Progressive supranuclear palsy (PSP) is a primary 4-repeat (4R) tauopathy characterized by the selective degeneration of specific neuronal populations in the brainstem, basal ganglia, and cerebral cortex. The disease presents clinically with vertical supranuclear gaze palsy, postural instability with early falls, axial rigidity, and progressive cognitive decline[1]. Understanding which neurons are selectively vulnerable in PSP — and why — is central to developing targeted therapies for this devastating condition.
The brainstem bears the heaviest neuronal burden in PSP. The substantia nigra pars compacta (SNpc) shows severe dopaminergic neuron loss, typically exceeding 80% at autopsy, which underlies the parkinsonian features of the disease[2]. Unlike Parkinson's disease, where SNpc degeneration is accompanied by Lewy body pathology, PSP neurons accumulate globose neurofibrillary tangles (NFTs) composed of hyperphosphorylated 4R tau[3].
The subthalamic nucleus (STN) undergoes particularly devastating neuronal loss in PSP, often exceeding 50%, making it one of the most severely affected regions[4]. STN neuron degeneration disrupts the indirect pathway of the basal ganglia motor circuit, contributing to the characteristic axial rigidity and postural instability. The pedunculopontine nucleus (PPN), which integrates locomotor and arousal signals, also suffers severe cholinergic neuron loss, directly contributing to gait freezing and falls[5].
Additional brainstem nuclei affected include the red nucleus, pontine nuclei, dentate nucleus of the cerebellum, and oculomotor nuclei (particularly the rostral interstitial nucleus of the medial longitudinal fasciculus, riMLF), whose damage produces the hallmark vertical gaze palsy[6].
In the globus pallidus, both internal (GPi) and external (GPe) segments show significant neuronal depletion. GPi output neurons, which form the primary inhibitory projection to the thalamus, are severely affected. The caudate nucleus and putamen show moderate neuronal loss with tau-positive inclusions in remaining neurons[7].
Cortical involvement varies by PSP subtype. In Richardson syndrome (PSP-RS, the classic form), frontal cortical neurons — particularly in the primary motor cortex, supplementary motor area, and prefrontal cortex — accumulate tau pathology. PSP with progressive nonfluent aphasia (PSP-PNFA) shows greater left perisylvian cortical involvement, while PSP with corticobasal syndrome (PSP-CBS) demonstrates asymmetric frontoparietal cortical degeneration[8].
PSP is defined by the selective accumulation of 4-repeat tau isoforms. Alternative splicing of the MAPT gene exon 10 produces tau isoforms with either 3 or 4 microtubule-binding repeats. In PSP, the 4R:3R ratio shifts heavily toward 4R, distinguishing it from Alzheimer's disease (mixed 3R/4R) and Pick's disease (3R predominant)[9].
The MAPT H1 haplotype, particularly the H1c sub-haplotype, is the strongest genetic risk factor for PSP (OR ~5.5), promoting increased exon 10 inclusion and 4R tau production[10]. This genetic predisposition likely enhances the propensity of susceptible neurons to accumulate pathological tau.
Neuronal tau inclusions in PSP form characteristic globose (rounded) neurofibrillary tangles, ultrastructurally composed of straight filaments 12-15 nm in diameter. This contrasts with the paired helical filaments (PHFs) of AD tangles. Cryo-EM studies have revealed that PSP tau filaments adopt a unique three-layered fold distinct from other tauopathies[11].
Multiple kinases contribute to pathological tau phosphorylation in PSP neurons. GSK-3β phosphorylates tau at multiple epitopes including Thr231 and Ser396. CDK5, activated by its pathological co-activator p25, phosphorylates tau at Ser202/Thr205 (the AT8 epitope used in neuropathological staging). DYRK1A and CK1 also contribute to the multi-site phosphorylation cascade[12]. Concurrently, the activity of protein phosphatase 2A (PP2A), the major tau phosphatase, is reduced in PSP brain tissue[13].
PSP neurons exhibit prominent mitochondrial complex I deficiency. Post-mortem studies show 30-40% reduction in complex I activity in PSP substantia nigra and striatum[14]. This bioenergetic deficit renders metabolically demanding neurons — particularly large projection neurons in the STN, SNpc, and PPN — especially vulnerable. Mitochondrial dysfunction amplifies oxidative stress, which in turn promotes tau phosphorylation via GSK-3β activation[15].
Activated microglia and astrocytes create a neuroinflammatory milieu that compounds neuronal vulnerability. Pro-inflammatory cytokines (TNF-α, IL-1β, IL-6) released by activated microglia promote tau phosphorylation and impair synaptic function. Tau-laden neurons release pathological tau species that further activate microglia, creating a feed-forward cycle of inflammation and neurodegeneration[16].
A distinctive feature of PSP is the prominent glial tau pathology. Tufted astrocytes — star-shaped astrocytic tau inclusions concentrated in motor cortex and striatum — are the pathological hallmark of PSP. Oligodendrocytes develop coiled bodies, and tau-positive threads appear in white matter tracts. This glial pathology disrupts the supportive microenvironment that neurons depend on for trophic support, metabolic coupling, and synaptic maintenance[17].
PSP neurons show impaired autophagy and lysosomal function. Accumulation of p62/SQSTM1 and LC3-positive puncta indicates failed autophagic clearance of tau aggregates. The transcription factor TFEB, a master regulator of lysosomal biogenesis, shows reduced nuclear translocation in PSP neurons, contributing to the inability to clear pathological tau[18].
PSP progression follows a stereotypical pattern of neuronal tau accumulation. Williams and colleagues proposed a staging scheme: early disease (stage 1-2) involves the STN, SNpc, and globus pallidus; intermediate disease (stage 3-4) extends to the pontine nuclei, dentate nucleus, and frontal cortex; advanced disease (stage 5-6) involves widespread cortical and brainstem regions[19]. Kovacs and colleagues refined this with a sequential distribution model highlighting initial pallido-nigro-luysial involvement with subsequent brainstem and cortical spread[20].
Fluid biomarkers reflecting PSP neuronal degeneration include elevated neurofilament light chain (NfL) in cerebrospinal fluid (CSF) and plasma, which correlates with disease severity and progression rate[21]. Tau PET imaging with second-generation tracers (e.g., [^18F]PI-2620) shows tracer retention in the basal ganglia and brainstem, though sensitivity remains limited compared to AD tau imaging[22]. MRI volumetry reveals characteristic midbrain atrophy — the "hummingbird sign" on sagittal views — and STN volume reduction on high-resolution imaging[23].
Understanding selective neuronal vulnerability in PSP guides therapeutic development across several strategies:
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