**3. Methods of isolation and analysis of extracellular vesicles**

Minimal experimental requirements for definition of EVs and their functions have been proposed [35], and isolated EVs should be characterized, and the morphology, protein composition, and functionality should be tested before any new enquiries are pursued. Whether the chosen isolation technique for the experiment consists in ultracentrifugation or any other technique, after collecting the sample it is necessary to perform two low-speed centrifugations as soon as possible after the sample collection [36]. The first low-speed centrifugation (300–800×g) removes cells, lipid droplets, and macromolecules from the sample, while the second low-speed centrifugation (2.500×g) removes platelets and apoptotic bodies. Cell removal is an important step; otherwise, the following high-speed centrifugations break the cells, leading to EV release and sample contamination [37].

**Differential ultracentrifugation** is the most widely used method for EV isolation [36], which involves multiple centrifugations at increasingly higher speeds obtaining a particle separation based on the sedimentation coefficient [38]. Establishing the appropriate speed and duration of centrifugation is a very important step in EV isolation [36]. Several inconveniences can occur using this technique such as the loss of certain subpopulations of EVs or simultaneous isolation of lipo/ protein aggregates [39, 40].

**Density gradient** ultracentrifugation is a method that isolates the particles by size and mass density [41], and its usefulness lies in the fact that it can isolate several subpopulations of EVs which are lost using differential ultracentrifugation; therefore, it increases the purity of the isolated EVs [42].

**Size exclusion chromatography** is an easy handling method by which a sizebased separation is achieved [43]. It allows the electron microscopy to be performed immediately after isolation and the proteins and lipoproteins are removed

**141**

**Figure 2.**

*generated from stem cells (D).*

*Part Two: Extracellular Vesicles as a Risk Factor in Neurodegenerative Diseases*

from the sample without losing any subpopulation, thus achieving a high-yield

**Precipitation kits** gained a lot of attention during the last years involving a concentration method based on the use of polyethylene glycol polymers. The price for the kits is low, the protocol is easy to perform, it is compatible with both low and high volumes of samples, and the method can be applied on large scale [45]. It must be taken into account that the precipitation kits are not the best method for EV isolation, having a low-yield purification because of the co-precipitations [37]. Anyway, for validating the results, it is recommended to use one of the ultracentri-

After the isolation step, a **general description of the protein composition** should be made even though there are no specific EV markers discovered yet. EVs are enriched in certain proteins such as tetraspanins (CD63, CD81, and CD9) and TSG 101 for exosomes, annexin V for ectosomes, etc. [46]. To exclude a contamination, the presence or absence of proteins that are not expected to be found in EVs, intracellular proteins like calnexin, cytochrome C, histones, GRP94, and Argonaute complex must be detected [35]. Western blot, flow cytometry, or mass spectroscopy

The next step consists in **individual characterization** of the EVs using at least

two methods: electron microscopy [35, 45], atomic force microscopy [47], or nanoparticle tracking analysis [48]. **Transmission electron microscopy** (TEM) is the most used method for visualization of EVs considering their nanoscale size (**Figures 1** and **2**). Negative staining [49], TEM on thin section from plastic

*Transmission electron microscopy: (A) ependymal cells (EC) facing the ventricular system of the mouse brain control the communication between cerebrospinal fluid and brain parenchyma; C—capillary. (B) Higher magnification of the square-marked area in (A) shows extracellular vesicles (arrows) close to cilia and microvilli of the ependymal cell (EC). Volume transmission may be mediated by multivesicular cargoes (encircled) which could be seen released from neurons in fetal mouse brain (C) or neurons from neurospheres* 

*DOI: http://dx.doi.org/10.5772/intechopen.86604*

fugation methods in parallel with this method.

can be used for this protein characterization step.

separation [44].

*Part Two: Extracellular Vesicles as a Risk Factor in Neurodegenerative Diseases DOI: http://dx.doi.org/10.5772/intechopen.86604*

from the sample without losing any subpopulation, thus achieving a high-yield separation [44].

**Precipitation kits** gained a lot of attention during the last years involving a concentration method based on the use of polyethylene glycol polymers. The price for the kits is low, the protocol is easy to perform, it is compatible with both low and high volumes of samples, and the method can be applied on large scale [45]. It must be taken into account that the precipitation kits are not the best method for EV isolation, having a low-yield purification because of the co-precipitations [37]. Anyway, for validating the results, it is recommended to use one of the ultracentrifugation methods in parallel with this method.

After the isolation step, a **general description of the protein composition** should be made even though there are no specific EV markers discovered yet. EVs are enriched in certain proteins such as tetraspanins (CD63, CD81, and CD9) and TSG 101 for exosomes, annexin V for ectosomes, etc. [46]. To exclude a contamination, the presence or absence of proteins that are not expected to be found in EVs, intracellular proteins like calnexin, cytochrome C, histones, GRP94, and Argonaute complex must be detected [35]. Western blot, flow cytometry, or mass spectroscopy can be used for this protein characterization step.

The next step consists in **individual characterization** of the EVs using at least two methods: electron microscopy [35, 45], atomic force microscopy [47], or nanoparticle tracking analysis [48]. **Transmission electron microscopy** (TEM) is the most used method for visualization of EVs considering their nanoscale size (**Figures 1** and **2**). Negative staining [49], TEM on thin section from plastic

#### **Figure 2.**

*Extracellular Vesicles and Their Importance in Human Health*

barrier (BBB), peripherally infused modified exosomes containing specific RNA were used to knockdown a specific gene in mouse brain [32–34]. Considering the extraordinary intricate cytoarchitecture of the brain, the presence of EVs in the adult brain is hard to be documented. Fetal brain and neurospheres contain cells which seem to release vesicles into the extracellular space (**Figure 1**). EVs are easier to be seen near ependymal cells floating in the ventricles from where they can be

*Transmission electron microscopy of the isolated extracellular vesicles: (A) negative staining and* 

Minimal experimental requirements for definition of EVs and their functions have been proposed [35], and isolated EVs should be characterized, and the morphology, protein composition, and functionality should be tested before any new enquiries are pursued. Whether the chosen isolation technique for the experiment consists in ultracentrifugation or any other technique, after collecting the sample it is necessary to perform two low-speed centrifugations as soon as possible after the sample collection [36]. The first low-speed centrifugation (300–800×g) removes cells, lipid droplets, and macromolecules from the sample, while the second low-speed centrifugation (2.500×g) removes platelets and apoptotic bodies. Cell removal is an important step; otherwise, the following high-speed centrifugations

**3. Methods of isolation and analysis of extracellular vesicles**

break the cells, leading to EV release and sample contamination [37].

therefore, it increases the purity of the isolated EVs [42].

**Differential ultracentrifugation** is the most widely used method for EV isolation [36], which involves multiple centrifugations at increasingly higher speeds obtaining a particle separation based on the sedimentation coefficient [38]. Establishing the appropriate speed and duration of centrifugation is a very important step in EV isolation [36]. Several inconveniences can occur using this technique such as the loss of certain subpopulations of EVs or simultaneous isolation of lipo/

**Density gradient** ultracentrifugation is a method that isolates the particles by size and mass density [41], and its usefulness lies in the fact that it can isolate several subpopulations of EVs which are lost using differential ultracentrifugation;

**Size exclusion chromatography** is an easy handling method by which a sizebased separation is achieved [43]. It allows the electron microscopy to be performed immediately after isolation and the proteins and lipoproteins are removed

**140**

protein aggregates [39, 40].

isolated [11].

**Figure 1.**

*(B) cryo-electron microscopy.*

*Transmission electron microscopy: (A) ependymal cells (EC) facing the ventricular system of the mouse brain control the communication between cerebrospinal fluid and brain parenchyma; C—capillary. (B) Higher magnification of the square-marked area in (A) shows extracellular vesicles (arrows) close to cilia and microvilli of the ependymal cell (EC). Volume transmission may be mediated by multivesicular cargoes (encircled) which could be seen released from neurons in fetal mouse brain (C) or neurons from neurospheres generated from stem cells (D).*

embedded EVs [49], can also be used to confirm the presence of the lipid bilayer of the isolated EV membrane and an election method to investigate EVs in tissue. **Cryo-TEM** [50] is a high resolution method to visualize the lipid bilayer. Electron tomography [4, 51] allows 3D reconstruction of the EVs with a very good imaging of the different types. For surface protein recognition, immuno-EM [52, 53] allows imaging of EV-specific markers.

**Flow cytometry** is a method based on measuring the signal of the light scattering from a structure passing through a laser beam. The smaller the particles, the less the light scattering, and therefore, conventional cytometry has a detection limit of approximately 200 nm [54]. Fluorescence-based detection is used to overcome this inconvenience [45, 55], the background noise being higher than the EV signal.

**Nanoparticle tracking analysis** involves the passing of a laser beam through a suspension that contains EVs and the scattering light is captured by a camera [48]. The Brownian movement of the EVs in the suspension is recorded, and according to their movement, the size can be measured [48].

The last step to fulfill the minimal experimental requirements involves the **functional assays** [35]. Multiple *in vitro* models can be designed for this step; co-incubating EVs with different culture cells and migration, proliferation, coagulation, and fibrinolysis may be quantified depending on the chosen model [45].

There is no gold-standard method yet, but researchers are encouraged to explore and to standardize their methods of isolation with the hope that someday, easy EV isolation will be possible.

## **4. Extracellular vesicles and cardiovascular risk for brain pathology**

All cells are capable of secreting specific arrays of EVs. Furthermore, the same cells may produce EVs by different biogenesis pathways, with different intracellular origins, of various sizes, with diverse composition and consequently, different functional properties [17]. Crucial feature for the normal functionality of the CNS and brain microenvironment homeostasis is sustained by vascular integrity which is highly dependent on the systemic status.

Several studies of patients with **stable coronary artery disease** have reported increased levels of circulating EVs which may influence the BBB integrity. Specific EV subpopulations, especially those of ECs origin, characterized by CD144+ , CD131<sup>+</sup> /annexin A5+ , or EVs containing miR-199a and miR-126, are currently researched as interesting biomarkers for cardiovascular risk and mortality in these patients [22, 56, 57].

Calcifications present in the atherosclerotic plaque [58] have a destabilizing effect in early lesions, favoring the rupture, but gain a potential protective effect in advanced lesions with heavy calcium deposits [59]. As several studies have shown, atherosclerotic plaque calcifications are associated with EVs of ECs, VSMCs, and macrophage origin. VSMCs can release EVs with low levels of calcification-inhibiting enzymes and annexin A6/phosphatidylserine nucleation complexes. Exposure of VSMCs to proinflammatory cytokines can stimulate the release of EVs that can mineralize when inhibitors of calcification are missing [60]. Also, ECs exposed to proinflammatory stimuli can release EVs rich in bone morphogenetic protein 2, promoting calcification in VSMs [61]. Alterations in local homeostasis of calcium and phosphate lead to the formation of macrophage-derived exosomes which stimulate mineralization, through an annexin-dependent mechanism [62].

Recent studies have also noted that in humans, advanced atherosclerotic plaques have a high content of procoagulant EVs, originating form leukocytes, erythrocytes, and VSMCs [63, 64]. In opposition to ectosomes, exosomes have shown

**143**

CD66+

*Part Two: Extracellular Vesicles as a Risk Factor in Neurodegenerative Diseases*

antithrombotic effects. In animal studies, platelet-derived exosomes suppressed platelet aggregation and occlusive thrombosis by inhibiting platelet CD36 and decreasing CD36-dependent oxidized LDL binding and macrophage cholesterol loading [65]. EVs influence the different mechanisms that lead to plaque destabilization and rupture. Intraplaque hemorrhages are produced by neovascularization originating from adventitial tissue, stimulated by plaque EVs, such as CD40+ vesicles of macrophage origin. Hemorrhages are also favored by leukocyte and ECs-EVs with fibrinolytic activity [66, 67]. Fibrous cap weakening is associated with VSMC apoptosis, induced by the presence of EVs, released in some pathological conditions [100]. Moreover, EVs can influence breakdown of matrix structural

Circulating levels of procoagulant EVs are higher in patients with **acute coronary syndromes** compared to healthy controls or patients with stable coronary artery disease [57, 69]. Circulating EVs alter endothelial-dependent NO mediated vasodilation, and endothelial EVs increase ECs thrombogenicity [70, 71]. Circulating EVs have also been investigated as prognostic markers in secondary prevention, in order to identify patients at high cardiovascular risk [56, 57]. Increased levels of CD11b+

leukocyte-derived EVs could be useful in identifying asymptomatic patients

Different neuronal cell types and molecules concur to regulate the improvement of brain vasculature [31, 80–82]. Each cell, including neurons and astrocytes [32, 83], is able to produce EVs enriched in specific proteins, lipids, and RNAs. EVs can stimulate targeted neural cells and surrounding neural tissues, which are important elements of vascular integrity preservation. The brain pathological condition changes the EV content profile of proteins and miRs [84]. A number of studies have shown that EVs regulate arterial stiffness [32, 85] which is linked to small vessel [32, 86–88], and platelet-derived EVs seem to be important players in the formation of cerebral microthrombi which lead to brain atrophy and consequent cognitive degeneration. It is believed that the prothrombotic nature of an elevated number of platelet-derived EVs reported in the acute phase of cerebral infarction may conduct to infarct progression [32, 84, 89, 90]. EV proteins cystatin C and CD14 have been shown to be related to cerebral white matter lesions and the progression of brain atrophy in patients with manifest vascular disease, suggesting a role for EVs in the

The role of cardiovascular disease risk factors in the occurrence and progression of cognitive impairment is widely accepted. There is a link between elevated levels of cholesterol and amyloid deposition in the brain, and the relationship between

The pathology of Alzheimer's disease (AD) consists in the extracellular amyloid

plaques formed by aggregated amyloid beta peptides and in the intraneuronal neurofibrillary tangles made of hyperphosphorylated tau proteins [91]. The

atherosclerotic injury and sporadic Alzheimer's disease is investigated.

**5. Extracellular vesicles in neurodegenerative diseases**

All these circulating EVs associated with coronary disease [74] may affect the vascular bed of the brain and disrupt the functionality of BBB. Aging and cardiovascular-associated disease are associated with BBB alteration [75] and blood circulating EVs may mediate early dysfunctions or progression of cerebral associated pathology. EVs associated with hypercholesterolemia [76] and atherosclerosis [77, 78] may have an impact on BBB function, and reducing the proinflammatory

/CD45+

/

EVs could identify individu-

*DOI: http://dx.doi.org/10.5772/intechopen.86604*

proteins through metalloproteinase interactions [68].

at high risk for plaque rupture [72], while CD3+

cytokines enrolling in EVs [79] may be beneficial.

etiology of structural brain changes [32].

als who will develop a major cardiovascular event [73].

#### *Part Two: Extracellular Vesicles as a Risk Factor in Neurodegenerative Diseases DOI: http://dx.doi.org/10.5772/intechopen.86604*

antithrombotic effects. In animal studies, platelet-derived exosomes suppressed platelet aggregation and occlusive thrombosis by inhibiting platelet CD36 and decreasing CD36-dependent oxidized LDL binding and macrophage cholesterol loading [65]. EVs influence the different mechanisms that lead to plaque destabilization and rupture. Intraplaque hemorrhages are produced by neovascularization originating from adventitial tissue, stimulated by plaque EVs, such as CD40+ vesicles of macrophage origin. Hemorrhages are also favored by leukocyte and ECs-EVs with fibrinolytic activity [66, 67]. Fibrous cap weakening is associated with VSMC apoptosis, induced by the presence of EVs, released in some pathological conditions [100]. Moreover, EVs can influence breakdown of matrix structural proteins through metalloproteinase interactions [68].

Circulating levels of procoagulant EVs are higher in patients with **acute coronary syndromes** compared to healthy controls or patients with stable coronary artery disease [57, 69]. Circulating EVs alter endothelial-dependent NO mediated vasodilation, and endothelial EVs increase ECs thrombogenicity [70, 71]. Circulating EVs have also been investigated as prognostic markers in secondary prevention, in order to identify patients at high cardiovascular risk [56, 57]. Increased levels of CD11b+ / CD66+ leukocyte-derived EVs could be useful in identifying asymptomatic patients at high risk for plaque rupture [72], while CD3+ /CD45+ EVs could identify individuals who will develop a major cardiovascular event [73].

All these circulating EVs associated with coronary disease [74] may affect the vascular bed of the brain and disrupt the functionality of BBB. Aging and cardiovascular-associated disease are associated with BBB alteration [75] and blood circulating EVs may mediate early dysfunctions or progression of cerebral associated pathology. EVs associated with hypercholesterolemia [76] and atherosclerosis [77, 78] may have an impact on BBB function, and reducing the proinflammatory cytokines enrolling in EVs [79] may be beneficial.

Different neuronal cell types and molecules concur to regulate the improvement of brain vasculature [31, 80–82]. Each cell, including neurons and astrocytes [32, 83], is able to produce EVs enriched in specific proteins, lipids, and RNAs. EVs can stimulate targeted neural cells and surrounding neural tissues, which are important elements of vascular integrity preservation. The brain pathological condition changes the EV content profile of proteins and miRs [84]. A number of studies have shown that EVs regulate arterial stiffness [32, 85] which is linked to small vessel [32, 86–88], and platelet-derived EVs seem to be important players in the formation of cerebral microthrombi which lead to brain atrophy and consequent cognitive degeneration. It is believed that the prothrombotic nature of an elevated number of platelet-derived EVs reported in the acute phase of cerebral infarction may conduct to infarct progression [32, 84, 89, 90]. EV proteins cystatin C and CD14 have been shown to be related to cerebral white matter lesions and the progression of brain atrophy in patients with manifest vascular disease, suggesting a role for EVs in the etiology of structural brain changes [32].

The role of cardiovascular disease risk factors in the occurrence and progression of cognitive impairment is widely accepted. There is a link between elevated levels of cholesterol and amyloid deposition in the brain, and the relationship between atherosclerotic injury and sporadic Alzheimer's disease is investigated.

### **5. Extracellular vesicles in neurodegenerative diseases**

The pathology of Alzheimer's disease (AD) consists in the extracellular amyloid plaques formed by aggregated amyloid beta peptides and in the intraneuronal neurofibrillary tangles made of hyperphosphorylated tau proteins [91]. The

*Extracellular Vesicles and Their Importance in Human Health*

their movement, the size can be measured [48].

highly dependent on the systemic status.

/annexin A5+

patients [22, 56, 57].

imaging of EV-specific markers.

isolation will be possible.

embedded EVs [49], can also be used to confirm the presence of the lipid bilayer of the isolated EV membrane and an election method to investigate EVs in tissue. **Cryo-TEM** [50] is a high resolution method to visualize the lipid bilayer. Electron tomography [4, 51] allows 3D reconstruction of the EVs with a very good imaging of the different types. For surface protein recognition, immuno-EM [52, 53] allows

**Flow cytometry** is a method based on measuring the signal of the light scattering from a structure passing through a laser beam. The smaller the particles, the less the light scattering, and therefore, conventional cytometry has a detection limit of approximately 200 nm [54]. Fluorescence-based detection is used to overcome this inconvenience [45, 55], the background noise being higher than the EV signal.

**Nanoparticle tracking analysis** involves the passing of a laser beam through a suspension that contains EVs and the scattering light is captured by a camera [48]. The Brownian movement of the EVs in the suspension is recorded, and according to

The last step to fulfill the minimal experimental requirements involves the **functional assays** [35]. Multiple *in vitro* models can be designed for this step; co-incubating EVs with different culture cells and migration, proliferation, coagulation, and fibrinolysis may be quantified depending on the chosen model [45].

**4. Extracellular vesicles and cardiovascular risk for brain pathology**

All cells are capable of secreting specific arrays of EVs. Furthermore, the same cells may produce EVs by different biogenesis pathways, with different intracellular origins, of various sizes, with diverse composition and consequently, different functional properties [17]. Crucial feature for the normal functionality of the CNS and brain microenvironment homeostasis is sustained by vascular integrity which is

Several studies of patients with **stable coronary artery disease** have reported increased levels of circulating EVs which may influence the BBB integrity. Specific EV subpopulations, especially those of ECs origin, characterized by CD144+

researched as interesting biomarkers for cardiovascular risk and mortality in these

Calcifications present in the atherosclerotic plaque [58] have a destabilizing effect in early lesions, favoring the rupture, but gain a potential protective effect in advanced lesions with heavy calcium deposits [59]. As several studies have shown, atherosclerotic plaque calcifications are associated with EVs of ECs, VSMCs, and macrophage origin. VSMCs can release EVs with low levels of calcification-inhibiting enzymes and annexin A6/phosphatidylserine nucleation complexes. Exposure of VSMCs to proinflammatory cytokines can stimulate the release of EVs that can mineralize when inhibitors of calcification are missing [60]. Also, ECs exposed to proinflammatory stimuli can release EVs rich in bone morphogenetic protein 2, promoting calcification in VSMs [61]. Alterations in local homeostasis of calcium and phosphate lead to the formation of macrophage-derived exosomes which stimulate

Recent studies have also noted that in humans, advanced atherosclerotic plaques

have a high content of procoagulant EVs, originating form leukocytes, erythrocytes, and VSMCs [63, 64]. In opposition to ectosomes, exosomes have shown

mineralization, through an annexin-dependent mechanism [62].

, or EVs containing miR-199a and miR-126, are currently

,

There is no gold-standard method yet, but researchers are encouraged to explore and to standardize their methods of isolation with the hope that someday, easy EV

**142**

CD131<sup>+</sup>

accumulation of the proteins induces an apoptotic response with neuronal loss and occurs especially in the cerebral cortex [92].

It has been observed that the pathological findings in AD have a typical spatial distribution suggesting a neuron-to-neuron spread of the amyloid and hyperphosphorylated tau proteins, which promote aggregation, acting as "seeds" [93]. Therefore AD is considered to have a prion-like model of propagation [94]. The immediate question that rises is: what is the mechanism of the propagation?

Amyloid beta is mainly formed extracellularly from the cleavage of APP by beta and gamma secretases, which are found at the level of the plasma membrane [95]. But in some degree, the secretases are present in endoplasmic reticulum and Golgi apparatus, and there is a certain intracellular production of amyloid beta [96]. It is removed from the cell via exosomes embedded in a multivesicular body as an alternative pathway to lysosomal degradation [97]. A new study suggests that exosomes containing amyloid beta are present in higher concentrations in the AD brain compared to the healthy brain [98]. Moreover, the study shows that exosomes are the carriers of the toxic amyloid beta from one neuron to another [98]. Also, it is thought that exosomes mediate the intercellular transfer of hyperphosphorylated tau protein, and the exosome-mediated tau protein induces the formation of neurofibrillary tangles [99].

The evolution of AD is insidious with an asymptomatic stage that lasts several years [100]. Although asymptomatic, the pathological changes in the brain are present in this stage [93]. These findings suggest the value of discovering biomarkers that can anticipate the onset of the clinical symptoms or can facilitate a window for the possibility of a future therapy that could stop the progression. Amyloid beta and hyperphosphorylated tau proteins are of great value as biomarkers when dosed from the cerebrospinal fluid [101]. Nevertheless, performing lumbar puncture in a wide population is almost impossible. Thereby, the discovery of new biomarkers is a valuable research theme.

Several types of miRs isolated from cerebrospinal fluid are differentially expressed in AD, such as miR-100, miR-146, miR-505, and miR-1274a [102]. The presence of several types of exosomal miRs isolated from serum (miR-361-5p, miR-93-5p, miR-335-5p, and miR-30e-5p) correlates with the neuropsychological evaluation and brain imaging [103]. It is to be mentioned that exosome-containing proteins like tau, apolipoprotein E, cystatin E, and HSP-90 alpha were isolated in the cerebrospinal fluid and were present in patients with AD [104]. This evidence proposes both miRs and protein-containing exosomes as a promising source of biomarkers for AD.

**Parkinson's disease** (PD) is a neurodegenerative disease that consists in the loss of dopaminergic neurons localized in the substantia nigra [105]. The pathology of the disease implies the deposition of Lewy bodies in the neurons which are mostly made of misfolded and aggregated alpha-synuclein protein [105]. The Braak staging explains the spatio-temporal dissemination of Lewy bodies into the neurons from caudal to rostral, starting in the medulla oblongata and spreading to the level of the cerebral cortex, damaging various structures on this way [106]. The starting point is thought to be either the enteric nervous system or the olfactory bulb [106]. Thereby, it is suggested that PD has a prion-like propagation [94]. Are exosomes responsible for carrying alpha-synuclein from neuron to neuron? The mechanism could be similar to the one described in AD, but there are fewer studies to draw certain conclusions regarding the involvement of exosomes in the pathogenesis of PD. Excessive intracellular alpha-synuclein is thought to be transported out of the cell via multivesicular body containing exosomes in a similar manner as in AD in an attempt to clean the intracellular space [107].

**145**

*Part Two: Extracellular Vesicles as a Risk Factor in Neurodegenerative Diseases*

proteins were also isolated in the CSF of PD patients [109, 112].

several diseases as well as in neurodegenerative diseases [117].

Recently, it was discovered that an important player in the field of neural diseases is EV derived from stem cells [118], mainly in the case of stroke [118–120]. In stroke pathophysiology, inflammation plays a significant role, circulating EV-activating immune cells. Neurons quickly depolarize and die, being next phago-

Because of their β1 and α2b integrin-enriched content, human neural stem cell-derived EV administration recovers both tissue and sensorimotor function and may protect the BBB integrity, in the preclinical mouse thromboembolic model of stroke [122, 123]. Similarly, multipotent mesenchymal stromal cells (MSCs), through their capacity to secrete soluble factors, play an important role in brain repair. It was demonstrated that MSC cargos modulate cell signaling in ischemic stroke by PI3K/Akt pathway activation [123, 124] and EVs facilitated secretion of miRs sustaining MSC neuroprotective effects in ischemic stroke as well. Previous research demonstrated that intravenous administration of bone marrow-MSCs containing exosomes transferred miR-133b to astrocytes and neurons into the ischemic boundary zone [120, 123], and MSCs cultured in the presence of extracts from rat ischemic brain induced increased expression of exosomal miR133b [123, 125]. Also, EVs released by human MSCs seem to have an anti-inflammatory effect on mast cells, by increased prostaglandin E2 (PGE2) synthesis and up-regulation of EP4 receptor which might prevent the rupture of intracranial aneurysms [126]. All these data suggest that EVs from various sources may contribute to the neurogenesis

cytosed by infiltrating circulating macrophages and microglia [84, 121].

and angiogenesis during brain repair processes in cerebral diseases.

**6. Extracellular vesicles' perspective use in brain pathology**

Studies of neuronal cell cultures expressing alpha-synuclein noticed that the protein is released by the cell free in the extracellular space but also incorporated in the exosomes [108]. Furthermore, neighboring cells take up the exosomes, and the transferred alpha-synuclein acts as seed for the formation of the aggregate [109]. Evidence to prove that in vivo alpha-synuclein is transferred by exosomes is not available yet, but it can be speculated that exosomes play an important role as

The use of EVs as a biomarker tool in PD is a promising field too [110]. Several miRs carried by exosomes were increased in the CSF of PD patients, such as miR-10a-5p, miR-153, and miR-409-3p, while some miRs such as miR-19b-3p and miR-1 were significantly reduced [111]. Exosomes containing alpha-synuclein and LRRK

The discovery of the EV involvement in several biological processes gave hope that some questions regarding neurodegenerative diseases will be answered. First of all, it is important to clarify which are the cellular mechanisms involved in the progression of the disease and if exosomes play any role. Based on the spatio-temporal spreading of the pathological proteins in the brain, an appealing theory is the prionlike propagation theory [113]. It is presumed that exosomes play an important role by facilitating the interneuronal transport of the proteins [114]. As well, there is a critical need in finding accessible biomarkers that can diagnose a neurodegenerative disease in the asymptomatic stage [115]. Dosing certain free proteins in biofluids can be an option, but several problems are experienced because of their low concentrations [115]. Therefore, a new approach is being attempted consisting in finding the proteins encapsulated in extracellular vesicles [116]. Micro-RNAs and different proteins carried by exosomes are attractive options for finding new biomarkers in

*DOI: http://dx.doi.org/10.5772/intechopen.86604*

in vitro.

#### *Part Two: Extracellular Vesicles as a Risk Factor in Neurodegenerative Diseases DOI: http://dx.doi.org/10.5772/intechopen.86604*

Studies of neuronal cell cultures expressing alpha-synuclein noticed that the protein is released by the cell free in the extracellular space but also incorporated in the exosomes [108]. Furthermore, neighboring cells take up the exosomes, and the transferred alpha-synuclein acts as seed for the formation of the aggregate [109]. Evidence to prove that in vivo alpha-synuclein is transferred by exosomes is not available yet, but it can be speculated that exosomes play an important role as in vitro.

The use of EVs as a biomarker tool in PD is a promising field too [110]. Several miRs carried by exosomes were increased in the CSF of PD patients, such as miR-10a-5p, miR-153, and miR-409-3p, while some miRs such as miR-19b-3p and miR-1 were significantly reduced [111]. Exosomes containing alpha-synuclein and LRRK proteins were also isolated in the CSF of PD patients [109, 112].
