Isolation of Murine Coronary Vascular Smooth Muscle Cells

Podsumowanie

The purpose of this protocol is to demonstrate the isolation and culture techniques of murine primary vascular smooth muscle cells (VSMCs) from the coronary circulation. Once VSMCs have been isolated, they can be used for many standard culture techniques.

Streszczenie

While the isolation and culture of vascular smooth muscle cells (VSMCs) from large vessels is well established, we sought to isolate and culture VSMCs from the coronary circulation. Hearts with intact aortic arches were removed and perfused via retrograde Langendorff with digestion solution containing 300 Units/ml of collagenase type II, 0.1 mg/ml soybean trypsin inhibitor and 1 M CaCl₂. The perfusates were collected at 15 min intervals for 90 min, pelleted by centrifugation, resuspended in plating media, and plated on tissue culture dishes. VSMCs were characterized by presence of SM22α, α-SMA, and vimentin. One of the main advantages of using this technique is the ability to isolate VSMCs from the coronary circulation of mice. Although the small number of cells obtained can limit some of the applications for which the cells can be utilized, isolated coronary VSMCs can be used in a variety of well-established cell culture techniques and assays. Studies investigating VSMCs from genetically modified mice can provide further information about structure-function and signaling processes associated with vascular pathologies.

Wprowadzenie

The goal of this method is to isolate vascular smooth muscle cells (VSMCs) from the murine coronary circulation for use in cell culture and standard cell culture assays. We developed this technique to assess the molecular mechanisms of vascular remodeling in diabetes. We have previously reported inward hypertrophic remodeling in the septal coronary arterioles in the db/db mouse model of diabetes¹. Due to the limited amount of tissue found in the murine septal coronaries, standard experimental techniques investigating protein changes (e.g. western blot) in db/db and control mice are difficult at best. In addition, we have previously shown that the angiotensin receptor blocker (ARB) losartan reduces the remodeling observed in db/db mice². Therefore, isolation of primary VSMCs from the coronary circulation allows us to further investigate changes in VSMC phenotype or activated signaling pathways in diabetic mice, which may be contributing to adverse coronary arteriole remodeling.

Numerous studies have elucidated canonical signaling pathways using VSMCs isolated from rodent aorta, rather than in each specific vascular bed. However, we have demonstrated vascular-bed specific remodeling in coronary, aortic, and mesenteric circulations of db/db mice¹, suggesting the VSMCs in each vascular bed may be different. Therefore, it is necessary to isolate VSMCs from each vascular bed in order to better understand the pathological changes occurring in each set of VSMCs. There are a plethora of different methods for isolating and culturing aortic VSMCs. However, currently, there is only one study that has been published on the isolation of VSMCs from the mouse coronary circulation³. Teng et al. was the first to report a method for isolating VSMCs from the mouse coronary circulation; however, we have amended the protocol significantly as they also isolated endothelial cells. Other labs have also used the protocol from Teng et al. to isolate coronary arterial myocytes and airway smooth muscle cells^4,5. The alterations we have incorporated will yield a population of cells highly enriched for VSMCs from the coronary circulation.

The retrograde perfusion of the isolated mammalian heart, or Langendorff technique, was established in 1897⁶ by Oscar Langendorff and is still widely used today for the isolation of cardiovascular cells. The technique presented here, coupled with the advancement of modern murine genetic modifications, provides a valuable tool for closer investigation of the molecular behavior of VSMCs from the coronary circulation.

Protokół

Ethics Statement: This study was conducted in accordance with the National Institutes of Health Guidelines, and it was approved by the Institution Animal Care and Use Committee at Nationwide Children's Hospital.

1. Preparation/Set up

Note: This isolation technique requires two Langendorff heating coils positioned side-by-side on a ring stand, and connected in parallel to a circulating water bath.

1. Turn on circulating water bath and adjust temperature to achieve a final temperature of 33-34 °C at the tip of the Langendorff cannula (the water bath used in this set up is set to 40 °C due to a 6-7 °C loss in temperature across tubing). Turn on the perfusion pumps and set perfusion rate to 0.5 ml/min.
   1. Clean both of the water-jacketed heating coils, attached tubing and 25 gauge cannula by flushing each with 50 ml of 70% ethanol, followed by 100 ml of autoclaved ultrapure water.
   2. Clear the heating coils by pushing air with a syringe and wash with 10 ml of Hank's Balanced Salt Solution (HBSS) without phenol red. Leave HBSS in the heating coils and tubing.
   3. Attach a sterile 10 ml luer-lock syringe filled with room temperature HBSS without phenol red to the tubing. Ensure that no air bubbles are trapped inside the tubing and heating coils when attaching the HBSS-filled syringe as this could cause air emboli during the digestion to negatively impact the VSMC isolation.
2. Remove the 25 gauge cannula from the heating coils and place on another sterile 10 ml syringe filled with ice-cold HBSS without phenol red. Keep this on ice until ready to use. Repeat for the other cannula.
3. Prepare Enzyme Digestion Solution.
   1. Weigh collagenase type 2 according to specific lot number for 75 ml of digestion solution to achieve a final concentration of 300 Units/ml.
   2. Dissolve collagenase in 75 ml of HBSS with phenol red. Next, add 1.5 ml of 0.1 mg/ml soybean trypsin inhibitor and 75 µl of 1 M CaCl₂ to the mixture.
4. If using the digestion solution immediately, warm it to 37 °C. If not, place it at 4 °C for up to 6 hr. This solution must be made fresh daily.
5. Prepare the stop solution/plating media.
   1. Add 100 ml heat-inactivated FBS, 5 ml of L-glutamine, 5 ml of non-essential amino acids, 5 ml of HEPES, and 1 ml of primocin to 500 ml of high glucose (4.5 g/L) DMEM. Filter sterilization is recommended.
   2. Aliquot 6 ml of the stop solution into each of twelve 15 ml conical tubes, numbered A1-A6 and B1-B6, and place at 4 °C. Aliquot 50 ml of stop solution into a 50 ml conical and place in 37 °C incubator.
      Note: This step can also be prepared the day prior to isolation if necessary. This stop solution will be used as the plating media following cell isolation.
6. Prepare two 1 ml syringes equipped with a 30 G needle with 100 µl of heparin (1,000 units/ml).
7. Cut a 5 cm piece of 5-0 surgical silk. Tie a loose overhand knot in the surgical silk with one end twice as long as the other. Place onto the 25-gauge cannula, but do not tighten. Repeat for the other 25 G cannula.
8. Fill four 35 mm sterile Petri dishes (#1-4) with 2 ml of sterile, ice-cold, HBSS without phenol red. Keep on ice.

2. Euthanasia, Heart Isolation and Cannulation

1. Before heart isolation, ensure that the digestion solution and 50 ml conical of stop solution are warm. Remove the HBSS-filled syringe with attached 25 G cannula from the ice and place in a burette clamp (or ring stand clamp) on a ring stand.
2. Anesthetize mice using 3% isofluorane. Confirm the mouse is anesthetized by a toe touch on each hind limb. If the leg twitches, the mouse is not yet anesthetized so wait 1 min and repeat the toe touch.
3. Expose the jugular vein by removing the fur and skin on the anterior of the neck with scissors. Next, use forceps to carefully remove any fat surrounding the jugular vein. After removing fat, slowly inject 100 µl of heparin (1,000 units/ml). Place a surgical sponge over the vein to avoid excessive bleeding.
4. After 1 min, open chest to expose heart, lift heart with curved forceps and excise it using scissors, making sure to keep the ascending aorta intact through the first brachiocephalic branch. Immediately place heart into a 35 mm dish (#1) with ice-cold HBSS without phenol red and rinse.
   Note: Perform the following 4 steps using a dissecting scope.
5. Position the 25 G cannula that is mounted on the ring stand at a 45° angle so that the tip is located just under the surface of ice-cold HBSS in dish #2 and is clearly visible through the dissecting microscope. Transfer the heart to dish #2.
6. Using Dumont forceps, expose the aorta by gently removing excess adipose via blunt dissection to prevent puncturing or tearing of the aorta. Next, use forceps to slide the aorta over the 25 G cannula.
7. Guide the cannula downward through the aorta, close to, but not beyond the aortic valve, which will compromise the integrity of the valve and therefore, the retrograde perfusion. Once the cannula is in place, slide the pre-tied silk over the aorta, and tighten. Tie a second knot to form a square knot around the aorta to secure the heart.
8. Once the aorta is securely tied, gently flush the remaining blood from the coronary circulation with the ice-cold HBSS in the syringe attached to the 25 G cannula. Take care to not push too much to avoid excessive coronary pressure. Only a very slow and gentle flush is required to complete the flush. Leak-free aortic cannulation can also be observed during this gentle flush.
9. Turn on the perfusion pump to begin the flow of HBSS. Remove the 25 G cannula (with the heart attached) from the HBSS-filled syringe, taking care to keep the cannula hub filled with HBSS, and connect it to the warm HBSS-filled heating coils. Begin perfusion of the heart with the perfusion pump at a rate of 0.5 ml/min for 8 min.
10. After the first heart is cannulated and is being perfused on the system, repeat steps 2.1-2.8 for the second heart. These isolations will be staggered for each heart therefore careful planning and timing are required.

3. Digestion

1. After flushing with HBSS, change the 10 ml HBSS syringe currently on the pump to one filled with 10 ml of pre-warmed digestion solution. Perfuse each heart with digestion solution for 12 min at a rate of 0.5 ml/min. Do not collect fractions stemming from this first digestion as this will contain any remnant blood and endothelial cells.
2. After 12 min, change the perfusion rate to 0.4 ml/min, place a 15 ml conical (tube A1 or B1, corresponding to the first or second heart for each digestion) filled with cold stop solution into an ice bucket beneath the heart in order to begin VSMC-enriched perfusate collection.
3. After 15 min, change the collection conical to tube A2 or B2 and spin conical tube A1 and B1 at 89 x g for 10 min immediately after collection of both fractions. When the syringe filled with the digestion solution on the pump has less than 1 ml of solution, replace with a freshly-filled 10 ml syringe of digestion solution.
4. After centrifugation, aspirate supernatant from each collection tube, leaving approximately 0.5 ml. Resuspend pellet from A1 with 2 mL of warm stop solution (or plating media). Add resuspension from A1 tube to B1 tube and place tube in 37 °C incubator with the cap loose.
5. Repeat steps 3.3 and 3.4 until all the tubes (through A6 and B6) are used for a total collection time of 90 min. At 80 min of digestion, cut open the heart apex to flush out any cells that may be trapped inside the ventricle and collect these cells in tube A6 and B6, respectively.
   Note: Occasionally the heart will fall off the cannula prior to the 90 min time point. If this occurs, retrieve the heart and place into a sterile 35 mm Petri dish filled with 2 ml of digestion solution. Cut the apex of the heart and gently rinse the heart with digestion solution. Next, filter the 2 ml of digestion solution through a sterile 100 µm cell strainer into a 50 ml conical and add to tube A6 or B6.
6. After each spin of subsequent tubes (A2 and B2), add the resuspended VSMCs to the previous collection tube (combined A1 and B1). Also, take care not to let the digestion solution in the pump run out and switch the 10 ml syringes as necessary throughout the digestion.
7. After all the tubes are combined, centrifuge the VSMC-rich suspension at 89 x g for 10 min.
8. Aspirate as much supernatant from collection tubes as possible. Resuspend the remaining pellet in 2 ml of plating media and plate on one 35 mm culture dish. Place culture dish in 37 °C incubator for 24 hr.

4. Cell Culture

Note: Complete the remaining steps in the biosafety cabinet.

1. After 24 hr, gently aspirate the plating media. The culture will normally have a large amount of debris. To wash the cells, add 2 ml of warm, sterile PBS and gently tap the dish against two fingers while rotating in a clockwise motion.
2. After rotating 360°, aspirate the PBS and repeat a second time. Aspirate the PBS and add another 2 ml of sterile, warm PBS. Check the culture dish under the microscope to make sure there is little to no debris on the plate. Cell confluence can also be determined at this time.
3. If debris remains in the culture dish, repeat step 4.2. If the culture dish is clear of debris, aspirate the PBS and add 2 ml of warm plating media.
4. After 24 hr, wash the cells again with warm, sterile PBS to remove any final debris or dead cells from the culture. Aspirate the PBS and place another 2 ml of warm plating media on the cells.
5. Check on the cells every day and feed every 48 hr with fresh warmed plating media. At this point, cells can be used for standard cell culture assays. VSMCs should be approximately 80% confluent 4-5 days after plating, although may take up to 7 days until the procedure is perfected. If splitting to subsequent passages, use a maximum of 1:4 35 mm dishes (or to a comparable area of culture dishes).

Wyniki

Due to the novel aspect of our coronary VSMC isolation technique, we sought to determine the purity of the cell isolation. Mouse coronary VSMCs were identified based on their morphology and immunofluorescence staining up to passage 2. Based on morphology of the cells in culture after the first wash, the isolation procedure effectively removes cardiac myocytes and endothelial cells. The VSMCs retain their morphology up to passage 2 (Figure 1). However, there is a possibili...

Dyskusje

The purpose of this study was to adapt existing cell isolation protocols to increase the yield of coronary vascular smooth from murine hearts. Most of the pioneering work in vascular smooth muscle biology was performed with cultured rat aortic smooth muscle cells. These studies provided fundamental knowledge of molecular mechanisms that control VSMC growth, migration and hypertrophy⁷. However, as the field progressed, it became apparent that VSMC phenotype and function was controlled by a number of vascular be...

Materiały

Name	Company	Catalog Number	Comments
Fetal bovine serum	Life Technologies	16140-071
HEPES 1M solution	Fisher	MT-25-060
Primocin - 20mL	Invivogen	ant-pm-2
DMEM (High Glucose, Sodium Pyruvate, L-Glutamine)	Life Technologies	11995-065
MEM NEAA 10 mM 100X	Life Technologies	11140-050
L-Glut 200 mM - Gibco	Life Technologies	25030-081
Sterile Cell Strainer 100um nylon mesh	Fisher	22363549
Nunclon Polystrene dish with lid, sterile, 35 mm	Fisher	12-565-91
Harvard Apparatus black silk suture 5-0	Fisher	14-516-124
Collagenase Type-2	Worthington Biochemical	LS004176
Soybean Trypsin Inhibitor 25mg	Sigma	T6522
Hanks' Balanced Salt Solution (HBSS) (1X), liquid (clear)	Life Technologies	14175-103
Hanks' Balanced Salt Solution (HBSS) (1X), liquid (phenol red)	Life Technologies	14170-161
5.0 ml heating coil with degassing bubble trap	Radnoti	158830
11 plus pump	Harvard Apparatus	70-2208
Circulating heated water pump			any brand will work