中国对虾SRAP分子标记体系正交优化及在遗传多样性分析中的应用  被引量：2

作　　者：陈华增[1,2] 李健[2] 何玉英[2] 李吉涛[2] 王清印[2] 

机构地区：[1]上海海洋大学水产与生命学院,201306 [2]中国水产科学研究院黄海水产研究所,青岛266071

出　　处：《渔业科学进展》2010年第6期43-53,共11页Progress in Fishery Sciences

基　　金：国家科技支撑计划专题(2006BAD01A13);国家自然科学基金课题(40706052);公益性行业专项(nyzx07-042);国家虾产业技术体系(nycytx-46)共同资助

摘　　要：利用正交设计L16(45)对影响中国对虾SRAP分子标记分析的5个因素(Taq酶,Mg2+,模板DNA,dNTP和引物浓度)在4个水平上进行了优化,筛选出各反应因素的最佳水平为:20μl反应体系中包含1.0UTaq酶,2.0mmol/L的Mg2+,40.0ng的模板DNA,0.125mmol/L的dNTP以及0.4μmol/L的引物,退火温度为53.5℃。研究表明,各因素的不同水平对扩增结果有显著影响,其中Mg2+影响最大,影响大小顺序依次为Mg2+,Taq酶,引物,dNTP和模板DNA。利用优化的SRAP分子标记体系对中国对虾"黄海1号"第12世代选育群体进行了遗传多样性分析,实验结果表明,此标记技术可作为中国对虾遗传分析的良好技术工具。遗传多样性分析共筛选出8对可以扩增出清晰稳定条带的引物组合,共获得171个位点,其中多态性位点154个,占90.08%;有效等位基因数为1.7741,期望杂合度均值为0.4219,Shannon多样性指数为0.6055。上述参数值均高于应用AFLP技术对前几代选育群体的遗传多样性分析结果。The orthogonal design L16（45）was used to optimize SRAP-PCR amplification system in marine shrimp Fenneropenaeus chinensis on four levels of five factors（Taq DNA polymerase,Mg2＋,DNA template,dNTP,and primer）.The results showed that the optimum concentrations were 1.0 U Taq enzyme,2.0 mmol/L Mg2＋,40.0 ng DNA template,0.125 mmol/L dNTP,and 0.4 μmol/L primer,respectively,in 20 μl SRAP-PCR system,and the annealing temperature was 53.5℃ via setting temperature gradient.Significant effects of each factor in different levels were observed and the concentration of Mg2＋ was the most dominant factor affecting the result of PCR,while Taq polymerse,primer,dNTP,and template DNA followed in terms of dominance.Then,the established amplification system was used to analyze the genetic diversity of the 12th generation of selected ＂Huanghai No.1＂ of F.chinensis.As a result,171 bands were generated with 8 primer sets,of which 154 bands were polymorphic bands,accounting for 90.08%.The effective number of alleles,genetic diversity and Shannon＇s information index were 1.774 1,0.421 9,and 0.605 5,respectively.The parameters obtained by SRAP were higher than those reported by authors applying AFLP technique.

关 键 词：中国对虾 正交设计 SRAP 遗传多样性 

分 类 号：S966[农业科学—水产养殖]