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In This Article

  • Summary
  • Abstract
  • Introduction
  • Protocol
  • Results
  • Discussion
  • Disclosures
  • Acknowledgements
  • Materials
  • References
  • Reprints and Permissions

Summary

The goal of this protocol is to perform in situ hybridization on adult coral samples that have been embedded in paraffin and sectioned onto glass slides. This is a qualitative method used to visualize the spatial expression of an RNA anti-sense probe in paraffin-embedded tissues.

Abstract

Corals are important ocean invertebrates that are critical for overall ocean health as well as human health. However, due to human impacts such as rising ocean temperatures and ocean acidification, corals are increasingly under threat. To tackle these challenges, advances in cell and molecular biology have proven to be crucial for diagnosing the health of corals. Modifying some of the techniques commonly used in human medicine could greatly improve researchers' ability to treat and save corals. To address this, a protocol for in situ hybridization used primarily in human medicine and evolutionary developmental biology has been adapted for use in adult corals under stress.

The purpose of this method is to visualize the spatial expression of an RNA probe in adult coral tissue that has been embedded in paraffin and sectioned onto glass slides. This method focuses on removal of the paraffin and rehydration of the sample, pretreatment of the sample to ensure permeability of the sample, pre-hybridization incubation, hybridization of the RNA probe, and visualization of the RNA probe. This is a powerful method when using non-model organisms to discover where specific genes are expressed, and the protocol can be easily adapted for other non-model organisms. However, the method is limited in that it is primarily qualitative, because expression intensity can vary depending on the amount of time used during the visualization step and the concentration of the probe. Furthermore, patience is required, as this protocol can take up to 5 days (and in many cases, longer) depending on the probe being used. Finally, non-specific background staining is common, but this limitation can be overcome.

Introduction

Corals are critical ecosystem builders and important for biodiversity in ocean and human health1,2,3. They are under threat due to climate change and other anthropogenic stressors, and many coral species are considered critically endangered. Thus, there is a significant need for cellular and molecular tools to diagnose corals under stress. Also, there is little understood about where genes are expressed within adult coral tissue, and therefore little understanding of the functions of these genes. To address this issue, we have adapted the in situ hybridization (ISH) protocol, commonly used in human medicine and evolutionary developmental biology, for use on paraffin-embedded tissue samples of adult corals. This technique is most powerful when used on adult corals that have undergone a stressful event such as exposure to heat stress. However, this technique can be used on a wide range of tissues and life stages in corals and is not limited to only heat-stressed corals4,6,7. Additionally, this technique can be used on tissues or cells of any metazoan as long as there is cDNA sequence information available.

The purpose of this method is to visualize RNA probes within adult coral tissue that has been preserved and embedded in paraffin and sectioned onto slides. This method is a powerful diagnostic tool that allows for the visualization of nucleic acids within adult coral tissue. Initially this method was developed for medical diagnostics, and it has since become a popular tool in fields such as developmental biology and evolutionary developmental biology8,9,10. ISH is also a critical method, particularly in non-model systems, when genomic and transcriptomic sequence data are available but spatial gene expression patterns are unknown. For diagnostic work in non-model systems, this technique is powerful because it can indicate which cells and tissues express a gene of interest and can lead to more targeted therapeutic approaches8,9,10,11,12. Lastly, this technique is qualitative and more powerful when paired with quantitative gene expression data11.

The approach outlined in this paper will be of interest to researchers who have already designed a digoxigenin (DIG)-labeled RNA probe (both the sense and antisense probes) and are now ready to perform in situ hybridization of the probes to a sample. To perform this method, two serial sections of a paraffin coral tissue will be needed for each probe being tested. One section will be used for the sense probe and the other for the antisense probe. The sense probe will be a control to indicate non-specific binding. If staining is observed in the sense probe, then the antisense probe is not specific to the RNA of interest. Probes can be designed for any gene expressed. In this protocol, several examples are used that were previously found to be expressed during heat stress in corals: FBJ murine osteosarcoma viral oncogene homolog B (Fos-B), Activator protein (AP1), and Tumor necrosis factor receptor 41 (TNFR 41)11. ISH using DIG-labeled RNA probes is preferred over using radioactive probes because their handling is much safer10. In addition, this technique is highly sensitive and can be performed on a wide range of tissues and embryos beyond heat-stressed adult corals13,14,15,16.

Protocol

1. Removal of Paraffin

Caution: Perform the following steps under a fume hood.

  1. Dewax the thin-sectioned paraffin-embedded slides with 100% xylene under the hood in glass Coplin jars for 10 min. Do not use plastic Coplin jars, as xylene melts plastic. Sterilize the Coplin jars in an autoclave before use.
  2. Prepare four sterile glass Coplin jars with the following: 100% ethanol, 80% ethanol, 70% ethanol and 60% ethanol. Dilute the ethanol with RNase-free water.
    1. Transfer the slides to the sterile glass Coplin jar with 100% ethanol and soak them for 10 min. After 10 min, empty the glass Coplin jar and replace with new 100% ethanol. Soak the slides again for 10 min.
    2. Transfer the slides to the sterile glass Coplin jar with 80% ethanol for 1 min.
    3. Transfer the slides to the sterile glass Coplin jar with 70% ethanol for 1 min.
    4. Transfer the slides to the sterile glass Coplin jar with 60% ethanol for 1 min.

2. Pretreatment of Slides for Preparation of RNA Probe Hybridization

  1. Perform the following washes at room temperature, unless specified otherwise. Perform room temperature washes on an orbital shaker at a slow speed. Use sterile slide mailers with room for up to five slides for the washing of the slides.
  2. Transfer the slides to a sterile slide mailer with 18 mL of 1x phosphate buffered saline (PBS). Wash for 5 min at room temperature.
  3. Pour off the 1x PBS, and immediately treat the tissue on the slides with proteinase K to enable probe penetration of the tissue. Add approximately 18 mL of proteinase K solution to the slide mailer (see Table 1 for working solution concentration). Incubate at 37 °C for 15 min. Do not shake.
    1. While the slides are incubating, prepare the prehybridization buffer (Prehybe Buffer). Place the Prehybe Buffer in a boiling water bath for 10 min, then cool on an ice bath for 5 min. For a recipe of Prehybe Buffer, see Table 1.
    2. Stop digestion of the proteinase K reaction by pouring out the proteinase K solution, and immediately add 18 mL of 0.2% glycine-PBS solution to the slide mailer. Let the slide mailer sit at room temperature for 5 min.
    3. Pour out the 0.2% glycine-PBS solution and add 18 mL of 2x saline sodium citrate (SSC) solution to each slide mailer. Wash the slides in the 2x SSC for 10 min at room temperature, with shaking at 100-150 rpm.

3. Prehybridization of Slides in Preparation for RNA Probe Hybridization

  1. While the slides are being washed with 2x SSC, obtain a new sterile slide mailer and put approximately 18 mL of Prehybe Buffer into the slide mailer. Place the slide mailer into the hybridization oven at hybridization temperature.
    NOTE: The hybridization temperature will depend on the probe being used but usually ranges from 50-60 °C.
  2. Once the 2x SSC wash is completed, pour out the 2x SSC, and place the slides within the slide mailer in the Prehybe Buffer in the hybridization oven for 1 h.

4. Hybridization of the RNA Probe

  1. While the slides are incubating with the Prehybe Buffer in the hybridization oven, prepare hybridization-probe solution.
    1. Dilute each probe in hybridization buffer (0.5 µL of probe with 24.5 µL of hybridization buffer).
      NOTE: The recipe for hybridization buffer is found in Table 1. An example of probe preparation and concentrations can be found in Traylor-Knowles et al.11.
    2. Place the diluted probe on an 86-90 °C heat block for 12 min, then cool for 1 min on ice.
  2. Remove the slide mailer from the hybridization oven and individually remove slides from the slide mailer using sterile tweezers. Lay the slides flat on a paper towel, and carefully wipe off excess Prehybe Buffer around the tissue samples. Be careful not to touch the samples, and work quickly to prevent drying of the tissue samples.
  3. Encircle the tissue with a PAP pen. Apply 25 µL of diluted probe solution with a pipette and cover the sample with a plastic coverslip.
    1. Place the samples in the slide moisture chamber with 4x SSC + 50% formamide solution in the bottom of the chamber.
    2. Once probes have been added to all the slides, place the slide moisture chamber into the hybridization oven for at least 24 h at a hybridization temperature of 50-60 °C. The incubation time can vary depending on the concentration of the probe but should be for a minimum of 24 hours.
  4. After overnight incubation with the diluted probes, remove the slide moisture chamber from the hybridization oven.
    1. Remove coverslips from each of the slides, being careful not to displace the tissue. In a 1000 µL pipette, add 1000 µL of 2x SSC solution and gently wash the slide off.
    2. Place the slide in a sterile slide mailer with 18 mL of 2x SSC solution for 5 min at room temperature. Pour out the solution and replace it with 18 mL of fresh 2x SSC. Repeat the incubation again for 5 min at room temperature with gentle shaking.
    3. Pour out the 2x SSC solution. Add 18 mL of 1x SSC solution and wash for 5 min at room temperature. Pour out the 1x SSC solution and replace it with 18 mL of fresh 1x SSC. Repeat the incubation for 5 min at room temperature with gentle shaking.
    4. Pour out the 1x SSC. Add 18 mL of 0.5x SSC and wash for 10 min at 42 °C without shaking. Pour out the 0.5x SSC and replace it with 18 mL of fresh 0.5x SSC. Wash again for 10 min at 42 °C without shaking.

5. Visualization of the RNA Probe

NOTE: For visualizing the probe, BM purple will be used during the development process. However, before this step, several washes are required to prepare the samples for staining.

  1. Wash the slides with 18 mL of alkaline phosphatase buffer (AP-buffer) without MgCl2 for 1 min. Pour out the AP-Buffer without MgCl2, and add 18 mL of 1x Boehringer-Mannheim blocking buffer diluted with maleic acid buffer. Incubate for at least 1 h at room temperature in a slide mailer with gentle shaking.
    NOTE: The Boehringer-Mannheim blocking buffer and maleic acid buffer used were premade and purchased in the DIG Wash and Block Buffer Set (available commercially).
    1. Alternatively, incubation overnight at 4 °C can be performed. A longer blocking period will lessen the appearance of non-specific binding.
  2. Prepare the 20 mL of diluted DIG anti-digoxigenin-AP Fab fragments (anti-DIG antibody = 2 µL of anti-DIG antibody + 20 mL 1x Boehringer-Mannheim blocking buffer). This is enough for use in 1 plastic slide mailer. More of this solution must be prepared if more than one slide mailer is to be used.
  3. Add the anti-DIG antibody to a new sterile slide mailer, and transfer the slides to the slide mailer with the anti-DIG antibody solution. Incubate at room temperature for 3 h with gentle shaking.
  4. After incubation, pour out the anti-DIG antibody and wash the slides in the slide mailer with 18 mL of AP-Buffer without MgCl2 for 5 min with gentle shaking.
  5. Pour out the AP-Buffer without MgCl2, and add 18 mL of AP-Buffer. Wash for 5 min with gentle shaking. After the 5 min incubation, pour off the AP-Buffer, replace it with 18 mL of fresh AP-Buffer, and wash for 5 min with gentle shaking.
  6. In the dark, pour out the AP-Buffer and add 18 mL of BM purple to the slide mailer. Incubate the slides at room temperature in the dark, checking for purple color development every ½ h. Reaction times for visualization will vary based on the probe that is being developed.
    NOTE: Instead of BM purple visualization, development solution can be made using 5-bromo-4-chloro-3-indolyl-phosphate (BCIP) and nitro blue tetrazolium (NBT). See Table 1 for instructions.
  7. Stop color development by transferring the slides to a new sterile slide mailer with 18 mL of Tris-EDTA (TE) buffer for 5 min at room temperature, in the dark.
  8. Pour off the TE buffer and add 18 mL of RNase-free water to the slide mailer and wash for 1 min, in the dark.
  9. Remove the slides from the water, and dry them around the edges of the tissue. Add glycerol mounting medium and place the coverslips. Store the slides at 4 °C until pictures are ready to be taken.

Results

After completing this protocol, identification of cells and tissues that are expressing the RNA probe of interest will be achieved. The representative results for this protocol are for AP-1, FosB, and TNFR41. These results, previously published by Traylor-Knowles et al.11, show spatial expression of RNA probes on adult corals that were exposed to heat stress. Two examples of different staining types are presented in Figure 1. ...

Discussion

The method described in this protocol has been modified from previous work in medical and evolutionary developmental research8,9,10,12,17. This protocol focuses on the nuances of an in situ hybridization with a DIG-labeled RNA anti-sense probe on adult corals, which have been preserved and embedded in paraffin. This method can be easily transferred to...

Disclosures

The authors have nothing to disclose.

Acknowledgements

This work was funded by award no. OCE-1323652 through the National Science Foundation Ocean Science Postdoctoral Fellowship and award no.1012629 from the Burroughs Wellcome Fund Postdoctoral Enrichment Program.

Materials

NameCompanyCatalog NumberComments
Denhardt's solutionAffymetrix70468 50 ML
Bioworld Alkaline phosphatase bufferFisher50-198-724
Slide mailersFisher12-587-17B
Bioworld Alkaline phosphatase bufferFisher50-198-724
50 mL Falcon tubesFisher14-959-49A
UltraPure Salmon Sperm DNA solutionInvitrogen15632-011
PBS - Phosphate-Buffered Saline (10X) pH 7.4InvitrogenAM9625
UltraPure DNase/RNase-Free Distilled Water, 10 x 500 mLInvitrogen10977-023
UltraPure DNase/RNase-Free Distilled Water, 10 x 500 mLInvitrogen10977-023
UltraPure Salmon Sperm DNA solutionInvitrogen15632-011
Slide white apex superior adhesiveLeica Biosystems3800080
PBS solution, pH 7.4Life Technologies10010072
Proteinase K, Molecular Grade, 2 mLNew England BiolabsP8107S
Super Pap Pen Liquid BlockerPromega22309
DIG Anti-Digoxigenin-AP Fab fragmentsRoche11093274910
BM Purple, 100 mLRoche11442074001
DIG Wash and Block Buffer SetRoche11585762001
NBT/BCIPRoche11681451001
Formaldehyde solution, 500 mL sizeSigma-Aldrich252549-500ML
SSC Buffer 20X concentrationSigma-AldrichS6639-1L
Acetic AnhydrideSigma-Aldrich320102-100ML
FormamideSigma-Aldrich47670-250ML-F
TriethanolamineSigma-Aldrich90279-100ML
Heparin sodium salt from porcine intestinal mucosaSigma-AldrichH3149-10KU
Xylenes, AR (ACS), For Histological UseVWRMK866806
EthanolVWREM-EX0276-4S
TE bufferVWRPAV6232
hybridization ovenVWR97005-252, 97005-254
Orbital shakerVWR89032-088

References

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  2. Chen, P. -. Y., Chen, C. -. C., Chu, L., McCarl, B. Evaluating the economic damage of climate change on global coral reefs. Global Environmental Change. 30 (Supplement C), 12-20 (2015).
  3. Hoegh-Guldberg, O., et al. Coral Reefs Under Rapid Climate Change and Ocean Acidification. Science. 318 (5857), 1742 (2007).
  4. Grasso, L. C., et al. Microarray analysis identifies candidate genes for key roles in coral development. BMC Genomics. 9 (1), 540 (2008).
  5. Miller, D. J., et al. The innate immune repertoire in Cnidaria - ancestral complexity and stochastic gene loss. Genome Biology. 8 (4), R59 (2007).
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  7. Anctil, M., Hayward, D. C., Miller, D. J., Ball, E. E. Sequence and expression of four coral G protein-coupled receptors distinct from all classifiable members of the rhodopsin family. Gene. 392 (1-2), 14-21 (2007).
  8. Darby, I. A., Hewitson, T. D. . In situ hybridization protocols. , (2006).
  9. Valentino, K. L., Eberwine, J. H., Barchas, J. D. . In situ hybridization. , (1987).
  10. Tautz, D., Pfeifle, C. A non-radioactive in situ hybridization method for the localization of specific RNAs in Drosophila embryos reveals translational control of the segmentation gene hunchback. Chromosoma. 98 (2), 81-85 (1989).
  11. Traylor-Knowles, N., Rose, N. H., Palumbi, S. R. The cell specificity of gene expression in the response to heat stress in corals. Journal of Experimental Biology. 220 (10), (2017).
  12. Wolenski, F. S., Layden, M. J., Martindale, M. Q., Gilmore, T. D., Finnerty, J. R. Characterizing the spatiotemporal expression of RNAs and proteins in the starlet sea anemone, Nematostella vectensis. Nature Protocols. 8, 900 (2013).
  13. Schnitzler, C. E., Simmons, D. K., Pang, K., Martindale, M. Q., Baxevanis, A. D. Expression of multiple Sox genes through embryonic development in the ctenophore Mnemiopsis leidyi is spatially restricted to zones of cell proliferation. EvoDevo. 5 (1), 15 (2014).
  14. Traylor-Knowles, N. G., Kane, E. G., Sombatsaphay, V., Finnerty, J. R., Reitzel, A. M. Sex-specific and developmental expression of Dmrt genes in the starlet sea anemone, Nematostella vectensis. EvoDevo. 6 (1), (2015).
  15. Barry, S. N., Crow, K. D. The role of HoxA11 and HoxA13 in the evolution of novel fin morphologies in a representative batoid (Leucoraja erinacea). EvoDevo. 8 (1), 24 (2017).
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