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Neuroscienze

Preparation of Newborn Rat Brain Tissue for Ultrastructural Morphometric Analysis of Synaptic Vesicle Distribution at Nerve Terminals

Published: June 07, 2019
doi:
10.3791/59694
,
1Department of Anesthesiology,University of Virginia Health System, 2Department of Anesthesiology,Universita’ degli Studi di Padova

Summary

We describe procedures for processing newborn rat brain tissue to obtain high-resolution electron micrographs for morphometric analysis of synaptic vesicle distribution at nerve terminals. The micrographs obtained with these methods can also be used to study the morphology of a number of other cellular components and their dimensional structural relationships.

Abstract

Our laboratory and many others have exploited the high resolving power of transmission electron microscopy to study the morphology and spatial organization of synaptic vesicles. In order to obtain high-quality electron micrographs that can yield the degree of morphological detail necessary for quantitative analysis of pre-synaptic vesicle distribution, optimal specimen preparation is critical. Chemical fixation is the first step in the process of specimen preparation, and of utmost importance to preserve fine ultrastructure. Vascular fixation with a glutaraldehyde-formaldehyde solution, followed by treatment of vibratome-sectioned specimens with osmium tetroxide, stabilizes the maximum number of molecules, especially proteins and lipids, and results in superior conservation of ultrastructure. Tissue is then processed with counterstaining, sequential dehydration and resin-embedding. En bloc staining with uranyl acetate (i.e., staining of vibratome-sectioned tissue before resin embedding) enhances endogenous contrast and stabilizes cell components against extraction during specimen processing. Contrast can be further increased by applying uranyl acetate as a post-stain on ultrathin sections. Double-staining of ultrathin sections with lead citrate after uranyl acetate treatment also improves image resolution, by intensifying electron-opacity of nucleic acid-containing structures through selective binding of lead to uranyl acetate. Transmission electron microscopy is a powerful tool for characterization of the morphological details of synaptic vesicles and quantification of their size and spatial organization in the terminal bouton. However, because it uses fixed tissue, transmission electron microscopy can only provide indirect information regarding living or evolving processes. Therefore, other techniques should be considered when the main objective is to study dynamic or functional aspects of synaptic vesicle trafficking and exocytosis.

Introduction

We describe methods for the preparation of newborn rat brain tissue to obtain high-quality electron micrographs for in-depth morphometric analysis of synaptic vesicle spatial distribution at nerve terminals1,2. The high-contrast micrographs that can be obtained by processing specimens following these methods can also be used to study the detailed morphology of a number of cellular components and their dimensional structural relations3,4.

The transmission electron microscope (TEM) is a powerful tool to study the morphology of organelles and other cellular structures quantitatively. As of this decade, there are no other methods of investigation that can provide the same degree of resolution of lipid membranes and organelles without immuno-tagging, with the exception of cryofixation by high pressure freezing. However, freeze substitution techniques are not widely used, and normally require expensive equipment and long preparation times.

In order to take advantage of TEM's high resolving power, optimal specimen preparation is of paramount importance. The main goals of specimen preparation are to preserve tissue structure with minimum alteration from the living state, enhance specimen contrast, and stabilize the tissue against extraction of cellular components during processing and exposure to the electron beam. Numerous protocols for TEM tissue preparation have been introduced and perfected by several laboratories over the years. Many of them have focused on methods for optimal visualization of synaptic vesicles5,6,7,8,9,10,11. Among a number of well-established, gold standard methods currently in use, we chose procedures for chemical fixation, post fixation, en bloc staining, sequential dehydration, resin embedding and post staining that aim to preserve optimal tissue structure and achieve excellent image contrast. Of note, preservation of fine ultrastructure can be particularly challenging when working with newborn rat brain tissue. In fact, the central nervous system of very young animals is characterized by a higher water content than the adult brain, more prominent enlargement of extracellular spaces, and looser connections between cells12. This makes newborn rat brain tissue profoundly sensitive to changes in osmolarity, and exquisitely prone to artifactual shrinkage and/or swelling when processed through sequential solutions of different tonicity12. Therefore, our methods employed solutions for specimen processing that are of osmolarity as close as possible to that of rat newborn brain. Our goal was to obtain high-quality, high-resolution electron microscopy images for quantitative assessment of synaptic vesicle spatial distribution at nerve terminals. Specifically, we sought to measure the number of vesicles within the nerve terminal, the distance of synaptic vesicles from the pre-synaptic plasma membrane, the number of vesicles docked at the pre-synaptic membrane, the size of synaptic vesicles and the inter-vesicle distances1.

Satisfactory chemical fixation is a prerequisite for obtaining high-quality electron micrographs that can provide the morphological detail necessary to study synaptic vesicle morphology and spatial organization. Although several modes of fixation exist, fixation of brain tissue by vascular perfusion is decidedly superior to other methods. Since fixation via vascular perfusion begins immediately after the arrest of systemic circulation, it shortens the interval between deoxygenation of the brain tissue and cross-linking of proteins with fixatives, resulting in minimum alterations in cell structure. Furthermore, it accomplishes fast and uniform penetration, because of the rapid flow of the fixative from the vascular bed to the extracellular and cellular compartments12,13,14. Primary fixation with glutaraldehyde, followed by secondary fixation (post-fixation) with osmium tetroxide, yields excellent preservation of the fine structure15,16,17. A mixture of glutaraldehyde and paraformaldehyde has the additional advantage of more rapid penetration into the tissue12.

Since biological tissues are not sufficiently rigid to be cut into thin sections without the support of a resin matrix, they need to be embedded in a medium before thin sectioning. Water-immiscible epoxy resins are commonly used as an embedding medium in TEM. When this type of matrix is used, all specimen's free water must be replaced with an organic solvent before resin infiltration. Water is removed by passing the specimen through a series of solutions of ascending concentrations of ethanol and/or acetone12. In this protocol, specimens are first flat embedded between flexible aclar sheets, then embedded in a capsule. The final result is tissue situated at the tip of a cylindrical resin block, which has the ideal geometry to be least affected by vibrations arising during microtome sectioning.

Staining with heavy metals to enhance endogenous tissue contrast is another important aspect of specimen preparation. Image contrast in TEM is due to electron scattering by the atoms in the tissue. However, biological materials consist largely of low atomic weight molecules (i.e., carbon, hydrogen, oxygen and nitrogen). Therefore, the generation of sufficient scattering contrast requires the incorporation of high atomic weight atoms into the cellular components of the tissue. This is achieved through staining of the specimen with heavy metals12,18,19. Osmium tetroxide, uranium and lead, which bind strongly to lipids, are the most common heavy metals used as electron stains.

Osmium (atomic number 76) is one of the densest metals in existence. It is both a fixative and a stain, although its primary role in TEM is as a reliable fixative12. Among various fixation protocols in use, the method of double fixation with glutaraldehyde followed by osmium is the most effective in reducing the extraction of cell constituents during specimen preparation. These two fixatives are used to stabilize the maximum number of different types of molecules, especially proteins and lipids, and result in superior preservation of tissue ultrastructure12,14,15,16,17.

Uranium (atomic number 92) is the heaviest metal used as electron stain, most typically in the form of uranyl acetate. Similarly to osmium, it acts as a stain and fixative, although its primary role in TEM is as a stain20,21. Nucleic acid-containing and membranous structures are strongly and preferentially stained with uranyl salts in aldehyde-fixed tissues22,23. Treatment of tissues with uranyl acetate after osmication and before dehydration results in stabilization of membranous and nucleic acid-containing structures, as well as enhanced contrast, and permits identification of some structural details that would not be easily detected in specimens stained with osmium alone12,24,25. It is thought that uranyl acetate may stabilize the fine structure by combining with reduced osmium that has been deposited on lipid membranes during osmication24. Maximum contrast is achieved when uranyl acetate is applied before embedding and as a post-stain in thin sections12.

Lead (atomic number 82) is the most common stain used for TEM and is mainly employed for post-staining of thin sections. Lead salts have high electron opacity and show affinity for a wide range of cellular structures, including membranes, nuclear and cytoplasmic proteins, nucleic acids and glycogen26,27. When the double staining method is employed (i.e., staining with uranyl acetate is followed by treatment with lead), the latter acts as a developer of uranyl acetate staining. For instance, lead post-staining of chromatin fixed with glutaraldehyde increases uranyl acetate uptake by a factor of three28,29,30,31,32. Lead also enhances the staining imparted by other metals such as osmium. It is thought that lead salts stain the membranes of osmium-fixed tissues by attaching to the polar group of phosphatides in the presence of reduced osmium33. A potential disadvantage of staining with both uranyl acetate and lead, especially for prolonged durations, is that many different structural elements are stained equally and non-specifically, and thus may not be easily distinguished from one another12.

The recent introduction of alternative light sources, such as in optical super-resolution photo-activated localization microscopy, has significantly improved light microscopy resolution34. However, because light microscopy relies on histochemical and immune-cytochemical methods to visualize individually-labelled proteins or enzymes, the power of TEM to display all structural elements at once remains unsurpassed for in-depth study of the morphology and dimensional relationships of tissue structures. In particular, no other technique can provide the morphological detail necessary to perform morphometric analysis of synaptic vesicle distribution at pre-synaptic nerve boutons. Nevertheless, it is important to note that electron micrographs capture the structure of the tissue after the organism dies, and therefore they cannot provide information regarding the dynamics of pre-synaptic vesicle trafficking and exocytosis. Hence, other tools, such as FM dye-live imaging and patch-clamp electrophysiology, should be considered when the main objective is to study dynamic and/or functional aspects of synaptic vesicle trafficking and exocytosis.

Protocol

All studies were approved by the Institutional Animal Care and Use Committee at the University of Virginia (Charlottesville, VA) and conducted in accordance with the National Institutes of Health guidelines.

1. Fixation by Vascular Perfusion

NOTE: A general description of the method for rat brain vascular perfusion has been already detailed in this journal13 and is beyond the scope of this protocol. However, the following steps are specific for the preparation of newborn rat brain tissue to obtain high-quality electron micrographs for quantitative analysis of synaptic vesicles distribution at pre-synaptic terminals.

  1. Prepare 4% paraformaldehyde
    1. Place 800 mL of 0.1 M Phosphate Buffer (PB) in a 2 L glass beaker on a stirring plate under a fume-hood. Heat to approximately 60 °C without boiling the buffer.
    2. Add 40 g of paraformaldehyde powder. Stir continuously
    3. While measuring pH, add small drops of 10 N NaOH until the solution clears. Final pH should be 7.2-7.4.
    4. Add remaining 0.1 M PB to a final volume of 1 L. Let cool, filter with a 0.45 μm membrane and store at 4 °C overnight.
      NOTE: Prepare fresh paraformaldehyde the day before perfusion.
      CAUTION: Inhalation of aldehyde vapors can cause nasal symptoms and airway irritation. Contact with skin causes dermatitis. Aldehydes should be handled in a fume-hood while wearing gloves, a protective gown and safety goggles
  2. Prepare Tyrode solution
    1. Place 1 L of distilled water in a glass beaker on a stirring plate. Add NaCl (8 g), KCl (0.15 g), CaCl2 (0.1 g), MgCl2 (0.006 g), NaH2PO4 (0.055 g), NaHCO3 (1 g) and dextrose (1 g) in the beaker.
    2. Stir continuously and measure pH. Keep pH between 7.2 and 7.4.
      NOTE: Tyrode solution is also commercially available.
  3. Mix 4% paraformaldehyde with glutaraldehyde at a final concentration of 2%. Add 40 mL of electron microscopy-grade 50% glutaraldehyde to 1 L of 4% paraformaldehyde. Mix well in a stirring plate
    NOTE: Approximately 100 mL of the paraformaldehyde-glutaraldehyde fixative solution is needed to perfuse the body of a newborn rat. Therefore, at least 10 newborn rats can be perfused with 1 L of fixative. Do not mix paraformaldehyde and glutaraldehyde until immediately before use. Bring all solutions to room temperature before perfusion.
  4. Once access to the left ventricle has been gained (see whole animal perfusion protocol13), flush the vascular system with Tyrode solution for 30 s at a perfusion pressure of 120 mmHg.
    NOTE: The success of the perfusion depends in part on the complete exclusion of blood from the vascular bed
  5. Flush with paraformaldehyde-glutaraldehyde solution at the same pressure for 10 min.
    NOTE: Maintenance of constant perfusion pressure is essential to avoid introduction of artifacts. In addition, the temperature of the perfusate should not be below the rat’s body temperature to avoid vasoconstriction
  6. Remove the fixed brain from the skull and place in fresh paraformaldehyde-glutaraldehyde fixative at 4 °C overnight.
    NOTE: The protocol can be paused here.

2. Brain Slicing

  1. Embed the fixed brain in 4% agarose and glue the brain-agarose block on a vibratome stage
    NOTE: Other laboratories have obtained good quality sections by achieving a stable block on the vibratome without agar support
  2. Section slices of 50 μm thickness. Set the microtome to low frequency and speed.
    NOTE: Sections can be stored in 0.1 M PB with 0.05% sodium azide at 4 °C for several years.
  3. Place the sections in 0.1 M PB in a Petri dish, examine the sections under a dissection microscope and select specimens for embedding
    NOTE: The protocol can be paused here.

3. Rinsing

NOTE: It is important to rinse the specimen after fixation with aldehydes and before post-fixation with osmium, since residual fixatives may produce osmium precipitates

  1. Pipette 0.1 M PB into a short, wide-mouth glass vial with cap. Place one specimen per each vial. Fully cover the specimen so that it does not dry.
    NOTE: Keep specimens in the same vial from this step through all the solution changes of fixation, dehydration and infiltration, until they are ready for flat embedding.
  2. Rinse the specimen in 0.1 M PB for 3 min x 2, then remove PB with a micropipette.
    NOTE: Since the brain of the newborn rat is profoundly sensitive to changes in osmolarity12,35,36,37, carry out the washings in the same vehicle as that used in the fixative mixture

4. Post-fixation with Osmium

  1. Preparation of osmium tetroxide (OsO4)
    NOTE: This Author’s lab utilizes OsO4 4% supplied in an aqueous solution in glass ampoules (5 mL of OsO4 4% in H2O). Other labs have used OsO4 crystals successfully. However, several hours are necessary to dissolve OsO4 crystals in a vehicle.
    1. Take 5 mL (one ampoule) of 4% OsO4/H2O, open it and place it in a brown glass bottle
      NOTE: OsO4 is a strong oxidizing agent and readily reduced by exposure to light. Reduction can be avoided during preparation by placing OsO4 in a brown glass bottle
    2. Add 5 mL of 0.2 M PB. This will yield 10 mL of 2% OsO4/0.1 M PB.
      NOTE: Since the brain of the newborn rat is profoundly sensitive to changes in osmolarity, use the same buffer to prepare aldehyde fixatives and OsO4 solution12,35,36,37
    3. Add additional 10 mL of 0.1 M PB. This will yield a final solution of 20 mL of 1% OsO4 in 0.1 m PB.
    4. Use a 20 mL syringe fitted with a long needle to draw 1% OsO4 and place it in a brown glass bottle or a scint vial covered with aluminum foil.
      CAUTION: OsO4 is extremely volatile and its fumes are toxic to nose, eyes and throat. All work should be performed in a fume-hood using gloves and protective clothing, and no body part should be exposed to OsO4. Handling and waste disposal should be done according to your institution’s guidelines. Store the unused OsO4 in a tightly stoppered brown glass bottle with Teflon liner on the glass stopper, wrap the bottle in double aluminum foil and store in a dessicator. In the presence of leaking fumes, OsO4 can discolor internal surfaces and contents of the refrigerator. Under the above mentioned storage conditions the OsO4 solution is stable for several months. When solutions get oxidized during storage, they turn gray, in which case they need to be disposed of.
  2. Add 1% OsO4 in 0.1 M PB in the specimen vial and let sit for 1 h. Extract OsO4 after 1 h with a micropipette.
    NOTE: Before applying OsO4 to the section, it is critical to unfold and flatten the specimen. Avoid application directly on top of the specimen, instead use the vial’s walls to gently drip OsO4 to the bottom of the vial. The specimen becomes brown and rigid shortly after OsO4 application. Handle gently from now on to avoid tissue damage

5. Rinsing

NOTE: It is important to rinse the specimen after post-fixation with OsO4 and before dehydration, since residual fixatives may react with dehydration agents37.

  1. Rinse with 0.1 M PB for 3 min x 3.
    NOTE: Since the brain of the newborn rat is profoundly sensitive to changes in osmolarity, carry out the washings in the same vehicle as that used in the fixative mixture12,35,36,37.
  2. Place the osmium solution and first two PB rinses into OsO4 waste and dispose of it according to your institution’s guidelines.

6. Sequential Dehydration and Staining with Uranyl Acetate

NOTE: This author’s laboratory uses water-immiscible epoxy resins for embedding. When epoxy resins are used, all specimen’s free water must be replaced with an organic solvent before infiltration by the embedding medium. Water is removed by passing the specimen through a series of solutions of ascending concentrations of ethanol and acetone12.

  1. Preparation of uranyl acetate (UA)
    1. Place a 200 mL volumetric glass flask containing 100 mL of EtOH 70% on a stirring plate.
    2. Add 4 g of UA to the flask. Wrap in aluminum foil (UA precipitates when exposed to light) and stir continuously.
      NOTE: UA dissolves slowly and incompletely in 70% EtOH. Allow undissolved crystals to settle down before using the solution. UA solution should be filtered with a 0.45 μm filter before use. UA can be prepared ahead of time and kept in a brown bottle wrapped in aluminum foil at 4 °C for months.
      CAUTION: UA is mildly radioactive and highly toxic. The inhalation of UA powder can cause upper respiratory tract disorders and disease of the lungs, liver and kidneys. UA is dangerous when ingested or when it comes in direct contact with skin and mucous membranes. All work should be performed in a fume-hood using gloves and protective clothing. Handling and waste disposal should be done according to your institution’s guidelines.
  2. Dehydrate in 50% EtOH for 1 min. Remove 50% EtOH before adding UA.
  3. Add 4% UA in 70% EtOH. Let sit for 1 h or overnight. If overnight, place in the refrigerator at 4 °C.
    NOTE:     Cap vial to avoid EtOH evaporation and cover with aluminum foil to avoid exposure to light. The protocol can be paused here.
    1. Dispose of UA waste and the two following rinses according to your institution’s guidelines
  4. Dehydrate in 70% EtOH for 1 min.
  5. Dehydrate in 90% EtOH for 5 min.
  6. Dehydrate in 100% EtOH for 5 min x 2.
  7. Rinse the specimen in acetone for 2 min x 3.

7. Infiltration and Embedding

NOTE: Tissues are not sufficiently rigid to be cut into thin sections without the additional support of a resin matrix. Therefore, infiltration and embedding must precede sectioning12.

  1. Preparation of EPON resin
    1. Use a 60 mL gavage syringe. Remove the syringe plunger and cap the syringe with a safety needle.
    2. Place the syringe with the open side up and add the volume of each ingredient of the resin mix incrementally. Add 22 mL of Embed-812 (resin). Add DDSA (hardener) to a total volume of 37 mL. Add NMA (hardener) to a total volume of 50.5 mL. Add 525 μL of DMP-30 (accelerator) with a pipette. Move the plunger of the pipette very slowly as DMP is very viscous.
      NOTE: it is important to add the embedding reagents in the order listed. The accelerator (DMP-30) must be added last. To obtain a cured block that has the desired characteristics, it is critical to use the exact amount of the hardener and the accelerator. Freshly prepared embedding mixtures are preferred.
    3. Put the plunger back and place the syringe on a rocker with continuous shaking for at least 30 min. Color will change from yellow to amber.
      NOTE: All ingredients must be mixed very thoroughly. Failure to do so results in uneven impregnation of the tissue specimen and a block of uneven hardness
  2. Mix 1 volume of EPON resin with 1 volume of acetone in a scint vial and shake to mix. Apply the 1:1 EPON:acetone mixture on the tissue after removing the last acetone rinse. Keep covered to avoid acetone evaporation. Remove the 1:1 mixture of resin and acetone after 2-4 h or keep overnight.
    NOTE: the protocol can be paused here.
  3. Replace the mixture of resin and acetone with full resin. Let sit for 4 h or overnight. Put all EPON waste in a collection container under the hood to be polymerized and disposed of later.
    NOTE: the protocol can be paused here.

8. Flat-embedding

NOTE: Specimens are flat-embedded between two aclar films in a sandwich-like fashion.

  1. Cut two rectangular pieces of clear aclar sheet. Wipe the films clean with EtOH 70%. Trim the sheets so that there is at least 1.5 cm of tissue-free plastic on every side of the section. The aclar sheet on top should have the same width as the bottom, and its height should be approximately two thirds of the bottom sheet.
  2. Slowly tilt the vial with the specimen and gently lift the tissue from the bottom of the vial.
  3. Use a micro flexible spatula and a fine brush to carefully move the section along the vial walls and transfer onto the aclar sheet.
    NOTE: Handle sections with caution to avoid specimen damage.
  4. Gently place the aclar sheet on top of the specimen.
    NOTE: Make sure there is enough resin between the two sheets to seal the sandwich
  5. Gently push out any trapped air bubbles without exerting direct pressure onto the section. Wipe out the excess EPON.
    NOTE: The elimination of air bubbles is important, as their presence makes visualization of the specimen difficult and weakens the stability of the resin bonds.
  6. Label the sheets with a solvent resistant pen and place in oven at 60 ͦC for 2-3 days to polymerize.
    NOTE: the protocol can be paused here.

9. Capsule Embedding

NOTE: Ultramicrotomes are supplied with chucks to hold cylindrical blocks obtained from embedding specimens in capsules. Cylindrical blocks have the ideal geometry to be least affected by vibrations arising during sectioning.

  1. Gently open the sandwiched aclar films. The specimen will adhere to one of the two aclar sheets.
  2. Use a solvent resistant pen to mark the side of the aclar sheet that contains the section. Mark near the tissue.
    NOTE: It is critical to perform this step before punching out the tissue of interest.
  3. Use a disc punch to obtain a circle sample of the section. The pen mark should be part of the punched out tissue.
  4. Prepare the cap of an embedding capsule side up on a capsule holder. Place a drop of resin on the cap.
  5. Place the punched disc inside the cap with the tissue section facing up. The pen mark will gleam when light is shined on the specimen.
  6. Insert a capsule into the cap and use fine tweezers to insert labeling. Roll and lower a printed 2 cm-long piece of paper into the capsule. Make the label to fit to the curvature of the side walls of the capsule. Wait for polymerization to be complete, so that the label becomes permanently embedded in the resin.
  7. Pour the embedding resin inside the capsule and fill until the edge of the capsule.
  8. Push the tissue specimen down to the bottom of the capsule with the aid of a pointed wooden stick and place in the oven at 60 °C for 2-3 days.
    NOTE: Take care not to press the tissue too hard, instead let it lie loosely so that a thin layer of the embedding medium is present between the tissue and the capsule surface. The protocol can be paused here.

10. Trimming of Block Face

NOTE: Small size and appropriate shape of the block face are prerequisites for satisfactory sectioning. Therefore, trimming of the specimen block is a necessity.

  1. Use a sharp one-edge razor blade. Clean with acetone immediately before use.
  2. Mount the capsule block in a block holder and place the block holder on the stage of a stereomicroscope.
    NOTE: The trimming procedure should be carried out under microscope binoculars and oblique illumination.
  3. Remove the aclar sheet from the tip of the capsule using a razor blade. The aclar sheet appears as a shiny layer under the light of the dissecting scope.
  4. Hold the razor blade at an angle of 45 degrees and make cuts down four sides of the capsule block.
    NOTE: Better control of the trimming is achieved if the blade is held with both hands.
  5. Make short cuts so that the block takes the form of a short pyramid with wall angles of approximately 45°.
    NOTE: The specimen face is supported much better if the sides leading to it are kept short. If the block tip is too thin and long, it will vibrate during thin sectioning. Ideally, the area of interest should be centered in the block face.
  6. Trim the tip of the capsule to discard superfluous tissue and only preserve the area of interest.
    NOTE: No part of the section should be without tissue, as variations in the density of the block face are a major cause of difficulty in sectioning. Ideally, the surface area of the capsule face should be no more than 1 mm2.
  7. Trim the capsule face in the shape of a scalene trapezoid. Because in a scalene trapezoid no side is equal, this shape is best to orient the area of interest relative to the rest of the specimen.
    NOTE: During sectioning, the trapezoid-shaped face is supported much better than that of any other shape.

11. Microtome Sectioning

NOTE: The majority of biological specimens are too thick in their natural state to be penetrated by an electron beam. Therefore, the material must be cut in thin sections that can be penetrated by the electron beam.

  1. Cut thin sections (silver interference color, 600-900 Å) on a ultramicrotome at planes parallel to the surface.
  2. Place the sections on grids. This author’s lab uses copper grids of 3.05 mm in outer diameter.
    NOTE: The protocol can be paused here.

12. Post-staining with Uranyl Acetate

  1. Prepare 2% UA in distilled water. Place a 200 mL volumetric glass flask containing 100 mL of distilled water on a stirring plate. Add 2 g of UA to the flask. Wrap in aluminum foil (UA precipitates when exposed to light) and stir continuously.
    NOTE: For details of UA preparation, see section 6 of this protocol.
  2. Place several individual drops of 2% UA on a clean sheet of dental wax in a Petri dish.
  3. Float the grid with the specimen (section side down) on a drop of UA for 25 min.
    NOTE: Float each grid on a separate drop of UA.
  4. Hold the grid at its edge with forceps and rinse twice under a gentle jet of boiled distilled water at room temperature from a plastic wash bottle.
    NOTE: Do not allow the grid to dry before staining with lead.

13. Post-staining with Lead

  1. Prepare a CO2-free chamber (CO2 in the air is the primary source of lead precipitation). Place a piece of filter paper soaked with 1 N NaOH in a Petri dish. Place a small sheet of clean dental wax on top of the filter paper and place several NaOH pellets on one side of the dish. Cover the dish.
    NOTE: Prepare this setup before the grids are stained with UA, so that the atmosphere in the chamber is free of CO2 and ready for lead staining by the time UA staining is complete.
  2. Make 4% NaOH. Add 0.2 g of NaOH to 5 mL of distilled water.
  3. Prepare Sato’s triple lead solution. To prepare 10 mL, add 0.1 g of lead nitrate, 0.1 g of lead citrate, 0.1 g of lead acetate and 0.2 g of sodium citrate into a glass bottle. Add 8.2 mL of distilled water and shake vigorously for 5 min. Sonicate for 30 s, then add 1.8 mL of freshly made 4% NaOH.
  4. Place several drops of Sato’s lead on the wax in the Petri dish.
  5. Place the grid stained with UA (section side down) on the drop of lead.
    NOTE: Each grid should be floated on a separate drop of lead. Each drop should be small enough to allow the grid to float on top of the dome of the drop instead of sliding down on the sides.
  6. Cover the dish and let stain for 5 min.
  7. Hold the grid at its edge with forceps and wash thoroughly under a gentle jet of boiled distilled water at room temperature from a plastic wash bottle.
  8. Blot dry the grid on filter paper and store the grid.
    NOTE: Make sure the section does not come in direct contact with the filter paper.

Representative Results

General criteria that are mostly accepted as indicative of satisfactory or defective preservation of specimen for TEM have been established. These criteria are exemplified in four selected electron micrographs (two examples of optimal preparation, two examples of defective preparation) that were obtained by treating young rat brain tissue following the methods described in this protocol.

In general, a good-quality electron micrograph appears as an orderly, distinct and overall grayish image. In a satisfactorily prepared specimen, spaces between membranes should be filled with granular material, and should not be empty. Similarly, no empty spaces should be found in the cytoplasmic ground substance or within organelles (compare Figure 1A and Figure 2A with Figure 3 and Figure 4). Nevertheless, it is important to note that the central nervous system of very young animals shows a certain degree of enlargement of extracellular spaces when compared to the adult brain, with looser connections between cells and an overall whiter, less electron-dense appearance. Membranes should be continuous, without distortion or breakage (Figure 1A and Figure 2A). The stroma of mitochondria should appear uniform and dense, with no empty spaces. Cristae should be intact and not swollen, and the mitochondrial outer double membrane should be unbroken (compare Figure 1A with Figure 3). To facilitate morphometric analysis of pre-synaptic vesicle organization, pre- and post- synaptic membranes need to be intact and essentially parallel to each other (see Figure 1). Synaptic vesicles should be traceable and bound by a continuous single membrane (see Figure 2).

Importantly, even when best practices are followed, treatment of the specimen with fixatives, stains and resins introduces artifacts. Since artifacts cannot be eliminated, it is critical to understand what process originates them, so that the appearance of the specimen can be interpreted with respect to the treatment that it underwent12. One example of an artifact — among several that can be generated during specimen preparation for TEM — is a myelin figure, a membranous lamellar inclusion that resembles myelin sheaths. Although myelin figures can be seen in pathologic conditions12, they most often result from extraction of membrane lipids during fixation with aldehydes (see Figure 4).

Figure 1
Figure 1: Electron micrograph representative of satisfactory preservation of cell structure (example 1). (A) Neuronal cell membranes are layered and without breaks. The cytoplasm is finely granular and without empty spaces. Mitochondria are neither swollen nor shrunk. Their outer double membrane is conserved, and internal cristae are intact. (B) Detail of panel A, exemplifying one method for measuring the distance of synaptic vesicles from the pre-synaptic membrane. Please click here to view a larger version of this figure.

Figure 2
Figure 2: Electron micrograph representative of satisfactory preservation of cell structure (example 2). (A) Synaptic vesicles are distinct and lined by an unbroken single membrane. To allow morphometric analysis of synaptic vesicle distribution, pre-synaptic and post-synaptic membranes need to be parallel and their continuity preserved. (B) Detail of panel A, exemplifying the counting of synaptic vesicles within the pre-synaptic terminal. Please click here to view a larger version of this figure.

Figure 3
Figure 3: Electron micrograph representative of defective preservation of tissue structure (example 1). Note the distortion and breakage of neuronal cell membranes and the presence of markedly enlarged extracellular spaces (marked with *). Mitochondria appear distended and have swollen cristae (marked with arrow). Please click here to view a larger version of this figure.

Figure 4
Figure 4: Electron micrograph representative of defective preservation of tissue structure (example 2). Note the presence of large white empty spaces within the cytoplasm (marked with ǂ), in place of finely granular cytoplasmic substance. Extracellular spaces appear enlarged. An artifactual membranous whorl (myelin figure), likely resulting from mobilization of lipids during fixation with glutaraldehyde, is marked with the acronym MF. Please click here to view a larger version of this figure.

Discussion

Handling of tissue sections during specimen preparation for TEM requires a considerable degree of finesse, concentration and patience. When using a micropipette to add and remove solutions, specimens can be sucked into the pipette tip by surface tension, so great care should be taken to avoid tissue damage by the pipette. Also, certain steps of the dehydration sequence can be as quick as 1 min, hence the operator needs to work swiftly to ensure that the next dehydration step is started on time and the specimen does not dry or wrinkle. One procedure that requires special attention is post-fixation with osmium. Sections become rigid after treatment with osmium and can be easily damaged. Before adding osmium, it is imperative that the sections are flattened at the bottom of the vial, else any fold will result in tissue fracture. Handling of osmicated tissue is particularly challenging when transferring sections onto aclar films for flat embedding. Special care is needed when lifting the specimen from the bottom of the vial to avoid fragmentation, and when pushing air bubbles out of the film sandwich. While it is important to push out any trapped air, as it makes visualization of the specimen difficult and weakens the stability of the resin bonds, direct pressure onto osmicated tissue can easily inflict damage. Another step that necessitates extra care is preparation of the resin mixture for specimen infiltration and embedding. EPON, the most widely used embedding resin, can be hardened with the addition of a hardener and an accelerator. It is imperative to use the exact amount of hardener and accelerator in order to obtain a cured block with the desired characteristics. Both gravimetric and volumetric methods have been described for measuring viscous resins. Although gravimetric methods have been traditionally considered more precise12, this Author's laboratory has had good success with volumetric modes (i.e., adding the volume of each ingredient of the resin mix incrementally by means of a gavage syringe). After the resin components have been carefully measured, they must be mixed very thoroughly to accomplish uniform impregnation, since they possess different viscosities and rates of polymerization. Failure to achieve complete mixing will result in a block of uneven hardness that is unsuitable for thin sectioning.

Marked changes in the tonicity of the solutions used to process sections of young rat brain can cause shrinkage and/or swelling of the extracellular space and cellular components12,35,36,37. During fixation, the best results are obtained when the osmotic pressure of the perfusate is kept as similar as possible to that of the tissue under study. Rat brain osmolality is approximately 330 mOsm. A 2% glutaraldehyde in 0.1 M PB solution is only slightly hypertonic (400-450 mOsm) and minimizes expansion of the extravascular space12. Notably, membranes remain sensitive to changes in the osmotic pressure of the rinsing and dehydration solutions after fixation with aldehydes. Therefore, it is also important to minimize the differences between the osmolarity of the fixative and the solutions used subsequently12,35,36,37. For this reason, the same vehicle (0.1 M PB, approximate osmolarity 440 mOsM) is used as a solvent for all solutions in this protocol. However, it should be noted that several different buffers have been used successfully during specimen preparation for TEM and no single buffer can claim universal superiority over the others. When buffers of lower tonicity are preferred, other laboratories have chosen to increase the osmolarity with electrolytes or non-electrolytes12.

Several steps in this protocol require the use of chemicals that can be toxic when not handled properly. The importance of working under a fume-hood and wearing personal protective equipment while handling aldehydes, osmium, uranium and lead compounds cannot be overstated. While automated contrasting systems can help attenuate some of the risk and are commercially available, they can be quite expensive and may not be affordable by laboratories that do not make routine use of TEM. Although the electron microscope laboratory can potentially be a hazardous place, specimen processing for TEM is overall safe when performed rigorously.

Recently, the introduction of super-resolution light microscopy has increased optical imaging resolving power to about 15 nm34. However, when the goal is to perform morphometric analysis of synaptic vesicle spatial organization at pre-synaptic terminals, no technique provides the same degree of morphological detail. Importantly, TEM is limited by the need for the specimen to be dead before it can be processed and visualized. Therefore, when the study objective is to investigate dynamic or functional aspects of synaptic vesicle trafficking and exocytosis, tools other than TEM should be considered.

Divulgazioni

The authors have nothing to disclose.

Acknowledgements

This manuscript was supported by NIH/NIGMS K08 123321 (to N.L.) and by funds from the Department of Anesthesiology at the University of Virginia. The Authors wish to thank Alev Erisir (Department of Biology, University of Virginia, Charlottesville, VA) for excellent training and technical assistance with TEM, and for her invaluable manuscript criticism. The Authors also thank the Advanced Electron Microscopy facility at the University of Virginia for technical assistance with specimen sectioning and post-staining.

Materials

4% Osmium tetroxide Electron Microscopy Sciences 19170 acqueous
50% Glutaraldehyde Electron Microscopy Sciences 16310 EM grade, acqueous
Aclar 33 C embedding film Electron Microscopy Sciences 50425-25 7.8 mil thickness, size 8"x10"
BEEM capsule holder Electron Microscopy Sciences 69916 holds size "00" capsules
BEEM embedding capsules Electron Microscopy Sciences 70021 size "00", flat
Butler block trimmer Electron Microscopy Sciences 69945-01
Camel hair paint brush Electron Microscopy Sciences 65576-01
Disc punch Electron Microscopy Sciences 77850-09
Embed 812 kit Electron Microscopy Sciences 14120
Lead acetate Electron Microscopy Sciences 17600
Lead citrate Electron Microscopy Sciences 17800
Lead nitrate Electron microscopy Sciences 17900
Leica UC7 ultracut microtome Leica
Micro scale Electron Microscopy Sciences 62091-23
Paraformaldehyde Electron Microscopy Sciences 19208 EM grade, granular
Precision Thelco laboratory oven Thelco 51221159
Sodium azide Sigma-Aldricht S2002
StatMark pen Electron Microscopy Sciences 72109-01
Tyrode solution Electron Microscopy Sciences 11760-05
Uranyl acetate Electron Microscopy Sciences 22400 powder
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Riferimenti

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Tags

Newborn Rat BrainUltrastructural Morphometric AnalysisSynaptic Vesicle DistributionNerve TerminalsTransmission Electron MicroscopyOsmium TetroxidePhosphate BufferUranyl AcetateSynaptic FunctionSynaptic DevelopmentAnesthetics

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Ferrarese, B., Lunardi, N. Preparation of Newborn Rat Brain Tissue for Ultrastructural Morphometric Analysis of Synaptic Vesicle Distribution at Nerve Terminals. J. Vis. Exp. (148), e59694, doi:10.3791/59694 (2019).
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