A total of 245 patients with possible autosomal recessive traits or negative family history were recruited from multiple hospitals in China from January 2012 to August 2021, which had excluded the previously reported recessive families (Yao et al., 2018). The criteria for the diagnosis of PFBC were as follows: 1) bilateral and symmetrical calcifications in the basal ganglia and/or dentate nucleus detected by CT scans; 2) a total calcification score (TCS) rates above the age-specific thresholds (Nicolas et al., 2013a); 3) absence of biochemical abnormalities, including serum concentration of calcium, phosphate, and parathyroid hormone; 4) secondary causes of brain calcification were excluded such as infectious, toxic, or traumatic causes. All sporadic patients were previously tested for variants of all AD-PFBC genes by Sanger sequencing, and no pathogenic variants were detected (SLC20A2, PDGFRB, PDGFB, and XPR1). For all patients, a complete neurological examination was performed by two neurologists. The calcifications in the cerebral locations were further evaluated with TCS (range from 0 to 80). In cases with biallelic MYORG variants, previous investigations were retrospectively analyzed based on a chart review where available: neuroimaging in all reported cases with CT (n = 3) and brain MRI (n = 1). We also recruited 200 individuals without brain calcification as normal controls. The study was approved by the institutional review board at the First Affiliated Hospital of Fujian Medical University. All subjects provided informed consent before inclusion.

We collected venous blood samples from all participants including all available family members. Genomic DNA was extracted from peripheral blood leukocytes using standard protocols. Polymerase chain reaction (PCR) was performed to amplify the coding exon (exon 2) of the MYORG gene (NM_020702.5), using the primers previously reported (Yao et al., 2018). The PCR products were purified and analyzed by Sanger sequencing with ABI 3730XL automated DNA-sequencing system. The sequence data were further analyzed and compared with reference MYORG coding sequences from the Human Genome database (NM_020702.5).

The identified variants that fulfilled the following criteria were included for further analysis: 1) excluded variants with frequencies exceeding 0.1% in the 1,000 Genomes Project (www.1000genomes.org), Exome Aggregation Consortium (ExAC, http://exac.broadinstitute.org/), or Genome Aggregation Database (gnomAD v2.1.1; http://gnomad.broadinstitute.org); 2) excluded synonymous variants and missense variants, which were predicted to be nonpathogenic in silico by Mutation Taster (http://www.mutationtaster.org/), Polyphen2 (http://genetics.bwh.harvard.edu/pph2/), or SIFT (http://sift.jcvi.org/). The evolutionary conservation of the affected amino acid among different species was estimated using HomoloGene (http://www.ncbi.nlm.nih.gov/homologene). All novel variants were independently classified by two investigators based on the American College of Medical Genetics and Genomics (ACMG) guidelines and the Association for Molecular Pathology (Richards et al., 2015).

We screened a total of 245 Chinese subjects including 21 subjects from 10 possibly autosomal recessive families and 224 sporadic cases. Eight MYORG variants were identified in six sporadic cases, while four of the eight variants were previously reported (c.103A > G, p.M35V; c.782_783GC > TT, p. R261L; c.1092_1097delCTTCGA, p.365_366delFD; and c.1967T > C, p. I656T) (Supplementary Figures S1A–D) (Yao et al., 2018; Forouhideh et al., 2019; Chelban et al., 2020; Chen et al., 2020). Notably, four novel variants in MYORG were identified: two nonsense variants (c.442C > T, p. Q148*; c.972C > A, p. Y324*) and two missense variants (c.1969G>C, p. G657R; c.2033C > G, p. P678R) (Figures 1A–D). The variants, c.442C > T and c.2033C > G, were separately found in a homozygous state in case 1 and case 4, while c.972C > A and c.1969G>C were identified in a heterozygous state in case 2 and case 3, respectively coupled with the previously reported variants (c.103A > G and c.782_783GC > TT) (Table 1).

None of the novel variants mentioned above were present in the 1000G, ExAC, or gnomAD (Table 1). In silico analysis predicted deleterious consequences using the Mutation Taster, SIFT, Polyphen2, and CADD software programs. The two missense variants were both located at the highly conserved positions and the glycosidase domain (Figure 2A). Based on the American College of Medical Genetics (ACMG) guidelines, the two nonsense variants were considered as “Pathogenic;” the missense variant c.2033C > G was considered as “Likely Pathogenic;” and c.1969G>C was considered as “Variants of Uncertain Significance” (Table 1). Four of the 224 sporadic PFBC (1.79%) carried variants in MYORG in this study.

The clinical manifestations of the patients with novel MYORG variants are summarized in Table 1. All four patients showed extensive calcification involving the basal ganglia, dentate nuclei, thalamus, and the subcortex in CT/MRI scans. Patients displayed a homogeneous clinical pattern and commonly experienced parkinsonism, dysarthria, ataxia, and vertigo. Detailed clinical and radiological findings of the patients are described as follows.

Case 1. The patient with a c.442C > T nonsense homozygous variant was a 73-year-old man who was admitted to the hospital because of dysarthria, gait impairment, and vertigo. These symptoms were experienced for 7 years. There was an initial progressive slurred speech, walked unsteadily, starting hesitantly with reduced up and down gaze, associated with profound bilateral bradykinesia, and a combination of ataxia and freezing. Progressive deterioration of dysarthria and bradykinesia became evident over the following years. He had difficulty in tandem walking and could not walk independently. A neurological examination revealed cerebellar dysarthria, supranuclear gaze palsy, bradykinesia, festinating gait, and mild rigidity in the lower limbs; no tremor was observed. His cerebral MRI at age 72 years showed high-intensity in the globus pallidus, thalamus, dentate nuclei, and subcortical white matter, suggesting moderate symmetrical calcification (Figures 2Ba–c). The patient reported no family history of brain calcification.

Case 2. The patient, carrying c.972C > A and c.103A > G heterozygous variants of MYORG, was a 47-year-old woman who had slurred speech with slow progression. She later developed dysphagia and forced laughter or crying. No other abnormalities were observed, including gait disorder, bradykinesia, involuntary movements, or psychiatric disorders. A neurological examination revealed dysarthria, forced laughter, and a positive Huffman’s sign. Her CT images (TCS, 43) showed severe calcification at the bilateral basal ganglia, thalamus, dentate nuclei, and subcortical white matter (Figures 2Bd–g). Unfortunately, her parents were unable to provide brain CT or blood samples.

Case 3. The patient who carried c.1969G>C and c.782_783GC > TT heterozygous variants was a 68-year-old female from Northern China. She presented with 23 years of vertigo and had a previous history of cerebral infarction, cerebral hemorrhage, hypertension, and coronary heart disease. A neurological examination was unremarkable. Laboratory tests showed normal levels of serum calcium, phosphorus, and parathyroid hormone. Her brain CT reported symmetrical calcification at the basal ganglia, thalamus, dentate nucleus, and corona radiata though a complete series of images was not available (Figure 2Bh). Unfortunately, we could not examine her parents because they have both passed away.

Case 4. The 62-year-old man carrying the homozygous c.2033C > G variant experienced disease onset at the age of 59, with slowly progressive gait unsteadiness, reduced up and down gaze and slurred speech. A neurological examination revealed mild dysarthria, bradykinesia, rigidity of the limbs, staggering in tandem gait, and poor pointing performance of the finger-to-nose test. No other abnormalities were found, including psychiatric disorder, seizure, memory disturbance, or involuntary movements. His CT images (TCS, 57) revealed prominent calcification in the basal ganglia, thalamus, dentate nuclei, cerebellar vermis, and subcortical white matter (Figures 2Bi–l). Extensive brainstem calcifications affecting the pons and mesencephalon were also observed. Moreover, cerebellar atrophy could also be witnessed in the CT images (Figures 2Bi-j). Unfortunately, brain CT and genetic screening of his parents were unavailable due to their death.