Mesenchymal stem cell-educated macrophages

Mesenchymal stem cells (MSC) are stromal cells with potent regenerative and immunomodulatory properties [1, 2]. They are found in multiple tissues, including bone marrow and adipose tissue [3] and are relatively easy to isolate and expand in culture. Their capacity to differentiate into multiple cellular lineages and their trophic effects on other progenitor cells has initiated interest in the use of these cells for regenerative therapy [4‐6]. However, analysis of the mechanisms involved in the reparative effects of MSC indicates that many of these effects may in fact relate to the immunomodulatory properties of MSC. It has been demonstrated that MSC ameliorate acute graft vs. host disease [7, 8], reduce the progression of kidney fibrosis by modulation of the early inflammatory response after injury [9, 10], and in experimental models show promise as a therapeutic treatment of immunological diseases including arthritis [11], hepatitis [12], and organ transplantation [13, 14].

MSC have the capacity to modulate the immune system via a plethora of mechanisms. They secrete anti-inflammatory factors such as TGF-β and hepatocyte growth factor [2], they inhibit lymphocyte proliferation via the expression of indoleamine 2, 3-dioxygenase (IDO) [15], and they express inhibitory co-stimulatory molecules such as programmed death ligand 1 (PD-L1) and TNF-related apoptosis-inducing ligand (TRAIL) [16, 17]. In addition, MSC modulate the immune system via indirect mechanisms by inducing immune cells to adapt a regulatory function. MSC induce regulatory T cells in vitro and in vivo[14, 18] and affect the differentiation and function of dendritic cells [19]. In recent years it has become clear that MSC also regulate the function of macrophages. Co-culture with MSC induces macrophages to adapt an enhanced regulatory phenotype via expression of increased levels of IL-10, reduced levels of TNF-α and IL-12, low co-stimulatory molecule CD86 and HLA class II while showing higher phagocytic activity [20, 21]. This effect of MSC is at least partially mediated by soluble mechanisms and prostaglandin E2 (PGE-2) has been indicated to be one of the factors involved [21].

The question is whether the in vitro effects of MSC on macrophages are operational in vivo. There is evidence that MSC infusion leads to increased levels of regulatory type monocytes/macrophages in the circulation [22]. This effect is accompanied by an increase in the abundance of regulatory macrophages present within inflamed tissue [22]. Furthermore, it has been shown that locally administered MSC attract macrophages and turn them into a regulatory phenotype [21, 23]. Thus in vivo administered MSC appear to have a similar effect on macrophages as their in vitro counterparts. The mechanisms involved, however, may be very different. There is accumulating evidence that, after administration, MSC are short-lived (Eggenhofer et al., in press). As transiently present MSC may themselves be incapable of secreting sufficient regulatory macrophages inducing factors, additional mechanisms may be important. Indeed, it has been demonstrated that the phagocytosis of dead MSC by macrophages induces them to adapt a more regenerative and immunomodulatory function [24]. This indicates that administered MSC may modulate macrophages function through initiating phagocytosis, while resident MSC that are around for a much longer period of time may modulate macrophages via the secretion of immunomodulatory factors and expression of cell surface molecules. In this respect it is interesting that throughout all tissues MSC are virtually ubiquitous. Tissue-resident MSC have the full capacity to locally induce regulatory macrophages. Studies into the influence of MSC on macrophages behavior are therefore relevant to assessments of MSC as a cell therapeutic product and also to examine the potentially exploitable effects of tissue-resident MSC.

MSC provide macrophages with signals that stimulate conversion to a regulatory phenotype. There are two conceivable applications for the generation of MSC-Mo, the first by inducing MSC-Mo through MSC therapy, and the second by the induction of MSC-Mo by tissue-resident MSC. Pre-clinical and clinical studies that aim to use or target MSC in organ transplantation should consider that MSC-Mo may have a vital role in mediating the effects of MSC.