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In This Article

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

Summary

The protocol describes a modification of the rapid Golgi method, which can be adapted to any part of the nervous system, for staining neurons in the hippocampus and medial prefrontal cortex of the rat.

Abstract

Golgi impregnation, using the Golgi staining kit with minor adaptations, is used to impregnate dendritic spines in the rat hippocampus and medial prefrontal cortex. This technique is a marked improvement over previous methods of Golgi impregnation because the premixed chemicals are safer to use, neurons are consistently well impregnated, there is far less background debris, and for a given region, there are extremely small deviations in spine density between experiments. Moreover, brains can be accumulated after a certain point and kept frozen until further processing. Using this method any brain region of interest can be studied. Once stained and cover slipped, dendritic spine density is determined by counting the number of spines for a length of dendrite and expressed as spine density per 10 µm dendrite.

Introduction

The method of using potassium dichromate and silver nitrate to label neurons was first described by Camillo Golgi1,2 and subsequently used by Santiago Ramon y Cajal to produce an immense body of work differentiating neuronal and glial subtypes. A recently published book with his illustrations is now available3. Following Ramon y Cajal's studies, which were published more than 100 years ago, very little Golgi impregnation was used. Golgi impregnation is a laborious process that allows three-dimensional visualization of neurons with a light microscope. There have been numerous modifications of the Golgi method over the years to make the method easier and the staining more consistent4. In 1984, Gabbott and Somogyi5 described the single section Golgi impregnation procedure which allowed for more rapid processing. This Golgi impregnation method requires perfusion with 4% paraformaldehyde and 1.5% picric acid, post-fixation followed by vibratome sectioning into a bath of 3% potassium dichromate. Sections are mounted onto glass slides, the four corners of coverslips glued so that when immersed in silver nitrate, diffusion is gradual. Coverslips are then popped off, sections are dehydrated, and eventually cover slipped permanently with mounting medium. This technique was successfully used to label neurons and glia6,7,8 in the hippocampus. The rapid Golgi method described here is an improvement because there is far less exposure to both potassium dichromate and silver nitrate and no paraformaldehyde and picric acid are used. In addition, although cells that were impregnated using modifications of the Gabbott and Somogyi5 method could be analyzed, often the sections were over-or under-exposed or fell off the slides during the dehydration step and generally, several experiments had to be pooled to have enough cells for analysis.

The present protocol describes the use of the Golgi staining kit (see Table of materials) to label dendrites and dendritic spines in the hippocampus and medial prefrontal cortex (mPFC) of the rat. The advantages of this method over previous ones are that it is rapid, there is less exposure to noxious chemicals for the researcher and there is consistent staining of neurons. The protocol described below has been used with minor modifications to assess dendritic spine density in the hippocampus and mPFC of the rat in many studies9,10,11,12,13,14,15.

Protocol

All experimental procedures are approved by the Sacred Heart University Institutional Animal Care and Use Committee and are in accordance with the NIH Guide for the Care and Use of Animals.

1. Isolation and infiltration of brain tissue

  1. Premix solutions A and B of the Golgi staining kit 24 h prior to use and keep in dark bottles and/or in dark. Make approximately 80 mL of solution A and B mix which is sufficient to change the solution after 24 h. Store in airtight bottles.
    NOTE: Perfusion with either saline or paraformaldehyde is not necessary.
  2. Sacrifice rats by guillotine following carbon dioxide euthanasia and remove brains within seconds. Rinse brains in saline if required but is not necessary.
    1. Place the brain, cortex down so that the hypothalamus is visible because the cuts are made anterior and posterior to it, on a non-porous surface. Cut into an anterior (contains the prefrontal cortex) and posterior (contains the hippocampus) block as shown in Figure 1.
  3. Place blocks into the premixed solutions of A and B, making sure that they are well immersed in the solution. Ensure that the volume of solutions A and B is sufficient to immerse the blocks. Store blocks in either brown bottles or clear bottles covered with foil (to keep light out) in the dark at room temperature.
  4. Replace solution after 24 h and keep in the dark for another 13 days at room temperature.
    NOTE: If used with mouse brains, there is no need to block, and the entire brain can be placed in the solution. If staining brain areas, which are different in size, the time in solutions A and B may have to be determined by trial and error.
  5. After two weeks the tissue is infiltrated well with solutions A and B, transfer the blocks to the cryoprotectant solution (solution C in the Golgi staining kit), and leave them for 48-72 h at 4 °C.
    NOTE: After cryoprotection, blocks may be frozen until further processing. Also, note that all solutions from the kit are collected and disposed of as hazardous waste.
  6. Freeze brain, cortex down, on a glass slide on dry ice. Once frozen either cut on the cryostat or store at -80 °C until sectioning using a cryostat.
    ​NOTE: Do not freeze in liquid nitrogen as this produces cracks in the tissue.

2. Sectioning of brain tissues

  1. Place a small amount of tissue medium on a pre-cooled cryostat chuck. Mount blocks on cryostat chucks by thawing one side of the block slightly in hand (gloved) and placing it on the tissue medium.
    NOTE: It is not necessary to embed the tissue. The block containing the hippocampus is somewhat easier to cut than the block with the prefrontal cortex because the latter is anterior to the corpus callosum and the two halves are separate.
  2. Cut 100 µm sections on a cryostat at -22 °C and mount onto subbed slides. Sections up to 150 µm of thickness can be used. Try to mount 3-4 coronal sections per slide as this decreases the number of slides that require processing. Use one of the following techniques to keep the sections frozen till they get on the slide.
    NOTE: These sections are not fixed in the usual way and therefore they tend to melt quickly. Allow the sections to melt on the slide. If they begin to melt before being placed on the slide, it is impossible to get them to be flat on the slide. There are several techniques to do this.
    1. Use a freezing spray on the knife and the block. Depending on the temperature and humidity in the room this may be necessary for every section. Use either the antiroll plate or a brush to keep the section flat while cutting.
      NOTE: Make sure to have enough freezing spray. Several cans can be used when cutting 20 blocks.
    2. Thaw mount, if possible, by using a room temperature slide and quickly appose it to the section. With practice, one can mount several sections at once. If this doesn't work, keep slides in the cryostat so they are very cold and transfer the section with cold forceps or a cold paintbrush and then thaw mount.
  3. Clean the knife with paper wipes between slices. If the knife requires more cleaning, use 100% ethanol (EtOH), and let it dry before cutting the next slice.
  4. Once mounted onto the slide, place the slide flat on cardboard slide trays and allow sections to dry at room temperature (for several hours to a maximum of 48 h) in the dark. Do not cover the slide tray. Ensure that the sections are completely dry before Golgi impregnation. Store flat, in the dark, on slide trays until Golgi impregnation.
    ​NOTE: Drying the sections does not cause any damage.

3. Staining and dehydration of brain tissue

  1. Perform staining in glass staining dishes. Mix solutions D and E immediately prior to staining. As per the protocol, add one part of solution D, one part of solution E, and two parts of distilled water. For glass staining dishes, make a 200 mL solution to completely submerge the sections. For Koplin jars, this requires less volume.
  2. Place slides in racks spaced far enough apart to allow solution access to sections.
  3. Place sections in distilled water for 4 min (2x) before placing them into the Golgi impregnation staining solution for 10 min. Change the staining solution every 70 sections. Change the distilled water when it turns yellow.
    NOTE: The timing for the staining step is critical. Too short does not allow enough staining and too long causes over staining, making the dendrites hard to separate when doing analysis. Once out of the staining solution the timing is less critical.
  4. Dehydrate the sections as follows: 70% EtOH (5 min), 95% EtOH (5 min; 2x), 100% EtOH (5 min; 2x), clearing agent (5 min; 3x). Change all solutions often, especially the 100% EtOH and clearing agent to ensure the sections remain anhydrous.
    NOTE: It is not necessary to go through a 50% EtOH step. Counterstaining is not needed for cell visualization because the Golgi impregnation provides sufficient contrast. The use of other clearing agents has not worked as well as the one used here (see Table of materials).
  5. Coverslip with glass coverslips that are 60 mm long with a generous amount of mounting medium. Make sure that there are, as few air bubbles as possible. If needed, carefully remove, and redo the coverslip (can be done even weeks later). Do this very slowly in order not to damage the section (can be done because of the large amount of mounting medium).
    NOTE: A large amount of mounting medium is somewhat messy but still necessary because enough mounting medium must be used to cover the thick 100 µm sections.
  6. To ensure that only one coverslip is placed on the sections, separate the coverslips in advance of the process.
  7. Once cover slipped, dry slides flat on any non-porous paper for 3-5 days, moving them slightly, especially after the first day, to avoid sticking. After 3-5 days transfer the slides to slide holders and, ideally, dry slides for at least 3 weeks before examining them. Keep slides flat to decrease the possibility of air bubbles forming.

4. Determination of dendritic spine density

  1. For analysis of dendritic spine density in pyramidal neurons of both the mPFC and the CA1 region of the hippocampus, examine the most lateral secondary basal dendrites and the most lateral tertiary apical dendrites as described in step 4.1.1 (Figure 2).
    1. Choose a dendrite, measure the length of the dendrite using an image analysis program, count the spines on the dendrites using a hand counter, and record both length and number of spines.
  2. Study and analyze six cells per region (mPFC, CA1) per brain. Quantify a minimum of six brains per group as previously described7,8. Choose neurons that meet the following criteria for analysis: cell bodies and dendrites are well impregnated; dendrites are distinguishable from adjacent cells and are continuous.
  3. Count the spines at 1000x (oil-immersion) by hand counting with a light microscope and measure dendritic length using an image analysis program. Calculate spine density by dividing the spine number by the length of the dendrite and express data as the number of spines/ 10 µm dendrite.
    NOTE: There are far more sophisticated methods for differentiating spine subtypes and dendritic architecture that can be used, but hand counting with a light microscope at 1000x can give a rapid result that can then determine if further investigation is necessary. Although every effort is made to consistently sample similar dendrites, there are variations in thickness that may affect the counting.

Results

Using the rapid Golgi method, cells are consistently well impregnated so that there are plenty of cells to analyze. This is a marked improvement over prior methods where experiments had to be pooled to have enough data for analysis. Therefore, more samples can be processed at once and brains can be stored frozen until processing. Examples of Golgi impregnated cells in the CA1 region of the hippocampus are shown at low and high power in Figure 3. Counting of spines in a given region yields co...

Discussion

The present protocol describes a method of Golgi impregnation that allows for rapid simultaneous processing of many sections. It is an improvement over previously described5 more labor-intensive methods and consistently yields impregnated neurons for analysis. In addition, there is less exposure to toxic chemicals used in Golgi impregnation. The most challenging part of the process is getting the sections to be flat on the slides, which takes considerable practice. Keeping everything as cold as po...

Disclosures

The authors have nothing to disclose.

Acknowledgements

This work was supported by Sacred Heart University Undergraduate Research InitiativeGrants.

Materials

NameCompanyCatalog NumberComments
Cardboard slides traysFisher Scientific12-587-10
Coverslips 24 x 60mmFisher Scientific12-545-M
FD Rapid GolgiStain kitFD NeurotechnologiesPK 401Stable at RT in the dark for months; Golgi staining kit
Freezing SprayFisher Scientific23-022524
HISTO-CLEARFisher Scientific50-899-90147clearing agent
NCSS SoftwareKaysville, UT, USA
PermountFisher ScientificSP-15-100mounting medium
Superfrost Plus Microscope slidesFisher Scientific12-550-15
Tissue Tek CTYO OCT CompoundFisher Scientific14-373-65Used to mount brains on cryostat chuck

References

  1. Pannese, E. The Golgi Stain: invention, diffusion and impact on neurosciences. Journal of the History of the Neurosciences. 8 (2), 132-140 (1999).
  2. Bentivoglio, M., et al. The Original Histological Slides of Camillo Golgi and His Discoveries on Neuronal Structure. Frontiers in Neuroanatomy. 13, 3 (2019).
  3. Swanson, L. W., Newman, E., Araque, A., Dubinsky, J. M. . The Beautiful Brain: The Drawings of Santiago Ramon y Cajal. , 208 (2017).
  4. Dall'Oglio, A., Ferme, D., Brusco, J., Moreira, J. E., Rasia-Filho, A. A. The "single-section" Golgi method adapted for formalin-fixed human brain and light microscopy. Journal of Neuroscience Methods. 189 (1), 51-55 (2010).
  5. Gabbott, P. L., Somogyi, J. The 'single' section Golgi-impregnation procedure: methodological description. Journal of Neuroscience Methods. 11 (4), 221-230 (1984).
  6. Gould, E., Frankfurt, M., Westlind-Danielsson, A., McEwen, B. S. Developing forebrain astrocytes are sensitive to thyroid hormone. Glia. 3 (4), 283-292 (1990).
  7. Gould, E., Woolley, C. S., Frankfurt, M., McEwen, B. S. Gonadal steroids regulate dendritic spine density in hippocampal pyramidal cells in adulthood. Journal of Neuroscience. 10 (4), 1286-1291 (1990).
  8. Woolley, C. S., Gould, E., Frankfurt, M., McEwen, B. S. Naturally occurring fluctuation in dendritic spine density on adult hippocampal pyramidal neurons. Journal of Neuroscience. 10 (12), 4035-4039 (1990).
  9. Frankfurt, M., Salas-Ramirez, K., Friedman, E., Luine, V. Cocaine alters dendritic spine density in cortical and subcortical brain regions of the postpartum and virgin female rat. Synapse. 65 (9), 955-961 (2011).
  10. Frankfurt, M., Luine, V. The evolving role of dendritic spines and memory: Interaction(s) with estradiol. Hormones Behavior. 74, 28-36 (2015).
  11. Bowman, R. E., Luine, V., Khandaker, H., Villafane, J. J., Frankfurt, M. Adolescent bisphenol-A exposure decreases dendritic spine density: role of sex and age. Synapse. 68 (11), 498-507 (2014).
  12. Bowman, R. E., et al. Bisphenol-A exposure during adolescence leads to enduring alterations in cognition and dendritic spine density in adult male and female rats. Hormones Behavior. 69, 89-97 (2015).
  13. Eilam-Stock, T., Serrano, P., Frankfurt, M., Luine, V. Bisphenol-A impairs memory and reduces dendritic spine density in adult male rats. Behavioral Neuroscience. 126 (1), 175-185 (2012).
  14. Inagaki, T., Frankfurt, M., Luine, V. Estrogen-induced memory enhancements are blocked by acute bisphenol A in adult female rats: role of dendritic spines. Endocrinology. 153 (7), 3357-3367 (2012).
  15. Jacome, L. F., et al. Gonadal Hormones Rapidly Enhance Spatial Memory and Increase Hippocampal Spine Density in Male Rats. Endocrinology. 157 (4), 1357-1362 (2016).
  16. Frankfurt, M. Bisphenol-A: a plastic manufacturing compound disrupts critical brain structures and impairs memory. Research Features. , (2021).
  17. Wallace, M., Luine, V., Arellanos, A., Frankfurt, M. Ovariectomized rats show decreased recognition memory and spine density in the hippocampus and prefrontal cortex. Brain Research. 1126 (1), 176-182 (2006).
  18. Wallace, M., Frankfurt, M., Arellanos, A., Inagaki, T., Luine, V. Impaired recognition memory and decreased prefrontal cortex spine density in aged female rats. Annals of the New York Academy of Science. 1097, 54-57 (2007).
  19. Bowman, R. E., Hagedorn, J., Madden, E., Frankfurt, M. Effects of adolescent Bisphenol-A exposure on memory and spine density in ovariectomized female rats: Adolescence vs adulthood. Hormones Behavior. 107, 26-34 (2019).
  20. Novaes, L. S., Dos Santos, N. B., Perfetto, J. G., Goosens, K. A. Environmental enrichment prevents acute restraint stress-induced anxiety-related behavior but not changes in basolateral amygdala spine density. Psychoneuroendocrinology. 98, 6-10 (2018).
  21. Trzesniewski, J., Altmann, S., Jäger, L., Kapfhammer, J. P. Reduced Purkinje cell size is compatible with near normal morphology and function of the cerebellar cortex in a mouse model of spinocerebellar ataxia. Experimental Neurology. 311, 205-212 (2019).
  22. Zemmar, A., et al. Oligodendrocyte- and Neuron-Specific Nogo-A Restrict Dendritic Branching and Spine Density in the Adult Mouse Motor Cortex. Cerebral Cortex. 28 (6), 2109-2117 (2018).

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