南方林业科学
南方林業科學
남방임업과학
Nanfang Forestry Science
2015年
2期
6-9,16
,共5页
叶金山%李万和%龚斌%杨春霞
葉金山%李萬和%龔斌%楊春霞
협금산%리만화%공빈%양춘하
南酸枣%ISSR-PCR%单因子实验%优化
南痠棘%ISSR-PCR%單因子實驗%優化
남산조%ISSR-PCR%단인자실험%우화
Choerospondias axillaris%ISSR-PCR%single factor experiment%optimization
以南酸枣叶片基因组DNA为模板,采用单因子实验方法对影响ISSR反应体系的dNTP、Mg2+、引物浓度、模板DNA、Taq酶等5个因子进行优化,结果表明,在20 L ISSR反应体系中,各反应物的最适含量为:2.5 mmol/L Mg2+、0.2 mmol/L dNTP、0.25~0.5 mol/L引物、20 ng DNA和0.5 U Taq聚合酶。利用该优化体系扩增85条ISSR引物,有65条有扩增产物,38条具有多态性,并且利用842引物扩增不同南酸枣DNA模板,扩增的目的条带清晰、多态性好、稳定性强,可以用于后期的南酸枣种质资源鉴定及遗传多样性研究。
以南痠棘葉片基因組DNA為模闆,採用單因子實驗方法對影響ISSR反應體繫的dNTP、Mg2+、引物濃度、模闆DNA、Taq酶等5箇因子進行優化,結果錶明,在20 L ISSR反應體繫中,各反應物的最適含量為:2.5 mmol/L Mg2+、0.2 mmol/L dNTP、0.25~0.5 mol/L引物、20 ng DNA和0.5 U Taq聚閤酶。利用該優化體繫擴增85條ISSR引物,有65條有擴增產物,38條具有多態性,併且利用842引物擴增不同南痠棘DNA模闆,擴增的目的條帶清晰、多態性好、穩定性彊,可以用于後期的南痠棘種質資源鑒定及遺傳多樣性研究。
이남산조협편기인조DNA위모판,채용단인자실험방법대영향ISSR반응체계적dNTP、Mg2+、인물농도、모판DNA、Taq매등5개인자진행우화,결과표명,재20 L ISSR반응체계중,각반응물적최괄함량위:2.5 mmol/L Mg2+、0.2 mmol/L dNTP、0.25~0.5 mol/L인물、20 ng DNA화0.5 U Taq취합매。이용해우화체계확증85조ISSR인물,유65조유확증산물,38조구유다태성,병차이용842인물확증불동남산조DNA모판,확증적목적조대청석、다태성호、은정성강,가이용우후기적남산조충질자원감정급유전다양성연구。
In order to optimize ISSR-PCR system for Choerospondias axillaris, different levels of concentration of dNTP, Mg2+, primer, template DNA and Taq DNA polymerase were trailed by single factor experiment. The results showed that the optimal ISSR-PCR system for Ch. axillaris contained 2.5 mmol/L Mg2+、0.2 mmol/L dNTP、0.25~0.5 mol/L primer、20 ng DNA和0.5 U Taq polymerase in 20 L PCR system. Furthermore, 65 primers could produce target bands among 85 ISSR primers, and including 38 polymorphic primers. With this optimal ISSR-PCR amplification system, high resolution, multiple polymorphic and good repeatability bands were gained on 6 different DNA templates, which indicated the stability and availability of this system. The ISSR-PCR system, which was established in this paper, could be used to study germplasm identification and genetic diversity of Ch. axillaris.
