Name: immunostaining of neurons in mouse brain slices following fluorescence in situ hybridization
Uploaded: 2025-04-28T12:01:57.000+00:00
Duration: 1 min 25 s
Description: Source: Baleriola, J., et. al., Detection of Axonally Localized mRNAs in Brain Sections Using High-Resolution In Situ Hybridization. J. Vis. ...

immunostaining of neurons in mouse brain slices following fluorescence in situ hybridization

Immunostaining of Neurons in Mouse Brain Slices Following Fluorescence In Situ Hybridization

Cover each slice with 100 to 200 microliters of blocking solution, containing three milligrams per milliliter BSA, 100 millimolar glycine, and 0.25% Triton X-100 in PBS. Cover each slide with parafilm, and incubate for 30 minutes at room temperature.Following the incubation, at 100 to 200 microliters of antibody diluted in blocking solution to the slides, an anti-choline acetyltransferase antibody is used here. After covering, the slides with parafilm, incubate for two days at four degrees Celsius. Make sure that brain slices don't dry out. If needed, reapply anti-chAT antibody solution to brain slices 24 hours after incubation.After washing the slides three times in 1X PBS for five minutes at room temperature, add 100 to 200 microliters of the appropriate Alexa conjugated secondary antibody to the slides. Cover with parafilm and incubate for one hour at room temperature while protected from light.After the hour has elapsed, wash the slides three times in 1X PBS for five minutes each as before, and then wash once with distilled water. Mount the slides with mounting medium containing DAPI. And then visualize the brain slices under the fluorescence microscope.

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All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee.<ol><li>FISH assay followed by immunohistochemistry using heat-induced antigen/RNA unmasking<ol style='list-style-type:decimal;'><li>Before starting, prepare all required material:<ol style='list-style-type:decimal;'><li>Heat the hybridization oven to 40 &#8451; and place a tray containing distilled water in the oven to create a humidified environment.</li><li>Take a slide box and place paper towels soaked in distilled water inside to humidify it. Then, place the slide box in the hybridization oven.</li><li>Remove the probes (both negative and target probes) from the fridge and heat them in the hybridization oven for 10 minutes. Then, let the probes cool down at RT.</li><li>Equilibrate amplification reagents AMP 1-4 (included in the Fluorescent Multiplex Reagent Kit) at RT.</li><li>Prepare antigen retrieval solution: 10 mM sodium citrate (pH 6), 0.05% Tween 20.&#160;Note: Solution can be stored at RT indefinitely and be used for future staining.</li><li>Prepare 1x wash buffer diluting the 50x stock solution (in the Fluorescent Multiplex Reagent Kit) in RNase-free or DEPC-treated water. NOTE: 1x wash buffer can be stored at RT for 1 month and be used for future staining. 50x wash buffer might precipitate. If so, heat 50x wash buffer at 40 &#8451; for 10 min before preparing the 1x solution.</li></ol></li><li>Remove slides from 100% ethanol and air-dry for 5 min at RT.</li><li>Prepare a coplin jar containing 50 ml of antigen retrieval solution. Immerse slides in antigen retrieval solution and boil them for 10 min in a microwave oven. NOTE: Alternatively place slides horizontally in a 100 mm diameter round glass dish containing 100 ml of retrieval solution.<ol style='list-style-type:decimal;'><li>Fill up a 1 L beaker with distilled water and place it in the microwave. NOTE:&#160;The water will &#8220;buffer&#8221; the heat when performing unmasking.</li><li>Place the slides in antigen retrieval solution inside the microwave. Boil slides at high power for 5 min. Immediately after samples have stopped boiling, heat slides again at high power for an extra 5 min.</li><li>Cool down slides at RT. NOTE: CRITICAL STEP: boiling duration and procedure should be determined by the user, depending on the microwave characteristics. The faster the boiling starts, the higher the chances of solution evaporation. In this case it is recommended that samples are boiled for shorter time periods more than twice to complete a total unmasking time of 10 min. On the contrary, if heating is performed at medium or low power, unmasking can be performed once for 10 min. However, if samples do not boil continuously for a total of approximately 10 min, this might result in partial unmasking of both the target RNA and protein to be detected.</li></ol></li><li>Wash slides three times with 1x PBS.</li><li>Add 2 - 3 drops (~100 &#956;l) of the&#160;dapB probe set to those brain slices used to assess background staining.&#160;NOTE: The&#160;dapB probe set targets a bacterial gene and should not recognize any mammalian RNA.</li><li>Add 2 - 3 drops of the targeting probe set to those brain slices used to detect the RNA of interest.&#160;NOTE: a probe set targeting residues 20 - 1,381 of the mouse&#160;Atf4 mRNA is used in this example.</li><li>Cover slides with parafilm to avoid probe evaporation, place them in the humidified slide box inside the hybridization oven, and incubate them at 40 &#8451; for 2 hrs. &#8203;NOTE: OPTIONAL: additional brain slices can be hybridized with a probe set targeting mouse&#160;Polr2A and used as positive controls.</li><li>Wash slides twice with 1x wash buffer for 2 min at RT.</li><li>Add 2 - 3 drops of amplification reagent AMP 1-FL to each brain slice, cover slides with parafilm, place them in the slide box, and incubate at 40 &#8451; for 30 min in the hybridization oven.</li><li>Wash slides twice with 1x wash buffer for 2 min at RT.</li><li>Add 2 - 3 drops of amplification reagent AMP 2-FL to each brain slice, cover slides with parafilm, place them in the slide box and incubate at 40 &#8451; for 15 min in the hybridization oven.</li><li>Wash slides twice with 1x wash buffer for 2 min at RT.</li><li>Add 2 - 3 drops of amplification reagent AMP 3-FL to each brain slice, cover slides with parafilm, place them in the slide box and incubate at 40&#160;&#8451; for 30 min in the hybridization oven.</li><li>Wash slides twice with 1x wash buffer for 2 min at RT.</li><li>Add 2 - 3 drops of amplification reagent AMP 4-FL to each brain slice, cover slides with parafilm, place them in the slide box and incubate at 40&#160;&#8451; for 15 min in the hybridization oven.</li><li>Wash slides twice with 1x wash buffer for 2 min at RT and twice with 1x PBS.</li><li>Add 100 - 200 &#956;l (or enough volume to completely cover slices) of a blocking solution containing 3 mg/ml BSA, 100 mM glycine, and 0.25% Triton X-100 in PBS (pH 7.4) to the slides, cover them with parafilm, and incubate for 30 min at RT.</li><li>Add 100 - 200 &#956;l of anti-ChAT antibody diluted in blocking solution (1/100) to the slides, cover them with parafilm, and incubate for 2 days at 4&#160;&#8451;. Make sure that brain slices don&#8217;t dry out. If needed, re-apply the anti-ChAT antibody solution to brain slices 24 hrs after incubation.</li><li>Wash slides three times in 1x PBS for 5 min at RT.</li><li>Add 100 - 200 &#956;l of the appropriate Alexa-conjugated secondary antibody (e.g., Alexa-594 donkey anti-goat for this particular example) to the slides, cover with parafilm, and incubate for 1 hr at RT.</li><li>Wash slides three times in 1x PBS for 5 min at RT.</li><li>Wash slides once with distilled water.</li><li>Mount slides with a DAPI-containing mounting medium.</li><li>Visualize brain slices under a fluorescence microscope.</li></ol></li></ol>

<figure class='table' style='width:540pt;'><table class='ck-table-resized'><colgroup><col style='width:26.85%;'><col style='width:25.74%;'><col style='width:21.11%;'><col style='width:26.3%;'></colgroup><tbody><tr><td style='height:58.0pt;width:145pt;'>Custom probe targeting residues 20-1381 of the mouse Atf4 mRNA (NM_009716)</td><td style='width:139pt;'>Advanced Cell Diagnostics</td><td style='width:114pt;'>-</td><td style='width:142pt;'>Probe</td></tr><tr><td style='height:58.0pt;width:145pt;'>Custom probe targeting residues 15-1256 of the human ATF4 mRNA (NM_001675.2)</td><td style='width:139pt;'>Advanced Cell Diagnostics</td><td style='width:114pt;'>-</td><td style='width:142pt;'>Probe</td></tr><tr><td style='height:14.5pt;width:145pt;'>Negative control probe-DapB</td><td style='width:139pt;'>Advanced Cell Diagnostics</td><td style='text-align:right;width:114pt;'>310043</td><td style='width:142pt;'>Probe</td></tr><tr><td style='height:29.0pt;width:145pt;'>Positive control probe-mouse Polr2A (optional)</td><td style='width:139pt;'>Advanced Cell Diagnostics</td><td style='text-align:right;width:114pt;'>312471</td><td style='width:142pt;'>Probe</td></tr><tr><td style='height:29.0pt;width:145pt;'>Goat polyclonal anti-ChAT antibody</td><td style='width:139pt;'>Millipore</td><td style='width:114pt;'>AB144P</td><td style='width:142pt;'>&#160;</td></tr><tr><td style='height:29.0pt;width:145pt;'>ProLong Gold mounting medium with DAPI</td><td style='width:139pt;'>Life Technologies</td><td style='width:114pt;'>P36935</td><td style='width:142pt;'>&#160;</td></tr><tr><td style='height:43.5pt;width:145pt;'>RNAscope Fluorescent Multiplex Reagent Kit (for fluorescence detection)</td><td style='width:139pt;'>Advanced Cell Diagnostics</td><td style='width:114pt;'>320850</td><td style='width:142pt;'>In situ hybridization kit</td></tr></tbody></table></figure>

<a href='https://app.jove.com/v/52799/detection-axonally-localized-mrnas-brain-sections-using-high'>Source: Baleriola, J., et. al., Detection of Axonally Localized mRNAs in Brain Sections Using High-Resolution In Situ Hybridization. J. Vis. Exp.&#160;(2015)</a>This video demonstrates the detection of mRNA within cholinergic axons in fixed mouse hippocampal slices using fluorescent in situ hybridization and antibody staining. Fluorescence microscopy reveals the spatial localization of probe-tagged mRNAs and choline acetyltransferase in cholinergic neurons.

Source: Baleriola, J., et. al., Detection of Axonally Localized mRNAs in Brain Sections Using High-Resolution In Situ Hybridization. J. Vis. ...

Take fixed and permeabilized mouse brain slices containing neurons, including cholinergic neurons expressing choline acetyltransferase.The slices are subjected to fluorescent in situ hybridization to detect target mRNAs localized to cholinergic axons, resulting in amplified signals using fluorescent probes, which are detected with fluorescence microscopy.Add a blocking solution containing proteins and a quenching agent. The proteins prevent non-specific binding, and the quenching agent neutralizes residual fixatives.Incubate with primary antibodies that target neuronal choline acetyltransferase.Wash with buffer to remove unbound antibodies.Incubate with fluorophore-conjugated secondary antibodies that bind to the choline acetyltransferase-bound primary antibodies.Wash with buffer to remove excess antibodies, then rinse in distilled water to remove buffer residues.Mount the slices with mounting media containing a nuclear stain to label the nuclei.Using fluorescence microscopy, image the slices to visualize the target mRNA signals and cholinergic axons stained with specific antibodies.

14 Views. Immunostaining of Neurons in Mouse Brain Slices Following Fluorescence In Situ Hybridization

Video: Immunostaining of Neurons in Mouse Brain Slices Following Fluorescence In Situ Hybridization - Experiment

Immunostaining to Visualize Murine Enteric Nervous System Development

The enteric nervous system is formed by neural crest cells that proliferate, migrate and colonize the gut. Following colonization, neural crest cells must then differentiate into neurons with markers specific for their neurotransmitter phenotype. Cholinergic neurons, a major neurotransmitter phenotype in the enteric nervous system, are identified by staining for choline acetyltransferase (ChAT), the synthesizing enzyme for acetylcholine. Historical efforts to visualize cholinergic neurons have been hampered by antibodies with differing specificities to central nervous system versus peripheral nervous system ChAT. We and others have overcome this limitation by using an antibody against placental ChAT, which recognizes both central and peripheral ChAT, to successfully visualize embryonic enteric cholinergic neurons. Additionally, we have compared this antibody to genetic reporters for ChAT and shown that the antibody is more reliable during embryogenesis. This protocol describes a technique for dissecting, fixing and immunostaining of the murine embryonic gastrointestinal tract to visualize enteric nervous system neurotransmitter expression.

The enteric nervous system is formed by neural crest cells that proliferate, migrate and colonize the gut. Neural crest cells differentiate into neurons with markers specific for their neurotransmitter phenotype. This protocol describes a technique for dissecting, fixing and immunostaining of the murine embryonic gastrointestinal tract to visualize enteric nervous system neurotransmitter expression.

The enteric nervous system is formed by neural crest cells that proliferate, migrate and colonize the gut. Following colonization, neural crest cells must ...

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Developmental Biology

Combining Multiplex Fluorescence In Situ Hybridization with Fluorescent Immunohistochemistry on Fresh Frozen or Fixed Mouse Brain Sections

Fluorescent in situ hybridization (FISH) is a molecular technique that identifies the presence and spatial distribution of specific RNA transcripts within cells. Neurochemical phenotyping of functionally identified neurons usually requires concurrent labelling with multiple antibodies (targeting protein) using immunohistochemistry (IHC) and optimization of in situ hybridization (targeting RNA), in tandem. A &#34;neurochemical signature&#34; to characterize particular neurons may be achieved however complicating factors include the need to verify FISH and IHC targets before combining the methods, and the limited number of RNAs and proteins that may be targeted simultaneously within the same tissue section.
Here we describe a protocol, using both fresh frozen and fixed mouse brain preparations, which detects multiple mRNAs and proteins in the same brain section using RNAscope FISH followed by fluorescence immunostaining, respectively. We use the combined method to describe the expression pattern of low abundance mRNAs (e.g., galanin receptor 1) and high abundance mRNAs (e.g., glycine transporter 2), in immunohistochemically identified brainstem nuclei.
Key considerations for protein labelling downstream of the FISH assay extend beyond tissue preparation and optimization of FISH probe labelling. For example, we found that antibody binding and labelling specificity can be detrimentally affected by the protease step within the FISH probe assay. Proteases catalyze hydrolytic cleavage of peptide bonds, facilitating FISH probe entry into cells, however they may also digest the protein targeted by the subsequent IHC assay, producing off target binding. The subcellular location of the targeted protein is another factor contributing to IHC success following FISH probe assay. We observed IHC specificity to be retained when the targeted protein is membrane bound, whereas IHC targeting cytoplasmic protein required extensive troubleshooting. Finally, we found handling of slide-mounted fixed frozen tissue more challenging than fresh frozen tissue, however IHC quality was overall better with fixed frozen tissue, when combined with RNAscope.

Combining Multiplex Fluorescence In Situ Hybridization with Fluorescent Immunohistochemistry on Fresh Frozen or Fixed Mouse Brain Sections

This protocol describes a method for combining fluorescence in situ hybridization (FISH) and fluorescence immunohistochemistry (IHC) in both fresh frozen and fixed mouse brain sections, with the goal of achieving multilabel FISH and fluorescence IHC signal. IHC targeted cytoplasmic and membrane attached proteins.

Fluorescent in situ hybridization (FISH) is a molecular technique that identifies the presence and spatial distribution of specific RNA transcripts within ...

In Situ Hybridization Combined with Immunohistochemistry in Cryosectioned Zebrafish Embryos

As a vertebrate, the zebrafish has been widely used in biological studies. Zebrafish and humans share high genetic homology, which allows its use as a model for human diseases. Gene function study is based on the detection of gene expression patterns. Although immunohistochemistry offers a powerful way to assay protein expression, the limited number of commercially available antibodies in zebrafish restricts the application of costaining. In situ hybridization is widely used in zebrafish embryos to detect mRNA expression. This protocol describes how to obtain images by combining in situ hybridization and immunohistochemistry for zebrafish embryo sections. In situ hybridization was performed prior to cryosectioning, followed by antibody staining. Immunohistochemistry and the imaging of a single cryosection were performed after in situ hybridization. The protocol is helpful to unravel the expression pattern of two genes, first by in situ transcript detection and then by immunohistochemistry against a protein in the same section.

In Situ Hybridization Combined with Immunohistochemistry in Cryosectioned Zebrafish Embryos

This protocol describes how to obtain images by combining in situ hybridization and immunohistochemistry of zebrafish embryonic sections. In situ hybridization was performed prior to cryosectioning, followed by antibody staining. It is useful to detect the expression patterns of two genes in zebrafish if there is a paucity of antibodies.

As a vertebrate, the zebrafish has been widely used in biological studies. Zebrafish and humans share high genetic homology, which allows its use as a ...

Immunostaining of Neurons in Mouse Brain Slices Following Fluorescence In Situ Hybridization

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Immunostaining of Neurons in Mouse Brain Slices Following Fluorescence In Situ Hybridization