We describe a mouse model of experimental cerebral malaria and show how inflammatory and microvascular pathology can be tracked in vivo using magnetic resonance imaging.
Cerebral malaria is a sign of severe malarial disease and is often a harbinger of death. While aggressive management can be life-saving, the detection of cerebral malaria can be difficult. We present an experimental mouse model of cerebral malaria that shares multiple features of the human disease, including edema and microvascular pathology. Using magnetic resonance imaging (MRI), we can detect and track the blood-brain barrier disruption, edema development, and subsequent brain swelling. We describe multiple MRI techniques that can visualize these pertinent pathological changes. Thus, we show that MRI represents a valuable tool to visualize and track pathological changes, such as edema, brain swelling, and microvascular pathology, in vivo.
Malaria is a significant global health problem.1 Severe malaria is characterized in part by cerebral involvement and is often a poor prognostic factor. Cerebral involvement is common in children under the age of five in areas of high malaria transmission and represents the major cause of malaria related death in that age group.1 While aggressive treatment can be life-saving, the detection of cerebral malaria, especially in early stages, can be difficult. The pathological processes involved in cerebral malaria include microvascular disruption and cerebral edema, which can lead to severe brain swelling. In this article, we present a magnetic resonance imaging (MRI) protocol that allows whole-brain in vivo imaging of experimental cerebral malaria (ECM). Whole-brain high-resolution imaging methods have been widely underutilized in this disease, even though little is known about how ECM initiates in the central nervous system or what specific mechanisms lead to the disease. In vivo MRI, covering the whole brain, represents an important research tool to gain a better understanding of ECM pathology. MRI is able to assess global cerebral brain swelling, which has recently been recognized to be an important predictor of death not only in ECM, but also in human cerebral malaria.2,3 Severe brain swelling occurs in fatal disease and represents one of several pathological features between the ECM models and human disease, a disease that is characterized by both inflammatory and microvascular alterations.4
ECM can be induced in CBA or C57BL mice through infection with lethal Plasmodium berghei ANKA.5 The onset of ECM typically occurs between days 6 and 10 post-infection and results in fitting, ataxia, respiratory distress, and coma, which lead to rapid death.4 The Rapid Murine Coma and Behavior Scale (RMCBS) is a helpful score to evaluate clinical symptoms of ECM. It consists of 10 parameters, each scored from 0 to 2, with a maximum possible score of 20.6 Recently, we showed good agreement between the severity of the RMCBS scores in ECM mice and pathological changes demonstrated by MRI.7 In this protocol, we describe ECM induction in mice and in vivo magnetic resonance imaging of mice with ECM.
All animal experiments reported in this article were conducted according to the Federation for Laboratory Animal Science Associations (FELASA) category B and the Society of Laboratory Animal Science (GV-SOLAS) standard guidelines and were approved by the local German authorities in Karlsruhe (Regierungspräsidium Karlsruhe, Germany). Please note that biosavety level 2 applies to mosquito and Plasmodium berghei ANKA sporozoite work.
1. Infection
2. Magnetic Resonance Imaging Setup
3. Imaging Protocol
NOTE: Choose imaging sequences from the protocol listed below according to the research questions to be addressed. All listed parameters are valid for the MRI software but might need to be adjusted if other software programs are used.
4. Image Processing and Analysis
In C57BL/6 mice, the first clinical symptoms of ECM can be observed between days 6 and 10 after infection with P. berghei ANKA sporozoites. ECM develops in 60 – 80% of infected mice and rapidly progresses to coma and death within 24 to 48 h. In contrast, mice that do not develop ECM die after the second week post-infection from severe anemia due to hyperparasitemia.12
In MRI imaging, the earliest signs of ECM are visible in the olfactory bulb, which belongs to the olfactory system of the mouse and is located in the rostral part of the brain.7,13 An increase in blood-brain barrier disruption (seen on contrast-enhanced T1-weighted images) and a fluid increase (increase of T2 signal on T2-weighted images, T2 relaxometry, and diffusion-weighted imaging) indicate early vasogenic edema in the olfactory bulb that is already present in mild disease (RMCBS score 20-16) and starts to spread as the severity of the disease increases. Relative T1 signal images help to detect subtle blood-brain barrier disruption (Figure 1). Blood-brain barrier disruption and vasogenic edema progress in a specific fashion. These pathological changes spread along the rostral migratory stream, a migrating route for neuroblasts, towards the brainstem, which is reached in very severe disease (RMCBS sore 9-0). On T2 maps, the severity of vasogenic edema can be quantified by drawing regions of interest into specific anatomical regions, as demonstrated in Figure 2. For each region, a T2 relaxation time that increases with increasing edema can be obtained. Along with vasogenic edema and blood-brain barrier disruption, brain swelling starts as the ECM severity increases. Brain volume indicative of edema starts to significantly increase in moderately sick mice as compared to baseline and further increases in severely sick mice (Figure 3).
Microvascular pathology, as evidenced by microhemorrhages and an increase of vessel susceptibility contrast (corresponding to slow flow), occurs after the first signs of blood-brain barrier disruption and vasogenic edema and can be visualized with T2*-weighted imaging. Microhemorrhages predominantly occur in the olfactory bulb (Figure 4). The number of microhemorrhages increases with progressive disease. With progressive disease microhemorrhages are also evident in cortex, basal ganglia, cerebellum, white matter and brainstem.
Decreased arterial patency is seen by time-of-flight angiography as a sign of macrovascular impairment in parallel to microvascular changes. Cerebral infarction is not a key finding in ECM. In very severe disease, however, focal areas of ADC decrease can be identified, indicating cerebral infarctions.
Figure 1: Blood-brain Barrier Disruption. (A) A representative coronal 3D T1-weighted image. An increase in T1 signal is visible in the central region of the olfactory bulb. (B) On the corresponding T1 relative signal image (T1 pre-contrast image subtracted from the T1 post-contrast image), contrast agent extravasation is easier to delineate. Contrast agent extravasation is visible in the frontal cortical regions (white arrows). Please click here to view a larger version of this figure.
Figure 2: T2 Relaxometry. Sample T2 maps at different heights from one severely sick mouse with an RMCBS score of 5 (A) and from the baseline scan (B) are displayed in color scale, in grey scale, and in grey scale with ROIs as colored overlays. Dark blue = RMS, green = cortex, turquoise = external capsule, yellow = basal ganglia, light blue = DMS, orange = thalamus, and red = brainstem Please click here to view a larger version of this figure.
Figure 3: Brain Volume Measurements. Brain volume significantly increases in moderately sick mice (RMCBS 15-10). Representative values of 10 mice are shown. Data is presented as the mean standard deviation. A paired Student's t-test was used to analyze the differences in brain swelling between groups. In moderately/severely sick mice, the brain volume was significantly increased compared to baseline (p = 0.021/0.001). Please click here to view a larger version of this figure.
Figure 4: Microhemorrhages. Representative T2*-weighted images of a mouse before the onset of blood-stage infection (A) and on day 8 after infection with an RMCBS score of 14 (B and C) are shown. In the first image, no microhemorrhges are evident (A), while in the second and third images, several microhemorrhages are visible, with a predominance in the olfactory bulb (B: plane coronal image; C: 3D projection with segmented microhemorrhages).
In this article, we describe a whole-brain MRI protocol to delineate changes in experimental cerebral malaria. We believe that MRI has been under-utilized in malaria research to date and hope that our protocols will aid other investigators. We would like to describe some additional points that may be helpful.
If severely sick mice are imaged, positioning is crucial. Due to increased intracranial pressure, mice are susceptible to death, and thus, the cervical spine should not be stretched. Anesthesia should also be kept to a minimum. If mice with mild disease are imaged, the best time point for MRI is 12-24 h prior to the expected onset of the first clinical symptoms. Mild vasogenic edema in the olfactory bulb is visible in mice that do not exhibit any clinical signs of ECM (RMCBS score of 20).
The length of the MRI protocol itself can be adapted according to the specific research question. The minimal protocol should include a T2-weighted sequence or T2 relaxometry and a T2*-weighted sequence in order to judge the presence of vasogenic edema and microhemorrhage load/microvascular impairment. To get good-quality images, motion artefacts should be kept to a minimum. Motion will be reduced through the proper positioning of the mouse and by keeping the breathing rate at about 60-80 breaths per min.
Other in vivo imaging methods, such as intravital microscopy, show promise in visualizing pathological alterations in ECM on a cellular level.14,15,16,17 Compared to MRI, intravital microscopy can offer high spatial resolution at the cost of only covering a limited cortical area. In contrast, MRI is able to cover the whole brain at a resolution of up to 80 µm. MRI can therefore guide further cellular investigations by identifying the predilection sites-the beginning of disease-as well as the stage of the disease, which can then be assessed using further methodologies. MRI findings in ECM can be compared to pathological alterations detected with MRI in human cerebral malaria. Both human and experimental cerebral malaria show vasogenic edema in areas of neurogenesis, as well as microvascular pathology, such as secondary cerebral infarcts in watershed areas.7,18 White and grey matter are affected in a similar fashion, and brain swelling in both human and experimental cerebral malaria involves the brainstem in severe disease, explaining the comatose state.2,7
We hope that in vivo imaging will help unravel the underlying pathological mechanism of cerebral malaria, which currently remains elusive. As edema and brain swelling are barely visible ex vivo, methods to visualize this pathology in vivo are key and will help to improve the evaluation of novel therapies and vaccinations.
The authors have nothing to disclose.
The expert technical assistance of Miriam Reinig is gratefully acknowledged. AH received funding from a postdoctoral stipend of the Medical Faculty of the University of Heidelberg. MP is supported by a memorial stipend from the Else-Kröner-Fresenius Foundation. AKM is a recipient of a maternity leave stipend by the DZIF Academy of the German Center for Infection Research (DZIF). JP is the recipient of a Heidelberg Research Center for Molecular Medicine (HRCMM) Career Development Fellowship. We furthermore gratefully acknowledge Julia M. Sattler and Friedrich Frischknecht for providing an exemplary movie of sporozoite movement.
Isoflurane | Baxter | 1001747 | for anesthesia |
Dotarem | Guebert | 1086923 | Gd-DTPA contrast agent; 0.5mmol/ml |
Amira (Image Processing Program) | FEI Group | Version Amira 5.3.2 | |
MATLAB | The MathWorks, Inc., | Release 2012b | |
FDT toolbox | FMRIB's Software Library | http://www.fmrib.ox.ac.uk/fsl/fdt/index.html |