Malaria is one the most serious infectious diseases of humans, with ∼500 million clinical cases annually. Most cases of severe disease are caused by Plasmodium falciparum, which is endemic in sub-Saharan Africa and throughout the tropics. Severe malaria is associated with a range of disease syndromes including respiratory distress, metabolic acidosis, hypoglycaemia, renal failure, and cerebral malaria (CM) [1]. The blood stage of the parasite is entirely responsible for malaria-associated pathology. Mature forms of P. falciparum blood-stage express parasitic proteins (such as P. falciparum erythrocyte membrane protein 1) on the surface of the infected erythrocyte, which allow them to bind to vascular endothelial cells and avoid clearance in the spleen. This process called sequestration induces obstructions in the blood flow and is postulated to result in hypoxia and haemorrhages that appear to be associated with the development of organ-specific syndromes such CM and placental malaria [1]. Many disease-association studies indicate that in addition to parasite sequestration, inflammatory responses also contribute to severe disease [1]. High TNF, IFN-γ, and IL-1β levels have been associated with disease severity [1]. The role of inflammatory cytokines in severe malaria is not completely understood, but they are thought to contribute to disease by up-regulating the expression of adhesion molecules such as ICAM-1 involved in the binding of parasitised red blood cells (pRBCs) to the vascular endothelium. Although parasite sequestration is the most common feature of patients succumbing to CM, postmortem examination has also revealed intra- and peri-vascular pathology including the presence of leukocytes within brain blood vessels [2]. These findings suggested that sequestration of host leukocytes might also contribute to the pathogenesis of some CM cases. Interestingly, recent findings revealed that increased levels of several inflammatory chemokines including MIP-1α and MIP-1β [3] and CXCL10 or IP-10 are associated with increased risk of severe malaria [4], suggesting a role for leukocyte trafficking in the etiology of human disease. Clearly, the analysis of intravascular inflammation predisposing to CM in humans is limited to the examination of post-mortem samples. Thus, murine malaria models constitute a valuable tool to obtain detailed mechanistic information, which cannot be deduced from human studies. Much useful evidence on the inflammatory processes (Figure 1) contributing to the induction of CM has been provided by the Plasmodium berghei ANKA model. This rodent infection has several features in common with human disease and is the best available model of severe malaria. Like in humans, pRBCs have been found to accumulate in brains of susceptible mice during infection. Numerous leukocytes are also present in brain blood vessels of these animals. This article summarizes the main lessons learnt from murine malaria studies and illustrates how emerging information on inflammatory pathways predisposing to disease might open new avenues for the development of therapeutic strategies to alleviate severe malaria. Figure 1 Inflammatory responses involved in the induction of ECM. Systemic and Organ-Specific Inflammation Mediated by Leukocytes Inflammatory responses mediated by cytokines such as TNF [5], IFN-γ [6], LT-α [7], and effector cells including CD4+T [8], CD8+T [9], [10], NKT [11], and NK cells [12] have been shown to contribute to the development of experimental CM (ECM). CBA and C57BL/6 mice, predisposed towards Type-1 responses, are susceptible to the ECM, whereas BALB/c mice are resistant. C57BL/6 and BALB/c mouse strains differ in the expression of molecules encoded by a genetic region called the Natural Killer Complex (NKC), and it has been shown that the differential expression of these receptors in CD1d-restricted NKT cells influences their immunological behaviour in response to malaria and accounts for the degree of susceptibility to ECM [11]. The expression of C57BL/6 NKC alleles, which is associated with disease severity, appears to favour enhanced IFN-γ responses to infection [11]. The role of T cells in the pathogenesis of ECM has been extensively investigated. Antibody depletion studies as well as infection of β2-microglobulin−/− mice demonstrated that CD8+ T cells contribute to the induction of ECM [8]. Cytotoxic CD8+ T cells have been found sequestered within brain blood vessels of P. berghei ANKA-infected mice [9], [10], and they appear to mediate CM via a perforin-dependent mechanism. The vast majority of inflammatory CD8+ T cells as well as CD4+ T cells and NK cells migrate to the brain of infected animals via a CXCR3-IP-10-dependent mechanism [13]–[15]. Brain-sequestered CD8+ T cells have been found to be specific for parasite-expressed model antigens [16]. Dendritic cells (DCs) are essential for the priming of T cell responses involved in the development of ECM [17]. Amongst these cells, CD8α+ conventional DCs are the main subset involved in the cross-presentation of parasite-expressed antigens to naive CD8+ T cells [16]. CD4+ T cells have also been found in brain blood vessels of CM-affected mice [10]. They are not as abundant as CD8+ T cells, and it is not clear if they are parasite-specific or not. Nevertheless, in vivo depletion of CD4+ T cells with antibodies or genetic deletion of MHC class II molecules [8] also results in protection of susceptible mice from ECM. Recent work demonstrated that IFN-γ production by CD4+ T cells is required for the recruitment of CD8+ T cells to the brain of infected animals [18]. NK cells are important mediators of IFN-γ responses to malaria in humans and mice. Specific depletion of NK cells protects mice from P. berghei ANKA-mediated severe disease [12]. NK cells were shown to stimulate the recruitment of CXCR3+ T cells to the brain of malaria-infected mice in an IFN-γ-mediated manner [12]. More specifically, NK cells appear to stimulate the DC-mediated priming of naive CD8+ T cells in response to P. berghei ANKA [19].