Impaired proteasome activity and neurodegeneration with brain iron accumulation in FBXO7 defect

Abstact FBXO7 is implicated in the ubiquitin–proteasome system and parkin‐mediated mitophagy. FBXO7defects cause a levodopa‐responsive parkinsonian‐pyramidal syndrome(PPS). Methods: We investigated the disease molecular bases in a child with PPS and brain iron accumulation. Results: A novel homozygous c.368C>G (p.S123*) FBXO7 mutation was identified in a child with spastic paraplegia, epilepsy, cerebellar degeneration, levodopa nonresponsive parkinsonism, and brain iron deposition. Patient’s fibroblasts assays demonstrated an absence of FBXO7 RNA expression leading to impaired proteasome degradation and accumulation of poly‐ubiquitinated proteins. Conclusion: This novel FBXO7 phenotype associated with impaired proteasome activity overlaps with neurodegeneration with brain iron accumulation disorders.


Introduction
Parkinsonism-pyramidal syndrome (PPS) is a complex movement disorder that may present in childhood associated with complex hereditary spastic paraplegia (SPG), young-onset parkinsonism, neurodegeneration with brain iron accumulation (NBIA) disorders, and inborn errors of metabolism. 1 FBXO7 deficiency (PARK15; MIM 260300) is a rare cause of PPS with 26 known patients since 2008. [2][3][4][5][6][7][8][9] Most of these patients develop spastic paraparesia and/or levodopa-responsive young onset parkinsonism with normal brain magnetic resonance imaging (MRI) and reduced dopamine uptake on DaTSCAN. [2][3][4][5][6][7][8][9] The F-box only pro-tein7 (FBXO7) gene encodes for a protein involved in ubiquitin-proteasome system (UPS) activity and mitophagy. FBXO7 protein is a subunit of a complex responsible for the phosphorylation-dependent ubiquitination, the SKP1/cullin-1/F-box protein (SCF) E3 ubiquitin ligase complex. FBXO7 acts as a substrate recruiter in this complex and has a regulatory role in proteasome through the direct interaction with the core proteasome subunit PSMA2, an essential protein required for a fully functional proteasome. Another role of FBXO7 protein is to provide an effective recruitment of parkin to damaged mitochondria and initiate mitophagy. [10][11][12][13] The genetic analysis of a child with a complex phenotype including epilepsy, progressive PPS with no response to levodopa, cognitive decline, and MRI features suggestive of NBIA revealed the novel homozygous FBXO7 c.368C>G (p.S123*) variant. We detected for the first time in patient's fibroblasts an impairment in ubiquitinprotein degradation and poly-ubiquitinated (poly-UB) proteins accumulation, (highlighting the essential role of the UPS activity of FBXO7 in human disease.

Methods
Used methodology is summarized in the main manuscript. Complete procedures and protocols are detailed in Supporting Information.

Consent and approval
All protocols complied with the ethics guidelines according to the Declaration of Helsinki and were approved by participating institutional review boards. The proband and relatives signed an informed consent for the study.

Genetic studies
Genetic test was performed in the proband using a customized gene panel. Because of second-grade parental consanguinity, homozygous variants were prioritized.

Cell culture and western-blot
Skin cultured fibroblasts from the patient and controls were grown in standard medium. FBXO7 expression and mitophagy-related proteins (PINK1, Parkin, K63 poly-UB, VDAC1) were studied by Western blot in homogenate and mitochondrial enriched fractions.

Nonsense-mediated mRNA decay (NMD) assay
Proband and control fibroblasts cultures were treated with emetine dihydrochloride hydrate, 14 a specific inhibitor of translation. RNA was extracted and retro-transcribed, and the resulting cDNAs underwent qPCR for the quantification of FBXO7 RNA expression.

Ubiquitin-proteasome system activity and expression assays
Chymotrypsin-like activity determination was done measuring fluorescence intensity after incubation of the proband and control fibroblasts' protein extract with a proteasome activity buffer and a fluorogenic substrate. Ubiquitinated-protein levels were quantified through a WB assay using an anti-UB antibody (Sigma-Aldrich, St. Louis, USA).

Electronic microscopy
Ultra-thin sections were examined under a transmission electron microscope FEI Tecnai Spirit BioTwin using a digital camera Morada (see Supplemental File).

Case Presentation
The proband is currently a 21-year-old girl born to healthy consanguineous parents from Morocco. After a normal perinatal history, she presented with mild global developmental delay followed by acute ataxia triggered by a viral gastroenteritis at 2 years. When she was 5 years old, valproate was started for absence epilepsy. She was lost to follow-up until the age of 12, when she was admitted to the intensive care unit due to acute parainfectious H1N1 encephalopathy. Neurological examination identified horizontal nystagmus, head tremor, dysmetria, lower limb spasticity, hyperreflexia, clonus, bilateral Babinski sign, and bladder dysfunction.
Between the age of 12 and 18 years the patient suffered progressive deterioration, including progressive spastic ª 2020 The Authors. Annals of Clinical and Translational Neurology published by Wiley Periodicals LLC on behalf of American Neurological Association paraparesia and gait loss at 13 years, language and cognitive regression, drug-resistant seizures, severe dysphagia, and optic neuropathy. At the age of 15, hypokinesia, rigidity, kinetic tremor, and upgaze limitation were identified. A trial with levodopa (100g/day) did not show a positive response (Video). Serial brain and medulla MRI studies from 10 to 17 years disclosed slight vermian atrophy progressing to cerebral and cerebellar atrophy, and a hot cross bun sign suggesting ponto-cerebellar tract degeneration. Excessive brain iron deposition in the pallidum and substantia nigra appeared as hypointense signal on iron-sensitive sequences at 15 years, which led us to suspect a causative relation with the onset of parkinsonian features ( Fig. 1). At 20 years, a brain DaTSCAN showed normal uptake.

Genetic findings
Data analysis of a custom gene panel identified two homozygous variants: c.100A>G (p.T34A) in DLD (NM_000108.4) and c.368C>G (p.S123*) in FBXO7 (NM_012179.3) ( Fig. 2A). In parallel, exome sequencing analysis revealed the same findings (data not shown). In silico predictors showed that DLD p.T34A (rs138002793; MAF = 5.1 9 10 -4 ) was probably benign. DLD enzyme activity assay in patient's fibroblasts was considered within the normal range of activity. According to these findings and the patient's clinical record, we ruled out the implication of DLD. Although gene panel data analysis disclosed a moderate number of single-exon CNVs in the proband, array-CGH found no pathological results (data not shown).

Functional studies
The novel FBXO7 c.368C>G (p.S123*) change would produce a very short protein where the only functional domain preserved would be the ubiquitin-like domain (Fig. 2B). Protein expression analysis showed the absence of FBXO7 protein in WB (Fig. 2C). mRNA expression was investigated by NMD assay confirming a significant decrease in FBXO7 mRNA in patient's fibroblasts compared to control (P < 0.05). Emetine incubation increased total mRNA in patient's fibroblasts up to control levels, thus confirming a NMD mechanism as a cause of loss of function effect (Fig. 2D).
Loss of FBXO7 is related to decreased proteasome activity. 10 A significant reduction of 20% in UPS activity was observed in patient's fibroblasts (Fig. 2E). We hypothesized that impaired UPS would not be able to degrade the poly-UB labeled proteins and we found an increase in these proteins in proband's fibroblasts (Fig. 2F).
FBOX7 is also involved in mitophagy. 12,13 Mitophagyrelated proteins studies showed no significant differences in mitochondrial enriched fractions in patient's fibroblasts (Fig. S1A). However, elevated mitochondrial proteins in mutant cells were observed, possibly due to accumulated mitochondria (Fig. S1B). Mitochondria analysis by electron microscopy revealed abnormal cristae morphology in ultra-thin sections images (Fig. S1C).
We observed a striking association between the onset of parkinsonian features and the occurrence of brain iron accumulation on MRI at 15 years. These findings, together with poor levodopa response and normal dopamine uptake suggested a likely postsynaptic degeneration condition overlapping with NBIA disorders. This contrasts previous reports showing a severe nigrostriatal dopaminergic defect in two patients carrying FBXO7 mutations. 3,4 Moreover, the patient suffered from cerebellar ataxia, oculomotor dysfunction, severe dysphagia, and cognitive decline. These features could be related to the progression of cerebellar atrophy and the appearance of a hot cross bun sign at the pons, also described in patients with multiple system atrophy or spinocerebellar ataxia. 15 Neither brain iron accumulation nor the hot cross bun sign have been reported in FBXO7 patients, mostly having normal structure or mild global brain atrophy on MRI (Table S1).
Previous FBXO7 patients with nonsense variants had the onset of core features within the second decade of life, and progression to severe parkinsonism, major disability or early death in five of 13 cases. [3][4][5][6]8,9 However, none of them developed epilepsy or cerebellar ataxia, two atypical features of our patient. On the other hand, patients with missense variants showed milder phenotypes, such as young onset parkinsonism or isolated SPG, probably due to a possible residual activity of FBXO7 7 (Table. S1).
The FBXO7 c.368C>G (p.S123*) nonsense mutation is located in the proximal region of the protein. According to our results, it would produce an aberrant mRNA, which was degraded by NMD, leading to a complete absence of FBXO7 protein and a loss of function effect. NMD is a well-known RNA quality control that limits the expression of mRNAs with premature termination codons. 16,17 Previously, two additional nonsense FBXO7 mutations (p.R498* and p.E470*) were reported. 3,9 The absence of expression of p.R498* was demonstrated in a human cell model, however, NMD process was discarded probably due to its location near the C-ter. 18 FBXO7 plays a regulatory role in proteasome and mitochondria. The FBXO7 knockdown in mice results in a decrease in UPS activity. 10 We have demonstrated that the UPS activity was reduced in FBXO7-PPS patient's fibroblasts, and as a consequence, the poly-UB proteins showed a trend to accumulate. Moreover, our findings suggest a likely mechanistic relationship between proteasome impairment and iron accumulation, previously observed in experimental models of PD. A mice model of PD induced by the proteasome inhibitor lactacystin showed loss of dopamine neurons, abnormal iron accumulation, and elevated iron regulatory protein 2 (IRP2) and divalent metal transporter 1 (DMT1) in the substantia nigra. 19 Also, the in vitro lactacystin dopamine cell line model showed an increase in labile iron, disruption in iron regulatory proteins, and aggregation of ubiquitinconjugated proteins, leading to cell premature death. 20 Taken together, these findings suggest that alterations in iron regulatory proteins due to proteasome dysfunction may lead to dopamine neuron degeneration.
In addition, PINK1/Parkin-mediated mitophagy is facilitated by FBXO7 and dependent on ubiquitin. 11,13,[21][22][23] We have not found differences in the expression of mitophagy-related proteins between mutant and healthy fibroblasts. However, elevated mitochondrial proteins in mutant cells were observed, possibly due to accumulated mitochondria.
Mitochondrial cristae alterations are associated with mitochondria impairment. 24 In a transgenic Drosophila model, the overexpression of FBXO7 leads to broken cristae and accumulated high-density material in the swollen mitochondria. 11 We observed abnormal mitochondrial cristae morphology in patient's fibroblasts, likely as a secondary consequence, since it is commonly seen in neurodegenerative diseases, including NBIA forms. [25][26][27] Our results have major limitations and should be interpreted with caution as they have been demonstrated in a single patient harbouring FBXO7 p.S123* mutation. Further studies are needed to clarify if proteosome impairment, mitophagy dysfunction, and iron accumulation are the main biological mechanisms leading to PPS in FBXO7 patients.
In conclusion, we describe a complex and severe FBXO7-related phenotype with a likely postsynaptic mechanism of neurodegeneration, which overlaps with other NBIA monogenic diseases. The absence of FBXO7 led to impaired proteasome degradation and accumulation of poly-ubiquitinated proteins, which highlights the essential role of the UPS in the disease mechanism.
analysis of the array-CGH. We are also in debt with Jos e M. Garcia-Verdugo, David Pla-Mart ın, and Candela Machuca-Arellano who helped us with the electronic microscopy, and with Francisco Garc ıa-Garc ıa who helped us with the statistical analysis.

Supporting Information
Additional supporting information may be found online in the Supporting Information section at the end of the article.
Video Segment A. The patient at 13 years old is in a wheelchair due to spastic paraplegia. Video Segment B. The patient at 15 years old has severe hypomimia, bradykinesia, and low amplitude kinetic tremor while throwing the ball. Video Segment C. Oculomotor features of patient at 16 years old are horizontal nystagmus and reduced upgaze during smooth pursuit. Video Segment D. Neurologic assessment at 21 years old reveals lower limbs hyperreflexia, bilateral Babinski sign, and Achilles clonus. On a second frame, we also observe upper limb bradykinesia, action tremor, and myoclonus. File S1. Additional information regarding materials and methods, a supplementary figure and a supplementary table are included in a supplementary material file.