Optimization for Reaction System and PCR program of Taraxacum mongolicum ISSR-PCR

LI Xi-feng1; QIU Tian-bao1; ZHANG Hong-mei2; HU Li-xin1; HU Chun-yue1; ZHENG Nan-nan1; TANG Lu1

doi:10.13422/j.cnki.syfjx.2012.16.089

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Optimization for Reaction System and PCR program of Taraxacum mongolicum ISSR-PCR

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- Optimization for Reaction System and PCR program of Taraxacum mongolicum ISSR-PCR
- Chinese Journal of Experimental Traditional Medical Formulae Vol. 18, Issue 16, Pages: 119-122(2012)
- 作者机构：
  
  1. 河南中医学院药学院
  2. 郑州大学医药科学研究院
- 作者简介：
- 基金信息：
- DOI：10.13422/j.cnki.syfjx.2012.16.089
  CLC： R450
- Published：2012
- 稿件说明：
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[1]李喜凤,邱天宝,张红梅,胡利欣,胡春月,郑楠楠,唐露.蒲公英ISSR-PCR反应体系及扩增程序的建立与优化[J].中国实验方剂学杂志,2012,18(16):119-122.

LI Xi-feng1, QIU Tian-bao1, ZHANG Hong-mei2, et al. Optimization for Reaction System and PCR program of Taraxacum mongolicum ISSR-PCR[J]. Chinese journal of experimental traditional medical formulae, 2012, 18(16): 119-122.
[1]李喜凤,邱天宝,张红梅,胡利欣,胡春月,郑楠楠,唐露.蒲公英ISSR-PCR反应体系及扩增程序的建立与优化[J].中国实验方剂学杂志,2012,18(16):119-122. DOI： 10.13422/j.cnki.syfjx.2012.16.089.

LI Xi-feng1, QIU Tian-bao1, ZHANG Hong-mei2, et al. Optimization for Reaction System and PCR program of Taraxacum mongolicum ISSR-PCR[J]. Chinese journal of experimental traditional medical formulae, 2012, 18(16): 119-122. DOI： 10.13422/j.cnki.syfjx.2012.16.089.

摘要

目的:优化蒲公英ISSR-PCR反应体系及扩增程序;筛选适合的引物

并确定最佳退火温度。方法:采用CTAB法提取蒲公英叶片的DNA

利用正交试验设计

从Taq酶MIX、模板DNA、引物3种因素2个水平

对蒲公英ISSR-PCR反应体系进行考察;采用单因素实验对其扩增程序进行优化。结果:确立了适合于蒲公英的最佳ISSR-PCR反应方法

即在25μL反应体系中

内含Taq酶MIX 15μL（1.25 U Taq DNA聚合酶

1.8 mmol.L-1 Mg2+

dNTPs各0.24 mmol.L-1）

0.3μmol.L-1引物

5 ng模板。在此基础上

从50条引物中筛选出16条扩增稳定、多态性丰富的ISSR引物

并通过梯度PCR试验

确定引物最佳退火温度。结论:采用单因子试验和正交设计方法可以快速建立ISSR-PCR反应体系

经过验证

证明该体系稳定可靠

可用于蒲公英遗传分析。

Abstract

Objective: To establish and optimize ISSR-PCR reaction system for Taraxacum mongolicum.Method: Based on the analysis of orthogonal design test

an orthogonal design was used to optimize the ISSR-PCR amplification system on T.mongolicum by three factors（Taq polymerase Mix

DNA template and primer） at two concentration levels

respectively.PCR program was optimized by single factor experiments.Result: The suitable PCR reaction system contained 15 μL Taq polymerase MIX（1.25 U Taq DNA polymerase

1.8 mmol·L-1 Mg2+

dNTPs 0.24 mmol·L-1）

0.3 μmol·L-1 primer and 5 ng template DNA in total 25 μL reaction solution.On this basis

16 primers were screened with stable amplification and rich polymorphism from 50 ISSR primers.The optimal annealing temperature for ISSR-PCR reaction was proposed by gradient PCR.Conclusion: It is a way to establisd the ISSR-PCR system for orthogonal design combining with single factor test.This optimized ISSR reaction system would provide the basis for the genetic analysis of T.mongolicum.

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