JoVE Journal > Immunology and Infection
Summary
Abstract
Protocol
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Materials
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Imunologia e Infecção

Isolierung und Charakterisierung von dendritischen Zellen und Makrophagen aus dem Mausdarm

Published: May 21, 2012
doi:
10.3791/4040
, , , ,
1Department of Pediatrics,Emory University, 2Department of Pathology & Laboratory Medicine,Emory University

Summary

Here, we detail a methodology for the rapid isolation of mouse intestinal dendritic cells (DCs) and macrophages. Phenotypic characterization of intestinal DCs and macrophages is performed using multi-color flow cytometric analysis while magnetic bead enrichment followed by cell sorting is used to yield highly pure populations for functional studies.

Abstract

Within the intestine reside unique populations of innate and adaptive immune cells that are involved in promoting tolerance towards commensal flora and food antigens while concomitantly remaining poised to mount inflammatory responses toward invasive pathogens1,2. Antigen presenting cells, particularly DCs and macrophages, play critical roles in maintaining intestinal immune homeostasis via their ability to sense and appropriately respond to the microbiota3-14. Efficient isolation of intestinal DCs and macrophages is a critical step in characterizing the phenotype and function of these cells. While many effective methods of isolating intestinal immune cells, including DCs and macrophages, have been described6,10,15-24, many rely upon long digestions times that may negatively influence cell surface antigen expression, cell viability, and/or cell yield. Here, we detail a methodology for the rapid isolation of large numbers of viable, intestinal DCs and macrophages. Phenotypic characterization of intestinal DCs and macrophages is carried out by directly staining isolated intestinal cells with specific fluorescence-labeled monoclonal antibodies for multi-color flow cytometric analysis. Furthermore, highly pure DC and macrophage populations are isolated for functional studies utilizing CD11c and CD11b magnetic-activated cell sorting beads followed by cell sorting.

Protocol

1. Dissection and Dissociation of Intestinal Epithelial Cells Preparation of reagents and equipment: Warm Ca2+/Mg2+-free PBS (CMF PBS) to room temperature. Warm Ca2+/Mg2+-free HBSS with 5% FBS (CMF HBSS/FBS) and 2mM EDTA to room temperature. Warm Orbital shaker to 37 °C. Note: Steps 1.1 to 1.7 must be performed as quickly as possible to minimize the extent of cell…

Discussion

Figure 3
Figure 3. Factors important for the optimization of cell yield and surface antigen expression. Cell yield and surface antigen expression are directly affected by the duration of tissue digestion, the specific characteristics of the collagenase, the degree of tissue mincing, and the presence or absence of inflammation, which may affect tissue integrity and cellularity. Prolonged tissue digestion may result in decreased cell viabili…

Declarações

The authors have nothing to disclose.

Acknowledgements

We thank Aaron Rae (Emory University Department of Pediatrics and Children’s Healthcare of Atlanta Flow Core) for cell sorting. This work was supported by NIH grant AA01787001, a Career Development Award from the Crohn’s and Colitis Foundation of America, and an Emory-Egleston Children’s Research Center seed grant to T.L.D.

Materials

Name of the Reagent Company Catalogue number Comments
1X PBS, Ca2+– and Mg2+-free      
Hank’s balanced salt solution (HBSS) with phenol red Fisher Scientific SH3001603  
Sodium bicarbonate Sigma S6014  
1M HEPES in 0.85% NaCl Lonza 17-737E  
Fetal bovine serum (FBS) Atlanta biologicals S11150H Heat-inactivated
0.5M EDTA (pH 8.0) Cellgro 46-034-CI  
Collagenase type VIII Sigma C2139  
DNase I Roche 14785000 Stock solution: 100mg/ml
LIVE/DEAD Fixable Aqua Dead Cell Stain Kit for 405 nm excitation Invitrogen L34957 Use at 1:1000
CD45-PerCP mAb (30F11) BD 557235 Use at 1:100
CD103-PE mAb (M290) BD 557495 Use at 1:100
FcγRIII/II mAb (2.4G2) BD 553141 Use at 1:200
CD11c-APC mAb (N418) eBioscience 17-0114-82 Use at 1:100
MHC-II (I-Ab)-Alexa Fluor 700 mAb eBioscience 56-5321-82 Use at 1:100
CD11b-eFluor 450 mAb (M1/70) eBioscience 48-0112-82 Use at 1:200
F4/80-PE-Cy7 mAb (BM8) eBioscience 25-4801-82  
CD11b microbeads Miltenyi Biotec 130-049-601  
CD11c microbeads Miltenyi Biotec 130-052-001  
50 mL conical tubes BD Falcon 352098  
Single mesh wire strainer Chefmate    
Small weigh boat Fisher Scientific 08-732-116  
100 μm cell strainer BD Falcon 352360  
40 μm cell strainer BD Falcon 352340  
5 mL polystyrene round-bottom tubes BD Falcon 352235 Use at 1:100
MaxQ 4450 benchtop orbital shaker Thermo Scientific    
LS MACS column Miltenyi Biotec 130-042-401  
LSR II BD    
FACSAria II BD    
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Referências

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Tags

IsolationCharacterizationDendritic CellsMacrophagesMouse IntestineInnate Immune CellsAdaptive Immune CellsToleranceCommensal FloraFood AntigensInflammatory ResponsesAntigen Presenting CellsDCsMacrophagesIntestinal Immune HomeostasisMicrobiotaIsolation MethodsDigestion TimesCell Surface Antigen ExpressionCell ViabilityCell YieldPhenotypic CharacterizationFluorescence-labeled Monoclonal AntibodiesFlow Cytometric AnalysisFunctional StudiesCD11cCD11b Magnetic-activated Cell Sorting Beads

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Geem, D., Medina-Contreras, O., Kim, W., Huang, C. S., Denning, T. L. Isolation and Characterization of Dendritic Cells and Macrophages from the Mouse Intestine. J. Vis. Exp. (63), e4040, doi:10.3791/4040 (2012).
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