Since both the clinical features and the mutation characteristics of SMA are obvious, the diagnosis of SMA is considered as relatively easy process. However, a recent review reported that the diagnostic process for SMA is not always simple, and there is usually a delay between the onset of clinical features and the diagnosis in all types of SMA [15]. At present, MLPA is the gold standard for clinical diagnosis of SMA. However, MLPA can only detect the deletion of SMN1 according to the gene copy number, not detect point mutations of SMN1. It is well known that about 4% of SMA patients bear one SMN1 copy with an intragenic mutation. Therefore, some SMA patients are inevitably misdiagnosed as carriers. In addition, the emergence of new therapies increases the need for early diagnosis of SMA, the approval of therapies and the neonatal screening programs urgently require a more detailed understanding of genetic variation [16]. In this study, Proband-3 was with one SMN1 copy and the SMN1 stop-gain mutation c.[271C>T], and the heterozygous deletion of SMN1 exon 7 was from her mother, and the SMN1 stop-gain mutation c.[271C>T] from her father. The SMN1 stop-gain mutation c.[271C>T] was never reported before, and it led to a amino acid change. Although MLPA results showed Proband-3 to be carrier, some SMA-related clinical features were occurred on her. Here, we suspected that Proband-3 might be a SMA patient caused by the heterozygous deletion of SMN1 exon 7 combined with the SMN1 stop-gain mutation c.[271C>T]. Simultaneously, c.[271C>T] might be involved in the onset of SMA. In addition, [2+0] genotype carriers are two SMN1 copies on one chromosome and with deletion of SMN1 on the other chromosome [17]. In this article, we found 2 patients (Proband-1 and Proband-2) whose one parent was carriers and the other parent with 3 SMN1 exon7 copies (Proband-1’s mother and Proband-2’s father). Based on our results we suspected that Proband-1’s mother and Proband-2’s father might be [2+0] genotype carriers.
SMN1 and SMN2 present on chromosome 5q13, and of the 5q13-linked SMA patients, 96.4% show homozygous absence of SMN1 exons 7 and 8 or exon 7 only, whereas 3.6% present a compound heterozygosity with a subtle mutation on one chromosome and a deletion/gene conversion on the other chromosome [6]. Due to the complexity of 5q chromosome structure, the mechanism of SMA has not been fully elucidated. For example, the rare variations in SMN2 have been described by several studies [18-20], and some scholars believe that the variations in SMN2 locus, such as the deletion of adjacent NAIP1 gene, will affect or even change the severity of SMA [21, 22]. With the development of bioinformatics, more and more mutations have been discovered in SMN1, and some of them possess significant clinical implications. Yamamoto et al [23] revealed 4 intragenic mutations (p.Ala2Val, p.Trp92Ser, p.Thr274TyrfsX32 and p.Tyr277Cys), and location of the mutations were associated with the clinical severity of SMA. Ronchi et al [24] described a novel SMN1 mutation that affected the donor splice site of exon 7 and resulted in an unusually severe SMA phenotype with rapid fatal outcome in an Italian infant. In this article, we found 6 SMN1 SNVs in 28 core families of suspected SMA patients, including 4 novel mutations c.[84C>T], c.[271C>T], c.[-39A>G] and g.[70240639G>C], which had never been previously reported. Besides, we identified more mutations combined with homozygous absence of SMN1 exons7 (Table 2). The 3 most frequent mutations were the insertion mutation c.[-41_-40insCTCT] in SPTA1 exon1 (rs111674514), the SNV c.[1001A>G] in FUT5 exon2 (rs778984), and the SNV c.[-117A>G] in MCCC2 exon1 (rs11746722). SPTA1 encodes the human erythroid alpha-spectrin, which is an actin crosslinking and molecular scaffold protein that links the plasma membrane to the actin cytoskeleton, and functions in the determination of cell shape, arrangement of transmembrane proteins, and organization of organelles [25, 26]. Mutations in SPTA1 can lead to a variety of hereditary red blood cell disorders, including elliptocytosis type 2, pyropoikilocytosis, and spherocytic hemolytic anemia [27, 28]. FUT5 encodes alpha1,3-fucosyltransferase in human, the down-regulation of FUT5 reduces the expression of sialyl-Lewis antigens and the adhesion and binding capacities of gastric cancer cells [29]. Gene transfer of alpha1,3-fucosyltransferase increased tumor growth of the PC-3 human prostate cancer cell line through enhanced adhesion to prostatic stromal cells [30]. Methylcrotonyl CoA carboxylase β (MCCβ) is encoded by MCCC2, and point mutations and deletion events in MCC2 can lead to MCC deficiency [31]. MCC deficiency is a rare autosomal recessive genetic disorder whose clinical presentations range from benign to profound metabolic acidosis and death in infancy, which is has something in common with SMA in some ways. MCCC2 locates on chromosome 5q13, which was the same as SMN1. Some studies indicated that SMN1 was the causative gene, and other genes on 5q13 region acted as modifier gene (such as SMN2, NAIP and GTF2H2), which were associated with disease severity [32]. The mutations rs111674514 in SPTA1, rs778984 in FUT5 and rs11746722 in MCCC2 have been identified previously, but the clinical significance remains uncertain. In this article, we found they were widely prevalent in SMA patients, and almost nonexistent in non-patients. Therefore, it suggested they might be involved in the morbidity of SMA.
One limitation of this study is the failure to use healthy children as control. The reason is that the children involving in this study are younger (0 to 12 years old), many parents are reluctant to let their healthy children participate in the study because of insufficient understanding of genetic testing. Another objective reason is that the cost of sequencing is high, so parents of healthy children are unwilling to pay for it. However, in terms of the rationality of the entire study, we really should add healthy children as control to make our research more complete, and that is what we will improve in the follow-up related studies. In contrast, using non-SMA patients with similar clinical characteristics of SMA as a control could exclude some genetic mutations that may lead to similar clinical characteristics of children with SMA, so as to make the object of this study more accurate. Using this population as a control can exclude other mutations that may cause dyskinesia, and only retain mutations unique to SMA patients.