infection and was marked as day 0. On day 5, cells were replated with fibroblast medium at 2 × 10⁵ cells per well in Matrigel-coated six-well plates. Culture medium was replaced with human ESC medium on day 6, and then changed to mTeSR1 medium in the following days. Cells were treated with 0.5 mm VPA (Sigma) for 10 d starting on day 5. Based on ESC-like colony morphology, iPSC colonies were picked around three to four weeks. The picked colonies were then expanded and maintained in Matrigel-coated plates with mTeSR1 medium.

Neural progenitor cells and neuronal differentiation

Neural progenitor cells were generated as previously reported with minor modifications (Yang et al., 2014). Briefly, iPSCs or ESCs were cultured in mTeSR1 medium with 10 μm RA and 0.5 mm VPA in Matrigel-coated 6-cm plates for 7 d. Cells were then digested with Versene and gently pipetted into small clumps supplemented with 10 μm Y-27632. Cell clumps were aggregated in KOSR medium for 4 d, followed by culturing in NSP medium for another week. The resulting neurospheres were then dissociated into single cells with Accutase (Innovative Cell Technologies), and maintained in neural progenitor cell medium. For MN differentiation (Tang et al., 2017; Sepehrimanesh and Ding, 2020), neural progenitor cells were plated into Matrigel-coated plates at a density of 3 × 10⁴ cells/cm² and transduced with a cocktail of two lentiviruses (1:1) expressing NEUROG2-IRES-GFP-T2A-Sox11 and ISL1-T2A-LHX3. Culture medium was replaced the next day with neuronal maturation medium. Neurons were dissociated with Accutase on day 6 and replated onto astrocyte-coated coverslips for long-term culture.

Immunostaining, confocal microscopy, and image analysis

Cultured cells at the indicated time points were fixed with 4% paraformaldehyde (PFA) in PBS for 15 min at room temperature (RT) and then permeabilized and blocked for 1 h in blocking buffer (PBS containing 0.2% Triton X-100 and 3% BSA). They were subsequently incubated overnight with primary antibodies in blocking buffer at 4°C, followed by washing and incubation with corresponding fluorophore-conjugated secondary antibodies. Cell nuclei were counterstained with Hoechst 33342 (HST; Thermo Fisher Scientific). Primary antibodies used in this study were choline acetyltransferase (CHAT; Millipore, AB144P, 1:200), GFP (Aves, GFP-1020, 1:1000), HB9 (DSHB, 81.5C10, 1:500), lamin A (LMNA)/LMNC (Abcam, ab40567, 1:300), LMNB1 (Proteintech, 12 987–1-AP, 1:500), MAB414 (BioLegend, 902901, 1:500), MAP2 (Sigma, M4403, 1:500), MAP2 (Abcam, ab5392, 1:10,000), NUP98 (Santa Cruz, sc-74 578, 1:200), NUP359 (Millipore, ABN1385, 1:100), SMI32 (BioLegend, 801701, 1:5000), SYN1 (Cell Signaling, 5297, 1:200), TUBB3 (Covance, MMS-435P, 1:2000), and TUBB3 (Covance, PRB-435P-100, 1:2000).

Confocal images were obtained with a Nikon A1R or Zeiss LSM700 (63×/1.4 NA) confocal microscope. Neurite length was measured with the ImageJ software and shown as relative length per neurite (Ding et al., 2013, 2016, 2018). Neurites with direct connections to the soma were counted and shown as primary branches per cell. For nuclear morphology assay, we zoomed in on individual nucleus by using the ImageJ software and defined the abnormal nucleus based on two criteria: (1) at least one obvious sharp angle or a deep invagination; and (2) at least half area of the nucleus losing the smooth outline. Signals of nuclei (HST) or nuclear lamins were used to distinguish the nucleus and cytoplasm.

Fluorescent in situ hybridization (FISH)

FISH was performed as described previously (Ding et al., 2020). Briefly, cultured cells were washed once with PBS, and fixed with 4% PFA for 30 min at RT. Cells were permeabilized with 0.2% Triton X-100 for 10 min, followed by two washes with PBS. Samples were equilibrated with hybridization buffer composed of 2× SSC, 10% dextran sulfate, 10 mm ribonucleoside-vanadyl complex (RVC; New England Biolabs) and 20% formamide. A mixture of digoxigenin (DIG)-labeled oligo-dT or dA probes (0.2 ng/µl) and yeast tRNA (0.2 µg/µl) were heated to 95°C for 5 min and immediately chilled on ice. Probes were then combined with equal volumes of 2× hybridization buffer and incubated with samples overnight at 37°C. Anti-DIG antibody (Sigma, 11333089001, 1:100) and corresponding fluorophore-conjugated secondary antibodies (Thermo Fisher Scientific) were used to detect oligo-dT signals. Anti-MAP2 (Abcam, ab5392, 1:10,000) antibody and HST were used to determine neuronal soma and nuclei, respectively. Fluorescence density of confocal images were analyzed with the ImageJ software. The “mean” values of the nucleus and the cytoplasm in each neuron were used to calculate the ratio of dT signal in nucleus to cytoplasm (Ding et al., 2020). We measured as large an area as possible for each neuron and employed an unbiased approach for data collection. The person who analyzed the images was completely blinded to the sample information.

Western blot analysis

Cells were lysed in lysis buffer composed of 50 mm Tris-HCl buffer (pH 8.0), 150 mm NaCl, 1% NP40, 1% Triton X-100, 0.1% SDS, 0.5% sodium deoxycholate, and protease inhibitor cocktail (Roche). Equal amounts of cell lysates (20 µg per lane) were used for SDS-PAGE and western blot analysis as previously described (Ding et al., 2018). Primary antibodies and dilutions were Actin (Sigma, A5441, 1:60,000), TOR1A (Cell Signaling, 2150, 1;1000), TUBB3 (Covance, MMS-435P, 1:10,000), LMNB1 (Proteintech, 12 987-1-AP, 1:2000), LMNB2 (Abcam, ab97513 1:1000), GLE1 (Abcam, ab96007, 1:2000), LAP2A (Abcam, ab5162, 1:2000), LAP2B (Thermo Fisher Scientific, A304-840A, 1:2000), and RANGAP1 (Cell Signaling, 36067, 1:1000).

Quantitative real-time PCR analysis

Total RNA was extracted from cultured cells using TRIzol (Life Technologies), and genomic contamination was removed using TURBO DNase (Life Technologies). cDNA synthesis reactions were performed using 0.5 µg of RNA from each sample with the SuperScriptIII First-Strand kit (Life Technologies) and random hexamer primers. Real-time PCR was performed in triplicate using primers, SYBR GreenER SuperMix (Invitrogen), and the ABI 7900HT thermocycler (Applied Biosystems). Target mRNA levels were normalized to the reference gene HPRT by 2^-ΔΔCt method as described previously (Ding et al., 2013, 2016, 2018). PCR primer sequences (from 5′ to 3′) were CTGGTGGATGGGGTCTCCTA (qTOR1A-F), GACACAGACAACGCGTGTTC (qTOR1A-R), AGGAAAGCGGAAGAGGGTTG (qLMNB1-F), and GCCTCCCATTGGTTGATCCT (qLMNB1-R).

Transmission electron microscopy (TEM)

Cells on Matrigel-coated glass coverslips were fixed overnight at 4°C with a solution composed of 4% PFA, 1% glutaraldehyde, 1.5 μm MgCl₂ and 5 μm CaCl₂ in 0.1 m cacodylate buffer (pH 7.4). Samples were then twice washed with cacodylate buffer, treated for 1.5 h at RT with 1% osmium tetraoxide (OsO₄; EMS) and 0.8% K3Fe(CN6) in cacodylate buffer, and prestained with 2% uranyl acetate in water for 2 h in the dark at RT. The subsequent steps of dehydration, infiltration, and embedding were the same as previously described (Li et al., 2016). The resin blocks were polymerized overnight at 60°C and sectioned with a diamond knife (Diatome) on a Leica Ultracut UCT 6 ultramicrotome (Leica Microsystems). Sections were poststained with 2% uranyl acetate in water and lead citrate. Images were acquired on a JEOL JEM 1200EX TEM equipped with a tungsten source at 120 kV using a Morada SIS camera (Olympus). The electron-dense areas immediately beneath the nuclear membrane were measured with ImageJ (NIH) and the ratio of electron-dense area to the nuclear perimeter was used to evaluate the thickness of nuclear lamina. By using the ImageJ software, we zoomed in on the nuclear member and quantified the number of nuclear pore complexes (NPCs) and the pore sizes.

Electrophysiology

Neurons cultured on astrocyte-coated glass coverslips for 35 d or longer were used for analysis. Whole-cell patch-clamp recordings were performed under visual guidance using GFP-fluorescence to identify GFP+ cells when cells were maintained at 30°C in a submersion chamber with tyrode solution containing 150 mm NaCl, 4 mm KCl, 2 mm MgCl₂, 3 mm CaCl₂, 10 mm glucose, and 10 mm HEPES at pH 7.4 (adjusted with KOH) and 300 mOsm. The recording pipettes (∼6–9 MΩ) were filled with an intracellular solution containing 0.2 mm EGTA, 130 mm K-gluconate, 6 mm KCl, 3 mm NaCl, 10 mm HEPES, 4 mm ATP-Mg, 0.4 mm GTP-Na, 14 mm phosphocreatine-di(Tris) at pH 7.2 and 285 mOsm. Series and input resistance were measured in voltage-clamp with a 400 ms, 10-mV step from a −60-mV holding potential (filtered at 30 kHz and sampled at 50 kHz). Cells were used for analysis only if the series resistance was <30 MΩ and was stable throughout the experiment. The input resistance ranged from 0.2 to 2 GΩ. Currents were filtered at 3 kHz, acquired and digitized at 10 kHz using Clampex10.3 software (Molecular Devices). Action potentials (APs) were recorded in current-clamp and elicited by a series of current injections ranging from −20 to 200 pA at 20-pA increments and 800 ms in duration. All current-clamp recordings were made at resting membrane potential or without any current injection. Data analysis was performed with Clampfit10.3 software (Molecular Devices). The AP trace immediately above threshold was used to determine the delay of first spike as the length of time and the start of current steps to the peak of AP. The same AP trace was used to measure AP threshold as the corresponding voltage when there was the sharpest change of the trace slope. The above indicated AP trace was also measured to determine maximum velocity of the rise and decay. AP frequency was obtained by dividing the maximum number of spikes during the current steps protocol with the step time duration (800 ms).

Statistical analysis

Unpaired two-tailed Student's t tests were used to compare one experimental sample with its control. One-way analysis of variance was used when comparing multiple samples, with either Tukey's (when comparing samples with each other) or Dunnett's (when comparing samples to a control) post hoc tests. Results are expressed as mean ± SD of at least three biological replicates, and p < 0.05 is treated as significant.