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In This Article

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

Summary

Here we describe a two-step cell digestion protocol for preparing a single-cell suspension of mouse carotid arteries.

Abstract

Carotid arteries are major blood vessels in the neck that supply blood and oxygen to the brain, but carotid stenosis occurs when carotid arteries are clogged by plaque. Revealing the cellular composition of the carotid artery at the single-cell level is essential for treating carotid atherosclerosis. However, there is no ready-to-use protocol for the preparation of single-cell suspensions from carotid arteries. To obtain a suitable protocol for the dissociation of normal carotid arteries at the single-cell level with less damage to cells, we designed a two-step digestion method by integrating the digestion process of collagenase/DNase and trypsin. Acridine orange/propidium iodide (AO/PI) dual-fluorescence counting was used to detect cell viability and concentration, and it was found that the single-cell suspension satisfied the requirements for single-cell sequencing, with the viability of cells over 85% and a high cell concentration. After single-cell data processing, a median of ~2500 transcripts per cell were detected in each carotid artery cell. Notably, a variety of cell types of the normal carotid artery, including vascular smooth muscle cells (VSMCs), fibroblasts, endothelial cells (ECs), and macrophages and dendritic cells (Mφ/DCs), were concurrently detectable. This protocol may be applied to prepare a single-cell suspension of blood vessels from other tissues with appropriate modifications.

Introduction

Atherosclerosis is a chronic inflammatory disease associated with risk factors such as high blood pressure, hyperlipidemia, and hemodynamics1. Carotid artery bifurcations are prone to hemodynamic changes and lead to carotid plaque formation. The clinical presentation of carotid atherosclerosis can be acute such as stroke and transient cerebral ischemia, or chronic such as recurrent transient cerebral ischemia and vascular dementia2. Mechanically, carotid plaque is the outcome of the interaction between different vessel wall cells and various blood cells under pathological conditions. Therefore, revealing the single-cell atlas of carotid vessels under physiological and pathological conditions is particularly important for preventing and treating carotid plaque development.

Single-cell RNA sequencing is one of the most powerful technologies of biological research because of its ultrahigh resolution and detection of cell heterogeneity from the same cell type of organisms3,4. Researchers have used single-cell RNA sequencing to conduct research in many fields, such as cardiovascular disease5 and cancer6. However, quickly and accurately separating tissues into single cells is still one of the main challenges. Enzymatic dissociation is a commonly used method that dominantly includes collagenase, papain, trypsin, DNase, and hyaluronidase. Specifically, collagenases are the major enzyme species for single-cell digestion, mainly hydrolyzing collagen components in connective tissues. Different collagenase types are applicable for the dissociation of different tissues, such as the mammary gland7, glomerulus8, iridocorneal angle9, knee joint10, aorta11, and lung12. Due to the unique physiological properties of different tissues, dissociation using the same method may cause many troubles in acquiring single cells, such as low cell viability, low cell number, and large cell debris. Therefore, the invention of digestion methods for different tissues is essential for preparing high-quality single-cell suspensions.

This protocol aims to develop a two-step cell digestion method to prepare a single-cell suspension of the carotid artery of wild-type mice. According to the characteristics of the carotid artery, we combined collagenase/DNase with trypsin to obtain a high-quality single-cell suspension of the mouse carotid artery because collagenase can hydrolyze collagen of the carotid tissues, which was further digested by trypsin into a single-cell suspension. Acridine orange/propidium iodide (AO/PI) dual-fluorescence counting was used to detect cell viability and concentration, and it was found that the single-cell suspension satisfied the requirements for single-cell sequencing, with the viability of cells over 85% and a high cell concentration. After single-cell data processing, four cell types, including vascular smooth muscle cells (VSMCs), fibroblasts, endothelial cells (ECs), and macrophages and dendritic cells (Mφ/DCs), were identified in normal mouse carotid arteries after digestion. The advantages of this protocol are that: 1) multiple cell types in the carotid artery can be identified, 2) cell viability is well preserved, and 3) it can be easily repeated without special equipment. This protocol is suitable for researchers who are interested in studying single-cell multiomics of the mouse carotid arteries. This protocol may also be helpful in the dissociation of other blood vessels with appropriate modifications.

Protocol

All animal procedures described below were approved by the Institutional Animal Care and Use Committee of Soochow University.

1. Reagents and materials preparation

  1. Utilize 1x PBS without calcium and magnesium and 2.5 U/mL heparin sodium salt to prepare the perfusion solution. Store at 4 °C, and precool on ice when used.
  2. Prepare dissociation reagent A that contains 125 CDU/mL collagenase II and 60 U/mL DNase I by diluting 1250 CDU/mL collagenase II and 3000 U/mL DNase I with HBSS. Store at 4 °C until use.
  3. Prepare dissociation reagent B that contains a final concentration of 0.12% trypsin by diluting 1 mL of 0.25% EDTA-free trypsin (without phenol red) into 1 mL of 1x PBS. Store at 4 °C until use.
  4. Prepare 10 mL of 1.5% FBS and 10 mL of 5% FBS in 1x PBS. Use 1.5% FBS to pool carotid arteries and keep on ice before use. Use 5% FBS to neutralize digestion and store at room temperature (RT).
  5. Get the experimental materials, including 1 mL syringes, 20 mL syringes with 26-G needles, six-well cell culture plates, 1.5 mL centrifuge tubes, 40 µm sterile cell strainers, and ice containers.

2. Equipment preparation

  1. Sterilize all the surgical equipment, including a stereoscopic microscope, dissecting scissors, micro-dissecting scissors, and fine-tip forceps.
  2. Turn on the automated cell counter and maintain it at RT.
  3. Turn on the water bath to 37 °C in advance.
  4. Precool the microcentrifuge to 4 °C before use.

3. Isolation of the mouse carotid artery

  1. Anesthetize the mouse using 1.25% tribromoethanol by intraperitoneal injection (0.24 mL for every 10 g of body weight) and flip the mouse to check if there is a righting reflex after 3 min. Then, euthanize the mouse by cervical dislocation and lay it on its back. Spray the mouse's skin with 75% alcohol.
  2. Use sterilized dissecting scissors to open up the skin and expose the chest cavity. Cut open the diaphragm.
  3. Continue cutting upward to the lower jaw and carefully remove excess connective tissues and fat, exposing the carotid artery.
  4. Cut the inferior vena cava of the mouse to make blood flow out of the closed circulation.
  5. Inject 20 mL of prechilled perfusion solution into the left ventricle with a syringe slowly and continuously.
    NOTE: If perfusion is successful, blood-rich organs such as the liver, spleen, and kidneys will turn gray-white.
  6. Peel off all the fat and connective tissues around the carotid artery with micro-dissecting scissors under a stereoscopic microscope.
    NOTE: This step should be done slowly and carefully to prevent damage to the carotid artery.
  7. Isolate the carotid artery from the mouse, wash with 1x PBS to flush the blood again, and transfer to six-well plates containing 1.5% FBS on ice.

4. Digestion of the carotid artery into single-cell suspension

  1. Use micro-dissecting scissors to dissect the carotid artery longitudinally and lay flat in another 6-well cell culture plate containing 1 mL of 1.5% FBS on ice.
  2. Flush the intima carefully with 1.5% FBS to remove the residual blood.
    NOTE: Flushing should be gentle and slow to avoid injuring endothelial cells.
  3. Cut each carotid artery into approximately 2 mm2 tissue pieces using microdissecting scissors in 1.5% FBS.
  4. Transfer these tissue pieces into a 1.5 mL centrifuge tube with 1 mL wide bore tips, centrifuge at 400 x g for 5 min at 4 °C to sink the tissues to the bottom.
  5. Discard the supernatant and resuspend the tissues in 500 µL of dissociation reagent A.
  6. Place the tube in a 37 °C water bath for 1 h. Pipette gently with a 1 mL pipette every 10 min.
  7. Add 500 µL of 5% FBS into the tube and mix well with a 1 mL pipette.
  8. Filter the cell suspension through a 40 µm sterile cell strainer into a new 1.5 mL centrifuge tube and centrifuge at 400 x g for 5 min at 4 °C.
  9. Remove the supernatant carefully and resuspend the cell pellet in 200 µL of dissociation reagent B.
  10. Place in a 37 °C water bath and digest for another 5 min. Gently pipette every 2 min during digestion to fully dissociate into a single-cell suspension.
  11. Use 200 µL of 5% FBS to terminate the digestion reaction, and centrifuge at 400 x g for 5 min at 4 °C.
  12. Discard the supernatant and resuspend the cell pellet in 100 µL of 1x PBS on ice.

5. Cell suspension examination and single-cell RNA sequencing

  1. Add 10 µL of AO/PI solution into 10 µL of single-cell suspension and gently mix with a 20 µL pipette.
  2. Pipette 20 µL of the mixture into the chamber slide and wait for 1 min.
  3. Load the slide into the automated cell counter instrument.
  4. Select the AO/PI Viability assay, then wait for the quality report.
  5. Use a single-cell 3ʹ reagent kit to generate single-cell gel beads in the emulsion on a single-cell controller and amplify the barcoded cDNA in a thermal cycler following the manufacturer's protocol.
    NOTE: Here, Chromium Single Cell 3ʹReagent Kits v3 was used.
  6. Perform sequencing on a sequencer with a paired-end 150 bp (PE150) reading strategy. Use a software application (Cell Ranger) to convert raw base call files to fastq files using the mkfastq pipeline. Then, use the Count Pipeline of Cell Ranger for performing alignment, filtering, barcode counting, and unique molecular identifier (UMI) counting to generate feature-barcode matrices13.
  7. Perform data dimensionality reduction and visualization with the R package Seurat14.
    1. First, the Read10X() function of Seurat reads in the output of the Cell Ranger pipeline and then uses the count matrix to create a Seurat object. Then, filter out the cells with expression of <200 or >4000 genes or a mitochondrial gene ratio that was more than 10% by the subset() function of Seurat.
    2. Use NormalizeData() and FindVariableFeatures() to normalize the data and identify 2000 highly variable features, respectively.
    3. Perform principal component analysis (PCA) on the scaled data, and cluster the cells with dims = 30 and resolution = 0.5. Finally, use the RunUMAP() function to visualize the single-cell datasets and FindAllMarkers() to find each cluster biomarker.

Results

This protocol describes a two-step cell digestion method for preparing a single-cell suspension of mouse carotid arteries (Figure 1). This two-step cell digestion method combines collagenase/DNase with trypsin to effectively dissociate the mouse carotid vascular wall to obtain high-quality single-cell suspensions for single-cell sequencing. After dissociation, the cell concentration and cell viability were calculated by an automated cell counter. The bright field showed the morphology of car...

Discussion

Here we provide a detailed protocol for the preparation of a high-quality single-cell suspension from the carotid artery of wild-type mice, in which a two-step digestion method integrating the digestion process of collagenase/DNase and trypsin was constructed. After the quality check of the single-cell suspension, we found that it satisfied the requirements for single-cell sequencing, with the viability of cells over 85% and a high cell concentration. Moreover, a variety of cell types in the carotid artery, including VSM...

Disclosures

The authors have no conflicts of interest to disclose.

Acknowledgements

This work was supported by grants from the Natural Science Foundation of China (82070450 to C.T.and 82170466 to L.Z.) and the fellowship of China Postdoctoral Science Foundation (7121102223 to F.L.).

Materials

NameCompanyCatalog NumberComments
0.25% EDTA-free trypsinBeyotimeC0205Dilute 1 mL of 0.25% EDTA-free trypsin into 1 mL of 1x PBS.
0.9% NaCl saline solutionBeyotimeST341Dilute the heparin sodium solution into a final concentration of 10 mg/mL
1 mL syringes SKJYLEANsk-r009To perform cardiac perfusion
1.5 mL centrifuge tubesKIRGENKG2211WTo centrifuge the tissue piece and cell suspension
20 mL syringesSKJYLEANsk-r013To perform cardiac perfusion
40 µm cell strainerJETBIOFILcss010040To filter undigested tissue fragments
AO/PI kitHengrui BiologicalRE010212To identify whether the cell is alive or dead
Automated cell counterCountstarMira FLTo analyze the cell morphology and cell viability of digested carotid vascular cells
Cell Ranger software10× Genomics3.0.2To process Chromium single-cell RNA-seq output and perform clustering and gene expression analysis
Chromium Single Cell 3'Reagent Kits v310× Genomics1000075To prepare single-cell RNA-seq libraries of single-cell suspension
Collagenase IISigma-AldrichC6885Dilute with HBSS to a final concentration of 125 CDU/mL
Deoxyribonuclease IWorthingtonLS002140Dilute with HBSS to a final concentration of 60 U/mL
Fetal bovine serum HyCloneSH30088.03Termination of the digestion reaction
Hank's balanced salt solution Gibco14175095Store at the room temperture
Heparin sodium saltSolarbio Life ScienceH8060Dilute with 0.9% NaCl to a final concentration of 10 mg/mL
MicrocentrifugeThermo Fisher Scientific75002560Applied for spining down the tissues and cell pellets
NovaSeq 6000 IlluminaN/ASequencer
Phosphate-buffered salineSolarbio Life ScienceP1000Used for cardiac perfusion and resuspension of cells
Seurat package- RSatija Lab3.1.2To performed dimensionality reduction, visualization, and analysis of scRNA-sequencing data
Six-well cell culture platesNEST703002Place the vascular tissue
Water bathJinghongDK-S22Keep the digestion temperature at 37 °C

References

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  13. You, Y., et al. Benchmarking UMI-based single-cell RNA-seq preprocessing workflows. Genome Biology. 22 (1), 339 (2021).
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  17. Kumar, S., et al. Isolation of endothelial cells from the lumen of mouse carotid arteries for single-cell multi-omics experiments. Journal of Visualized Experiments. 176, e63128 (2021).

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Single cell SuspensionMouse Carotid ArteriesSingle cell SequencingVascular Tissue DissociationCarotid StenosisCarotid AtherosclerosisTwo step Digestion MethodCollagenase DNaseTrypsinCell ViabilityCell ConcentrationVascular Smooth Muscle Cells VSMCsFibroblastsEndothelial Cells ECsMacrophages And Dendritic Cells M DCs

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