Overview

Idiopathic intracranial hypertension (IIH) is a neurological disorder characterised by papilloedema, in the absence of an identifiable secondary cause on neuroimaging (including venous sinus thrombosis); with an elevated lumbar puncture opening pressure and normal cerebrospinal fluid (CSF) constituents [1]. IIH typically affects obese women between the ages of 15 and 45 [2].

Headache is the commonest reported symptom which for the majority has a migrainous phenotype which significantly impacts on quality of life [3, 4]. Other commonly reported symptoms include visual manifestations such as transient visual obscurations in 68% of cases [5, 6], diplopia as a result of cranial nerve VI palsy [7], pulsatile tinnitus, dizziness, and back and neck pain [2]. A cardinal feature of IIH is the presence of papilloedema (swelling of the optic disc secondary to raised ICP) [8]. The pathophysiological basis for the appearance of papilloedema is thought to be secondary to axoplasmic stasis resulting from impaired transport due to raised intracranial pressure (ICP) [9]. Papilloedema can lead to visual loss which can necessitate emergency surgical intervention [10] and is reported to cause visual loss in up to 25% of cases [11, 12].

Clinical approaches to management are variable internationally but recently (2018) the first consensus guidelines have outlined a standardised approach to investigation and management of adult IIH [1, 10, 13]. Whilst treatment options are limited in choice and efficacy, there are now an increasing number of randomised clinical trials in this disease area [5, 14,15,16,17].

This review article is based on previously conducted studies identified by searches on the electronic databases of States National Library of Medicine (PubMed), Medline and the Cochrane Library, from listing until 1st April, 2019. The following descriptors were used to include articles for review: IIH; pseudotumour cerebri; pathophysiology; aetiology; intracranial pressure; preclinical models; CSF secretion; animal models. The articles were limited to those in English language. Abstracts were reviewed and relevant full articles were obtained but case reports and letters to the editor were excluded. Only preclinical models were included as clinical models are out of scope and not included in this review. Reference lists from articles were also examined for further citations.

The aim of this review is to inform the readership of the current literature pertaining to pathophysiological mechanisms identified in IIH and how preclinical models are allowing the field to gain mechanistic insights into IIH. Ultimately this may allow identification of targeted therapeutics to be developed.

Epidemiology of IIH

Previously the incidence of IIH was estimated at between 0.5 and 1.0 per 100,000 people [2], however, the incidence has been increasing. The largest cohort study to date of 23,182 new IIH cases reported a 108% increase from 2.26 per 100,000 in 2002 to 4.69 per 100,000 in 2016 [18]. The highest incidence was seen in females aged 25 years and was 15.2 per 100,000. More recently a UK population-based matched cohort study demonstrated a 350% increased incidence over the last decade to an incidence of 9.0 per 100,000 in 2019 [19]. Increased incidence is rising in line with increased obesity rates [18]. Obesity has long been an associated risk factor for typical IIH [2], and incidence of IIH has been noted to reflect country specific obesity rates [20].

IIH has a significant financial impact. IIH costs were estimated at $444 (£345.5) million in the United States in 2011 [21]. Recently health economic evaluation of UK hospital costs incurred from IIH were reported to rise from £9.2 ($12.3) million in 2002 to £49.9 ($64.0) million in 2014, and projected costs to UK hospital services at £462.7 ($593.6) million by 2030 [18]. Rising costs are predominantly driven by high hospital attendance rates, as well as scanning and procedure rates, as well as indirect costs such as absence from work or reduced work capacity.

There are many unanswered questions in IIH. Patients and professionals have voiced their opinions on the research priorities in IIH through a James Lind Alliance Research priority setting partnership. Identifying the aetiology of IIH was placed as the number one priority [22] (Table 1).

Table 1 Summary of the top ten priorities for IIH research.

The pathophysiology of IIH has been speculated for over a century and many causative factors have been postulated [23,24,25]. There have been a number of key advances over the last decade with a focus on identifying disease specific biomarkers. IIH biomarkers may represent either cause or consequence of the disease and their validity and interpretation is enhanced though understanding their mechanistic role. Preclinical models are a useful tool to enhance our understanding of IIH disease pathophysiology and underpinning mechanisms. The number of preclinical models is growing and their relevance, utility and interpretation requires careful scrutiny.

Here we aim to update the current thinking on IIH pathophysiology and provide a guide to the preclinical models which evaluate CSF secretion, CSF absorption and animal models pertinent to IIH.

Pathophysiology overview

The pathophysiology of IIH has been speculated over time. Due to elevated ICP much of the literature surrounding the disease has focussed on hypersecretion of CSF and/or a reduction of CSF absorption through the arachnoid granulations or the glymphatic system [26]. To understand central nervous system fluid dynamics, a basic understanding of normal anatomy and physiology is important. There are three main barrier sites between the brain and the blood: the blood–brain barrier, the blood–CSF-barrier and the arachnoid epithelium as shown in Fig. 1.

Fig. 1: Schematic diagram of main transport proteins of CSF secretion within choroid plexus epithelia and the putative pathway of CSF secretion and absorption.
figure 1

The diagram shows the CSF and ISF movement between the brain barriers from secretion to absorption of both fluids. Fluid movement is shown by the blue arrows between the BBB (brain capillary endothelium) (1); BCSFB (CP epithelium) (2a) into the brain compartments and absorption through the arachnoid barrier (3) back into the blood. Evagination of the arachnoid membrane into the lumen of the vein and therefore the dural vessel allows the communication between CSF in the SAS and blood. CSF also passes through the SAS to the olfactory bulbs and then drains into nasal lymphatics by passing through the cribriform plate and along channels adjacent to olfactory nerves and into the blood (4). The exchange of fluid between the CSF in the SAS and the ISF in the brain parenchyma allows these fluids to drain into the cervical lymph nodes through the glymphatic pathway (5). The highlighted region (2b) of the diagram depicts the CP with the net transport of Na+, HCO3 , Cl and water, from basolateral (blood) to apical (CSF) membranes, with schematic locations of ion transporters Na+-K+-ATPase, NKCC1, HCO3− and Cl channels are localised to the apical CSF facing membrane. NHE1, NCBE and AE2 transporters are expressed on the basolateral blood facing membrane. AQP-1 water channels are expressed on both sides of the CP epithelium. Blood–brain barrier (BBB), blood cerebrospinal fluid barrier (BCSFB), carbonic anhydrase (CA), choroid plexus (CP), interstitial fluid (ISF), subarachnoid space (SAS).

CSF secretion

Approximately 80% of CSF is produced by the epithelial cells of the choroid plexus, organs that reside in the cerebral ventricles, with 20% being secreted by the ventricular ependymal and the brain tissue itself [27, 28]. The functional unit of the choroid plexus is the choroid plexus villus, which comprises of central fenestrated capillaries surrounded by choroid plexus epithelial cells, where through the formation of tight junctions, the choroid plexus villus constitutes the blood–CSF-barrier and controls CSF composition.

Choroid plexus epithelial cells have critical roles related to directed transport processes from blood into the CSF, removal of substances out of the brain, and for CSF production [27]. The pressure required for the circulation of CSF is maintained by a hydrostatic pressure gradient between the choroid plexus (highest pressure at site of CSF formation) and the arachnoid granulations (lowest pressure at site of CSF absorption) [29].

The total volume of CSF within adult humans is ~140 ml and the rate of secretion by each choroid plexus is 0.2 ml/min [27, 30] or 500 ml per day [31].

Fluid secretion by choroid plexus epithelial cells depends on the unidirectional transport of ions, facilitated by transport proteins that are found in the apical (lumen) and basolateral (blood) membranes of the cells [28] (Fig. 1), generating an osmotic gradient which induces net water movement [32]. Fluid secretion by these cells involves the sodium–potassium ATPase pump (Na+-K+-ATPase), epithelial sodium channel, chloride channel (CIC-2) and aquaporin-1 water channel (AQP-1) located on the apical membrane, driving the efflux of Na+, Cl, K+, HCO3 and H2O into the CSF [27]. Chloride–bicarbonate exchanger (AE2) and sodium–bicarbonate co-transporters (NCBn1, NCBE), are located on the basolateral membrane and drive the accumulation of Na+, Cl and HCO3 into the cytoplasm of the choroid plexus epithelial cells, eventually resulting in CSF secretion [27].

However, conventional osmotic forces may not account for the known production rate of CSF and the molecular mechanisms underlying CSF production remain under investigation [31]. The osmotic processes are being facilitated by AQP-1, and studies have revealed that AQP-1 knockout mice decrease CSF secretion and ICP but do not fully ameliorate CSF secretion [33]. Studies have reported the novel concept of the cotransport of water involving the Na+-K+-2Cl cotransporter (NKCC1), contributing to approximately half of the CSF production [31]. This suggests NKCC1 transporters action upon water and CSF secretion works independently of AQP-1 and explains why AQP-1 knockout does not fully prevent CSF secretion [31, 34].

In vitro—models of CSF secretion

In vitro CSF secretion assays fall into two generic groups; those that directly assess CSF secretion and those that assess surrogates of CSF secretion.

Porcine choroid plexus cultures have been previously (1998) utilised to assess CSF secretion in vitro and has the potential to screen molecules that alter CSF secretion [35]. However, pigs are not standard model organisms. The assay has not been reliably replicated in other centres. Rodent choroid plexus does not provide sufficient material in primary cultures to make such an assay ethically viable, or increase throughput due to the amount of animals that need to be sacrificed.

As such Na+-K+-ATPase activity at the choroid plexus is utilised in vitro as a surrogate of CSF secretion [36,37,38,39], and the physiological rationale behind this is clear. Inhibiting Na+-K+-ATPase inhibits CSF secretion in vivo by up to 80% of baseline, thus Na+-K+-ATPase activity is intrinsically linked to CSF secretion [39]. These assays directly assess ionic movement, and ATPase activity. Importantly, these models are predictive of the in vivo effects of drugs [38, 40]. However, these assays only measure end points and thus are prone to variability. More recently a novel Na+-K+-ATPase activity assay assessed ATPase activity in real-time through live cell imaging, and reduced variability provided data comparable to other assays [41].

As NKCC1 channels have been demonstrated to contribute to CSF secretion [31], assessing the activity of the NKCC1 channel, and other channels proposed to directly transport water, would allow a more complete understanding of how molecules alter CSF secretion [42]. But the impact of each of the myriad of ion channels on overall CSF production is not fully understood.

In vivo models of CSF secretion

The main aim of in vivo models is to measure CSF secretion rates within physiological parameters. However, a number of models have been studied previously and are highlighted in Table 2.

Table 2 In vivo models of CSF secretion.

In summary, CSF secretion rate experiments are interpreted by the classic hypothesis of CSF hydrodynamics [43]. The advantages of these techniques include marker substances such as Dextran can only be diluted by newly formed CSF in the case of the ventriculo-cisternal perfusion technique [43]. The aqueductal method allows for a closed system, which permits the CSF pressure between the ventricular and subarachnoid spaces in a physiological range [44, 45]. However, in most cases the techniques used are not performed under physiological conditions (normal CSF secretion rate: 7 μl/min in cats [45], 2 μl/min in rats [46]), which can limit their interpretation. Also, air and CSF absorption from the CSF has to be prevented [43]. Therefore, a novel method is necessary to determine the physiology and pathophysiology of CSF dynamics.

CSF absorption

There are three main routes of CSF absorption: arachnoid granulations, nasal and dural lymphatics and the glymphatic system [47,48,49,50,51].

CSF absorption by arachnoid granulations

Each choroid plexus secretes CSF into the ventricle in which it is situated. The ependymal epithelium, which lines the ventricles, is in contact with the CSF. The CSF and the interstitial fluid of the brain parenchyma are separated by the perivascular space that surrounds the large blood vessels (Figs. 2 and 3) [49, 52]. There is a constant directional flow of CSF from the cerebral ventricles to the subarachnoid space. The openings of the subarachnoid space into the dural venous system through arachnoid granulations have classically thought to be the primary site of CSF absorption back into the blood [2, 27, 29, 53]. Hydrostatic pressure is maintained in the subarachnoid space allowing the flow of CSF into the dural sinus. As the opening is valvular, the blood cannot cross in the opposite direction [54, 55].

Fig. 2
figure 2

Human choroid plexus H&E stained (×40).

Fig. 3: Adult rat brain and the site of injection into the lateral ventricle for ventriculo-cisternal perfusion and variable rate infusion.
figure 3

a Ventriculo-cisternal perfusion: aCSF (containing blue dextran) was perfused into each lateral ventricle of the rat brain. The solutions were collected every 10 min from the Cisterna magna and the absorbance was read on a spectrophotometer. The increase in dilution of the blue dextran within the aCSF as it passes through each ventricle indicates an increase in CSF secretion over the course of experiment. b Variable rate infusion: aCSF was perfused into one lateral ventricle of the rat brain at increasing perfusion rates. A separate cannula, attached to a pressure transducer, was inserted into the other lateral ventricle and pressure readings were taken every 10 min. The increase in dilution of the blue dextran within the aCSF for each sample indicates an increase in CSF secretion over the course of experiment; therefore as it is a closed system this would lead to an increase in pressure. Artificial cerebrospinal fluid (aCSF).

Although debated, venous sinus stenosis has been reported to be present in over 90% of IIH patients; resulting in compressed venous sinus causing decreased CSF absorption within the arachnoid granulations and increased ICP [56]. Current treatments involve the use of venous sinus stenting using the introduction of flexible stents that navigate the intracranial venous circulation to increase CSF drainage and lower ICP [56, 57]. Venous stenosis has also been reported to be reversed following LP with CSF drainage [58].

CSF absorption by the nasal and dural lymphatic system

A second pathway of CSF absorption occurs through two sites of the lymphatic system: nasal cavity and lymphatic vessels. At least 50% of CSF drains to lymph nodes in rodents and non-human primates [51, 59], and the lymphatic drainage pathways are well developed in humans [59]. In both humans and rodents, resin injection studies have demonstrated that CSF passes through the subarachnoid space to the inferior aspect of the olfactory bulbs and then drains into nasal lymphatics by passing through the cribriform plate and along channels adjacent to olfactory nerves, highlighting the nasal lymphatics as a likely site of CSF drainage [50, 59].

More recently, studies have demonstrated CNS lymphatic vessels in the dura mater [47, 60]. These are in contact with the CSF and facilitate its drainage, where damage to these vessels impairs CSF flow and absorption as evidenced in ageing mammals being associated with an accumulation of toxic amyloid beta protein in the brain parenchyma [60, 61]. In addition, it has been postulated that lymphatic spaces may be present at the optic nerve head in papilloedema [62].

CSF absorption by the glymphatic system

A third route of fluid clearance through paravenous drainage pathways involves the exchange of fluid between the CSF in the subarachnoid space and the interstitial fluid in the brain parenchyma [49]. These glial lymphatics or ‘glymphatics’ facilitate the passive movement of both CSF and interstitial fluid from the cranium to the periphery through a pressure gradient, facilitated by aquaporin-4 on astrocytes [63, 64].

The relative contribution of each of these pathways to normal physiology and in the disease state of IIH is unknown.

In vitro—models of CSF absorption

In vitro assessment of CSF absorption is an under developed area with few dedicated assays available. In vitro and ex vivo CSF absorption showing unidirectional fluid movement from the apical to basolateral aspects has been demonstrated in cadaveric human arachnoid granulation tissue [65, 66]. Such an assay has the potential to screen for molecules that alter CSF absorption at the arachnoid granulations. However, the rarity of human arachnoid granulation tissue for culture and the absence of arachnoid granulations in rodents make such an assay impractical as a routine laboratory technique.

The association of other structures, such as the nasal and dural lymphatics with CSF drainage, presents the possibility to utilise assays to assess fluid transports across a monolayer of lymphatic endothelial cells to provide a surrogate assay for CSF drainage. In addition, the demonstration that the glymphatic system contributes to CSF absorption suggests that assessing in vitro fluid transport in cultured astrocytes could provide a surrogate for glymphatic CSF absorption [49]. The above assays exist and as such should be explored, providing a potential screening mechanism that could complement in vivo assessment of glymphatic CSF drainage [67].

In vivo—models of CSF absorption

Few models of CSF absorption have been studied previously, as described in Table 3, but are essential in determining the mechanism upon which CSF is drained from the brain under physiological parameters (normal CSF pressure: 11.9 cmH2O in cats [68]; 9.5 cmH2O in rats [69]).

Table 3 In vivo models of CSF absorption.

The variable rate infusion technique is useful to study the effects of mediators upon resistances to CSF absorption but is particularly invasive. However, both imaging techniques are less invasive and are useful tools to study CSF lymphatic absorption in order to understand this pathway in CNS disease models [48].

Effects of obesity and gender on CSF dynamics in IIH

Obesity and female gender are known risk factors of IIH [23]. Studies by Newborg were the first to document diet as a treatment for IIH in open label case series [70]. Variable weight loss occurred in following a low calorie and low sodium diet, and resulted in improvement in IIH symptoms and papilloedema [70]. Other studies found a weight loss of 6% in female IIH patients with obesity resulted in recovery of papilloedema and visual field dysfunction in 74% of cases [71]. Re-evaluation after 3 months, following maintenance of a low energy diet with no evidence in weight gain, showed that reduced ICP and papilloedema were maintained [72]. Reducing weight is considered the optimal approach to decrease ICP and modify the underlying disease in IIH [1, 2, 72].

Obesity and female gender have also been suggested to impair CSF absorption pathways [26, 73]. Some studies have noted reduced CSF absorption in those with IIH [73]. Other studies used isotope methods which evaluated CSF circulation and absorption, and cisternographic findings to show an increased arachnoid resistance to CSF efflux might be present in those with IIH [74].

Further studies suggested thrombosis in the arachnoid granulations, increased thrombotic gene expression, and increased resistance to CSF absorption through inflammation of the arachnoid granulations in female IIH patients is potentially aggravated by thrombophilic exogenous oestrogens [75]. The risk factor of prothrombotic effects may be hypothesised to cause increased resistance to CSF absorption and consequently elevated ICP but this has not been substantiated.

Hormones and IIH

Retinoids (vitamin A), steroid hormones such as corticosteroids and sex steroids have all been hypothesised to alter CSF dynamics [26].

Retinoids

Studies have described the intake of large quantities of vitamin A causing secondary intracranial hypertension symptoms [76,77,78] and vitamin A pharmacological therapies have been associated with elevated CSF pressure in adults [79]. Indeed IIH patients have been identified to have altered retinoid metabolism by several studies [80, 81]. However, a definitive evaluation conducted using samples from the Idiopathic Intracranial Hypertension Treatment Trial, which was noted for its accurate quantitative assessment of vitamin A metabolites, demonstrated that although IIH patients have mild abnormalities in retinoid metabolism, these abnormalities were not altered following resolution of symptoms suggesting that vitamin A toxicity is unlikely to contribute to the aetiology of IIH [78].

Glucocorticoids

Glucocorticoids (GCs) are pleotropic steroid hormones where cortisol is the major physiologically active GC in humans. It has previously been demonstrated that, following weight loss in IIH patients, reductions in the global capacity to activate GCs through reduction in 11β-hydroxysteroid dehydrogenase type 1 (11β-HSD1), is associated with reduced ICP [82]. This coupled with the expression of 11β-HSD1, the enzyme that gates tissue level activation of GCs, at choroid plexus epithelial cells, suggests that GCs could modulate ICP [83]. Indeed, elevated levels of cortisol in the choroid plexus epithelium driven by 11β-HSD1 drives apical Na+ channels to increase movement of Na+ and therefore water molecules into the CSF, thereby driving CSF secretion and ICP [82, 84].

Of interest, in an embryologically related tissue, the ocular ciliary body, where the mechanisms of fluid secretion (aqueous humour) is analogous to that of CSF secretion at the choroid plexus, demonstrated inhibition of 11β-HSD1 [84, 85]. Of note, activity of 11β-HSD1 in patients with IIH correlates significantly with ICP changes. However, there are a lack of human studies evaluating the systemic and central nervous system GC phenotype in IIH patients compared with matched controls.

Leptin

Leptin is an adipokine that circulates in serum at levels proportionate to body fat and modulates appetite and energy balance [86, 87]. Leptin is a product of the Obese (Ob) gene and when absent, results in profound obesity in rodents and humans [88, 89]. Leptin elicits its action centrally in the hypothalamus where leptin is delivered via the blood–brain barrier and the CSF, where the organ responsible for leptin transport in the CSF is the choroid plexus [90].

Due to the association of IIH and obesity, leptin levels have been assessed in both the serum and CSF in IIH patients [86, 91,92,93,94]. There is however no consensus as to the leptin phenotype in IIH due to conflicting study designs (Table 4). However, the majority of studies reported increased serum leptin, and the largest study assessing CSF leptin reported increased CSF leptin in IIH. In addition, this study demonstrated that CSF leptin levels positively correlate with lumbar puncture opening pressure in non-IIH patients, suggesting leptin could modulate ICP [86]. Indeed, chronic leptin exposure increases Na+-K+-ATPase activity in renal tubule cells [95, 96]. As Na+-K+-ATPase activity increases CSF secretion at the choroid plexus, it may be hypothesised that leptin increases CSF secretion; however, there is currently no direct evidence to support this theory.

Table 4 Leptin levels in serum and CSF of IIH patients compared with controls.

Oestrogen and progesterone

Given that IIH is predominantly a disease of women, the levels of the female sex hormones progesterone and oestrogens have been assessed. Studies of these sex hormones and IIH demonstrate inconclusive results, confounded by small cohorts and use historical assays (n = 5–51 IIH patients, 1991–2013) [26, 97, 98]. These studies were also hampered through the use of radioimmunoassay, which are noted to have low reliability, a poor lower limit of sensitivity as well as issues with cross reactivity of some metabolites leading to unspecificity [99].

Historical case series evaluating the use of hormonal contraceptives have suggested a possible causal role in IIH through several case studies [26]. However a recent longitudinal meta-analysis (n = 53) suggests that the use of hormonal contraceptives confers no additional risk to the development of IIH [100]. It should also be noted that oral contraceptives are a hugely heterogenous group of medications. They differ in the oestrogen effects, sex hormone binding globulin effects and progestogenic effects. In some the progestogen components have mild anti-androgenic effects; others have mild proandrogenic effects while others have direct anti-androgenetic effects. The net effect is also further complicated by differing dosages used across populations. Thus, case series analyses that evaluate the effect of hormonal contraceptives as a whole in IIH, without consideration for contraceptive subtype cannot be reliably interpreted.

Animal experimentation suggest both oestrogen and progesterone decrease Na+-K+-ATPase activity thus potentially reduce CSF production [101]. However, the direct effect of these hormones on ICP has yet to be established.

Androgens

The importance of androgens in the pathophysiology of IIH has recently come to the fore following the discovery that IIH is characterised by a unique androgen excess signature which modulates CSF dynamics.

Androgens are sex steroids that are primarily generated in ovarian thecal cells and activated peripherally by the skin, liver and adipose tissue [102]. The cardinal disease of female androgen excess, polycystic ovary syndrome (PCOS) is prevalent in IIH with some case series reporting up to 57% of patients presenting with PCOS [75, 103]. In female-to-male gender reassignment patients, testosterone therapy has been suggested to cause raised ICP and papilloedema which goes into remission temporally with testosterone withdrawal [104,105,106]. Indeed, young onset (<25 years of age) female IIH patients are associated androgen excess [98].

Steroid metabolite analysis using liquid chromatography–tandem mass spectrometry was performed in serum, urine and CSF of patients with IIH (n = 70), PCOS (n = 60) and in patients with simple obesity (n = 40) matched for age, gender and BMI. IIH women showed a pattern of androgen excess distinct to that observed in PCOS and simple obesity, with increased serum testosterone, and increased CSF testosterone and androstenedione. 11-oxygenated androgens, which are adrenal derived and a major contributor to androgen excess in PCOS, were not deranged in IIH [107]. In addition, specific to IIH, systemic steroid metabolism measured in 24 h urine samples using gas chromatography–mass spectrometry demonstrated a net increase in systemic 5α-reductase activity, an important reaction in androgen activation [107].

The study also demonstrated that IIH was uniquely characterised by elevated CSF levels of the active androgen testosterone as well as its precursor androstenedione [107].

The choroid plexus epithelial cells express the androgen receptor as well as the key enzymatic machinery for androgen metabolism. Furthermore testosterone has the capacity to increase Na+-K+-ATPase activity in rodent choroid plexus cells, a surrogate marker of CSF secretion [36] suggesting testosterones capacity to increase ICP, thus potentially pathogenicity in IIH [41]. Interestingly, systemic androgen production is reduced following weight loss in IIH patients and concurrent resolution of symptoms [82]. This suggests that adipose tissue could be in part driving the androgen excess phenotype, but this has yet to be assessed.

Androgen excess is a key driver of increased cardiovascular risk [108,109,110,111,112,113]. In a population-based matched cohort study patients with IIH were found to have doubled risk of cardiovascular disease compared to age, gender and BMI matched control subjects [19]. This supports a concept that IIH is a complex disease characterised by systemic metabolic dysregulation. Interestingly, increased centripetal fat drives the risk of metabolic syndrome and cardiovascular disease [114,115,116]. IIH is characterised by a centripetal fat distribution which correlates with ICP [117].

Moving towards an in vivo IIH model

Obesity in rodents has been postulated to model IIH. Although there are several available models of rodent obesity, to our knowledge only one has assessed the role of obesity with regards to ICP. Obese Zucker rats, who have a dysfunctional leptin receptor, have raised ICP when compared with lean controls [40]. However, the ICP recordings of over fed rats, that develop obesity over 4 weeks, showed a tendency to correlate positively with weight gain, but this did not reach significance [40]. ICP recordings were achieved using an epidural ICP probe thereby utilising minimally invasive in vivo ICP monitoring and suggests that obesity could elevate ICP [40]. The advantages and disadvantages of this technique as well as other in vivo models of ICP are described in Table 5.

Table 5 Advantages and disadvantages of in vivo ICP monitoring models.

Thus assessing the capacity of other models of obesogenesis should be assessed with regards to ICP. Other models of obesity need to be explored.

Conclusion

This paper has explored the current pathophysiological mechanisms identified in IIH. Due to the nature of this descriptive review there are inherent limitations in the methodology, for example it did not critically grade each article for bias, and only those published in English have been included. It does however serve to provide the clinician with an in-depth understanding of the complex processes that are now thought to have influence on our patients. The last decade has seen major advances in understanding IIH. Systemic metabolic dysregulations may be a key causal driver in disease pathogenesis with a unique androgen excess profile recently identified in IIH and implicated in CSF dysregulation. A twofold increase in cardiovascular disease risk in IIH further supports re-classifying IIH as a systemic disease. Mechanistic studies, through the use of preclinical models, are vital to further advance the understanding of IIH. An in vivo model to fully explain IIH has yet to be established and in the interim the use of preclinical models provide a fundamental resource to facilitate mechanistic evaluations as well as evaluation of potential novel therapeutics. However, these models all have clear pros and cons which are vital to grasp in order to critically interpret the ensuing study results.

DH | National Institute for Health Research (NIHR)—NIHR-CS-011-028 [Sinclair].

RCUK | Medical Research Council (MRC)—MR/K015184/1.

Summary

What was known before

  • The aetiology of IIH has long been speculated.

  • The role of increased CSF secretion or decreased CSF drainage as a cause of elevated ICP is debated.

  • Although biomarkers have been identified in IIH, studies are small and have previously lacked a mechanistic evaluation.

  • There are limited in vitro and in vivo models of IIH to evaluate underlying mechanisms in IIH.

What this study adds

  • A unique androgen excess profile which modulates CSF dynamics has been identified in IIH.

  • Androgens modulate CSF secretion via the choroid plexus, affecting ICP regulation, and are highlighted as the most important therapeutic target in IIH.

  • In vitro and in vivo models of CSF dynamics are emerging and growing in sophistication in their ability to inform regarding underlying aetiology in IIH.

  • Understanding the pros and cons of these preclinical models is vital to enable accurate interpretation of the ensuing results.

  • There is currently no in vivo model to fully explain IIH.