Nepal Journal of Biotechnology. D e c .  2 0 1 6  Vol. 4, No. 1: 37-42   ISSN 2091-1130(Print)/ISSN 2467-9319 (online) 

 
ORIGINAL RESEARCH ARTICLE 

©NJB, Biotechnology Society of Nepal    37        Nepjol.info/index.php/njb 

Multiplex Ligation Dependent Probe Amplification Based 
Mutation Analysis of Dystrophin Gene in Nepalese Patients 

with Duchenne Muscular Dystrophy 
Kushal Shrestha1, Smita Shrestha2, Mr. Saroj Khatiwada3, Bishnu Acharya4, Sulochana Manandhar5, Rohit Kumar 

Pokharel6,7 * 
1Central Department of Biotechnology, Tribhuvan University, Kirtipur, Nepal. 
2Central Department of Biotechnology, Tribhuvan University, Kirtipur, Nepal. 

3Department of Biochemistry, Modern Technical College, Lalitpur, Nepal. 
4Muscular Dystrophy Foundation-Nepal (MDF-Nepal), Lalitpur, Nepal. 

5Center for Molecular Dynamics-Nepal (CMDN), Nepal. 
6Muscular Dystrophy Foundation-Nepal (MDF-Nepal), Lalitpur. 

7Department of Orthopedics and Trauma surgery, IOM, Tribhuvan University, Kathmandu, Nepal. 

Abstract 
Duchenne muscular dystrophy (DMD) is X-linked recessive neuromuscular disorders caused due to mutation in 

dystrophin gene, leading to progressive muscle weakness. This study was done to identify mutation in 

dystrophin gene in Nepalese patients with DMD using Multiplex Ligation Dependent Probe Amplification 

(MLPA) assay in Nepal. Twenty one patients from different regions of Nepal, who were clinically diagnosed as 

DMD were enrolled in the study. Peripheral blood samples were collected in EDTA vials, gDNA was extracted, 

and deletion mutation in the dystrophin gene was analysed using Multiplex Ligation Dependent Probe 

Amplification (MLPA) assay. 

Exon deletion mutation in the dystrophin gene was observed in 14 (66.6%) out of 21 DMD cases. The most 

common exon deletion was observed and confined in exon 7-14 and 45-53 of dystrophin gene. The location of 

deletion in dystrophin gene is apparently non-random with a preponderance found in the hot spot regions. Use of 

MLPA is useful in detecting copy number changes in DMD proband and suspected carriers in Nepal. 

Keywords: Duchene muscular dystrophy, Multiplex ligation dependent probe amplification, Mutation, Nepal. 

*Corresponding Author 
Email: pokharel.rohit@gmail.com 

 

Introduction 
Duchenne and Becker muscular dystrophies (DMD & 

BMD) are X-linked recessive neuromuscular 

disorders with incidence of 1 in 3,500 and 1 in 30,000 

live male births, respectively [1]. DMD is 

characterized by progressive muscle weakness with 

onset at 3-5 years of age, leading to loss of 

ambulation by 10-12 years of age without treatment. 

Respiratory, orthopaedic, and cardiac complications 

emerge with age, and without intervention, the mean 

age at death is around 19 years [2]. 

Both DMD and BMD are caused by mutations in the 

dystrophin gene (MIM 300377), one of the largest 

known human genes, spanning about 2.4 Mb of 

genomic DNA [3]. The most common mutations in 

the DMD gene are the deletion or duplication of one 

or more exons [3]. Mutations lead to an absence of or 

defect in the dystrophin protein, which results in 

progressive muscle degeneration leading to loss of 

independent ambulation by the age of 13 years. 

Variable phenotypic expression relates mainly to the 

type of mutation and its effect on the production of 

dystrophin [4]. 

Muscular dystrophy is diagnosed on the basis of 

clinical examination, raised creatine phosphokinase 

(CPK) level, muscle biopsy and dystrophin gene 

mutation analysis. The genetic tests commonly used 

to identify dystrophin mutations are multiplex 

polymerase chain reaction (mPCR), multiplex 

ligation dependent probe amplification (MLPA), 

single condition amplification/internal primer, and 

multiplex amplifiable probe hybridization [5]. 

Mutation analysis of dystrophin gene in DMD/BMD 

has been performed in several countries [2, 3]. 

However, no such studies have been performed in 

Nepal. MLPA, a simple and cheaper genetic test to 

detect duplication/ deletion mutation, could be a 

better tool for genetic diagnosis of DMD in Nepalese 

patients; thereby assisting in timely diagnosis, 

treatment and management. We conducted present 

study among clinically diagnosed DMD patients to 

find the mutation pattern in dystrophin gene using 

MLPA and test the efficacy of MLPA in identifying 

mutation in DMD patients in the Nepalese context. 



Nepal Journal of Biotechnology. D e c .  2 0 1 6  Vol. 4, No. 1: 37-42  Shrestha et al.  

  

 

 

©NJB, Biotechnology Society of Nepal    38        Nepjol.info/index.php/njb 

Materials and Methods  
The study was conducted among 21 clinically 

diagnosed DMD patients from different regions of 

Nepal, who were referred to Muscular Dystrophy 

Foundation-Nepal (MDF-Nepal). Diagnosis of DMD 

was done on the basis of clinical presentations and 

markedly elevated serum creatine phosphokinase 

(CPK) levels. Proper genetic counselling was done, 

and consent was taken from each patient and their 

parents. 

Peripheral blood samples (5 ml) were collected from 

each patient in EDTA vials and transported to 

laboratory of Central Department of Biotechnology, 

Tribhuvan University, Kirtipur maintaining cold 

chain. The samples were stored at -200 C until 

analysis. Genomic DNA was isolated from blood, as 

recommended by the MRC-Holland, by using the 

extraction method of the QIAamp DNA mini kit [6]. 

The absorbance of DNA samples were measured at 

230 nm, 260 nm and 280 nm using the UV 

spectrophotometer to check for purity of DNA 

samples required for MLPA assay. 

A commercial MLPA kit (MRC Holland) with probes 

of P034 (DMD exons 1-10, 21-30, 41-50, and 61-70) 

and P035 (DMD exons 11-20, 31-40, 51-60, and 71-79) 

was used to detect DMD deletion/duplication in 

DMD patients according to the manufacturer’s 

recommended protocol (Amsterdam, Netherlands). 

50-250 ng of genomic DNA, in a volume of 5 µL Tris-

EDTA, was denatured at 980 C for 5 min, cooled 

down, and then mixed with MLPA P034 or P035 

probemix. The mixture was then heated to 950 C for 5 

min and incubated at 600 C overnight for probe 

hybridization. After 16 hours, ligation was 

performed with Ligase-65 enzyme at 540 C for 15 min 

and Ligase-65 enzyme was inactivated at 980 C for 5 

min. Then, PCR amplification was performed with 

specific SALSA FAM PCR primers (5’-

GGGTTCCCTAAGGGTTGGA-3’). After that, the 

mixture was separated by capillary electrophoresis 

and then analyzed using ABI-310 Genetic Analyzer 

[7]. 

The Genescan analysis software in the ABI-310 

Genetic Analyzer analyzed the raw data to quantify 

the DNA fragments and determine the size of the 

fragments by comparing them to fragments in a size 

standard. The electropherograms of test samples 

were analyzed by comparing with the peak pattern 

of the male and female reference samples. The novel 

software Coffalyser.net was used to analyze the data 

obtained after the capillary electrophoresis run which 

was further confirmed by visual assessment by 

overlaying two fragment profiles and comparing the 

relative intensities of fragments. The relative peak 

ratio (RPR) of every single exon was plotted to its 

corresponding bar chart [8]. Absence of peaks 

corresponding to two or more contiguous exons was 

taken to represent a genuine deletion. The absence of 

only one peak in males, corresponding to a single 

exon, were also recorded which are yet to be 

investigated further by applying the novel methods 

as PCR primer flanking the exons in question or by 

sequencing. The framedness of the mutation in 

probands were also estimated by using the 

dystrophin exonic deletions/duplications reading 

frame checker 1.9 as recommended by MRC Holland. 

The data from the study was entered into ms excel 

and analyzed using SPSS version 11.0. 

Results  
The mean age of DMD patients at the time of study 

was 11.4 years (age range from 8-18 years). All the 

patients had very high serum CPK level (median: 

6245 U/L, range:  2100-32890 U/L). The genomic 

DNA extracted from samples had concentration 

range within 27-59 μg/mL. The ratio of the optical 

density (OD) of DNA samples at 260 nm and 280 nm 

ranged from 1.5-2.0 with mean OD 1.76. Among the 

21 samples of DMD analyzed by MLPA assay, 

deletions were observed at various exons of 

dystrophin gene in 14 samples. Seven samples 

however did not have any deletion or duplication in 

the exons. Thus, MLPA tool could detect mutations 

in about 66.6% (14 of 21 samples). The most prevalent 

exonic deletion regions were found to be confined in 

the exon 7-14 and 45-53. Deletion mutations at 

different exons observed in samples are shown in 

table 1. Similarly, electropherograms of control 

sample and test sample after MLPA assay with 

SALSA probe mix P034 and P035 are shown in figure 

1. 

As indicated by the dystrophin exonic deletions/ 

duplications reading frame checker 1.9, all the 14 

samples with detection of deletion mutation were 

detected by MLPA assay have out of frame 

mutations suggesting that the samples were those of 

DMD patients. But the confirmation of the 

framedness is yet to be made by gene sequencing, 

and the 7 samples with negative MLPA result need 

further genetic testing like sequencing. 



Nepal Journal of Biotechnology. D e c .  2 0 1 6  Vol. 4, No. 1: 37-42  Shrestha et al.  

  

 

 

©NJB, Biotechnology Society of Nepal    39        Nepjol.info/index.php/njb 

 
Table 1: Exon deletions detected by MLPA assay in 
DMD patients 

Case  Age 
(years) 

Serum 
Creatine 
kinase level 
(U/L) 

Exon 
deletions 

Phenotype  

1 5 12122 48-50 DMD 

2 7 3412 52 DMD 

3 6 14467 10-43 DMD 

4 8 1287 52 DMD 

5 9 11580 45 DMD 

6 5 24200 51-53 DMD 

7 14 22000 45-50 DMD 

8 5 21887 46-49 DMD 

9 12 2700 52 DMD 

10 11 2100 51 DMD 

11 8 4328 12-14 DMD 

12 9 3220 51 DMD 

13 6 9123 45 DMD 

14 7 6245 7-9 DMD 

 
Discussion 
In Nepal, DMD/BMD patients are generally 

diagnosed late due to the lack of complete 

understanding of the disease, poor screening of 

paediatric group for muscular dystrophy and lack of 

genetic diagnostic facilities in the country. Most of 

the cases are diagnosed on the basis of history given 

by the parents, positive clinical signs of DMD and 

very high CK level in the blood. For the diagnosis at 

the gene level clients usually go to or the sample is 

send outside Nepal, which is not accessible and 

affordable to many of the parents. This study to 

detect deletion mutation in DMD using MLPA is first 

genetic pilot study in Nepal.  

Among the 21 samples of clinically diagnosed DMD 

patients, deletion of dystrophin exon was found in 14 

samples (66.6%). However, 7 samples (33.3%) did not 

show any deletion or duplication. Thus, MLPA was 

efficient in accurately confirming mutations in about 

67% of all the cases. A number of studies have found 

MLPA assay to be highly sensitive diagnostic assay 

to identify mutation in DMD and BMD patients [9]. 

In the study to evaluate the efficacy of MLPA 

technique in comparison with the traditional 

multiplex PCR assay in detection of exon deletions 

and duplications of the DMD gene by Lai et al., 

MLPA was able to detect all the known deletions and 

duplications; it detected four additional mutations 

that had been missed by multiplex PCR  [10]. In a 

study in China amongst 70 DMD/BMD patients, 

MLPA detected exonic deletions in 42 patients (60%), 

exonic duplications in 7 patients (10%) and 21 

patients (30%) showed normal results [11]. 

In the present study, only exons deletion was 

observed. No exon duplication was found. We found 

most prevalent exonic deletion regions to be confined 

in the exons 7-14 and 45-53. One, 3, 4, 6 and 44 exons 

deletion was observed in 7, 4, 1, 1 and 1 patients 

respectively. No novel mutations were identified in 

this study. In a study in Iranian DMD/BMD patients, 

30.9 % of patients had single exon deletion, while 

group and contiguous exon deletions were identified 

in 41% of the patients [12]. The most numerous exon 

deletions included exons 45-50, and two exons 3-5 

and 41-43 duplications (1.4 %) was observed in a 

BMD and a DMD patient, respectively [12]. In a 

study in Polish DMD/BMD patients, Zimowski et al. 

identified 110 deletions, 22 duplication (in one 

patient two different duplications were detected) and 

2 point mutations. Deletions involved mainly exons 

45-54 and 3-21, whereas most duplication involved 

exons 3-18 [13]. It has been found that deletions 

account for approximately 60-65% of mutations and 

duplications for 5-10% in DMD/BMD. The 

remaining cases are mainly point mutations (30-35% 

of the cases). Although deletions encompass all 79 

exons, two deletion hotspots (exons 45-55 and exons 

2-19) are recognized [14]. 

Identification of exon deletion is important to design 

gene therapy by exon skipping method that is an 

emerging therapy for DMD that can transform DMD 

into BMD is based on the recovery of reading frame 

induced by alternative splicing of antisense 

oligonucleotides [15]. More patients may benefit 

from individual exon skipping therapies following a 

comprehensive understanding of the correlation 

between genotypes and phenotypes under the 

guidance of large-scale genetic epidemiological 

studies [16]. Similarly identifying disease at earlier 

stage could help in better management of patients 

and thus better life quality. 

This was the first genetic study on DMD in Nepal. 

The location of deletion in dystrophin gene is 

apparently non-random with a preponderance found 

in the hot spot regions in Nepalese population as 

well. Use of MLPA is useful in detecting copy 

number changes in DMD proband and suspected 

carriers. 

 



Nepal Journal of Biotechnology. D e c .  2 0 1 6  Vol. 4, No. 1: 37-42  Shrestha et al.  

  

 

 

©NJB, Biotechnology Society of Nepal    40        Nepjol.info/index.php/njb 

 

A 

B

A 

C

A 



Nepal Journal of Biotechnology. D e c .  2 0 1 6  Vol. 4, No. 1: 37-42  Shrestha et al.  

  

 

 

©NJB, Biotechnology Society of Nepal    41        Nepjol.info/index.php/njb 

Figure 1. Electropherogram of control sample and test sample after MLPA. Fig. 1A and Fig. 1B are for normal control 
sample with P034 and P035 respectively. Fig. 1C and Fig. 1D are for DMD patient with deletion in dystrophin gene with 
P034 and P035 respectively. 

 

Competing Interest 
None  

Acknowledgement 
We appreciate the parents and DMD boys who gave 

consent to take part in this study. We acknowledge 

the support of MDF-Nepal for counseling parents 

and probands, providing the detail information 

about the clients and also bearing the cost of some 

chemicals for gDNA extraction and charge of genetic 

analyzer. We express our gratitude to Prof. Masafumi 

Matsuo, M.D; Ph.D. from Kobe, Japan for providing 

us the MLPA kits, which pioneered the genetic 

testing of DMD cases in Nepal for the first time. We 

thank Prof. Tribikram Bhattarai, former head of 

department of Biotechnology, Tribhuvan University 

and current head Prof. Dr. Rajani Malla for 

encouraging and providing the laboratory for the 

study. We also thank Intrepid Nepal Pvt Ltd.; Centre 

for Molecular Dynamics (CMDN), Thapathali-11, 

Kathmandu, Nepal, for allowing us to use the 

Genetic analyzer at the center. 

Author’s Contribution 
KS, SS and RKP designed the study and collected 

samples. KS, SS, SK, BA and SM engaged in sample 

collection and conducted laboratory analysis. SK 

performed statistical analysis and wrote the 

manuscript. KS, SS and RKP revised the draft. All 

authors read and approved the final version of the 

manuscript. 

References 
1. Hegde MR, Chin EL, Mulle JG, Okou DT, Warren 

ST, Zwick ME: Microarray-based mutation 
detection in the dystrophin gene. Hum Mutat. 
2008, 29(9):1091-99. 

2. Li X, Zhao L, Zhou S, Hu C, Shi Y, Shi W, et al: A 
comprehensive database of Duchenne and 
Becker muscular dystrophy patients (0-18 years 
old) in East China. Orphanet J Rare Dis. 2015; 10:5. 
doi: 10.1186/s13023-014-0220-7. 

3. Santos R, Gonçalves A, Oliveira J, Vieira E, Vieira 
JP, Evangelista T, et al: New variants, challenges 
and pitfalls in DMD genotyping: implications in 
diagnosis, prognosis and therapy. J Hum Genet. 
2014, 59(8):454-64. 

4. Bushby K, Finkel R, Birnkrant DJ, Case LE, 
Clemens PR, Cripe L, et al: Diagnosis and 
management of Duchenne muscular dystrophy, 
part 1: diagnosis, and pharmacological and 
psychosocial management. Lancet Neurol. 2010, 
9(1):77-93. 

5. Flanigan KM, Dunn DM, von Niederhausern A, 
Soltanzadeh P, Gappmaier E, Howard MT, et al: 
Mutational spectrum of DMD mutations in 
dystrophinopathy patients: application of 
modern diagnostic techniques to a large cohort. 
Hum Mutat. 2009, 30(12):1657-66. 

6. MLPA, General protocol, MRC-Holland, MLPA, 
protocol version MDP-v002, last update 23-01-
2012. 

D

A 



Nepal Journal of Biotechnology. D e c .  2 0 1 6  Vol. 4, No. 1: 37-42  Shrestha et al.  

  

 

 

©NJB, Biotechnology Society of Nepal    42        Nepjol.info/index.php/njb 

7. Chen C, Ma H, Zhang F, Chen L, Xing X, Wang S, 
et al: Screening of Duchenne Muscular 
Dystrophy (DMD) Mutations and Investigating 
Its Mutational Mechanism in Chinese Patients. 
PLoS ONE. 2014, 9(9):e108038. 

8. Wang X, Wang Z, Yan M, Huang S, Chen TJ, 
Zhong N: Similarity of DMD gene deletion and 
duplication in the Chinese patients compared to 
global populations. Behav Brain Funct. 2008, 4:20. 
doi: 10.1186/1744-9081-4-20. 

9. Stuppia L, Antonucci I, Palka G, Gatta V: Use of 
the MLPA Assay in the Molecular Diagnosis of 
Gene Copy Number Alterations in Human 
Genetic Diseases. Int J Mol Sci. 2012, 13(3): 3245-
76. 

10. Lai KKS, Lo IFM, Tong TMF, Cheng LYL, Lam 
STS: Detecting exon deletions and duplications 
of the DMD gene using Multiplex Ligation-
dependent Probe Amplification (MLPA). Clinical 
Biochemistry. 2006, 9 :367-72. 

11. Long F, Sun W, Ji X, Li XH, Liu XQ, Jiang WT, Tao 
J: Clinical application of multiplex ligation-
dependent probe amplification for the detection 
exonic copy number alterations in the 
Dystrophin gene. Zhonghua Yi Xue Yi Chuan Xue 
Za Zhi. 201,28(6):699-704. 

12. Zamani GR, Karami F, Mehdizadeh M, Movafagh 
A, Nilipour Y, Zamani M. Analysis of dystrophin 
gene in Iranian Duchenne and Becker muscular 
dystrophies patients and identification of a novel 
mutation. Neurol Sci. 2015. doi:  10.1007/s10072-
015-2290-2. 

13. Zimowski JG, Massalska D, Holding M, Jadczak S, 
Fidziańska E, Lusakowska A, et al: MLPA based 
detection of mutations in the dystrophin gene of 
180 Polish families with Duchenne/Becker 
muscular dystrophy. Neurol Neurochir Pol. 2014, 
48(6):416-22. 

14. Nouri N, Fazel-Najafabadi E, Salehi M, 
Hosseinzadeh M, Behnam M, Ghazavi MR, et al: 
Evaluation of multiplex ligation-dependent 
probe amplification analysis versus multiplex 
polymerase chain reaction assays in the detection 
of dystrophin gene rearrangements in an Iranian 
population subset. Adv Biomed Res. 2014, 3: 72.  
doi: 10.4103/2277-9175.125862. 

15. Cirak S, Arechavala-Gomeza V, Guglieri M, Feng 
L, Torelli S, Anthony K, et al: Exon skipping and 
dystrophin restoration in patients with 
Duchenne muscular dystrophy after systemic 
phosphorodiamidate morpholino oligomer 
treatment: an open-label, phase 2, dose-escalation 
study. Lancet. 2011, 378(9791):595-605. 

16. Mitrpant C, Fletcher S, Wilton SD: Personalised 
genetic intervention for Duchenne muscular 
dystrophy: antisense oligomers and exon 
skipping. Curr Mol Pharmacol. 2009,2(1):110-21