The validation of miR-30a:BDNF 3′-UTR interaction with luciferase reporter assays in two different cell lines, and its higher relative expression in neurons that are able to synthesize BDNF compared with some of the other candidate miRNAs, including miR-195, suggest that miR-30a is more likely to be a potential regulator of neuronal BDNF expression. To pursue this further, we used a lentivirus-based system to overexpress miR-30a precursor in cultured neurons (derived from E14.5 rat forebrain progenitor cells, see Materials and Methods) (Fig. 4A) and then assayed BDNF protein by ELISA. A lentivirus expressing miR-NSC30 (Fig. 4D) was also included in these experiments. Transduction efficiencies were verified with GFP expression and included a majority of cells (on average, 60%) (Fig. 4A). Cultures transduced with miR-30a showed a 2–4-fold increase in mature miR-30a levels, as measured by qRT–PCR (Supplementary Material, Fig. S4). There was a significant, ~30% decrease in BDNF protein levels in neuronal cultures overexpressing miR-30a (Fig. 4B). In contrast, the control—which was identical to miR-30a except for three mutations in the seed sequence (Fig. 4C and D)—did not alter neuronal BDNF levels. Notably, miRNAs exhibiting partial complementarity to their mRNA target (such as miR-30a:BDNF 3′-UTR, Fig. 4C), predominantly block translation, but additional mechanisms involving mRNA decay have also been reported (1). Therefore, we assayed BDNF mRNA in our cultures, and no changes were observed (Supplementary Material, Fig. S4). We conclude that miR-30a exerts an inhibitory effect on BDNF translation in neurons.

Small RNAs (<200 nt) were isolated by using the mirVANA PARIS kit (Ambion), according to the manufacturer's instructions and treated with DNase I for 30 min at 37°C. Then, samples were incubated at RT (room temperature) for 2 min in DNase I inactivating buffer (Ambion—RNAqueous kit), followed by centrifugation (13 000g) for 1.5 min and supernatant was stored at −80°C. The mirVANA PARIS kit was also used for the extraction of large (>200nt) RNA that was used for measurement of BDNF mRNA. The mirVANA PARIS kit (Ambion) was used for total or small RNA isolation from rat neuronal cultures and the RNAqueous Micro kit (Ambion) was used for total RNA extraction in HEK-293 cells. All samples were treated with DNase I to avoid DNA contamination. For determination of RNA quality RNA RIN were calculated using the Agilent 2100 bioanalyzer and according to manufacturer's instructions.

³²P-UTP-labeled probes (mirVana miRNA Probe Construction Kit, Ambion) reverse antisense to the mature miRNAs and 5S rRNA were used in conjunction with the solution hybridization assay according to manufacturer's instructions (mirVana miRNA detection kit). Briefly, the small RNA sample was mixed with the probe and after hybridization in solution, samples were subjected to RNase digestion. The radiolabeled protected fragments of the probe after RNase inactivation and precipitation were separated in a denaturing polyacrylamide gel. Probe-specific sequences (without linker sequence) were as follows: 5′-CTTCCAGTCGAGGATGTTTACA-3′ (this is the reverse complement of the mature mir-30a-5p); 5′-ACTAGAGCCTTCGATT-3′ (this is the reverse complement of a conserved region within the 5S rRNA).

For LNA-ISH, 20 µm thick sections of immersion-fixed (human) or perfusion-fixed (mouse) cerebral cortex were mounted on SuperFrost-Plus slides (VWR), air-dried, then subjected to the following procedure with sterile solutions (DEPC-treated water): Washed with 1× PBS 3 × 5 min each, fixed with 4% paraformaldehyde in 0.1 M phosphate buffer for 15 min at RT, then washed again in 1× PBS 3 × 5 min each, then protein was denatured using 0.2 M HCL/1×PBS for 10 min at RT, then washed with 1×PBS 3 × 5 min, then treated with 0.25% acetic anhydride/0.1 M triethanolamine/1×PBS for 10 min at RT, washed again at 1× PBS 3 × 5 min, then prehybridized in 50–100 µl hybridization buffer/per section for 2 h at a specific temperature depending on probe based on the formula T_m probe −21°C, with T_m provided by probe vendor (Exiqon) and shown in Supplementary Material, Table S2. Each probe is a 5′-digoxigenin-labeled, 2′-O, 4′-C methylene bicyclonucleoside monomer-containing oligonucleotide (LNA, phosphoramidite). Sequences are reverse complement to the mature miRNAs (Supplementary Material, Table S2). The 20 ml of hybridization buffer was made of 50% deionized formamide/2×SSC/10% dextran sulfate/500 µg/ml sperm DNA/0.25 mg/ml yeast t-RNA/0.2 mg/ml BSA/50 µg/ml heparin/2.5 mm EDTA/0.1% Tween-20 in 2.3 ml DEPC-H₂0. After absorbing the prehybridization buffer with a kimwipe, 50–100 µl of hybridization buffer containing 0.17–0.25 µM of probe were added to each section and slides were covered with RNAse-free coverslips (HybriSlip, Molecular Probes) and incubated overnight at the specific temperatures (see above) in a humidified chamber. The following day, sections were washed twice in 2×SSC at RT for 15 min on a shaker, then washed in 1×SSC at 37°C for 15 min, then washed twice with 2×SSC/formamide, then with 0.1×SSC for 30 min at the probe-specific temperature (see above), then washed with 0.1×SSC for 15 min at RT, then incubated with buffer I (0.1% Tween-20/0.1 M Tris–HCL, pH 7.5/150 mm NaCl) for 10 min at RT, then with blocking solution [10% normal goat serum/1% blocking reagent (Roche) in buffer I] for 30 min at RT, then incubated with anti-digoxigenin-alkaline phosphate-conjugated antibody (goat, Roche) diluted 1:1000 in blocking solution (150 µl/slide) and parafilm-covered slides were incubated in a humidified chamber on shaker for 3 h at RT. Sections were then washed in buffer I 3 × 15 min each, then incubated in buffer III (0.1 M Tris–HCL, pH 9.5/0.1 M NaCl) at RT for 10 min, then 500 µl of color substrate solution (CSS) were added to each slide (CSS = nitroblue tetrazolium/BCIP stock solution (Roche) diluted 1:50 in buffer III) at RT under light-protected conditions overnight. Slides were then washed in TE buffer at RT for 10 min, then washed with 1×PBS at RT for 10 min, then with ddH₂0 at RT for 10 min. Finally the slides were coverslipped with 100 µl of VectaMount mounting medium (Vector Labs) for each slide, and were stored under light-protected conditions at RT for microscopic studies. Additional sections were first processed by LNA-ISH as described above, and then subjected to immunohistochemical labeling with the mouse monoclonal anti-NF-H (anti-SMI-32 antibody, Covance) and FITC-conjugated goat-anti mouse antibody, followed by diaminobenzidine (DAB)-based peroxidase detection with Vectastain ABC (Vector Labs).

Protein was extracted with the mirVANA PARIS kit according to manufacturer's instructions and after centrifugation the supernatants were used for estimation of total protein with BCA micro-kit (Pierce). BDNF levels were essayed with enzyme-linked immunosorbent assay (ELISA) and with the use of BDNF ELISA kit (Chemicon) according to manufacturer's instructions.

Sections, 8–10 µm thick, were cut from frozen unfixed postmortem human tissue blocks (adult PFC—BA10) on a cryostat (Leica) on plain non-coated glass slides, stored at −80°C, than before staining they were dried for 2 min, fixed in 100% acetone for 2 min, air dried for 30 s, then washed in PBS and processed for immunohistochemistry with the mouse monoclonal anti-NF-H (anti-SMI-32 antibody, Covance) and FITC-conjugated goat-anti mouse antibody, with intermittent washing steps. This staining procedure was limited to altogether <100 min, and then sections were transferred to a Arcturus Veritas microdissection instrument (Molecular Devices) in order to collect somata of layer III NF-H immunoreactive pyramidal neurons, as defined by triangular shape and prominent, vertically oriented apical dendrite. As a control, tissue from deeper white matter was collected. Cells were collected in pools of 500–1000, using the CapSure MacroLCM Caps (Arcturus) collection caps and then transferred to RNase-free Eppendorf tubes and stored at −80°C until further processed. RNA was extracted with the mirVana miRNA isolation kit (Ambion). In particular, the plastic membrane containing harvested cells was removed from the CapSure cap and immersed into 300–400 µl of the kit's lysis-binding buffer, then incubated in the same solution at 42°C for 30 min with intermittent vortexing, in order to remove the laser-captured tissue from the membrane. The yield was ~5 ng/µl small RNA/pool. For dissection of upper and deeper cortical layers, superficial cortical gray matter (approximately upper one-fifth of gray matter) and white matter from frozen unfixed postmortem tissue (n = 5, ages 30, 38, 56, 61, 68 years of age) was removed and the upper (roughly corresponding to parts of layers II and III) and lower one-third (roughly corresponding to parts of layers V and VI) of the remaining gray matter tissue was used for protein and RNA extraction.

Chromatin immunoprecipitation in postmortem tissue from human PFC of different age was done as described previously (38) by using 70–100 mg of tissue and with the primers shown in Supplementary Material, Table S2.

Ambion's pMIR-REPORT luciferase reporter plasmid was engineered to include a 551 bp fragment of human BDNF 3′-UTR (1500–2051 nt, Genbank ID NM_170735) at the 3′ end of the luciferase gene. Lipofectamine 2000 (Invitrogen) was used for transfection of HEK293 cells in 24-well plates. CMV-driven vectors containing chicken beta-actin promoter (CAG-RmiR plasmids) and expressing miRNA precursors (750 ng per well) were cotransfected with the luciferase reporter plasmid (150 ng per well) containing the 551 nt fragment of BDNF 3′-UTR and with Ambion's pMIR-REPORT β-galactosidase plasmid (100 ng per well) to control for transfection efficiency. Luciferase and β-galactosidase assays (Promega) were used to calculate the normalized luciferase expression. As controls 750 ng of vector expressing miR-NSC30 precursor with 3 bases difference in the seed sequence (see also below) or 750 ng of an EGFP expressing vector (control reference) were used. The overexpression of the mature miRNAs was measured with qRT–PCR and from at least two replicates.

The pGIPZ self-inactivating lentiviral empty vector was purchased by Open Biosystems. Two sets of 111 bp oligos that encode the human miR-30a precursor or the miR-30a precursor with 3 bases difference in the seed sequence of the 5p mature miRNA (NSC30) and that contain XhoI and EcoRI restriction enzyme overhangs (purchased by IDT Integrated DNA Technologies) were annealed and initially ligated into a double digested (XhoI, EcoRI) self-inactivating retroviral vector pSM2c by Open Biosystems (Purchased by the shRNA Library Core Facility of UMass Medical School). After PCR and subsequent digestion this product was then ligated to the pGIPZ self-inactivating lentiviral empty vector. The final products (called pmiR30 and NSC30) are designed to drive expression of tGFP (turbo GFP) and the miRNA precursor molecule, through the same CMV RNA polymerase II promoter. The expected mature miRNA of the miR-NSC30 precursor molecule is not predicted to target BDNF mRNA at any region (RNA hybrid software). Standard methodologies were used for preparation of rat forebrain neuronal cultures from precursor cells (38), for viral production and infection (60). The production of the mature miR-30a was assayed with qRT–PCR. In addition, transduction efficiency was estimated by measuring GFP expression 4 days post-infection with epi-fluorescence microscopy (Nikon Eclipse E600). An average of 60% transfection efficiency was observed.