CX3CL1 Pathway as a Molecular Target for Treatment Strategies in Alzheimer’s Disease

Given all the above, the role of CX3CL1 in in vivo and in vitro AD models has been investigated, achieving controversial results. It can be stated that discrepancies among the findings obtained depend on several factors. Firstly, regarding the in vivo studies using different AD animal models, the typology of mice utilized has been found to sharply influence the findings obtained. In general, suppressing CX3CL1 signalling in Aβ pathology models (i.e., hAPP, APP-PS1 and CRND8 mice) and tau pathology models (hTau mice) gives rise to opposite results due to a Janus behaviour of CX3CL1 toward Aβ and tau aggregate deposition [39,40]. Indeed, the chemokine signal normally reduces the amyloid clearance (by inhibiting microglial phagocytosis), favouring amyloid aggregate deposition, but avoids tau phosphorylation, protecting from neurofibrillary tangle accumulation [40,51,52]. Consequently, suppressing the CX3CL1 signal in Aβ pathology mouse models results in ameliorating Aβ burden, but it does worsen tau phosphorylation and exacerbates cognitive deficits in tau-pathology mouse models [19,46]. In addition, differential expression of CX3CR1 throughout the brain influences Aβ deposition and toxicity [53]. Another main flaw affecting the studies on this topic is that detailed knowledge about different soluble versus membrane-bound FKN isoform functions is lacking. This increased discrepancies and confounders among the experiments and findings and prompted some authors to investigate the most common commercial peptides used as FKN reagents in scientific research from a pharmacologic point of view [31]. Interestingly, the authors concluded that findings from the studies on FKN in neurodegenerative diseases should be taken with a grain of salt and great caution is needed in selecting peptides as well.

Another main factor influencing the unidirectionality of the results is using animal models per se. AD mouse models often present transgenic tau overexpression that leads to a forceful, extreme inflammation, artificially altering experimental processes and results, compared to the milder inflammatory response by microglia that is more likely to occur in the brain, especially in the early stage of disease [54,55,56]. This advantage should be added to the most known one, which is the simplified nature of in vivo models compared to humans, resulting in possible difficulties in translating findings and conclusions from preclinical to clinical models. Finally, the administration route of some molecules that have been found to be either potential targets for treatment or stimulating factors for some pathways involved in the disease pathogenesis (as is the case for CX3CL1) remains a challenging issue. Stereotactic injections, viral vectors and the use of mesenchymal stem cell-derived products represent the most common methods for molecule administration among AD studies experiments, calling attention to the need to identify novel strategies for administering molecules of interest [9].

That said, the main findings from the studies addressing a possible role for CX3CL1 in AD pathogenesis and, most importantly, as a target for AD treatment can be summarized as follows.

Recently, Guo et al., investigated the effect of bone marrow mesenchymal stem cell (BMSC)-derived CX3CL1 on SH-SY5Y neuroblastoma cells under Aβ1-42 inducement. They found that BMSC-derived CX3CL1 inhibited cell damage induced by Aβ1-42, as defined by axonal length, cell growth and synaptic protein expressions. In addition, the authors described the putative mechanism underlying their results, that is, the TXNIP/NLRP3 pathway [42]. However, the authors pointed out that the experiments were insufficient to explain either the involvement of BMSC-derived CX3CL1 axis in brain inflammation or which CX3CL1 isoform, between the membrane-bound and the soluble ones, was responsible for reducing Aβ1-42-induced injury in SH-SY5Y cells.

Dworzak et al., performed complex analyses, including both in vivo and in vitro AD models, starting from the assumption that CX3CR1 can be expressed by neurons and microglia in some contexts, having different influences on the local response to Aβ deposition. Examination of differences between neuronal and microglial CX3CR1 was defined as synaptic toxicity and dysfunction induced by Aβ deposition. Using primary cultures of CX3CR1-/- neurons and microglia, the authors demonstrated that Aβ peptide composition and conformation affects synaptic transmission per se, and that neuronal CX3CR1 is more present within the hippocampus compared to the cortex, making its deficiency protective toward neurotoxicity. The authors suggested that hippocampal neurons are more prone to Aβ toxicity due to the high, selective presence of CX3CR1 in this brain area [53]. However, considering the controversy around the presence of CX3CR1 on neurons, with some authors [35,57,58] reporting selective microglial expression of the receptor, Dworzak's findings should be interpreted with caution.

Bolos et al., examined whether microglia could carry out tau internalization through a CX3CR1-mediated mechanism, by treating primary cultures from the cerebral cortex of 2-day-old mice with phosphoTau Cy5 and control Cy5. Immunofluorescence analysis showed that CX3CR1 mediates tau internalization by microglia, as measured by calculating the amount of Cy5 positive area within microglial cells [59].

At the beginning of the investigations on the CX3CL1/CX3CR1 axis in AD, the focus has been the CX3CR1 receptor for a long time, with many studies performed using CX3CR1 deficient AD mouse models [38,39,40,59]. Lee et al., reported CX3CR1 deficiency reduced Aβ deposition and neuronal loss in APP-PS1 and R1.40 mouse models of AD, along with the reduction in microglia surrounding Aβ plaques, as demonstrated by immunohistochemical analysis using the CD68 microglial marker [40]. The experiments of Lee et al., contributed to confirming much information about FKN, such as its capability of modulating inflammation in the brain and the regulation of phagocytosis activity in microglia, that nowadays are fully established. Bhaskar et al., reported CX3CR1 deficiency worsened tau phosphorylation and brain inflammation in the tau-pathology mouse model of AD hTau mice [39], confirming that different experiments give rise to different effects, either beneficial or detrimental, depending on the mouse model used. Successive experiments have focused on the role of FKN signalling regardless of the CX3CR1 receptor. In 2019, Fan et al., examined the role of the CX3CL1 C-terminal fragment (CX3CL1ct), which is the intracellular domain that is produced after two sequential cleavages of the transmembrane chemokine by BACE and γ secretase [32]. The experiments were performed by generating the mouse models of AD 5xFAD, in which amyloid deposition and neuronal loss were found to diminish significantly due to increased neurogenesis. Authors concluded that overexpression of CX3CL1ct enhances SGZ and SVZ neurogenesis via activation of transcriptional factors of some genes involved in neurogenesis, with TGFβ3, bone morphogenetic protein (BMP) and Smad being the most implicated pathways. Importantly, the authors described the back-signalling mechanism through which CX3CL1ct is translocated in the nucleus, where it induces the regulation of the above-mentioned transcription factors. The importance of these results is that the authors proved the beneficial effect of the chemokine in AD models and showed stimulation of neurogenesis to be independent of the receptor CX3CR1, which moved the focus of investigations from neuron-to-glia communication signalling pathways toward the expression levels of BACE in neurons and the production of the sole chemokine C-terminal fragment in these cells [32]. Subsequent analysis of Fan et al., was carried out using transgenic Tg mice overexpressing CX3CLK1 and a PS19 AD mouse model, confirming that FKN enhances neurogenesis via Smad signalling and showing that the CX3CL1ct reduces neuronal loss and improves cognitive function, as defined by learning and memory process, in AD mice [60].

Hickman et al., analyzed PS1-APP mice heterozygous for CX3CR1 (PS1-APP-CX3CR1+/−), documenting that CX3CR1 deficiency is associated with the reduction in Aβ levels, plaque burden and improved cognitive function [61]. Due to the ability of CX3CL1 to enhance the production of some molecules involved in Aβ degradation, the authors suggested that targeting CX3CL1/CX3CR1 signalling could be considered a useful way to delay the progression of AD by increasing neuronal Aβ clearance and reducing Aβ levels [61]. Li et al., performed their experiments using adenovirus-mediated gene transduction of BMSCs to deliver exogenous CX3CL1 and Wnt3a in APP/PS1 mice [62]. While CX3CL1 alone did not improve cognitive function, MSCs carrying CX3CL1 and Wnt3a ameliorated memory and learning [62]. Importantly, Li's experiment demonstrated a direct link between cognitive functions and microglial neurotoxicity, confirming that microglia status (baseline or quiescent, activated and primed) sharply affects brain function in health and diseases, and this status is influenced upstream by CX3CL1/CX3CR1 signals. This all gives strength to the hypothesis that baseline quiescent microglia can influence per se the destiny of healthy and AD people in many conditions, such as ageing, and through various mechanisms, including the FKN pathway [63]. Finneran et al. [64] isolated the chemokine domain and mucin-like stalk fragment of CX3CL1 and cloned it into a pTR2-MCS vector to gain mutant tau Tg45 mice. The authors evaluated the impact of soluble CX3CL1 expression on cognition in tau rTg450 mice after the onset of cognitive deficits by intraparenchymal injections of FKN in the ventricular system through adeno-associated virus serotype 4. They documented that soluble FKN overexpression significantly improved cognitive performance but did not reduce tau hyperphosphorylation. Opposite findings were achieved by Bolos et al., who demonstrated that CX3CR1 deficiency was associated with impaired uptake and degradation of tau by microglia, although it should be noted that CX3CR knockout mice were used in Bolos' experiments instead of mutant tau Tg45 mice. In addition, an interesting mechanism was highlighted by Bolos et al., consisting of a competition between tau protein and the natural ligand of CX3CR1, FKN. Using affinity chromatography, the authors showed that the amount of tau internalization in vitro is reduced in the presence of CX3CL1, highlighting that microglia strongly influence tau internalization via CX3CR1 [59]. However, this event happens at the cost of disturbing the signalling of CX3CL1 and causing the activation of microglia [59]. Actually, Nash et al., had previously reported overexpression of FKN in AD mouse models. In their experiments, APP/PS1 and Tg4510 mice were treated with adeno-associated virus serotype 9 expressing FKN along with a viral control vector expressing green fluorescent protein (GFP) instead of CX3CR1.

Results showed decreased tau pathology in Tg4510 mice and no changes in Aβ deposition in APP/PS1 mice treated with FKN. Based on these findings, the authors, with enthusiasm, proposed CX3CR1 as a good target for AD treatment [65]. To address the issue of different activity and signals between the soluble and membrane-bound isoforms of CX3CL1, Lee et al., performed in 2014 an experiment on CX3CL1-deficient APPPS1 mice and crossed them with a mouse line expressing only soluble CX3CL1. Findings revealed that soluble CX3CL1 signalling does not influence fibrillar Aβ deposition and tau phosphorylation, while the membrane-bound isoform reduces Aβ and increases tau phosphorylation, being responsible for AD hallmark-related changes in CX3CL1 deficient mice. In addition, the authors observed enhanced phagocytosis and activation of microglia, postulating that the absence of membrane-bound FKN causes the reduction in Aβ deposition thanks to the p38 mitogen-activated protein kinase (MAPK)-mediated activation of microglia and the macrophage scavenger receptor 1 (MSR-1)-dependent phagocytosis [66].

In 2018, Bemiller et al., evaluated the effects of expressing only the chemokine domain of CX3CL1 on tau pathology and behavioural function. The authors used a mouse line expressing soluble FKN presenting only the chemokine domain of CX3CL1, crossed with tau pathology mouse models of hTau. Results showed that the chemokine domain of CX3CL1 fails to decrease both tau pathology and microglial activation [67], suggesting that this fragment of Cx3CL1 downregulates CX3CR1 expression by microglia and increases tau pathology. In addition, the authors confirm the hypothesis that neuron-microglia crosstalk mediated by CX3CL1/CX3CR1 signalling can cause, when dysfunctional or disrupted, the quiescent baseline status of microglia, giving rise to a phenotype of these cells, known as the primed phenotype, that loses protective ability toward neurons, acquires aggressive and neurotoxic behaviour and, in turn, underlies neuron damage and loss [63].

Even considering the above-mentioned flaws of these studies, it could be sound to hypothesize that a promising target for AD treatment could be searched for within the CX3CL1 signalling pathway and, generally, among molecules influencing microglia phenotypes.