青海大学学报(自然科学版)
青海大學學報(自然科學版)
청해대학학보(자연과학판)
JOURNAL OF QINGHAI UNIVERSITY (NATURAL SCIENCE EDITION)
2015年
3期
32-35
,共4页
青杂7号%纯度鉴定%杂交种%SSR%甘蓝型油菜%碱裂解法
青雜7號%純度鑒定%雜交種%SSR%甘藍型油菜%堿裂解法
청잡7호%순도감정%잡교충%SSR%감람형유채%감렬해법
Qingza No .7%purity inspection%hybrid%SSR%Brassica napus L.%alkaline lysis meth-od
为了建立准确高效的青杂7号杂交种种子纯度鉴定方法,并促进青杂7号的推广。本研究选用青杂7号的恢复系、不育系及F1杂交种,利用60对SSR引物对其进行分析并利用大田制种群体对标记进行验证。同时对碱裂解DNA快速提取方法进行了优化。结果表明:得到的1对SSR共显性标记P49,该标记的鉴定结果与大田鉴定结果基本一致,但SSR标记检测方法比大田检测更快更准确;优化的DNA快速提取方法提取的DNA可以稳定扩增出清晰可见的条带,可以应用于鉴定油菜杂交种纯度,进一步加快了油菜杂交种纯度鉴定的速度。
為瞭建立準確高效的青雜7號雜交種種子純度鑒定方法,併促進青雜7號的推廣。本研究選用青雜7號的恢複繫、不育繫及F1雜交種,利用60對SSR引物對其進行分析併利用大田製種群體對標記進行驗證。同時對堿裂解DNA快速提取方法進行瞭優化。結果錶明:得到的1對SSR共顯性標記P49,該標記的鑒定結果與大田鑒定結果基本一緻,但SSR標記檢測方法比大田檢測更快更準確;優化的DNA快速提取方法提取的DNA可以穩定擴增齣清晰可見的條帶,可以應用于鑒定油菜雜交種純度,進一步加快瞭油菜雜交種純度鑒定的速度。
위료건립준학고효적청잡7호잡교충충자순도감정방법,병촉진청잡7호적추엄。본연구선용청잡7호적회복계、불육계급F1잡교충,이용60대SSR인물대기진행분석병이용대전제충군체대표기진행험증。동시대감렬해DNA쾌속제취방법진행료우화。결과표명:득도적1대SSR공현성표기P49,해표기적감정결과여대전감정결과기본일치,단SSR표기검측방법비대전검측경쾌경준학;우화적DNA쾌속제취방법제취적DNA가이은정확증출청석가견적조대,가이응용우감정유채잡교충순도,진일보가쾌료유채잡교충순도감정적속도。
In order to establish the technology for seed purity inspection of Qingza No .7 and promote the extension of Qingza No .7.The fertile lines, sterile lines and F1 of Qingza No.7 were selected and 60 pairs of simple sequence repeat ( SSR) primers were used for analyzing .The populations of field seed producing were used to verify .At the same time , the alkaline lysis method is optimized . One co-dominant marker P49 was identified and the result was consistent with field identification . The co-dominant marker P49 was more efficient to distinguish false hybrids compared with field ob-servation method. Fragments can be steadily amplified from the DNA extracted by the modified alka-line lysis method .It is confirmed that the modified alkaline lysis method is suitable to be applied in the large-scale hybrid seed purity inspection of rapeseed , which would speed up hybrid seed purity inspection of rapeseed with SSR marker .