An improved allele-specific PCR primer design method for SNP marker analysis and its application

BACKGROUND: Although Single Nucleotide Polymorphism (SNP) marker is an invaluable tool for positional cloning, association study and evolutionary analysis, low SNP detection efficiency by Allele-Specific PCR (AS-PCR) still restricts its application as molecular marker like other markers such as Simp...

Descripción completa

Detalles Bibliográficos
Autores principales: Liu, Jing, Huang, Shunmou, Sun, Meiyu, Liu, Shengyi, Liu, Yumei, Wang, Wanxing, Zhang, Xiurong, Wang, Hanzhong, Hua, Wei
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2012
Materias:
Methodology
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3495711/
https://www.ncbi.nlm.nih.gov/pubmed/22920499
http://dx.doi.org/10.1186/1746-4811-8-34
_version_ 1782249553005641728
author Liu, Jing
Huang, Shunmou
Sun, Meiyu
Liu, Shengyi
Liu, Yumei
Wang, Wanxing
Zhang, Xiurong
Wang, Hanzhong
Hua, Wei
author_facet Liu, Jing
Huang, Shunmou
Sun, Meiyu
Liu, Shengyi
Liu, Yumei
Wang, Wanxing
Zhang, Xiurong
Wang, Hanzhong
Hua, Wei
author_sort Liu, Jing
collection PubMed
description BACKGROUND: Although Single Nucleotide Polymorphism (SNP) marker is an invaluable tool for positional cloning, association study and evolutionary analysis, low SNP detection efficiency by Allele-Specific PCR (AS-PCR) still restricts its application as molecular marker like other markers such as Simple Sequence Repeat (SSR). To overcome this problem, primers with a single nucleotide artificial mismatch introduced within the three bases closest to the 3’end (SNP site) have been used in AS-PCR. However, for one SNP site, nine possible mismatches can be generated among the three bases and how to select the right one to increase primer specificity is still a challenge. RESULTS: In this study, different from the previous reports which used a limited quantity of primers randomly (several or dozen pairs), we systematically investigated the effects of mismatch base pairs, mismatch sites and SNP types on primer specificity with 2071 primer pairs, which were designed based on SNPs from Brassica oleracea 01-88 and 02-12. According to the statistical results, we (1) found that the primers designed with SNP (A/T), in which the mismatch (CA) in the 3(rd) nucleotide from the 3’ end, had the highest allele-specificity (81.9%). This information could be used when designing primers from a large quantity of SNP sites; (2) performed the primer design principle which forms the one and only best primer for every SNP type. This is never reported in previous studies. Additionally, we further identified its availability in rapeseed (Brassica napus L.) and sesame (Sesamum indicum). High polymorphism percent (75%) of the designed primers indicated it is a general method and can be applied in other species. CONCLUSION: The method provided in this study can generate primers more effectively for every SNP site compared to other AS-PCR primer design methods. The high allele-specific efficiency of the SNP primer allows the feasibility for low- to moderate- throughput SNP analyses and is much suitable for gene mapping, map-based cloning, and marker-assisted selection in crops.
format Online
Article
Text
id pubmed-3495711
institution National Center for Biotechnology Information
language English
publishDate 2012
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-34957112012-11-13 An improved allele-specific PCR primer design method for SNP marker analysis and its application Liu, Jing Huang, Shunmou Sun, Meiyu Liu, Shengyi Liu, Yumei Wang, Wanxing Zhang, Xiurong Wang, Hanzhong Hua, Wei Plant Methods Methodology BACKGROUND: Although Single Nucleotide Polymorphism (SNP) marker is an invaluable tool for positional cloning, association study and evolutionary analysis, low SNP detection efficiency by Allele-Specific PCR (AS-PCR) still restricts its application as molecular marker like other markers such as Simple Sequence Repeat (SSR). To overcome this problem, primers with a single nucleotide artificial mismatch introduced within the three bases closest to the 3’end (SNP site) have been used in AS-PCR. However, for one SNP site, nine possible mismatches can be generated among the three bases and how to select the right one to increase primer specificity is still a challenge. RESULTS: In this study, different from the previous reports which used a limited quantity of primers randomly (several or dozen pairs), we systematically investigated the effects of mismatch base pairs, mismatch sites and SNP types on primer specificity with 2071 primer pairs, which were designed based on SNPs from Brassica oleracea 01-88 and 02-12. According to the statistical results, we (1) found that the primers designed with SNP (A/T), in which the mismatch (CA) in the 3(rd) nucleotide from the 3’ end, had the highest allele-specificity (81.9%). This information could be used when designing primers from a large quantity of SNP sites; (2) performed the primer design principle which forms the one and only best primer for every SNP type. This is never reported in previous studies. Additionally, we further identified its availability in rapeseed (Brassica napus L.) and sesame (Sesamum indicum). High polymorphism percent (75%) of the designed primers indicated it is a general method and can be applied in other species. CONCLUSION: The method provided in this study can generate primers more effectively for every SNP site compared to other AS-PCR primer design methods. The high allele-specific efficiency of the SNP primer allows the feasibility for low- to moderate- throughput SNP analyses and is much suitable for gene mapping, map-based cloning, and marker-assisted selection in crops. BioMed Central 2012-08-24 /pmc/articles/PMC3495711/ /pubmed/22920499 http://dx.doi.org/10.1186/1746-4811-8-34 Text en Copyright ©2012 Liu et al.; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License ( http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Methodology
Liu, Jing
Huang, Shunmou
Sun, Meiyu
Liu, Shengyi
Liu, Yumei
Wang, Wanxing
Zhang, Xiurong
Wang, Hanzhong
Hua, Wei
An improved allele-specific PCR primer design method for SNP marker analysis and its application
title An improved allele-specific PCR primer design method for SNP marker analysis and its application
title_full An improved allele-specific PCR primer design method for SNP marker analysis and its application
title_fullStr An improved allele-specific PCR primer design method for SNP marker analysis and its application
title_full_unstemmed An improved allele-specific PCR primer design method for SNP marker analysis and its application
title_short An improved allele-specific PCR primer design method for SNP marker analysis and its application
title_sort improved allele-specific pcr primer design method for snp marker analysis and its application
topic Methodology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3495711/
https://www.ncbi.nlm.nih.gov/pubmed/22920499
http://dx.doi.org/10.1186/1746-4811-8-34
work_keys_str_mv AT liujing animprovedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT huangshunmou animprovedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT sunmeiyu animprovedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT liushengyi animprovedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT liuyumei animprovedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT wangwanxing animprovedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT zhangxiurong animprovedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT wanghanzhong animprovedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT huawei animprovedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT liujing improvedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT huangshunmou improvedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT sunmeiyu improvedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT liushengyi improvedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT liuyumei improvedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT wangwanxing improvedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT zhangxiurong improvedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT wanghanzhong improvedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication
AT huawei improvedallelespecificpcrprimerdesignmethodforsnpmarkeranalysisanditsapplication

Ejemplares similares