Long-range PCR sequencing as a novel approach in genetic—analysis of MYH3: A preliminary result
Background and objective: Genetic diagnosis of large genes are usually complicated by large transcript size, complexity of the gene region and the high level of gene variations. Long-range PCR is a flexible, fast, efficient and cost-effective choice for sequencing large candidate genomic regions,...
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| Main Authors: | , , |
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| Format: | Article |
| Language: | English |
| Published: |
2015
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| Subjects: | |
| Online Access: | http://eprints.unisza.edu.my/5190/1/FH02-FP-17-09400.pdf http://eprints.unisza.edu.my/5190/ |
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| Institution: | Universiti Sultan Zainal Abidin |
| Language: | English |
| Summary: | Background and objective: Genetic diagnosis of large genes are usually complicated by large
transcript size, complexity of the gene region and the high level of gene variations. Long-range
PCR is a flexible, fast, efficient and cost-effective choice for sequencing large candidate
genomic regions, especially when combined with next-generation sequencing (NGS) platforms.
This article aims to develop and optimise novel mutation screening assay for MYH3 gene which
is 40 kb in size by directly sequencing four LR-PCR products using Illumina MiSeq sequencing
platform.
Methods: Genomic DNA was isolated from 1 mL of peripheral blood was extracted using
GeneAll DNA extraction kit (GeneAll, Korea), following the manufacturer’s protocol. Four sets
of primers that span the entire gene were synthesised. MaxTaq DNA Polymerase (Vivantis) was
used to amplify each amplicons with cycling conditions; 94 °C for 2 min, 94 °C 12, annealing
temperature for 30, 68 °C for 10 mins, 68 °C for 7 min for a total of 35 cycles. The amplified
amplicons were pooled together and library was prepared using Nextera XT DNA Sample
Preparation Kit (Illumina Inc., CA, USA). Pooled library was generated by mixing all libraries
equally for high-throughput sequencing on MiSeq™ Benchtop Sequencer (Illumina Inc., CA,
USA). The sequence was aligned to the hg19 assembly of the genome with BWA enrichment
analysis tool (Illumina Inc., CA, USA) and variants were called using Variant Studio (Illumina
Inc., CA, USA). Only variants with at least 6-fold read coverage and a phred scale SNP ≥30
were included for further analysis.
Results: The four 10 kb amplicons were successfully amplified with annealing temperatures;
63.1, 62.4, 64.7 and 64.7 ºC respectively, employing standard PCR cycling method within a short
period of time. Targeted sequencing using Illumina MiSeq paired-end sequence resulted in
11,947,785 reads (98.05%) of which 99.8% could be aligned with the human genome. This
provided 99.8% coverage of the sequence at a minimum sequencing depth of 6×. With this method, a total of 2,280 known variants and 848 unknown variants were detected, which will be
subjected to further downstream analysis.
Conclusions: Current method enables amplification of the entire gene with four reactions, each
generating product sizes of 10 kb circumventing the need for specific PCR amplification of
individual exons. LR-PCR allows direct sequencing and screening methods for detecting genetic
variations, achieving high sensitivity and improved intronic coverage with a faster turnaround
time and lower costs, and providing a reliable tool for complex genetic analyses. |
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