Isolation, Culture, and Polarization of Murine Bone Marrow-Derived and Peritoneal Macrophages




© Springer Science+Business Media New York 2015
Vicente Andrés and Beatriz Dorado (eds.)Methods in Mouse AtherosclerosisMethods in Molecular Biology133910.1007/978-1-4939-2929-0_6


6. Isolation, Culture, and Polarization of Murine Bone Marrow-Derived and Peritoneal Macrophages



Inés Pineda-Torra , Matthew Gage1, Alba de Juan2 and Oscar M. Pello1, 3  


(1)
Division of Medicine, Centre for Clinical Pharmacology, University College London, 5 University Street, London, WC1 E6JF, UK

(2)
Walter Brendel Center for Experimental Medicine, Ludwig-Maximilians-Universität, Marchioninistr. 27, 81377 Munich, Germany

(3)
Department of Hematology, John Goldman Centre for Cellular Therapy, Hammersmith Hospital, 150 Du-Cane Road, London, W12 0HS, UK

 



 

Inés Pineda-Torra (Corresponding author)



 

Oscar M. Pello (Corresponding author)



Abstract

Macrophages are the most specialized phagocytic cells, and acquire specific phenotypes and functions in response to a variety of external triggers. Culture of bone marrow-derived or peritoneal macrophages from mice represents an exceptionally powerful technique to investigate macrophage phenotypes and functions in response to specific stimuli, resembling as much as possible the conditions observed in various pathophysiological settings. This chapter outlines protocols used to isolate and culture murine bone marrow-derived and peritoneal macrophages. Furthermore, we describe how these macrophages can be “polarized” to obtain specific macrophage subsets with special relevance to atherosclerosis.


Key words
Bone marrow-derived macrophagesPeritoneal macrophagesMacrophage polarizationAtherosclerosis



1 Introduction


Macrophages are phagocytic immune cells that play essential roles in homeostasis and orchestrate multiple responses to pathogens [1]. These cells acquire specialized phenotypes and functions depending on their microenvironment and, indeed, several macrophage subtypes have been identified and characterized over the last decade [2]. In the context of atherosclerosis, macrophages are crucial components of atherosclerotic plaques and contribute to the pathogenesis of the disease from its initial stages throughout the progression of the atheroma, and up to the final stages when the plaque becomes vulnerable and may rupture into the bloodstream [3]. During this process, macrophages contribute to a variety of functions depending on their phenotype, which in turns depends on their microenvironment. In an oversimplified classification, Th1 pro-inflammatory cytokines such as IL-2, IL-12, IFNγ, and TNFα and β lead to the activation of macrophages towards the so-called classical inflammatory phenotype (CAMs or M1 macrophages). In addition, Th2 cytokines such as IL-4 and IL-13 as well as anti-inflammatory molecules like IL-10 and TGFβ activate macrophages towards an alternative phenotype (AAMs or M2 macrophages). While M1s have been described to be involved in the secretion of inflammatory cytokines and vasoactive molecules contributing to atheroma growth, M2 cells participate in a wide range of processes including apoptotic cell clearance or the release of anti-inflammatory molecules and are generally considered anti-atherosclerotic [4, 5]. Although IL-4 is considered “the original” cytokine promoting M2 polarization, its role in atherosclerosis still remains ambiguous, as it has been shown to be involved in both, pro- and anti-atherosclerotic mechanisms [6].

The physiological and pathophysiological processes macrophages participate in make them a very interesting therapeutic target for inflammatory diseases, including atherosclerosis and cancer. Although in recent years there have been major advances in the use of noninvasive techniques to investigate the mechanisms underlying cardiovascular diseases, the systematic study of macrophages in a living organism, specifically within the aorta or a blood vessel by these techniques, is not yet technically feasible [7]. Thus, the isolation and culture of macrophages, which may be subjected to different stimuli ex vivo, has been a very useful and widespread tool to investigate the phenotype and functions of a particular subtype of macrophages. The number, purity and ease of culture of these cells make them a very attractive in vitro model. To investigate in culture the (dys)regulated pathways within a specific macrophage subtype that are playing a role in a particular pathological condition such as atherosclerosis, macrophages are usually activated with IFNγ plus LPS (CAMs or M1) or with IL-4, IL-13, and IL-10 (AAMs or M2) [8]. Due to the complex stimuli milieu present within the atheroma, it is not surprising that other macrophage subtypes have also been described in response to other molecules that affect the pathogenesis of atherosclerosis, including oxidized-LDLs (Mox macrophages) [9], CXCL4 (M4 macrophages) [10], or heme/haemoglobin (Mhem macrophages) [11].

In this chapter we describe the most common protocols used to isolate and differentiate cultured murine bone marrow-derived macrophages and peritoneal macrophages, and outline how these macrophages are traditionally “polarized” to obtain the M1 and M2 subsets that may be relevant to atherosclerosis and other inflammatory diseases.


2 Materials




1.

Purified-recombinant proteins



(a)

Murine macrophage colony-stimulating factor (M-CSF or CSF-1). Alternatively, noncommercial L929-M-CSF conditioned medium (LCM) prepared as indicated in Subheading 3.1.

 

(b)

Murine interleukin 4 (IL-4).

 

(c)

Murine interferon γ (IFNγ).

 

(d)

Lipopolysaccharide (LPS).

 

 

2.

High-glucose DMEM medium (with stable l-glutamine).

 

3.

RPMI-1640 medium with l-glutamine.

 

4.

Sterile phosphate-buffered saline (PBS) 1× suitable for cell culture.

 

5.

Sterile-filtered penicillin/streptomycin (P/S) (10 mg/mL).

 

6.

Sterile-filtered gentamycin (10 mg/mL) in deionized water.

 

7.

Fetal bovine serum (FBS).

 

8.

Complete DMEM medium: High-glucose DMEM, 10 % FBS, 5 % P/S.

 

9.

Complete RPMI medium: RPMI-1640 medium with l-glutamine, 10 % FBS, 2 % P/S.

 

10.

Differentiation medium: DMEM with stable glutamine + 20 % FBS + 30 % LCM + 20 μg/mL gentamycin (see Notes 1 and 2 ).

 

11.

Low (≤10 EU/mL) endotoxin FBS (FBS-LE).

 

12.

Trypsin–EDTA (0.25 % in PBS).

 

13.

Vacuum filter units, 0.45 μm.

 

14.

Sterile dissection tools: scissors, scalpel, and forceps.

 

15.

Needles, 25 gauge.

 

16.

Syringes, 5–10 mL.

 

17.

Sterile 1.5, 15, and 50 mL tubes.

 

18.

Centrifuge/microcentrifuge.

 

19.

Tissue culture T-75 cm2 and T-175 cm2 filter cap flasks.

 

20.

Tissue culture dishes (100 × 20 or 150 × 20 mm).

 

21.

Tissue culture sterile polysterene pipettes (10 mL, 2 mL).

 

22.

Plates (6-well) for macrophage culture.

 

23.

Humidified incubator with 5 % CO2 at 37 °C.

 

24.

Red blood cell lysis buffer (RBC lysis buffer).

 

25.

Mice: mouse models of atherosclerosis.

 

26.

70 % Ethanol in distilled water.

 

27.

Freezing medium: 90 % FBS + 10 % dimethyl sulfoxide (DMSO).

 

28.

Activation medium M1: 10 % FBS-LE, 20 μg/mL gentamycin, 20 ng/mL IFNγ, 100 ng/mL of LPS.

 

29.

Activation medium M2: 10 % FBS-LE, 20 μg/mL gentamycin, 20 ng/mL IL-4.

 

30.

Hemacytometer.

 


3 Methods


Before starting the methods please read carefully Notes 3 and 4 .

Sep 17, 2016 | Posted by in SUGERY, ORTHOPEDICS & ANESTHESIA | Comments Off on Isolation, Culture, and Polarization of Murine Bone Marrow-Derived and Peritoneal Macrophages

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