Fourteen SMA patients and their parents, from 13 unrelated families, were enrolled in this study. All patients met the diagnostic criteria of proximal SMA, with their clinical data provided in Table 1. Of these cases, three were diagnosed as type I SMA, nine were type II SMA, and two were type III SMA. Case 9 was the younger sister of case 8. Genomic DNA and total RNA from these individuals were isolated from peripheral venous blood using phenol-chloroform extraction and an RNeasy Kit (Qiagen, Germany), respectively. Samples of the parents of cases 1 and 7 were not available. This study was approved by the Ethics Committee of the Capital Institute of Pediatrics, and informed consent was obtained from all subjects.

Conversion means deletion of SMN1 owing to conversion of SMN1 sequences to SMN2 with the copy number of SMN2 increasing. ND, not detected. §Novel mutation; #,these patients had been reported 22 ; †, Walk in waddling gait ;case 8 and case 9 are siblings.

Cloning and sequencing of reverse transcription polymerase chain reaction (RT-PCR) amplicons was carried out to analyze subtle mutations. First-strand cDNA synthesis was performed with 0.5 μg of total RNA, random primers, and M-MLV Reverse Transcriptase (Invitrogen, USA) in accordance with the manufacturer’s instructions. Specific PCR primers (SMN575 13 and 541C1120 4 ), were used to amplify the SMN gene (exons 1–8) using LA Taq polymerase (TAKARA, Japan) and cDNA template. Thermal cycling conditions involved an initial denaturation step for 5 min at 94°C, followed by 30 cycles of 45 s at 94°C, 50 s at 60°C, and 60 s at 72°C, with a final extension step at 72°C for 10 min. Amplicons were subcloned into the pGEM-T Easy cloning vector (Promega, USA) according to the supplier’s protocol. SMN1and SMN2 subclones were differentiated using restriction enzymes (DraI and DdeI) 25 . Around 5 ~ 8 SMN1 and 2 ~ 3 SMN2 clones for each case were sequenced. Mutations were further confirmed by direct sequencing of the amplified products from SMN genomic DNA samples.

MLPA analysis was performed to detect copy numbers of SMN1 and SMN2 in all cases using a SALSA MLPA kit (P021-A1; MRC-Holland, Amsterdam, The Netherlands) according to the manufacturer’s recommendations. This SALSA kit contained 16 probes specific for the SMA critical region (5q12.2–q13.3). Among these, two specific probes for the C→T transition in exon 7 (C for SMN1 and T for SMN2) and two specific probes were for the G→A transition in exon 8 (G for SMN1 and A for SMN2) were included. In addition, the SALSA kit contained 21 control probes mapping to other autosomes. After MLPA treatment, products were run on the ABI 3730 automatic sequencing system (Applied Bio-Systems, USA). Four healthy individuals carrying two SMN1 copies were the normal controls, with eight carriers (parents of the patients with a homozygous SMN1 deletion) as the single copy SMN1 reference. For each sample, raw data [relative peak area (RPA)] were analyzed and compared with normal controls using Gene marker version 1.75 software. This software is able to calculate the RPA for each probe and to compare RPAs with those derived from normal controls. All samples were analyzed at least twice. A ratio with normal controls in the range 0.7–1.3 indicated a normal copy number (two copies), a ratio less than 0.7 indicated one copy, a ratio between 1.3–1.6 was indicative of three copies, and a ratio equal to 0 indicated zero copy.

The allele-specific primer, Y277CR (5′-CTG AGT GAT TAC TTA CCA TAC-3^′), was designed to identify only the mutant allelic sequence, and was coupled with the upstream primer SMNE6F 12 . This was applied in an allele-specific PCR (AS-PCR) to screen for the p.Tyr277Cys mutation in 150 control individuals. Simultaneously, alignment analysis of SMN proteins from six different species was performed using Clustal X version 1.8 to analyze levels of conservation for tyrosine 277.

Total RNA (0.5 μg) was isolated from the peripheral blood of patients and controls, and used to synthesize first-strand cDNA as described earlier. The cDNAs were amplified using primers SMN575 13 and 541C1120 4 in a 50-μl reaction with a 60°C annealing temperature for 30 cycles as the section of “Analysis of subtle mutations in SMN1 ”described. In general, SMN transcripts yielded three products, full-length SMN1 (fl-SMN1, 1259 bp), full-length SMN2 (fl-SMN2, 1259 bp) and SMN2 isoform lacking exon 7 (Δ7-SMN2, 1205 bp). The SMN1 transcripts could be distinguished from SMN2 transcripts by digestion with the restriction enzyme DdeI. Following digestion, there was a 1259-bp fragment corresponding to fl-SMN1, a 1136-bp fragment corresponding to fl-SMN2, a 1082-bp fragment indicative of Δ7-SMN2 and a 123-bp fragment from SMN2. The transcripts and their products after DdeI digestion were separated on a 6% polyacrylamide gel at 500 volts for 2 h. Gels were stained with silver stain.

Three plasmids (fl-SMN1, fl-SMN2 and GAPDH) were constructed as external standards. Amplified SMN1 and SMN2 were obtained using normal control cDNA and primers SMN-F (5^′-GCT GAT GCT TTG GGA AGT ATG TTA-3^′) and SMN-R (5′-TCA ACT GCC TCA CCA CCG TGC TGG-3′), specific for exons 6 and 8, respectively. The primer pair for amplification of GAPDH was GAPDH_exst-F and GAPDH_exst-R, as previously described 26 . Amplicons for SMN1/SMN2 (395 bp) and GAPDH (133 bp) were cloned into the pGEM-T Easy cloning vector (Promega, USA). Cloned inserts were all verified by sequencing. Plasmid DNA was extracted and quantified by absorbance using a NanoDrop 2000 (Thermo, USA). Based on plasmid length and concentration, the copy number of each plasmid can be calculated. These plasmids were serially diluted across a range (10³–10⁸ copies) and used as external standards to construct the standard curve.

A qPCR assay to quantify SMN transcripts was conducted as described by Tiziano et al. 26 . The primers and MGB-probes were designed using Primer Express v1.5 software (Applied Biosystems, USA), with sequences provided in Table 2. The fl-SMN1 and fl-SMN2 transcripts were amplified using the same primer pair (SMN_mgb-F and SMN_mgb-R). Full-length transcripts of the two genes were distinguished by two different Taqman MGB probes on the basis of the C→T transition located in exon 7. For GAPDH, the primers (GAPDH_abs-F and GAPDH_abs-R) and MGB probe sequence were the same as those described in Tiziano et al. 26 described. All reactions (20 μl) were carried out using a 7500 Real-Time PCR System (Applied Biosystems, USA) and contained 2× GoldStar TaqMan Mixture (KANGWEI, China), 20 ng of cDNA, 0.4 μl of each primer (10 pmol/μl), and 4 pmol of the SMN1, SMN2 or GAPDH probe. The thermal cycling conditions involved 2 min at 50°C then 10 min at 95°C, followed by 40 cycles of 15 s at 95°C and 1 min at 60°C. Each sample was assayed in duplicate and repeated at least twice. Evaluation of data was performed using 7500 Software SDS version 1.4.

The bases C and T in bold are specific for SMN1 and SMN2, respectively. The primers and probe sequences of GAPDH are described by Tiziano FD et al. 26 .

Transcript levels for fl-SMN1, fl-SMN2 and GAPDH were expressed as copies per nanogram of total RNA. Expression levels of fl-SMN1, fl-SMN2, and fl-SMN were normalized to GAPDH. Statistical analysis was carried out using SPSS 19.0. A parametric test (t-test) was used to compare the transcript levels between normal controls and carriers, as well as between carriers and patients. Correlation between SMN2 gene copy numbers and fl-SMN2 transcript levels were analyzed by a gerneral linear model(one-way ANOVA). A p-value less than 0.05 was regarded as significant.

The numbers of SMN1 and SMN2 copies in the 14 patients analyzed by MLPA are presented in Table 1. All patients carried only one copy of SMN1. Patients 3, 7, 11, 12, and 14 carried three copies of SMN2. The remaining patients had two copies of SMN2.

Six subtle mutations were identified in the present study (Table 1). Five mutations (p.Ser8LysfsX23, p.Leu228X, p.Ser230Leu, p.Glu134Lys, and p.Arg288Met) were detected in more than one patient. A novel mutation (p.Tyr277Cys) located in exon 6 of SMN1 was identified for the first time (Figure 1A). The p.Arg288Met mutation has been previously described 22 . No subtle mutations were detected in two of the patients carrying one copy of SMN1.

AS-PCR was performed to screen for the novel p.Tyr277Cys mutation in control individuals (Figure 1B). This mutation was not observed in the 150 control individuals. Sequence alignment of six different species showed that the Tyr277 residue was highly conserved (Figure 1C).

A DdeI digest of SMN transcripts assay was carried out to qualitative analysis the SMN transcript in all the patients with subtle mutations. Following DdeI digestion, three obvious products (fl-SMN1, fl-SMN2 and Δ7-SMN2) were detected, without obviously truncated or prolonged transcripts in most patients (Figure 2). While in patients carrying the p.Arg288Met mutation, the fl-SMN1 transcript (1259 bp) was rare, but the undigested Δ7-SMN1 fragment (1205 bp) was more prominent (Figure 2). An undigested Δ7-SMN1 fragment was also observed in their father with the p.Arg288Met mutation.

The SMN cDNA (from exon 1 to exon 8) of patients with p.Arg288Met were amplified and subclone to the pGEM-T vector. After screening the SMN1 clones and sequencing, we found that all 5 subclones of SMN1 from these patients had lost the entire sequence of exon 7 (Figure 3), while three full-length SMN clones belong to the sequences of SMN2. This result was consistent to the result of DdeI digest of SMN transcripts assay. The p.Arg288Met mutation produces a transcript of Δ7-SMN1 other than the transcript of fl-SMN1, it implies that it might cause the skip of exon 7 of SMN1 gene.

To evaluate the effect of subtle mutations on fl-SMN1 levels, we compared fl-SMN1 levels in patients with that of normal controls, and with healthy carriers (Table 3 and Figure 4). The fl-SMN1 levels in normal controls and healthy carriers were 23.77 ± 7.74 and 9.47 ± 5.39, respectively. The difference between these two groups was statistically significant (t = 5.296, P = 0.000). The fl-SMN1 transcript levels in all patients were significantly decreased compared with normal controls (t = 7.839, P = 0.000). Compared with healthy carriers carrying one copy of SMN1, patients with the p.Glu134Lys or p.Ser230Leu mutation showed no significant difference (t = 1.769, P = 0.094 and t = 1.660, P = 0.115, respectively), patients with the novel p.Tyr277Cys mutation presented a slight decrease in fl-SMN1 transcript levels (t = 2.337, P = 0.032), while the patients with the p.Ser8LysfsX23, p.Leu228X, and p.Arg288Met mutations were significantly reduced (t test, P = 0.000). Especially for the patients carrying p.Arg288Met, fl-SMN1 transcript levels were almost undetectable (0.017 ± 0.15).

fl -SMN1, GAPDH ,and corrected fl- SMN1 indicate transcript levels, measured as no. of molecules per nanogram of total RNA. Superscripted a means that the t-test was carried out between controls and carriers; Superscripted b means the t-test was performed between carrier and the patients with subtle mutations.

Although there was no correlation between fl-SMN2 transcript level and SMN2 copy numbers (one-way ANOVA, F = 0.391, P = 0.679) in normal controls and healthy carriers, the fl-SMN2 transcript level was increased along with SMN2 copy numbers (Figure 5). The fl-SMN2 transcript levels in patients are presented in Table 1, with no significant differences (F = 1.029, P = 0.430). Total fl-SMN transcript levels (fl-SMN1 + fl-SMN2) were used to assess the correlation between the fl-SMN levels and the clinical severity. The fl-SMN transcript levels in normal controls and healthy carriers were 34.4 ± 7.1 and 21.7 ± 12.7, respectively, with a significant difference (t = 2.596, P = 0.017). The fl-SMN transcript levels in all patients were significantly decreased compared with normal controls (t = 7.060, P = 0.000). Mean fl-SMN transcript levels in type I (n = 2) and type II (n = 8) were 11.27 ± 6.8 and 11.67 ± 6.34, respectively. For type III (n = 2) patients, a slight increase in levels could be observed (20.00 ± 9.43). Because the number of types I and III patients were low, statistical analysis of fl-SMN transcript levels was only carried out between type II patients and healthy carriers, with a significant difference observed (t = 3.046, P = 0.009).