Abstract
Ischemic stroke is rarely confined to gray matter, and primary white matter injury occurs in a significant proportion of human strokes. In preclinical investigations searching for stroke therapies, the emphasis is shifting away from primary neurotoxicity to the secondary injury phase, which occurs in a time window that is more amenable to treatment in hospital. This phase is characterized by a prominent inflammatory response in the brain that can last for hours to days. This chapter focuses on the intersection of inflammation and white matter injury in experimental models of ischemic stroke. We first describe the main rodent models and methods used to monitor white matter damage, and discuss we prefer some approaches. Next, we describe the main immune cells involved in animal models of ischemia, how to monitor them, and present key findings. We then summarize the limited literature addressing the intersection of ischemic stroke, white matter injury, and inflammation in adult and neonatal rodent ischemia models, and finally comment on specific needs for further research.
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Keywords
- White Matter
- Middle Cerebral Artery Occlusion
- Myelin Basic Protein
- White Matter Tract
- Transient Ischemia
These keywords were added by machine and not by the authors. This process is experimental and the keywords may be updated as the learning algorithm improves.
1 Introduction
1.1 Statement of the Problem
This entire book focuses on white matter; ranging from structure and distribution in the central nervous system (CNS), to methods for monitoring injury and repair, and mechanisms underlying white matter injury. Many types of CNS insult in patients and in animal models are considered, and several chapters deal specifically with stroke in patients, and with ischemia in animal models. Ischemic stroke is much more prevalent than hemorrhagic stroke (Adams et al. 1993) and is the leading cause of long-term disability in the USA and the second leading cause of death worldwide (Kelly-Hayes et al. 1998; Lopez and Mathers 2006). Primary ischemic stroke can be global (usually the result of cardiac arrest or an aortic occlusion) (Traystman 2003) or focal, if caused by a transient or permanent occlusion of a major cerebral artery or one or more deep blood vessels (so-called lacunar stroke) (Durukan and Tatlisumak 2007). Intracerebral hemorrhage (ICH) results from rupture of small brain arteries or arterioles, and accounts for the remaining 10–15 % of strokes in Western populations (Anderson et al. 1994). Up to 30–40 % of ischemic strokes spontaneously undergo hemorrhagic transformation (Wang and Lo 2003), and ICH patients are at a high risk of developing global ischemia (Qureshi et al. 2009). In addition, ischemic stroke is a risk factor when treating hemorrhage with the blood-clot promoter; factor VIIa, the only drug used for treating ICH. While factor VIIa can decrease hematoma expansion (Diringer et al. 2008; Mayer et al. 2005, 2008), the outcome is often unimproved (Mayer et al. 2008; Lin et al. 2012).
The only effective drug treatment for ischemic stroke patients is the thrombolytic, tissue plasminogen activator (tPA). While tPA can, in limited cases, produce a remarkable reperfusion of damaged tissue, its use is limited by the need to inject it within the first 3–4.5 h of stroke onset (Wang et al. 2004). Because most patients are not in hospital and assessed in that time window, only about 5 % of patients can currently benefit from tPA therapy (del Zoppo 1998). This has spawned a huge and ongoing effort to identify new therapeutic targets and drugs. Hundreds of chemicals that target early neurotoxicity have been identified, and dozens have proven promising in preclinical studies in rodents but have been ineffective in improving survival or functional outcomes in clinical trials (Brott and Bogousslavsky 2000; Ginsberg 2009; Lakhan et al. 2009). This failure has led to deeper consideration of potential shortcomings of experimental approaches and models used in preclinical stroke research (Braeuninger and Kleinschnitz 2009; Dirnagl 2006; O’Collins et al. 2006). Several reports from European and North American Stroke Consortia (Stroke Therapy Academic Industry Roundtable) (Endres et al. 2008; Meairs et al. 2006; Fisher 1999) have emphasized that most experimental studies target events that are too early to be “drug-able,” are restricted to healthy, young male rodents, lack relevant comorbidities (e.g., hypertension, diabetes), monitor infarct size as their primary outcome measure, and have been highly neurocentric. Most stroke research has explored neural cell death and neural cell repair (Petty and Wettstein 1999). Many studies have relied on showing treatment-related changes in neuron apoptosis (e.g., TUNEL, caspase 3 activation), damaged (e.g., Fluorojade) or remaining neurons (e.g., NeuN staining). Recommendations from stroke consortia for improving preclinical studies include: (1) focus more on white matter injury; (2) identify strategies to protect vascular and glial cells, not just neurons; (3) focus more on aged animals; (4) develop small animal models of lacunar stroke and compare mechanisms of damage with large vessel occlusion; and (5) identify and understand neuroimmune interactions and develop therapeutic strategies to target inflammation. This chapter will address several of these recommendations for preclinical studies.
1.2 Why Study Inflammation and White Matter Injury After Ischemic Stroke?
Historically, white matter was thought to be less susceptible to stroke than gray matter (Marcoux et al. 1982). More recent advances in imaging technology have led to a paradigm shift. Development of neuroimaging techniques, such as magnetic resonance imaging (MRI) and Diffuse Tensor Imaging, has provided the means to map networks of white matter in the human brain at the macroscopic level. Resulting clinical observations have shown that ischemic stroke is rarely confined to gray matter (Goldberg and Ransom 2003), and primary white matter injury occurs in about 25 % of human strokes (Matute et al. 2013). At the microscopic level, more recent research has demonstrated the sensitivity of the major cellular components of white matter to ischemia. Several animal models have shown the susceptibility to ischemic damage of oligodendrocytes, the myelin forming cells of the CNS (reviewed by (Arai and Lo 2009)), myelin and axons (Petty and Wettstein 1999; Hughes et al. 2003; Irving et al. 2001; Lively and Schlichter 2012; Medana and Esiri 2003; Moxon-Emre and Schlichter 2010, 2011; Pantoni et al. 1996). Thus, white matter is now considered an important contributor to stroke outcome, and a tractable therapeutic target.
A second paradigm shift has been the change in focus of preclinical investigations searching for new post-stroke therapies. The emphasis is moving away from the rapidly occurring primary neurotoxicity to the secondary injury phase, which occurs in a time window that is amenable to treatment in hospital. This secondary phase is characterized by a prominent inflammatory response within and surrounding the core infarct that can last for many hours to days (Emsley and Tyrrell 2002; Jin et al. 2010; Zhang and Stanimirovic 2002). However, inflammation is complex. Understanding its temporal-spatial development and which components are harmful versus beneficial will be essential for developing better therapeutic strategies. Figure 19.1 illustrates the commonly proposed time course of events after stroke in humans.
1.3 Scope of This Chapter
Much of this book is devoted to white matter damage after acute injury, including ischemic stroke and intracerebral and subarachnoid hemorrhage. Thus, we will not review findings that focus solely on white matter damage. Instead, the chapter will focus on the intersection of inflammation and white matter injury in the context of experimental models of ischemia. In focusing on ischemic stroke (the vast majority), the chapter begins by describing the main models used to monitor white matter injury in experimental stroke studies (mainly rodents). We describe methods used to monitor white matter damage in these models, and provide some figures to illustrate why we prefer some approaches over others. Because this is the only chapter in this book that explicitly deals with inflammation, we then provide a brief primer on inflammation. This section describes the main immune cells involved in animal models of ischemia, how to monitor them, and key findings. Then, we summarize the limited literature concerning the intersection of all three elements (ischemic stroke, white matter injury, inflammation) in both adult and neonatal rodent ischemia models. The wrap-up section comments on needs for further research.
In selecting literature related to this chapter, we searched the PubMed database up to March 2013. As shown in Fig. 19.2, the search began with original and review articles that contained all three topics: transient focal ischemia + white matter + inflammation. Remarkably, only two publications were found. We then broadened the search using combinations of multiple search terms, and included studies that examined inflammation and white matter damage in neonatal hypoxia–ischemia and adult chronic ischemia models.
2 Animal Models Used to Study White Matter Injury After Ischemia
2.1 White Matter Locations in the Brain
It is often noted that the ratio of white matter to gray matter in the human brain is 60:40, but much lower in the rat (14:86) and mouse (10:90) (Krafft et al. 2012). While this might be considered an impediment to studying white matter injury, rodents have several brain regions with high densities of white matter (Johnson et al. 2012). Several of these regions are commonly used to study white matter damage in rodents. The corpus callosum is comprised of white matter tracts (nerve fibers) that connect the two cerebral hemispheres, transferring and integrating information from the left and right hemispheres (Bruni and Montemurro 2009). The internal capsule is a compact band of fibers that lies deep in the brain, separating the caudate nucleus from the putamen. It consists of projection fibers that relay information from the cortex and spinal cord, brain stem, and subcortical structures (Bruni and Montemurro 2009). The optic nerve, formed by axons of retinal ganglion cells, carries information from the retina to the thalamus and other subcortical nuclei (Perry and Cowey 1984; Perry et al. 1984). Other white matter-dense brain regions include, but are not limited to, the anterior commissure, cingulum, extreme capsule, and external capsule (Bruni and Montemurro 2009). Some brain regions such as the striatum provide an excellent template for studying white and gray matter injury side-by-side. As Fig. 19.3 illustrates, the striatum contains a large number of myelinated axon bundles that are surrounded by nerve cell bodies and dendrites, and astroglial and microglial cells. We have exploited this structure in rats to simultaneously analyze inflammation, neuronal death, and damage to myelin and axons after both ischemic and hemorrhagic stroke (Lively and Schlichter 2012; Moxon-Emre and Schlichter 2010, 2011; Lively et al. 2011; Wasserman and Schlichter 2007, 2008; Wasserman et al. 2008).
2.2 Ischemia Models Used to Study White Matter Damage
It is clear that no animal model can fully recapitulate all components of human stroke (Durukan and Tatlisumak 2007; Howells et al. 2010). Most preclinical studies are conducted in small animals, especially rodents (Durukan and Tatlisumak 2007), and almost all results relevant to this chapter come from rats and mice. While mouse models facilitate using transgenic animals, which are of limited availability in rats (Durukan and Tatlisumak 2007), we mainly exploit rats for several reasons. The cerebrovascular anatomy and physiology is reasonably similar between rats and humans (Macrae 1992). In the most commonly used mouse model of ischemia (middle cerebral artery occlusion (MCAo), discussed below), the infarct size is highly variable and shows strain-dependence that is not seen in rats (Carmichael 2005). The positive correlation between brain size and amount of white matter (Zhang and Sejnowski 2000) and larger brain size of rats yields more material for analysis. The larger size is especially useful when one seeks to analyze several parameters or stains, and to quantify differences across brain regions.
2.2.1 Vessel Occlusion
Middle cerebral artery occlusion. Most human ischemic strokes occur in the area surrounding the middle cerebral artery (MCA). A rodent model of MCAo was developed early and has since been refined (Koizumi et al. 1986; Robinson et al. 1975). Robinson et al. (1975) used craniotomy to expose the MCA and distally ligated the artery, which produced an ischemic lesion that extended into the cortex. Now, a more commonly used method for occluding blood flow is to advance an intraluminal suture through the internal carotid artery (ICA) until it reaches the origin of the MCA (del Zoppo et al. 1992). With this method, transient ischemia is produced by removing the suture to allow reperfusion. The duration of MCAo needed to produce a significant nonlethal lesion is variable. The common duration for rat is 60, 90, or 120 min (Carmichael 2005), and usually results in neuron death throughout the striatum and into the dorsolateral cortex, but not in contralateral brain regions (Garcia et al. 1995). Based on the distribution of injury, the MCAo model is useful for simultaneously analyzing damage that is mainly isolated to gray matter (in the cortex), white matter (in the corpus callosum), or occurs in both (in the striatum). Despite its popularity, an important limitation of the MCAo model is the variable size and location of the infarct (Liu and McCullough 2011). Some of the variability seen in the literature can be attributed to differences in size and quality of the suture/filament used (Kuge et al. 1995); silicone-coated thread induces a larger lesion than uncoated thread (Laing et al. 1993). When using mice, some strains demonstrate substantially larger infarcts after MCAo than others (Connolly et al. 1996a). Other limitations of the MCAo model are the risk of subarachnoid hemorrhage (Carmichael 2005), and the added difficulty in aged animals, which have less flexible blood vessels and higher mortality (Liu and McCullough 2011).
Anterior choroidal artery occlusion. Occlusion of the anterior choroidal artery (AchAo) can be obtained by advancing an intraluminal suture through the ICA to a region proximal to the MCA (He et al. 1999). As illustrated in detail in their follow-up paper the infarct location is similar in MCAo and AchAo (He et al. 2000). The main differences are that after AchAo, the infarct is generally smaller but nearly always encompasses the internal capsule. Thus, AchAo reliably produces ischemia in a white matter-dense region, and facilitates studies of deep lacunar strokes with a less-distributed lesion than MCAo.
2.2.2 Vasoconstriction
An increasingly popular model uses injection of the potent vasoconstrictor, endothelin-1 (ET-1). ET-1 is a naturally occurring, 21 amino acid peptide produced by endothelial cells, which binds to the endothelial receptors, ETA and ETB (Verhaar et al. 1998). There are several advantages of this model over vessel occlusion models. Provided the potency of each ET-1 batch is tested, the injected dose can be titrated to obtain different degrees of transient ischemia, and lesion sizes that are relatively reproducible. For instance, with moderate amounts of ET-1 injected directly into the brain parenchyma, a reduction of cerebral blood flow (CBF) of ~60 % for up to 3 h has been reported (Hughes et al. 2003).
ET-1 is sometimes applied to the MCA to cause constriction, instead of ligating the artery in rats (Gresle et al. 2006; Robinson et al. 1990). Importantly, stereotaxic ET-1 injection can be used to produce a focal infarct in brain regions that are selected to focus on white matter (e.g., corpus callosum, internal capsule), gray matter (e.g., cortex), or both (e.g., striatum) (Sozmen et al. 2012). When injected into white matter-rich regions, ET-1 produces hallmarks of white matter injury seen in humans, including axonal damage, demyelination, inflammation, and glial scar formation (Hughes et al. 2003; Lively and Schlichter 2012; Moxon-Emre and Schlichter 2010). Figure 19.4 shows the development of a typical infarct after ET-1 injection into the anterior striatum (putamen + caudate) of the rat, and illustrates sample sites for quantitative spatial analysis.
There are few mouse studies using ET-1 injection to evoke transient ischemia, and the results have been inconsistent. Injecting ET-1 into the striatum failed to induce ischemia in multiple strains of mice, and increasing the dose increased mortality without inducing a lesion (Horie et al. 2008). Another study showed a dose-dependent increase in infarct size in mouse brain subjected to multiple focal injections of ET-1 (Sozmen et al. 2009). Differences in expression of endothelin receptor subtypes might be a confounding factor. Mouse brain expresses a lower proportion of ETA receptors, which evoke the vasoconstriction needed to produce ischemia, than ETB receptors, which generally cause vasodilation (but see below) (Sozmen et al. 2012; Wiley and Davenport 2004). The possibility was raised that the larger proportion of ETB receptors interferes with induction of ischemia in the mouse brain (Sozmen et al. 2012). That differences in ET-1 affinities are responsible is unlikely: the K d for ET-1 binding is 0.12 nM for ETB and 0.6 nM for ETA receptors (Haynes et al. 1995). A further complication is that in humans, ETB receptors can mediate both vasodilation and vasoconstriction (Haynes et al. 1995; Clozel et al. 1992; Seo et al. 1994). This might explain the finding that although the rat striatum contains mainly ETB receptors (Tayag et al. 1996), a focal ET-1 injection reliably produces an ischemic infarct (described above). Further research is needed to clarify the regional and cell-specific expression, and roles of the ET-1 receptor subtypes in rodents. Nevertheless, focal ET-1 injection into the rat CNS is a widely accepted model of transient ischemia that can create reproducible lesions restricted to a desired region of the brain (Sozmen et al. 2012).
2.2.3 Neonatal Hypoxia–Ischemia Models
The most commonly used model of ischemic injury in immature rodents is the hypoxia–ischemia (HI) model (Vannucci and Hagberg 2004). To induce ischemia, the common carotid artery is permanently ligated, and the whole body is temporarily exposed to hypoxia (often 8 % oxygen for up to 3 h). This procedure reduces CBF to the ipsilateral brain region by 40–60 %, and then CBF returns to normal immediately after re-exposure to normoxic conditions (Vannucci et al. 1988). Unlike adult rodents, ligation or hypoxia alone does not induce ischemia in neonates: both are required (Vannucci and Hagberg 2004). The resulting infarct is large but restricted to the ipsilateral hemisphere; damage to the contralateral hemisphere is rare (Towfighi et al. 1995; Vannucci and Vannucci 1997). On the ipsilateral side, the infarct extends through the cerebral cortex, striatum, thalamus, hippocampus, and most importantly for the topic of this chapter, the subcortical white matter. HI is exploited as an animal model of cerebral palsy (Johnston et al. 2005), a disorder seen in about 1/300 8-year-old children in the USA (Kirby et al. 2011). Several modifications of the HI model have also been used, including bilateral carotid ligation or variations in the duration of hypoxia. In this chapter, we will restrict discussion to rodent models using unilateral ligation followed by 6–8 % oxygen.
2.2.4 Optic Nerve Ischemia
The myelinated axon tracts that make up the optic nerve have proven extremely useful for studying mechanisms underlying white matter injury. Much of the stroke-related mechanistic work has used isolated optic nerves subjected to varying periods of oxygen-glucose deprivation (OGD) to simulate ischemia (Arai and Lo 2009). However, the optic nerve is one of the most vulnerable white matter regions following experimental chronic ischemia (Wakita et al. 1994). ET-1 has been injected into the microvasculature of the optic nerve in vivo (Cioffi et al. 1995), and some consider the resulting ischemia and white matter injury to be a good model of human glaucoma (Cioffi 2005).
2.3 Methods Used to Monitor White Matter Damage After Ischemia
As mentioned above, neuronal axons and the myelin sheath are both susceptible to ischemic injury.
Despite their intimate connections, the timing and mechanisms underlying damage to these structures differs. The vulnerability of oligodendrocytes to ischemic injury can lead to myelin loss and prevent its repair. Therefore, to comprehensively examine white matter injury after ischemia, it is important to distinguish myelin from axons (both healthy and damaged) and to monitor oligodendrocytes.
2.3.1 Staining Healthy and Damaged Myelin
Histological stains for myelin have been in use for many years, with loss of staining indicating white matter pathology. Healthy myelin can be labeled with colorimetric stains, such as the lipid soluble dyes, Luxol Fast Blue (LFB) (Kluver and Barrera 1953; Salthouse 1962) and Sudan Black B (Stilwell 1957) but these dyes provide low contrast and resolution (Schmued et al. 2008). There are several recent improvements in myelin labeling that are less expensive than antibody-based methods. Gold-chloride and, especially, the improved gold-phosphate complex (“Black-Gold”) provide excellent contrast under bright-field and dark-field illumination (Wasserman and Schlichter 2008; Schmued et al. 2008). If fluorescence is required, FluoroMyelin™ stain is attractive because it can be combined with immunohistochemistry in fixed tissue. For live imaging, FluoroMyelin™ Red is a vital dye that labels myelinated axons (Monsma and Brown 2012).
The use of antibody-based immunohistochemistry for detecting myelin damage has become popular because it can provide excellent contrast and allows use of multiple stains. The most commonly used protein target is myelin basic protein (MBP), which constitutes up to 30 % of myelin in the CNS (Sternberger et al. 1978). A reduction in antibody staining for MBP has been used to monitor myelin damage or loss in animal models of transient ischemia (Irving et al. 2001; Lively and Schlichter 2012; Moxon-Emre and Schlichter 2010; Souza-Rodrigues et al. 2008) and HI (Carty et al. 2008; Villapol et al. 2011). A cautionary note in relying solely on MBP labeling is that the staining can appear faint if healthy myelinated axon bundles are very tightly packed (Sternberger et al. 1978). If so, then the swelling of damaged axon bundles might actually increase the MBP labeling. An important advance that overcomes this limitation is the immunological detection of degraded MBP (dMBP) (Matsuo et al. 1997). We prefer this approach and, as shown in Fig. 19.5, have found that the increase in dMBP labeling coincides temporally and spatially with loss of MBP after transient ischemia evoked by injecting the vasoconstrictor, ET-1, into the rat striatum.
2.3.2 Identifying Damaged Axons
For histological assessment of axon pathology, the Bielschowski silver impregnation method was developed many years ago (Nauta 1952). This stain labels degenerating axon terminals, and although it is still in use, it is capricious and cannot be used for co-labeling (Castellani et al. 2007). With increased understanding of axon pathology, new markers of damaged axons continue to be identified. For instance, when fast axonal transport is disrupted in injured axons, there is swelling and accumulation of proteins and organelles. Accumulation of amyloid precursor protein (APP) can be readily detected by immunohistochemistry (Fig. 19.6). APP is considered a more reliable indicator of early axon injury than traditional silver stains (Ferguson et al. 1997; Gentleman et al. 1995; Smith et al. 2003) but accumulation does not indicate whether axons are terminally damaged or can recover. As shown in Fig. 19.6, we recently found that the matricellular molecule, SC1/hevin, identifies early axon damage after transient ischemia (and other forms of acute damage) much like APP (Lively and Schlichter 2012). Another indication of damage is loss of integrity of the axon cytoskeleton, which can be monitored using antibodies raised against neurofilaments (e.g., NF200) (Lively and Schlichter 2012; Moxon-Emre and Schlichter 2011; McCracken et al. 2002). In the brain, the heavy neurofilament chain is considered the most highly phosphorylated protein, and changes in its phosphorylation state have been used to detect axon damage (reviewed in (Petzold 2005)). Nonphosphorylated heavy neurofilaments can be detected using the SMI-32 antibody (Sternberger and Sternberger 1983), which labels damaged axons in humans following cerebral ischemia (Leifer and Kowall 1993). The interpretation of changes in SMI-32 staining intensity might be complicated. After transient forebrain ischemia in rats, an increase in SMI-32 intensity was seen in swollen, degenerating axons in the core of the infarct, and the staining gradually decreased as white matter damage progressed (Gresle et al. 2006). However, at the inside edge of the lesion (delineated by ballistic light analysis), increased staining was also seen in morphologically normal-appearing axons. The authors suggest that SMI-32 immunohistochemistry might distinguish the edge of the peri-infarct region.
2.3.3 Monitoring Oligodendrocyte Damage
The microtubule-associated protein, Tau-1, might be a good early indicator of oligodendrocyte pathology. After transient (Valeriani et al. 2000) and permanent ischemia (Valeriani et al. 2000; Irving et al. 1997), Tau-1 immunoreactivity increases rapidly (<1 h) and transiently (1–3 days) in oligodendrocytes within the infarct. However, the fate of the Tau-1-labeled cells is unclear and they are not necessarily lost (Gresle et al. 2006). Tau-1 is normally present in healthy axons so it is necessary to either show lack of co-labeling with a neuron marker, or the presence of co-labeling with an oligodendrocyte marker. Loss of oligodendrocytes can be assessed using markers of mature oligodendrocytes, including antibodies directed against 2′, 3′cyclic nucleotide 3′ phosphodiesterase (CNPase) (Sprinkle et al. 1983) and adenomatous polyposis coli (APC) protein (Bhat et al. 1996). For a comprehensive review of oligodendrocyte markers used during development, please see (Baumann and Pham-Dinh 2001).
3 A Primer on CNS Inflammation After Ischemia
3.1 Overview
The brain is highly vascularized, and when healthy, is protected by the blood–brain barrier (BBB) from cells and molecules of the circulatory system (reviewed in (Engelhardt and Sorokin 2009)). This isolation from blood and lymphatic systems contributed to the long-standing notion that the CNS is immune-privileged (Streilein 1993). However, tissues that are at high risk of infection generally possess resident macrophages (e.g., Kupffer cells in the liver, “dust cells” in the lung) that are positioned to rapidly respond, and to help recruit blood-borne immune cells into the injured tissue. The CNS is no exception: it possesses microglia, resident macrophage-like cells that rapidly respond to a wide variety of insults, and with a myriad of outcomes (discussed below). After a stroke, the BBB integrity is compromised and CNS inflammation then involves “activation” and extravasation of blood-borne innate immune cells (neutrophils, monocytes). The innate immune system can respond rapidly because, unlike the adaptive immune system mediated by T and B lymphocytes, it does not require antigen recognition, processing, cell priming, and proliferation. Thus, it is expected that within minutes of arriving at the damage site, resident microglia and infiltrating innate immune cells (neutrophils, macrophages) can begin to secrete inflammatory mediators. From in vitro work, we (Kaushal et al. 2007; Kaushal and Schlichter 2008; Sivagnanam et al. 2010) and many others (Colton and Gilbert 1987; Mao et al. 2007; Piani et al. 1991; Smith et al. 1998) have shown that activated microglia and macrophages can produce pro-inflammatory molecules, excitatory amino acids, lipases, proteases, and reactive oxygen and nitrogen species.
When considering acute inflammation after stroke, the damage-induced (“danger”) response is generally more relevant than a pathogen-induced (“stranger”) response. However, stroke often occurs in an inflammatory environment (Jin et al. 2010; Chapman et al. 2009; Denes et al. 2010; Drake et al. 2011; McColl et al. 2009; Whiteley et al. 2009), with comorbidity arising from bacterial infection, atherosclerosis, hypertension, diabetes, or obesity (Drake et al. 2011; Fischer et al. 2006).
Inflammation in peripheral tissue or within the brain is thought to be an important determinant of stroke outcome (Kleinig and Vink 2009). In rodent models of transient ischemia, a wave of inflammation occurs within the brain during the first week: microglial activation is seen early, followed by infiltration of blood-borne immune cells (macrophages, neutrophils) (Moxon-Emre and Schlichter 2010; Stevens et al. 2002). Infiltration of blood-borne immune cells is mediated by their interactions with endothelial cells through receptors that include the lymphocyte adhesion receptor α4 integrin; and significantly, blocking this interaction reduced the infarct volume and improved the neurological outcome after transient MCAo (Becker et al. 2001; Relton et al. 2001).
Animal models are widely used to study inflammation after transient ischemia; for detailed reviews, see (Jin et al. 2010; Ceulemans et al. 2010; Jordan et al. 2008; Wang et al. 2007). Often called a “double-edged sword,” there is strong evidence that inflammation can both contribute to secondary damage and to post-stroke recovery. A simplistic view has been that early inflammatory responses are directed toward destroying damaged cells, and later responses help resolve the pro-inflammatory state, promoting tissue recovery and repair. There are many recent reviews on microglia (Kettenmann et al. 2011; Luo and Chen 2010; Saijo and Glass 2011) and macrophages (Van Dyken and Locksley 2013; Wynn et al. 2013) summarizing that these cells can function as antigen-presenting cells, phagocytose damaged cells and debris, and produce a plethora of cytokines, chemokines, proteases, and growth factors that affect themselves and other cells. Here, we will not catalogue individual inflammatory molecules and cell functions. Instead, we will briefly present methods for monitoring the most relevant inflammatory cells, and then present an overview of findings on inflammation in rodent models of transient focal ischemia.
3.2 Methods to Assess Inflammation in Ischemia Models
3.2.1 Monitoring Neutrophils
After transient ischemia, neutrophils have been identified using routine hematoxylin and eosin (H&E) staining, by recognizing cells with a unique multi-lobed nucleus (Phillips et al. 2000; Williams et al. 2003; Zhao et al. 2009). Limitations are that the staining resolution is relatively low, especially in densely packed tissues, and it is not conducive to double- and triple labeling. The extent of neutrophil infiltration after ischemia (and other types of injury) is most commonly monitored by biochemical detection of myeloperoxidase (MPO) activity, which is high in activated neutrophils (Barone et al. 1991; Batteur-Parmentier et al. 2000; Beray-Berthat et al. 2003; Bradley et al. 1982; Lerouet et al. 2002). A major limitation of this indirect detection is its inability to reveal spatial and cell-specific MPO expression. This problem can be overcome by exploiting anti-MPO antibodies, as has been done by us and numerous others in animal models of transient ischemia (Moxon-Emre and Schlichter 2010; Justicia et al. 2003; Matsuo et al. 1994). Immunodetection is more sensitive than the biochemical assay (Zhang and Chopp 1997) and can be paired with other cell-specific antibodies to identify the cellular source (Weston et al. 2007). This is important because MPO can also be expressed by activated macrophages and microglia, as shown after transient MCAo (Zhang and Chopp 1997). MPO levels increase when microglia and macrophages become phagocytic, and they can also phagocytose neutrophils that contain MPO (Weston et al. 2007). In mice, neutrophils have also been labeled in situ by an antibody against the Ly6G antigen, which is commonly used in fluorescence-activated cell sorting (FACS) analysis (Gelderblom et al. 2009). Two papers used antibodies against unknown neutrophil antigens: HB199 (Hughes et al. 2003) and MBS-1, with antigen retrieval (Souza-Rodrigues et al. 2008).
3.2.2 Monitoring Microglia and Macrophages
In the healthy adult brain, resting microglia can be readily distinguished from other cell types by their tiny cell bodies and highly ramified processes, and by immunohistochemical staining (reviewed in (Kettenmann et al. 2011)). There are several markers that are widely used to detect microglia: the “integrin alpha M” subunit (ITGAM), which is also known as CD11b, complement component receptor 3 alpha (CR3A), and macrophage-1 alpha antigen (Mac-1A) (Akiyama and McGeer 1990; Robinson et al. 1986); “ionized calcium binding adapter molecule 1” (Iba1) (Imai et al. 1996; Ito et al. 1998); and the surface glycoprotein, F4/80 (Perry et al. 1985). ITGAM and F4/80 also label dendritic cells (Whiteland et al. 1995), endogenous macrophage-like cells that are mainly in myelinated fiber tracts (e.g., corpus callosum, striatal axon bundles, fimbria) and at sites of interstitial fluid drainage (i.e., perivascular space, interface between choroid plexus and cerebral spinal fluid) (reviewed in (Colton 2013)). Microglia (and infiltrating macrophages) can also be identified by lectin staining, notably Griffonia simplicifolia B4 isolectin (IB4) and tomato lectin; however, these stains are less specific and also label blood vessels (Acarin et al. 1994; Streit and Kreutzberg 1987). Figure 19.7 illustrates some markers we exploit for labeling resting microglia in the healthy rat brain, and both activated microglia and macrophages after transient ischemia.
After acute brain damage, some of the markers are up-regulated (Isaksson et al. 1999; Ito et al. 2001) but the continuing challenge is to discriminate microglia from blood-derived macrophages in damaged tissue.
Guillemin and Brew (Guillemin and Brew 2004) have reviewed biochemical and morphological similarities and differences between activated microglia and macrophages. The key issues are that microglia respond to injury by retracting their processes and can adopt a rounded morphology that closely resembles perivascular macrophages and infiltrating macrophages, and all three cell types share many markers. Because of the difficulty in distinguishing between these cells in the damaged brain, we prefer using the combined term, “activated microglia/macrophages.” Matters are further complicated because the commonly used marker, CD11b, is also present on neutrophils. After infiltrating the brain following transient ischemia, neutrophils can also label with IB4 (Matsumoto et al. 2007), although staining might also reflect phagocytosis by neutrophils of microglia and/or macrophages. CD11b is part of an integrin complex on leukocytes, whose interaction with adhesion molecules on endothelial cells allows cell extravasation. Consequently, CD11b inhibition has been tested as a means of reducing stroke damage. Intravenous injection of a function-blocking anti-CD11b antibody at the time of reperfusion after MCAo, reduced neutrophil infiltration, infarct volume, and neurological deficits (Chen et al. 1994). This was presumed to result from reduced neutrophil infiltration but the possibility that macrophage infiltration and microglial activation were affected was not addressed. Another antibody often used as a pan-macrophage marker is CD68 (also known as ED1), which was initially thought to label an intracellular antigen (Dijkstra et al. 1985). Later, ED1 was shown to be a lysosomal marker whose increased expression correlates with the amount of phagocytic activity (Damoiseaux et al. 1994). In the acutely damaged rat brain, ED1 labels phagocytic microglia and macrophages (Moxon-Emre and Schlichter 2010, 2011; Wasserman et al. 2008; Hansen et al. 2001) (and see Fig. 19.7). In an attempt to differentiate between microglia and macrophages, an alternative approach has been to use FACS analysis. It is most common to co-label with CD11b and the antigen, CD45 (also known as leukocyte common antigen [LCA]), which is a protein tyrosine phosphatase. Resting microglia are CD11b+CD45low; whereas, infiltrating macrophages are CD11b+CD45high (Ford et al. 1995). One limitation is that CD45 can be up-regulated in activated microglial cells, which then closely resemble invading macrophages (Kettenmann et al. 2011; Sedgwick et al. 1991). Moreover, because all information about spatial localization of the cells is lost, FACS analysis is not useful for addressing the relationship between specific immune cells and white matter damage.
3.2.3 Monitoring Lymphocytes and Other Immune Cells
When examining lymphocytes, it can be useful to first monitor the presence of both activated T and B cells by staining with an antibody directed against CD25 (the IL-2 receptor alpha chain) (Whiteland et al. 1995). More specific markers can be used to distinguish between T and B cells. B cells can be labeled for CD45R/B220 (Whiteland et al. 1995), Ki-B1R antigen (Koch et al. 2008), CD19 or Pax5 (Ward et al. 2006); and the pan-T cell marker, CD3, is very useful for showing their presence in rodent tissues (Ward et al. 2006). All of these markers can be used both for immunohistochemistry on brain sections and for FACS analysis. Immunohistochemistry is of limited use for identifying T cell subtypes and double labeling is usually required. For example, CD4 labels helper T cells, and CD8 labels cytotoxic T cells and NK cells (Whiteland et al. 1995), but in rats, both have been reported to label macrophages and dendritic cells (Gibbings and Befus 2009). To further discriminate T cell subtypes, it is better to use FACS analysis (Liesz et al. 2011).
3.3 Findings on Brain Inflammation in Rodent Models of Ischemia
Here, we will address the intersection of inflammation and ischemia, with emphasis on the major immune cells involved, and animal models using vessel occlusion or vasoconstriction, which are more closely aligned with human ischemic stroke seen in the clinical setting. Microglia, macrophages, and neutrophils are the most abundant types of immune cells found in the ischemic infarct (Gelderblom et al. 2009), and consequently, have been the focus of most experimental stroke studies.
3.3.1 Results on Neutrophils
Circulating blood leukocytes are thought to have a more prominent and damaging role in transient ischemia, which is followed by reperfusion, than in permanent ischemia, in which blood flow is arrested. Reperfusion after transient ischemia increases endothelial cell expression of adhesion molecules that attract circulating neutrophils, and this recruitment can further clog blood vessels (Connolly et al. 1996b; del Zoppo et al. 1991; Hartl et al. 1996; Prestigiacomo et al. 1999). The prevailing view is that neutrophils are the first hematogenous cells to infiltrate the ischemic infarct. For instance, using the ET-1 model of transient ischemia, we (Moxon-Emre and Schlichter 2010) and others (Souza-Rodrigues et al. 2008) observed peak neutrophil levels at 1 day, and they were undetectable by 7 days. However, another study reported a complete absence of neutrophils (Hughes et al. 2003). The reasons for this discrepancy are not clear but might reflect the labeling methods; i.e., different antibodies, occasional use of antigen retrieval (Sect. 19.3.2.1). The idea that neutrophils are harmful after ischemia is long-standing. The extent of ischemic injury correlates with the increase in neutrophil numbers (Weston et al. 2007). Neutrophils express several pro-inflammatory mediators, and although activated neutrophils are short-lived (1–3 days) (Moxon-Emre and Schlichter 2010; Lerouet et al. 2002; Matsuo et al. 1994; Weston et al. 2007), they can contribute to the early rise in cytokines, reactive oxygen species, and matrix metallopeptidases (MMPs) that can exacerbate BBB breakdown and tissue damage (Justicia et al. 2003; Hartl et al. 1996; Nguyen et al. 2007).
The most compelling evidence comes from studies that have depleted the pool of circulating neutrophils or inhibited their extravasation (reviewed in (Hartl et al. 1996)). Antibody-mediated neutrophil depletion has been exploited in several studies of cerebral ischemia (Matsuo et al. 1994; Gautier et al. 2009; Harris et al. 2005; Petrault et al. 2005). We used this method in a study of ICH in the rat striatum, and showed how blood neutrophil depletion affects their density in the lesion (Moxon-Emre and Schlichter 2011). Several studies implicate neutrophils in BBB breakdown, edema, and infarct volume (Matsuo et al. 1994; Gautier et al. 2009) but others reported that neutrophil depletion did not affect the infarct size (Beray-Berthat et al. 2003; Yilmaz et al. 2006). One possible explanation is that the contribution of neutrophils to ischemic damage might be region dependent. After transient MCAo, MPO activity was elevated for up to 3 days in the cortex and striatum of adult rats (Weston et al. 2007). Depleting neutrophils with vinblastine reduced MPO activity in the cortex and striatum, but oxidative stress and infarct volume decreased only in the cortex (Beray-Berthat et al. 2003). This is consistent with neutrophils being more abundant and long-lasting (up to 15 days post-ischemia) in the cortex than in the striatum (Weston et al. 2007). However, while increased MPO activity reflected accumulation of neutrophils, the sustained elevation at later times reflected neutrophil phagocytosis by microglia and macrophages (Weston et al. 2007).
In considering neutrophils as a potential target for reducing stroke damage, it is important to note their interactions with capillary endothelial cells, which regulate the BBB and control neutrophil infiltration (reviewed in (Tonnesen 1989)). Endothelial cells are more resistant to ischemic insults than neurons but are still vulnerable, and their damage can contribute to BBB breakdown and secondary injury (Won et al. 2011). A salient in vitro study that exposed bovine endothelial cells to OGD showed that they express inducible nitric oxide synthase (NOS-2) and produce nitric oxide (NO), which contributes to their OGD-induced apoptosis (Xu et al. 2000). However, not all sources of NO are detrimental. There is evidence that toxicity depends on the cellular source, type of NO synthase used (e.g., inducible versus constitutive), and timing. Some studies suggest that NO production very early after transient ischemia is beneficial. That is, infarct volume and neutrophil infiltration increased if the NOS inhibitor, L-NAME (NG-nitro-l-arginine methyl ester), was injected intraperitoneally immediately (but not 1 h) after the onset of ischemia (Batteur-Parmentier et al. 2000). That study suggested that high NO might limit neutrophil entry. Transgenic mice lacking constitutive endothelial NOS had larger infarcts after focal ischemia (Huang et al. 1996). A recent study has challenged the accepted view that neutrophils infiltrate the brain parenchyma after transient MCAo. Neutrophils did accumulate but remained in the capillary lumen or perivascular space in mice and in samples from human stroke patients (Enzmann et al. 2013). These studies have contributed to an ongoing debate concerning whether the contribution of neutrophils to stroke pathology has been overestimated (Kalimo et al. 2013).
3.3.2 Results on Microglia and Macrophages
A burgeoning area of experimental stroke research (reviewed in (Weinstein et al. 2010)) is the roles of macrophage-related innate immune cells: microglia, macrophages, and dendritic cells. Their roles are widely debated. A serious confounding factor is that most studies have failed to discriminate between activated microglia and macrophages (Sect. 19.3.2.2). Both cell types have the capacity to produce molecules and perform functions that can potentially either exacerbate damage or aid in repair. In vitro studies show that purified populations of microglia can produce pro-inflammatory cytokines (e.g., tumor necrosis factor (TNF)-α, interleukin (IL)-1β), and reactive oxygen and nitrogen species that can be cytotoxic (Wang et al. 2007; Hanisch and Kettenmann 2007). Conversely, microglia can produce anti-inflammatory cytokines (e.g., IL-10, TGFβ) that dampen the inflammatory response, and growth factors and neuroprotective molecules that can promote neuron survival and repair (Turrin and Rivest 2006; Wang and Dore 2007). In vivo studies are just beginning to discriminate their roles using selective monocyte depletion, genetic labels, and chimeric or parabiotic animals.
As CNS-resident cells, microglia have the potential to respond rapidly to ischemic events, including the initial insult to neurons, and the timing of events has sometimes been used to implicate microglia. After transient MCAo, one study concluded that microglia progress to the phagocytic state before macrophages enter (Schilling et al. 2005). As noted (Sect. 19.3.2.2), ED1 is up-regulated in phagocytic microglia and macrophages. Using the ET-1 injection model in rats, one study saw accumulation of ED1-labeled cells at 1 day, with maximal accumulation at 3 and 7 days (Souza-Rodrigues et al. 2008), while we (Moxon-Emre and Schlichter 2010) and others (Hughes et al. 2003) did not see them at 1 day. The timing of macrophage entry after stroke is uncertain, possibly reflecting different stroke models, but certainly because of identification issues. After transient MCAo in rats, round, Iba1+ cells were present in the infarct at 12–24 h and interpreted as “may be blood-borne macrophages” (Ito et al. 2001). However, there was no proof of their identity. A similar study claiming monocyte infiltration as early as 1 day used H&E staining and showed cells accumulating in the lumen of blood vessels (Clark et al. 1994). The timing of extravasation was not determined and the authors stated that macrophages were abundant in the infarct by 3 days. A better approach is to systemically inject super-paramagnetic iron oxide nanoparticles, which are endocytosed by blood-borne monocytes and can be detected by MRI in the brain. Using this method after cortical photo-thrombotic stroke in rats, blood-derived macrophages were detected in the ischemic infarct only after 5–8 days (Kleinschnitz et al. 2003). Based on their late entry, the authors postulate that after stroke, macrophages are involved in remodeling functions rather than acute responses.
Another major issue in considering potential roles of activated microglia and macrophages is defining what is meant by “activation.” For microglia it is essential to move beyond conventional descriptions of morphological changes, and instead, assess their biological functions. Recent attempts to better define microglial activation have used macrophage activation as a starting point (Luo and Chen 2010; Boche et al. 2013; Colton 2009; Noda and Suzumura 2012). Over the past decade, up to five modes of macrophage activation have been proposed to describe their responses, with each mode depending on the stimulus and affecting different inflammatory mediators and cellular functions (reviewed in (Van Dyken and Locksley 2013; Gordon 2003; Varin and Gordon 2009)). In the absence of microbe infiltration, classical and alternative activation are especially relevant to stroke. While classical activation is evoked by bacterial lipopolysaccharide, it is postulated to occur after exposure to “danger” signals during early stroke events. Classical activation results in secretion of reactive oxygen and nitrogen species and pro-inflammatory mediators. Alternative activation induces anti-inflammatory molecules that antagonize the actions of the pro-inflammatory mediators produced during classical activation. Thus, it is thought to be involved in tissue remodeling and repair. Experimentally, alternative activation can be evoked by IL-4 and IL-13. The analogy between activation of macrophages and microglia is probably too simplistic. Monocytes are blood-borne cells that mature into macrophages in multiple tissues, while microglial cells normally reside behind the BBB. These very different chemical and structural environments will undoubtedly influence the specific responses and contributions of these two cell types to brain pathology.
Because blood-derived macrophages are absent from the healthy brain, it is much easier to analyze functions of “resting” microglia. Several studies have addressed motility, and we now know that the ramified processes of resting microglia are actually very active in sensing the environment. The processes make contact with various neural tissue elements, including neurons, astrocytes, and blood vessels, and engulf tissue particles that are then retrograde-transported to their somata (Nimmerjahn et al. 2005). The ramified processes of microglia monitor synaptic conditions, and their motility is modulated by neuron activity. Live imaging using two-photon microscopy shows that cortical microglia make brief (~5 min) contacts with synapses as often as once an hour, and the frequency decreases during reduced neuron activity (Wake et al. 2009). There is evidence that multiple neurotransmitters affect microglial motility. In an ex vivo retinal explant model, glutamatergic neurotransmission through AMPA and kainate receptors maintained microglial branching complexity and increased process motility indirectly through purinergic signaling (Fontainhas et al. 2011). Ionotropic GABAergic neurotransmission had the opposite effects; it decreased branching complexity and reduced process motility. Changes in motility of microglial processes occur after ischemia. One study addressed this in the peri-infarct region after photo-thrombotic focal ischemia in the mouse somatosensory cortex (Wake et al. 2009). As early as 30 min after ischemia, the duration of contact between microglia and synapses increased, and was often followed by loss of the presynaptic terminal. A recent study found that after 60 min of focal ischemia, there was an increase in microglial branching complexity (hypertrophy) in the ischemic striatum but a decrease in number of contacts per microglia in the cortex (Morrison and Filosa 2013). However, following reperfusion for 8 or 24 h, progressive retraction of microglial processes (de-ramification) occurred in both regions.
Phagocytosis is an important function of microglia and macrophages after stroke; indeed, microglia were once considered the brain’s “garbage men.” The bulk of the evidence is that microglial cells can rapidly transform into active phagocytes, in some cases before macrophages have even begun to enter the brain. One such study depleted peripheral monocytes using clodronate-loaded liposomes, and then subjected the rats to photo-thrombotic focal ischemia (Schroeter et al. 1997). Accumulation of phagocytic cells in the peri-infarct area was mainly microglia at 3 days but both microglia and macrophages at 6 days. A study of transient MCAo in mice used a transgenic, bone-marrow chimera in which blood-borne monocytes were labeled with green fluorescent protein (GFP) (Schilling et al. 2005). Microglial activation, as judged by morphological changes of unlabeled cells, was seen as early as 1 day, was coincident with phagocytosis of neuronal debris, and preceded macrophage infiltration, which began on day 2. By 7 days, massive accumulation of these cells was observed in the infarct, but macrophages accounted for only 20 % of the cells. Using the ET-1 injection model in rats, our laboratory also observed huge numbers of activated microglia/macrophages in the infarct by 7 days, but we could not distinguish between the two cell types (Moxon-Emre and Schlichter 2010). It has been postulated that a protective role of microglia is to phagocytose infiltrating neutrophils, thereby reducing toxic molecules in the extracellular space (Denes et al. 2007; Neumann et al. 2008). However, it is also possible that by releasing inflammatory molecules during phagocytosis, microglia might damage bystander neurons. Given that most acute neuron death (gray matter injury) has already occurred by the time the majority of macrophages infiltrate, the question is: What are macrophages doing? Do they perpetrate delayed white matter damage? Are they mainly involved in repair mechanisms? These questions and others highlight the need to determine, in time and space, the distribution of the two cell types, what molecules they produce, and what specific cellular functions they perform.
3.3.3 Results on Lymphocytes and Other Immune Cells
The peripheral immune system is suppressed after stroke, perhaps as an attempt to offset the inflammatory reactions occurring in the brain, and T lymphocytes are thought to be involved in this process (Planas and Chamorro 2009). However, there is a continuing debate concerning the degree to which lymphocytes enter the brain after stroke and whether they contribute to brain pathology. An early study reported T cell infiltration in the rat cortex as early as 1 day following photo-thrombotic stroke (Jander et al. 1995). FACS analysis and immunohistochemistry have identified both T and B cells in the ischemic hemispheres of mice 3 days after transient MCAo (Stevens et al. 2002; Gelderblom et al. 2009). Some findings suggest that T cells play a more prominent role in the evolving stroke damage, and they have been receiving more attention in experimental stroke research (reviewed in (Brait et al. 2012)). Transgenic mice in which “recombination activating gene 1” (RAG1) is deleted are deficient in both T and B cells, and RAG1-null mice had 70 % smaller ischemic infarcts at 24 h after reperfusion than their wild-type counterparts. If RAG1-null mice were reconstituted with CD3+ T cells, the ischemic infarcts were larger and comparable to wild-type mice; whereas, reconstitution with B cells did not affect the infarct size (Kleinschnitz et al. 2010).
Differences in stroke models, subclasses of T cells examined and gender contribute to controversies about the role of T cells. A transient increase in natural killer T cells (NKT) cells (but not NK cells) has been identified by FACS analysis in the ipsilateral mouse hemisphere 3 days after transient MCAo (Gelderblom et al. 2009) but their role is unknown. As expected, T cells infiltrate better after reperfusion in a transient ischemia model, but surprisingly, the brains of male mice contained more T cells (Brait et al. 2010). On the one hand, there is evidence for a beneficial role of regulatory T cells (Treg) in a permanent MCAo model in mice. Depletion of Treg cells using a CD25 function-blocking antibody increased the infarct size, microglial “activation,” neutrophil invasion, levels of pro-inflammatory cytokines in the brain and blood, and neurological deficits (Liesz et al. 2009). Conversely, a detrimental role was seen in mice after transient MCAo. Selective genetic depletion of Treg cells in DEpletion of REGulatory T cells (DEREG) mice reduced the infarct size and improved neurological outcome scores (Kleinschnitz et al. 2012). Intriguingly, that study found that Treg cells can exacerbate ischemic brain damage by causing dysfunction of the microvasculature, rather than through their typical immunosuppressive functions. Roles of other T cell subsets are beginning to be investigated. After transient MCAo, mice lacking CD4+ or CD8+ T cells had smaller infarct volumes, which correlated with less leukocyte adhesion and recruitment as early as 4 h after reperfusion (Yilmaz et al. 2006). Given that an adaptive immune response generally takes days to develop, this rapid effect is surprising and the mechanism is unknown. Related studies of T cell roles after ischemia in other organs, such as liver (Zwacka et al. 1997) and kidney (Yokota et al. 2002) further demonstrate their complexity, and highlight the need to clarify their roles in cerebral ischemia. We lack studies of the contributions of T cells to white matter injury after stroke; however, future investigations can be informed by studies that associate specific T cell subsets with white matter damage in multiple sclerosis (Scheikl et al. 2010; Walker et al. 2011).
4 Intersection of Inflammation and White Matter Damage After Transient Ischemia
4.1 Adult Rodents
The preceding section addressed the intersection of inflammation and transient ischemia (see Venn diagram in Fig. 19.2), focusing on the immune cells involved. Here, we add the third component: white matter damage. Much of the limited information about effects of inflammation on white matter injury after ischemia is based on the correlation of microglia and macrophage accumulation in regions of white matter damage.
As one of surprisingly few groups that address this three-way intersection, we have exploited the transient focal ischemia model induced by a single 400 pmol ET-1 injection into the anterior striatum (putamen + caudate) of adult Sprague–Dawley rats. In our first study, having determined that saline injection alone caused minimal damage at each time point, we quantitatively compared changes in the core and edge of the infarct with the undamaged contralateral striatum (Moxon-Emre and Schlichter 2010). We showed that neutrophils (strongly immunoreactive for MPO) were present in the ischemic infarct at 1 day following the insult, and were no longer detected by 7 days. When present, neutrophils were inside and around MBP-labeled myelinated white matter tracts. As previously discussed (Sect. 19.3.2.2), after microglia had rounded-up we could not readily distinguish them from macrophages, and therefore used the collective term: activated microglia/macrophages. [See Fig. 19.7 for examples of staining for CD11b, Iba1, ED1.] As shown in Fig. 19.8, by 3 days after ischemia, Iba1-labeled activated microglia/macrophages began to infiltrate MBP-labeled white matter tracts in the infarct. By 7 days, there was a massive infiltration of Iba1-labeled cells into white matter tracts that were damaged, as judged by loss of MBP signal. By co-immunolabeling adjacent serial sections for MBP and dMBP, we were further able to show that the infiltrated bundles were damaged. A similar study of transient ischemia injected a much smaller dose of ET-1 (10 pmol) into the striatum of adult Wistar rats (Souza-Rodrigues et al. 2008), and did not include quantitative analysis. Qualitative similarities include progressive loss of MBP staining in striatal axon bundles that was most prominent by 7 days; infiltration by 1 day of neutrophils (labeled with MBS-1); and later accumulation, at 3 and 7 days, of ED1-positive cells in the ischemic infarct. However, we must be cautious in comparing the results because that study did not show the infarct, report its volume, or show the position of the sample site. It also did not compare the locations of neutrophils or microglia/macrophages in the infarct, or their spatial relation to the damaged white matter.
We know very little about the specific activation state of the microglia/macrophages or their contribution to the evolving white matter injury. However, in the two studies just described, their increased expression of the lysosomal marker, ED1 (see Fig. 19.7), suggests that they are actively phagocytic; perhaps removing myelin debris. Both microglia and macrophages can phagocytose myelin in vitro (Smith 1993; Trotter et al. 1986). Myelin degradation products have been found in vivo within lesion-associated cells in the corpus callosum of cuprizone-fed mice (Olah et al. 2012). The authors concluded that these were microglia because this model of demyelination and re-myelination apparently has minimal involvement of peripheral immune cells.
More information comes from models of neonatal hypoxia–ischemia (Sect. 19.2.2.3) and adult chronic ischemia. In humans, chronic hypo-perfusion resulting from blocked vessels or impaired vascular function is thought to underlie vascular dementia (Roman et al. 2002), and is associated with neurodegeneration, impaired cognitive processes and psychiatric disorders (reviewed in (Farkas et al. 2007)). The main animal model of chronic hypo-perfusion uses bilateral common carotid artery occlusion (BCCAo) in adult rats, which results in memory impairment (Ohta et al. 1997). Two earlier studies used this model to correlate inflammation with white matter damage, as judged by LFB (Wakita et al. 1994) or by ultra-structural changes, including large vacuoles in swollen axons, and myelin sheaths that were irregular and loosely wrapped (Farkas et al. 2004). In the latter study, there was a prolonged (13 weeks) accumulation of CD11b+ cells in the corpus callosum, internal capsule and, most notably, in the optic tract (Farkas et al. 2004). The white matter damage correlated with accumulation of CD11b+ microglia (macrophages?), often in close proximity to damaged fibers (Farkas et al. 2004), and with infiltration of CD4+ and CD8+ lymphocytes (Wakita et al. 1994).
Accumulation of major histocompatibility complex (MHC) class I-labeled cells began as early as 1 day, was much more prominent in white matter than gray matter, and preceded the appearance of white matter lesions (Wakita et al. 1994). These cells were called “microglia” at the earlier time points (1–3 days). At 1 day, the white matter infiltrating cells had shortened processes, hypertrophic somata, and increased staining for MHC class I (Wakita et al. 1994). By 3 days, the bundle-infiltrating cells began to express MHC class II (Ia) antigen and LCA (CD45). Their numbers increased with time to a peak at 7–14 days, at which time they were round, looked like foamy macrophages, and from this time on, the authors called them “microglia/macrophages.” In a recent study that did not directly correlate inflammation with white matter damage, increased numbers of MHC class II-labeled microglia (macrophages?) were detected at 13 weeks after BCCAo in the hippocampal fimbria of rats exhibiting spatial memory impairments (Choi et al. 2011).
Several studies have used drugs to target inflammation following BCCAo. Rats that received intraperitoneal injections of the immunosuppressant, cyclosporin A, had less white matter damage, as judged by LFB and Bielschowsky silver stain (Wakita et al. 1995). The white matter tracts also contained fewer “microglia/macrophages” that were immunostained for LCA, MHC class I or II antigens. A very similar study by the same group used the immunosuppressant, FK506, and found similar results; i.e., less white matter damage and fewer bundle-infiltrating microglia/macrophages (Wakita et al. 1998). A third BCCAo study tested a 2 week treatment with the anti-inflammatory compound, minocycline (Cho et al. 2006). They found reduced white matter injury (LFB, Bielschowsky silver, MBP staining) in the corpus callosum and optic tract, and reduced microglia (and macrophage?) activation, as measured by the CD11b+ area in the corpus callosum. Similarly, after MCAo in adult mice, axon damage and oligodendrocyte death were reduced by melatonin, which is considered to act an anti-inflammatory agent (Lee et al. 2005).
4.2 Neonatal Rodents
Although there are few investigations of the specific intersection between ischemia, inflammation, and white matter damage in neonatal animals, there are more publications than for adult animals. Neonatal stroke studies almost entirely exploit the HI model in rodents, which causes damage to both white and gray matter (Calvert and Zhang 2005). White matter damage is often assessed as the degree of myelin loss, axonal damage, and oligodendrocyte death (Carty et al. 2008; Villapol et al. 2011; Biran et al. 2006; Deng et al. 2008; Uehara et al. 1999; Wang et al. 2013). Subcortical white matter damage correlates with decreased numbers of immature (Carty et al. 2008; Wang et al. 2013) and mature oligodendrocytes (Carty et al. 2008; Villapol et al. 2011). Several HI studies have monitored inflammation concomitantly with white matter injury and have shown an increase in numbers of microglia/macrophages in white matter tracts. For instance, after HI in neonatal rats, white matter injury was accompanied by a 2–3 fold increase in the number of microglia (macrophages?) (IB4 or CD11b labeled), which were assumed to be “activated” (Biran et al. 2006). However, their specific activation states have not been defined and, for the reasons addressed in Sect. 19.3.3.2, it is not known whether these two immune cells play similar or different roles.
It is well known from in vitro studies from our lab (Kaushal et al. 2007; Kaushal and Schlichter 2008; Sivagnanam et al. 2010; Fordyce et al. 2005; Khanna et al. 2001; Schlichter et al. 2010) and others (Colton and Gilbert 1987; Mao et al. 2007; Piani et al. 1991; Smith et al. 1998; Lai and Todd 2008; Rock et al. 2004) that activated neonatal microglia can produce neurotoxic molecules. Less is known about their products and roles in white matter injury in vivo. Several studies of neonatal HI have directly addressed correlations between inflammatory cell numbers and white matter damage. Evidence that these cells directly contribute to white matter damage is the phagocytosis of immature oligodendrocytes in damaged white matter, as judged by colocalization of the microglia/macrophage marker, Iba1, and the immature oligodendrocyte marker, O1 (Biran et al. 2006). This is expected to hamper recovery and remyelination. In the corpus callosum of rat pups, a decrease in the density and activation of microglia (macrophages?) (Iba1 staining) accompanied a decrease in myelin loss (MBP staining intensity) and increase in premyelinating (O4+ cells) and immature oligodendrocytes (O1+ cells) (Carty et al. 2008). More recently, when the density of microglia (macrophages?) (tomato lectin staining) was reduced by melatonin administration, there was a decrease in HI-evoked white matter damage (MBP loss) and an increase in mature oligodendrocytes (APC-labeled cells) (Villapol et al. 2011).
Several studies support the view that inflammation, microglia/macrophage activation, and specific pro-inflammatory molecules contribute to white matter damage after neonatal HI. Some studies have begun to target functions of specific inflammatory mediators. Increased expression of the potentially toxic cytokines, IL-1β, and TNF-α, was seen in the rat corpus callosum after HI (Deng et al. 2008; Wang et al. 2013; Brochu et al. 2011; Carty et al. 2011). Administering the IL-1 receptor antagonist reduced white matter injury in the internal capsule (Girard et al. 2012). IL-1β can be processed to its active form by MMP9 (Schonbeck et al. 1998) and, after HI in MMP9-null mice, there were fewer activated microglia (macrophages?) (IB4 staining) in the damaged white matter, which was judged by loss of MBP (Svedin et al. 2007). MMPs are regulated by several “tissue inhibitors of metallopeptidases” (TIMPs), and there is evidence from knockout mice that TIMP-3 contributes to TNF-α-dependent death of immature oligodendrocytes after MCAo in the adult (Yang et al. 2011). Cyclooxygenase-2 (COX-2) is an interesting target because it is inhibited by nonsteroidal anti-inflammatory drugs (such as aspirin and ibuprofen), and it increases after ischemic stroke in humans, rodents, and nonhuman primates (reviewed in (Candelario-Jalil and Fiebich 2008)). In rats, COX-2 was found in activated microglia (macrophages?) (Bauer et al. 1997), and the nonsteroidal anti-inflammatory drug, ibuprofen, inhibited COX-2 induction after HI (Carty et al. 2011). In mice, the pro-inflammatory cytokine, IL-18, was markedly increased in microglia and astrocytes after HI, and IL-18-null mice had less subcortical white matter damage (Hedtjarn et al. 2002, 2005). Several anti-inflammatory drugs reduced white matter damage in rodent HI models. Ibuprofen reduced IL-1β and TNF-α, and increased the amount of intact myelin (MBP stained) and immature (O1+) and mature oligodendrocytes (O4+) (Carty et al. 2011). White matter damage (loss of MBP) was also reduced by minocycline (Carty et al. 2008) and melatonin (Villapol et al. 2011).
5 Future Studies Needed
In 2010, we published our first paper on inflammation and white matter damage after focal ischemia in rat (Moxon-Emre and Schlichter 2010). At that time we stated that: “Despite substantial progress in understanding the pathogenesis of neuronal injury after stroke, most preclinical studies have failed to consider damage to the white matter. Only recently have stroke studies begun to focus on the secondary injury phase and prominent inflammatory response, which is delayed, prolonged, and more amenable to treatment than acute neurotoxicity.” White matter is increasingly recognized as a vulnerable region following ischemia (reviewed in (Petty and Wettstein 1999)); thus, we were surprised how little was known about the spatial and temporal progression of white matter damage. As described in Sect. 19.4.1, only two studies had addressed inflammation and white matter damage after transient ischemia in adult rodents (Hughes et al. 2003; Souza-Rodrigues et al. 2008), and they came to different conclusions about the infiltration of neutrophils and microglia/macrophages into the ischemic infarct. Thus, we set out to quantitatively analyze the temporal and spatial coevolution of white matter damage and inflammation using ET-1 injection to produce a transient, focal ischemic stroke in the rat striatum (Moxon-Emre and Schlichter 2010). ED1-labeled microglia/macrophages selectively infiltrated damaged white matter tracts in the rat striatum as early as 3 days after focal ischemia, but remained outside undamaged white matter tracts. As the Venn diagram in Fig. 19.2 illustrates, we found no additional publications addressing the intersection of inflammation and white matter damage after transient ischemia in adult rodents. This dearth of experimental animal research means there are many important aspects to address in future. Here, we will briefly discuss a few that are especially relevant to the material in this chapter.
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1.
While the ET-1 model of ischemia has shown that microglia/macrophages infiltrate damaged white matter tracts, we do not know their specific activation state or what functions they are carrying out (Sect. 19.3.2.2). We do not know if, or how, this infiltration affects neurotransmission, neuron survival, repair, or ultimate behavioral outcomes. We know little, if anything, about whether other inflammatory cells (e.g., lymphocytes, dendritic cells) contribute to white matter damage after transient ischemia (Sect. 19.3.2.3). We know almost nothing about how the inflammatory response affects white matter damage in aged or hypertensive animals, which are better models of most human strokes than using young, healthy animals.
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2.
Very few studies have quantified specific responses in transient ischemic stroke models. We need more detailed information on position- and time-dependent changes in the staining intensity or area of damaged white matter, whether it is myelin or axon damage, the density or numbers of specific immune cells, inflammatory molecules they are producing, and how these responses are changed by treatments.
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3.
As addressed throughout this chapter (e.g., Sect. 19.3.2), a major challenge is distinguishing activated microglia from infiltrating macrophages. Over the years, several experimental manipulations have been used in an attempt to distinguish their contributions. Several studies have ablated circulating monocytes using clodronate-loaded liposomes (Schroeter et al. 1997; Kanematsu et al. 2011; Mawhinney et al. 2012) or by bone marrow irradiation (Schilling et al. 2005). The recent development of knock-in fluorescent protein reporter mice for the fractalkine receptor (CX3CR1+/GFP) and chemokine receptor 2 (CCR2+/RFP) promises to help differentiate endogenous microglia from invading macrophages (Mizutani et al. 2012).
-
4.
Recent insights into the ontogeny of microglia show that parenchymal CNS microglial cells develop earlier than previously thought, and from a surprising location: the embryonic yolk sac (Ginhoux et al. 2010). This site of origin differs from bone-marrow derived macrophages. A better understanding of their development and possible differential gene expression might provide insight into how to distinguish between activated microglia and infiltrating macrophages. There is some controversy about the potential of peripheral macrophages to replenish microglia after CNS injury. In transgenic mice engineered to allow ganciclovir-mediated depletion of proliferating microglia (CD11b-HSVTK transgenic mice), circulating Iba1+ macrophages entered the brain, responded to ATP gradients and migrated towards sites of kainate-induced neuron death (Varvel et al. 2012). Unlike native resting microglia, which are highly ramified and have small somata, the infiltrating macrophages had large somata and short, irregular processes. This suggests that infiltrating macrophages remain as a distinct population. In future, identifying molecular expression profiles underlying the unique morphological and developmental differences might be useful in distinguishing microglia from macrophages.
-
5.
It has been postulated that white matter is particularly vulnerable to inflammatory mediators (Coleman and Perry 2002). This means that inflammation after stroke might damage white matter at times and in locations where frank loss of neurons is not seen. Our discovery (Sect. 19.2.3.2) that SC1/hevin is a new early marker of axon damage might prove very useful. Its spatiotemporal expression correlated with microglia/macrophage infiltration of white matter bundles, and it showed aging-related differences in the progression of white matter damage (Lively and Schlichter 2012).
-
6.
In neonatal HI models, attempts have been made to more closely evaluate the intersection of ischemia, white matter damage, and inflammation (Sect. 19.4.2). Most studies have been correlational, showing that white matter damage in a lesioned area was accompanied by an increase in microglia/macrophage numbers. While several studies used broad-spectrum anti-inflammatory drugs (minocycline, ibuprofen, melatonin), further research is needed to address the mechanisms. As for adult animals, an over-arching need is to parse out specific aspects of the inflammatory response, and determine whether they exacerbate the damage, aid in repair, or both.
Abbreviations
- AchAo:
-
Anterior choroidal artery occlusion
- AMPA:
-
2-Amino-3-(3-hydroxy-5-methyl-isoxazol-4-yl)propanoic acid
- APC:
-
Adenomatous polyposis coli
- APP:
-
Amyloid precursor protein
- ATP:
-
Adenosine triphosphate
- BBB:
-
Blood–brain barrier
- BCCAo:
-
Bilateral common carotid artery occlusion
- CBF:
-
Cerebral blood flow
- CNS:
-
Central nervous system
- COX-2:
-
Cyclooxygenase-2
- CR3A:
-
Complement component receptor 3 alpha
- dMBP:
-
Degraded myelin basic protein
- eNOS:
-
Endothelial nitric oxide synthase
- ET-1:
-
Endothelin-1
- FACS:
-
Fluorescence-activated cell sorting
- GABA:
-
Gamma-aminobutyric acid
- GFP:
-
Green fluorescent protein
- H&E:
-
Hematoxylin and eosin
- HI:
-
Hypoxia–ischemia
- IB4 :
-
Isolectin B4
- Iba1:
-
Ionized calcium binding adapter molecule 1
- ICA:
-
Internal carotid artery
- ICH:
-
Intracerebral hemorrhage
- IL:
-
Interleukin
- ITGAM:
-
Integrin alpha M
- LCA:
-
Leukocyte common antigen
- LFB:
-
Luxol fast blue
- Mac-1:
-
Macrophage-1 alpha antigen
- MBP:
-
Myelin basic protein
- MCAo:
-
Middle cerebral artery occlusion
- MHC:
-
Major histocompatibility complex
- MMP:
-
Matrix metallopeptidase
- MPO:
-
Myeloperoxidase
- MRI:
-
Magnetic resonance imaging
- NKT:
-
Natural killer T cells
- NO:
-
Nitric oxide
- NOS:
-
Nitric oxide synthase
- OGD:
-
Oxygen-glucose deprivation
- RAG1:
-
Recombination activating gene 1
- TGFβ:
-
Transforming growth factor beta
- TIMP:
-
Tissue inhibitor of metallopeptidase
- TNF-α:
-
Tumor necrosis factor alpha
- tPA:
-
Tissue plasminogen activator
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Schlichter, L.C., Hutchings, S., Lively, S. (2014). Inflammation and White Matter Injury in Animal Models of Ischemic Stroke. In: Baltan, S., Carmichael, S., Matute, C., Xi, G., Zhang, J. (eds) White Matter Injury in Stroke and CNS Disease. Springer Series in Translational Stroke Research, vol 4. Springer, New York, NY. https://doi.org/10.1007/978-1-4614-9123-1_19
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