miR-132 Enhances Dendritic Morphogenesis, Spine Density, Synaptic Integration, and Survival of Newborn Olfactory Bulb Neurons

An array of signals regulating the early stages of postnatal subventricular zone (SVZ) neurogenesis has been identified, but much less is known regarding the molecules controlling late stages. Here, we investigated the function of the activity-dependent and morphogenic microRNA miR-132 on the synaptic integration and survival of olfactory bulb (OB) neurons born in the neonatal SVZ. In situ hybridization revealed that miR-132 expression occurs at the onset of synaptic integration in the OB. Using in vivo electroporation we found that sequestration of miR-132 using a sponge-based strategy led to a reduced dendritic complexity and spine density while overexpression had the opposite effects. These effects were mirrored with respective changes in the frequency of GABAergic and glutamatergic synaptic inputs reflecting altered synaptic integration. In addition, timely directed overexpression of miR-132 at the onset of synaptic integration using an inducible approach led to a significant increase in the survival of newborn neurons. These data suggest that miR-132 forms the basis of a structural plasticity program seen in SVZ-OB postnatal neurogenesis. miR-132 overexpression in transplanted neurons may thus hold promise for enhancing neuronal survival and improving the outcome of transplant therapies

miR-132 sequestration <i>in vivo</i> truncates dendritic development leading to synaptic input deprivation.

<p>(<b>A and B</b>) Representative reconstructions of SCR-SP- (A) and 132-SP-expressing (B, green) newborn neurons at 6 wpe in the GCL. (<b>C and D</b>) Plots of the summed dendritic length (C) and bar graphs of the total dendritic length (D) of SCR-SP-(black) and 132-SP-expressing (B, green) newborn neurons (n = 22 and 25 neurons, respectively). (<b>E</b>) Confocal images of spines in fluorescent neurons containing: SCR-132 (black) or 132-SP (green). (<b>F</b>) Comparison of normalized spine density. N = 3 mice for each condition. (<b>G</b>) Bar graph of the mean frequency of GABA_A PSCs in SCR-SP (black) and 132-SP (green) neurons (n = 18 and 16 neurons, respectively). (<b>H</b>) Representative examples of EPSCs in neurons containing SCR-SP and 132-SP. Scale bar: 10 pA/30 s. (<b>I and J</b>) Bar graphs of the mean amplitude (I) and frequency (J) in neurons containing SCR-SP (black, n = 11 cells) and 132-SP (green, n = 11 cells). Scale bar in A–B: 50 µm; in E: 10 µm.</p

Validation of the specificity of miR-132 sponge vectors and experimental diagram.

<p>(<b>A</b>) Schematic of vectors encoding GFP containing 20 tandem, miR-132-binding sites in its 3′UTR (orange bars) to “sponge” out miR-132 (132-SP) and a control vector encoding mutant GFP containing 20 random sites in its 3′UTR (SCR9-SP). (<b>B</b>) Schematic of a sensor vector encoding RFP containing perfectly complementary miR-132 binding sites (blue bars). (<b>C</b>) Confocal images of Neuro-2A cells transfected with the sensor vector and SCR-SP or 132-SP. Scale bar: 70 µm. (<b>D</b>) Diagram of our experimental paradigm. DNA constructs were introduced into the lateral ventricle of P0–P1 pups for electroporation into neural progenitor cells. 4–6 weeks post-electroporation, fluorescently tagged, synaptically integrated newborn neurons were analyzed.</p

miR-132 overexpression at synaptic integration promotes long-term neuronal survival.

<p>(<b>A</b>) qRT-PCR of miR-132 fold-change normalized to control RNA U6 from the ipsilateral bulbs containing pSico¹³²-expressing neurons (red) and from the contralateral bulbs (black) at 5 weeks post-tamoxifen (wpt) injections given 2 wpe (N = 5 mice each). (<b>B and C</b>) Plots of the summed dendrite length (B) and bar graphs of the total dendritic length (C) of pSico^SCR (n = 47) and pSico¹³²-containing neurons (n = 51) at 5 wpt injections given at 7 dpe (i.e. 6 wpe). (<b>D</b>) Bar graphs of the frequency of GABAergic PSCs in pSico^SCR- and pSico¹³²-containing neurons at 5 wpt (n = 13 black and 15 red, respectively). (<b>G</b>) Sample images illustrating the density of pSico^SCR and pSico¹³² neurons in OB coronal sections. (<b>H and I</b>) Bar graphs of absolute (H) and normalized (I) RFP⁺ (<i>i.e.</i> pSico^SCR, black and pSico¹³², red) neuron density in the GCL (N = 8 and 9 mice, 3–4 images per mouse, respectively). Scale bar: 100 µm.</p

miR-132 overexpression promotes dendritic morphogenesis and synaptic integration <i>in vivo</i>.

<p>(<b>A and B</b>) Representative reconstructions of SCR-132 (A) and miR-132-expressing (B, red) newborn neurons at 8 wpe in the GCL. <b>(B)</b> Plots of the summed dendritic length of SCR-132-(black) and miR-132 expressing (B, red) newborn neurons (n = 38 and 55 neurons, respectively). <b>(C)</b> Bar graphs of the percentage (%) of control for the total dendritic length of miR-132 overexpressing neurons (red). A break in the Y-axis was inserted between 5 and 60 µm. ). <b>(D)</b> Confocal images of spines in fluorescent neurons containing: SCR-132 (black) or miR-132 (red). <b>(E)</b> Bar graphs of the normalized spine density. N = 3 mice for each condition. <b>(F)</b> Representative traces of GABAergic postsynaptic synaptic currents (PSCs) in SCR-132- and miR-132-containing neurons. <b>(G and H)</b> Bar graphs of the frequency (E) and amplitude (F) of GABAergic PSCs in SCR-132- and miR-132-containing neurons (n = 10 black and 15 red, respectively). Scale bar: 100 pA/500 ms in F.</p

miR-132 is expressed in newborn SVZ neurons at the onset of synaptic integration.

<p>(<b>A–D</b>) <i>In situ</i> hybridization images of miR-132 with TOPRO-3 (red) overlay (red, A), miR-132 (B), miR-1 (C), and miR-9 (D) in a sagittal section containing the SVZ, RMS and OB. (<b>E–G</b>) Higher magnification of miR-132, miR-1 and miR-9 images in the granule cell layer (GCL). Scale bars: 100 µm (A–D) and 30 µm (E–F). The image in (E) comes from the boxed region in (A). (<b>H</b>) Bar graphs of miR-132 qRT-PCR fold changes in the RMS_OB and GCL compared to the SVZ.</p