Methods for Cell-attached Capacitance Measurements in Mouse Adrenal Chromaffin Cell

Podsumowanie

After exocytosis, fused plasma membrane is retrieved through a process known as endocytosis. This mechanism reforms new synaptic vesicles for the next round of release. Individual endocytic events are captured and analyzed through the use of the cell-attached capacitance recordings in mouse adrenal chromaffin cells.

Streszczenie

Neuronal transmission is an integral part of cellular communication within the brain. Depolarization of the presynaptic membrane leads to vesicle fusion known as exocytosis that mediates synaptic transmission. Subsequent retrieval of synaptic vesicles is necessary to generate new neurotransmitter-filled vesicles in a process identified as endocytosis. During exocytosis, fusing vesicle membranes will result in an increase in surface area and subsequent endocytosis results in a decrease in the surface area. Here, our lab demonstrates a basic introduction to cell-attached capacitance recordings of single endocytic events in the mouse adrenal chromaffin cell. This type of electrical recording is useful for high-resolution recordings of exocytosis and endocytosis at the single vesicle level. While this technique can detect both vesicle exocytosis and endocytosis, the focus of our lab is vesicle endocytosis. Moreover, this technique allows us to analyze the kinetics of single endocytic events. Here the methods for mouse adrenal gland tissue dissection, chromaffin cell culture, basic cell-attached techniques, and subsequent examples of individual traces measuring singular endocytic event are described.

Wprowadzenie

Synaptic transmission is mediated by exocytosis of neurotransmitter-containing synaptic vesicles, and these vesicles must undergo local endocytic recycling within the nerve terminal to maintain neuronal communication in the long term. Given the essential role of synaptic transmission in the brain, understanding the molecular machinery that constitutes the synaptic vesicle cycle is an essential foundation towards a better comprehension in cellular communication as a whole. Among cell model systems, the adrenal chromaffin cell has provided some of the most definitive insight into the molecular machinery underlying synaptic vesicle recycling. Exocytosis, the final step in neurotransmitter release, has been immensely studied and examined through the use of the adrenal chromaffin cell^1,2. In fact, most of the molecular players that orchestrate the formation, targeting, docking, and fusion of secretory granules have been identified due to application of diverse techniques in chromaffin cells¹. Furthermore, by providing an opportunity to allow for single-vesicle resolution of the protein machinery involved in exocytosis, the chromaffin cell remains a powerful model to address the questions of vesicle fusion³.

Cell-attached capacitance measurements were first utilized in resolving single-vesicle fusion during exocytosis³. Exocytosis of vesicles as small as ~60 nm in diameter have been demonstrated to be detected by cell membrane admittance measurements with the patch clamp technique in the cell attached configuration^4-7. Admittance is defined as a measure of how easily a circuit or device will allow a current to flow; it is the inverse of impedance. Thus, admittance measurements provide an understanding of the membrane capacitance. This is accomplished by the incorporation of the vesicular membrane into the plasma membrane; this incorporation reveals changes in surface area⁸. Each fusing vesicle causes a stepwise increase in membrane capacitance^9,10. Additionally, this admittance measurement provides the membrane conductance and the fusion pore conductance during an exocytotic event³. As this technique has provided a unique tool at identifying single-vesicle kinetics during exocytosis, our lab has recently applied this concept to detect endocytosis of single vesicles^11,12.

Our specific interest is clathrin-mediated endocytosis (CME), which has been considered as a fundamental housekeeping component in many cells¹³ and as a main pathway for synaptic vesicle endocytosis in neuronal terminals^14,15. CME is known to be biologically important, however, its kinetics remain not well understood due to technical limitations in monitoring singular endocytic events. Given the similarities in exocytic mechanisms between chromaffin cells and neurons¹, it is plausible that the fission mechanisms in chromaffin cells may likely apply to synaptic vesicle endocytosis in neurons. The cell-attached capacitance measurements have been utilized to monitor individual endocytic events and analyze the fission kinetics, which most methods are unable to resolve. In our cell-attached recordings, a sine wave at 20 kHz is superimposed over the holding potential, and the output current is separated into membrane conductance in one channel and membrane capacitance in the other channel from a two-phase lock-in amplifier^16-18. From the changes in the membrane conductance and capacitance, one can calculate the kinetics of the fission-pore, which likely corresponds to the tubular membrane neck that connects the internalizing vesicle to the plasma membrane prior to vesicle pinch-off. Collectively, this technique gives us the opportunity to examine the regulatory mechanisms of vesicle fission during CME.

Protokół

NOTE: The entire procedure was conducted in accordance with the guidelines of the National Institutes of Health, as approved by the Animal Care and Use Committee of the University of Illinois at Chicago.

1. Solutions and Culture Media Preparations

1. Keep all the solutions at -20 °C for up to six months. Keep the culture media at 4 °C for up to 3 months.
2. Prepare 100 ml of culture media by mixing 1 ml of pen-strep solution and 1 ml of ITSX (Insulin-Transferrin-Selenium-Supplementation) to 100 ml with DMEM.
3. Prepare enzyme solution by mixing 250 ml of DMEM, 2.5 ml of 100 mM CaCl₂, and 2.5 ml of 50 mM EDTA.
4. Prepare inactivation solution by mixing 225 ml of DMEM, 25 ml of FBS, 625 mg of albumin, and 625 mg trypsin inhibitor.
5. Prepare a Locke’s Solution of 154 mM NaCl, 5.6 mM KCl, 5.0 mM HEPES, 3.6 mM NaHCO3, 5.6 mM glucose. Adjust the pH to 7.3 with NaOH.
6. Prepare a poly-d-lysine (PDL) solution of 50 mg/ml. Use a final concentration of 1 mg/ml to coat coverslips.
7. Prepare an extracellular solution of 140 mM NaCl, 5 mM KCl, 2 mM CaCl₂, 1 mM MgCl₂, 10 mM HEPES-NaOH, and 10 mM glucose. Adjust the pH to 7.3 with NaOH with an osmolarity of ~310 nmol/kg.
8. Prepare a pipette solution of 50 mM NaCl, 100 mM TEACl, 5 mM KCl, 2 mM CaCl₂, 1 mM MgCl₂, and 10 mM HEPES. Adjust pH to 7.3 with NaOH with an osmolarity of ~290 nmol/kg.

2. Adrenal Gland Isolation

1. Autoclave a pair of large and small dissection scissors and two pairs of forceps. Wear gloves during the whole process and place the dissecting tray on an ice bucket.
2. Use mice taken at Day 0-3. Euthanize animals with a pressurized CO₂ tank followed by decapitation.
3. Utilize the smaller set of scissors to cut down the back of the pup following the spine from cervical to caudal region. Be sure to cut superficially under the skin and not pierce into the body cavity.
4. Next, peel skin away from spine so that musculature is exposed to have a clear view of the spinal column. From here, make a transectional cut at the cervical spinal cord and then make two parallel cuts along the sides of the spine.
5. With one pair of forceps holding the main body of the animal, use the other pair of forceps to grab spinal column and peel back spine till kidneys are exposed.
6. At this moment, visualize the adrenal glands on the top of the kidneys. Then carefully place the two glands from each animal into a conical tube filled with Locke’s solution.
   NOTE: Sometimes the glands will stick to the forceps. If this is the case, gently use another pair of forceps to aid in the removal of the glands from the forceps and into the Locke’s solution. The glands can be kept in this condition for up to 2 hr.

3. Tissue Digestion

1. In the meantime, bubble the enzyme solution with 5% CO₂ + 95% O₂ for 15 min prior to use. Ensure that the equilibrated solution turns from a bright pink color into pinkish/orange color.
2. Add the papain to the freshly bubbled enzyme solution at a final concentration of 20-25 unit/ml. Incubate each pair of glands from each animal for 40-60 min at 37 °C in the enzyme solution with papain.
3. Add 75% of inactivation solution to each tube and incubate at 37 °C for another 10 min. This incubation inactivates the enzyme activity of papain.
4. After the 10 min incubation with the inactivation solution, gently transfer the glands into a newly labeled tube and then wash the glands 3x with culture media.

4. Cell Dissociation and Plating

1. After washing, place the two glands into 200 µl of the culture media and then gently titrate the glands up and down through the pipette tip with a 200 µl pipette until there is no longer a large piece of tissue in the solution.
   NOTE: When titrating, maintain glands at the bottom of the tube with a downward force from the 200 µl pipette tip and engage the tissue gently and slowly. Be certain to use slow, continuous strokes, never pipetting fast or abrupt.
2. Add an additional 250 µl culture media to bring the total volume of culture media up to 450 µl.
3. Plate 60 µl of this cell-containing solution onto each of seven 12 mm PDL-pre-coated coverslips, which are placed in a 60 x 15 mm culture dish.
4. Once plated, place the dish into the incubator that is set to 37 °C and maintained with a steady flow/supply of 5% CO₂ for 30 min to ensure an environment for cell viability. After incubation, gently add 5 ml of pre-warmed culture media into the culture dish and return the dish back into the incubator for 24 hr prior to cell-attached recordings.
   NOTE: Typically, the cells can be used for electrophysiological recordings for up to 4 days.

5. Cell Identification and Gigaohm Seal Formation

1. Place the 12 mm coverslip into extracellular solution. Since the whole adrenal glands are used for cell preparation, mix the chromaffin cells (typically very bright with a brownish/beige coloring and a near perfect circular form (Figure 1) in culture with cortical cells (smaller and dimmer than chromaffin cells).
2. Pull the patch pipettes in four stages using a programmable P-97 puller. Dip the pipette tip into a melted wax, which will help to reduce the capacitance of the glass and then fire polish the tip to “blow-away” this wax from inside of the pipette tip.
   NOTE: When filled with patch pipette solution, patch pipettes typically have a resistance of ~2 MΩ.
3. Approach the patch pipette close to the cell within several microns. To achieve a cell-attached configuration, look for any slight cell deformation during the approach of the patch pipette closer to the cell. Apply gentle suction until a GΩ seal is achieved.

6. Cell-Attached Capacitance Recordings

1. Once a GΩ seal is revealed, make cell-attached recordings through the use of an EPC-7 plus patch-clamp amplifier and a two-phase analog lock-in amplifier (see attached table of equipment). Apply a sinewave with amplitude of 50 mV (r.m.s.) and frequency of 20 kHz from the lock-in amplifier.
2. Set the output filter of the lock-in amplifier at 1 msec time constant and 24 db. Set the phase of the lock-in amplifier such that transient capacitance changes produced by gentle suction pulses appear only in the patch capacitance (Im) trace with no projection into the patch conductance (Re) trace (Figure 2).
   NOTE: Please see the details for the calibration of the system in reference 19.
3. Identify typical capacitance changes by “downward” steps (Figure 3).
   NOTE: A solid recording will be viewed as a “staircase” type resemblance with many downward steps, which indicates internalizing single vesicles. The patching process serves as a mechanical stimulation since action current can be typically recorded from most cells.
4. Name files as individual folders including date: mm/dd/year and each cell-attached recording as its own individual numbering (xx) within that file.

Wyniki

The cell viability and the quality of gigaohm seal are critical in determining the quality of the cell-attached capacitance recordings. Therefore, it is critical to procure an effective and efficient cell culture prior to electrophysiological recordings, and typical viable cells are illustrated in Figure 1. Practice and time will be helpful in achieving a gigaohm seal with high quality. If one can clearly see cell deformation when the patch pipette is approaching the cell as described in protocol Step 5....

Dyskusje

Cell-attached capacitance measurements require several critical steps in order to successfully obtain recordings with high quality: 1) viable and healthy cells prepared from adrenal glands; 2) PDL coating of the coverslips; 3) gigaohm seal formation; 4) noise level of the system; and 5) phase correction.

For animal surgery, modifications one can potentially make is to adjust the surgical approach to best suit dexterity and to prevent damage during dissection. Additionally, sufficient practice ...

Materiały

Name	Company	Catalog Number	Comments
Poly-D-Lysine	Sigma	P0899
DMEM		15066024	Keep out of UV
Dulbecco’s Modified Eagle Medium	Life Technologies
Cover Glass	Carolina Biological	633029	12 mm
Penicillin Streptomycin	Life Technologies	15140122	100 ml
Insulin-Trans-Sel-X	Life Technologies	51500056	Only thaw on ICE!
Papain	Worthington	39S11614
EPC-7 plus patch amplifier	HEKA
BNC-2090 data acquisition board	National Instruments
Igor data acquisition software	Wavemetrics
P-97 pipette puller	Sutter Instruments
Microforge	Scientific Instruments
Borosilicate glass capillaries	Sutter Instruments	B150-110-10	Outer diameter: 1.5 mm Inner diameter: 1.10 mm Length: 10 cm