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1.
选用36个随机引物对"寒丰A"、"寒丰B"、"8204A"、"8204B"、"R161"等5份杂交粳稻亲本材料进行RAPD扩增,对其中特异RAPD标记片段进行克隆和测序.根据获得的特异DNA序列设计序列特征扩增区(SCAR)特异的引物,将18个RAPD标记转化成6个稳定的SCAR标记.用这些SCAR标记对亲本和杂种F1代单株进行检测,实验室检测种子纯度的结果与海南田间种植的结果基本一致.此外,应用水稻细胞质雄性不育特异的1对PCR引物,分辨出2对不育系/保持系亲本:"寒丰A"与"寒丰B"、"8204A"与"8204B".  相似文献   

2.
利用RAPD分子标记对番茄杂交种纯度的鉴定研究   总被引:9,自引:0,他引:9  
李丽  郑晓鹰  E.Klocke 《广西植物》2003,23(2):149-154,148
应用RAPD(RandomlyamplifiedpolymorphicDNA)分子标记对番茄京丹1号和毛粉802的F1代杂交种纯度进行鉴定的实验研究。该项研究使用了10个碱基的单随机引物和10个碱基的双随机引物进行扩增。在60个单引物扩增反应中获得7个京丹1号父本特有的核酸标记片段。但在14个双随机引物对京丹1号和毛粉802杂交组合的扩增反应中获得了7个京丹1号F1代杂交种特有的核酸标记片段和5个毛粉802父本特有的标记带。实验结果显示,双引物的扩增反应对鉴定双亲亲缘关系极近的杂交种纯度较单引物扩增反应更有效。其中,京丹1号的14个标记片段在北京蔬菜研究中心,种子纯度检测室又进行了重复扩增实验。实验结果为87%的RAPD标记可以在使用不同的PCR仪和不同来源的Taq酶的实验条件下得到。RAPD分子标记技术对鉴定双亲亲缘关系极近的杂交种纯度是真实可靠的。  相似文献   

3.
以F1代苦瓜杂交种如玉11号及其亲本为材料,利用RAPD及SRAP两种分子标记技术对这3种苦瓜基因组DNA进行比较分析,以获得该杂交种及其亲本(或母本)差异目的基因片段。经过多次对该3种苦瓜叶片DNA提取,PCR扩增及其PCR产物的琼脂糖凝胶电泳分析,在供试的46个RAPD引物及121对SRAP引物中,筛选出1个RAPD引物及1对SRAP引物能区分该苦瓜杂交种及其母本种子,通过进一步验证分析,证明该两种分子标记的特异引物可作为如玉11号苦瓜杂交种子的纯度鉴定之用。  相似文献   

4.
利用Operon系列引物筛选到1个与HB红花性状基因连锁的RAPD标记OPA15^1160,对差异条带进行克隆与核苷酸测序,根据测序结果设计SCAR引物,在HB红花近等基因系及其白花轮回亲本中进行PCR扩增程序优化和鉴定,筛选出一对引物可稳定扩增出与HB红花性状基因连锁的特异片段,获得了与HB红花性状基因紧密连锁的SCAR标记HB^-330。利用具黄色花瓣紫红色基斑的海岛棉与粉红花瓣的红叶棉等种质材料以7LHB红花近等基因系与白花轮回亲本杂交的F1、BC1F1、F2群体,对该SCAR标记的特异性与准确性进行了鉴定与验证,在红花植株中扩增出了330bp大小的片段而在白花植株中未扩增出,证明该标记准确性高、重复性好。HB红花是通过远缘杂交转自野生二倍体比克氏棉的性状,已成功地应用于性状标记杂交棉育种。该SCAR标记不仅为HB红花标记杂交种的纯度鉴定提供了有效技术手段,也为新品种保护提供了技术支持,促进了红花性状杂交种的分子标记辅助育种进程。  相似文献   

5.
水稻苯达松敏感致死基因的RAPD标记和SCAR标记   总被引:9,自引:0,他引:9  
利用RAPD技术对水稻品种农林 8号 (含苯达松抗性基因Ben)和其突变体农林 8号m (含苯达松敏感致死基因ben)进行标记 ,从 36 0个 10bp寡核苷酸随机引物中筛选出 5个引物产生的 7个RAPD标记。经对多态性标记的克隆和序列分析 ,再设计PCR引物 ,将其中 4个RAPD标记OPG18/ 94 3、OPG18/ 972、OPD10 / 12 4 8和OPF0 3/ 1198转化成SCAR标记SCAR/G18/ 883、SCAR/G18/ 890、SCAR/G18/ 919/ 94 8、SCAR/D10 / 12 37、SCAR/F0 3/ 1186。通过对农林 8号×农林 8号mF2 分离群体 32 0个单株的连锁分析及在 1对含ben基因的近等基因系H12 1和Hben12 1中验证 ,标记SCAR/G18/ 883、SCAR/G18/ 890、SCAR/G18/ 919/ 94 8与Ben或ben基因共分离 ,SCAR/D10 / 12 37与Ben基因的遗传距离为 (14 .8± 2 .1)cM。经Southernblotting分析并结合F2 代分离比例表明 ,标记OPG18/ 94 3、OPG18/ 972及其转化的SCAR标记在基因组中为单拷贝序列 ,且OPG18/ 94 3和OPG18/ 972为一对等位STS位点。这是首次报道与ben或Ben基因相连锁的分子标记。本研究为利用分子标记辅助ben基因的转育及利用图位克隆技术分离ben基因提供了有用的分子标记。  相似文献   

6.
陕油8号种子纯度的RAPD鉴定研究   总被引:5,自引:0,他引:5  
从杂交油菜“陕油8号”及其亲本中提取基因组DNA,用100个RAPD随机引物进行扩增,从中筛选出3个可将亲本和子代区分的引物BA208、BA1090、BA497。BA208产生亲本互补的特征带BA208-1050bp、BA2081250bp;BA1090产生母本特征带BA1090-700bp,BA497产生父本特征带BA497-870bp,上述谱带均在子代中出现。以BA208产生的特征谱带作为分子标记对杂交油菜种子纯度鉴定得到了一致的结果,并与大田纯度检测结果一致。BA497可将“陕油8号”与当地4个主栽品种有效区分。此外,还对双引物共同鉴定杂交种子纯度问题进行了初步探讨。  相似文献   

7.
利用RAPD技术对水稻品种农林8号(含苯达松抗性基因Ben)和其突变体农林8号m (含苯达松敏感致死基因ben)进行标记,从360个10 bp寡核苷酸随机引物中筛选出5个引物产生的7个RAPD标记.经对多态性标记的克隆和序列分析,再设计PCR引物,将其中4个RAPD标记OPG18/943、OPG18/972、OPD10/1248和OPF03/1198转化成SCAR标记SCAR/G18/883、SCAR/G18/890、SCAR/G18/919/948、SCAR/D10/1237、SCAR/F03/1186.通过对农林8号×农林8号m F2分离群体320个单株的连锁分析及在1对含ben基因的近等基因系H121和Hben121中验证,标记SCAR/G18/883、SCAR/G18/890、SCAR/G18/919/948与Ben 或ben基因共分离,SCAR/D10/1237与Ben基因的遗传距离为(14.8±2.1) cM.经Southern blotting分析并结合F2代分离比例表明,标记OPG18/943、OPG18/972及其转化的SCAR标记在基因组中为单拷贝序列,且OPG18/943和OPG18/972为一对等位STS位点.这是首次报道与ben或Ben基因相连锁的分子标记.本研究为利用分子标记辅助ben基因的转育及利用图位克隆技术分离ben基因提供了有用的分子标记.  相似文献   

8.
葡萄感霜霉病基因的分子标记(英文)   总被引:4,自引:0,他引:4  
 在葡萄抗病育种中 ,幼苗期排除感霜霉病的后代具有特别重要的意义 .用 BSA,RAPD和SCAR方法研究了葡萄感霜霉病基因的分子标记 .分析了两个种间杂交组合 [毛葡萄 (抗病 )×欧洲葡萄 (感病 ) ]88- 1 1 0和 88- 84与 88- 1 1 0的 F1代自交或互交所得的 3个 F2 代 ,以及欧洲葡萄品种和中国野生葡萄种 .共筛选了 2 80个随机引物 .引物 OPO1 0产生了一个 RAPD标记 OPO1 0 - 80 0与葡萄感霜霉病主效基因紧密联锁 .将该 DNA片段克隆并测序 .OPO1 0 - 80 0的实际长度为 835bp,所以 OPO1 0 - 80 0应为 OPO1 0 - 835.据其两端序列 ,设计了一对长度为 2 6bp和 2 8bp的特异引物分别扩增上述试材 ,获得了与该 RAPD标记相同大小的一条带 ,将 RAPD标记转化为 SCAR标记SCO1 0 - 835.并证实了此 SCAR标记的通用性 ,该 SCAR标记可用于葡萄抗病育种中杂种后代对霜霉病的抗病与感病性鉴定 .  相似文献   

9.
回收、纯化由引物OPB07(5’-GGTGACGCAG-3’) OPB18(5’-CCACAGCAGT-3’)扩增而得的杉木(Cunninghamia lanceolata(Lamb.)Hook)种子随体染色体特异性RAPD(随机扩增的DNA多态性分析)片段OPB07-18907,将该片段克隆至pUCm-T载体,转化受体菌后筛选出阳性克隆,并对插入片段进行测序,根据序列特点设计两对SCAR(序列特异性扩增区)引物,PCR结果显示,这两对引物的4种组合都可以扩增出属于随体染色体的特征带,适宜退火温度为57℃。成功将特异RAPD标记OPB07-18907转化为稳定的SCAR标记。开发随体染色体SCAR标记目的是:一方面能在分子水平上鉴定微分离的杉木随体染色体,另一方面,也可以将杉木已构建的遗传图谱中连锁群与染色体进行对应。探讨了该SCAR标记对杉木核型分析的作用。  相似文献   

10.
利用SRAP分子标记对12份甜瓜材料进行亲缘关系鉴定和F1代杂交种进行纯度检测。结果表明:从40对引物中筛选出13对多态性好的引物,共扩增出78条带,多态性带的比例为50%;聚类分析结果显示,12份甜瓜材料的相似系数在0.263~0.921之间,可将该12份甜瓜材料分为2大类,进一步细分为5类。利用引物Me15-Em7和Me3-Em16对‘红绿早脆’100S杂交种进行纯度检测,杂交种纯度为77%。研究为甜瓜品种间亲缘关系及种子纯度检测提供了可靠的理论依据。  相似文献   

11.
A simpler and better method for purity testing of hybrid pepper seed was developed. The simplest method for extracting genomic DNA, the NaOH method, was chosen. Two RAPD markers identifying male and female parents were also developed, and the PCR products of male- and female-specific RAPD markers were cloned and sequenced. From these sequences, new longer primers were constructed for conversion into SCAR markers. In blind tests the RAPD and SCAR markers were able to reliably detect contaminating exotic seeds. These PCR-based markers are therefore directly applicable for purity testing by seed companies. In addition, the PCR products of the SCAR markers could be identified by direct staining methods such as ethidium bromide and pellet painting without electrophoresis.  相似文献   

12.
SSR与SRAP标记在玉米品种鉴定中的比较研究   总被引:4,自引:0,他引:4  
利用SSR标记和SRAP标记对19个玉米品种及8份莱农15样品进行了分析,比较了2种标记的分辨能力及在亲缘关系和杂交种纯度鉴定中的表现.与SSR标记相比,SRAP标记用于玉米品种鉴定扩增住点数量更多,PIC值更高,具有更高的分辨率;在亲缘关系分析方面,SSR检测的遗传距离变幅更大,2种标记计算的遗传距离呈极显著正相关,分类结果基本一致;在杂交种纯度检测中,SRAP标记的期望位点在杂交种群体中检测率高于SSR标记相应位点,检测杂交种纯度结果更接近田问种植鉴定,因而准确度更高.SRAP在玉米品种鉴定中具有一定的优势,可作为SSR标记技术的有益补充,特别是在杂交种纯度鉴定中应用.  相似文献   

13.
RAPD (Random Amplified Polymorphic DNA) and ISSR (Inter Simple Sequence Repeats) markers were used to analyse the genetic divergence between the regenerated plants derived from callus cultures and the original maize line A188. Analysis of polymorphism by using 38 RAPD- and 10 ISSR-oligonucleotide primers showed that the differences between eight examined somaclones and the original line ranged from 6.5 to 23%. As confirmed using new primers, the regenerants derived from callus cultures grouped into two clusters according to their origin. The regenerants isolated from calluses grown for eight months differed from one another and the original line to a larger extent than the regenerants obtained from two-month callus cultures. In some somaclones, molecular marking of the regenerants revealed specific RAPD and ISSR fragments that were absent in other somaclones or the original maize line. On the basis of six specific fragments (five RAPD and one ISSR), SCAR (Sequence Characterized Amplified Region) markers were developed. Specific polymorphism revealed with random primers was completely confirmed using five SCAR markers. Polymorphism of one SCAR marker differed from that revealed with random primers. Five SCAR fragments were inherited as simple dominant traits. One SCAR fragment displayed codominant inheritance.  相似文献   

14.
RAPD (Random Amplified Polymorphic DNA) and ISSR (Inter Simple Sequence Repeats) markers were used to analyse the genetic divergence between the regenerated plants derived from callus cultures and the original maize line A188. Analysis of polymorphism by using 38 RAPD- and 10 ISSR-oligonucleotide primers showed that the differences between eight examined somaclones and the original line ranged from 6.5 to 23%. As confirmed using new primers, the regenerants derived from callus cultures grouped into two clusters according to their origin. The regenerants isolated from calluses grown for eight months differed from one another and the original line to a larger extent than the regenerants obtained from two-month callus cultures. In some somaclones, molecular marking of the regenerants revealed specific RAPD and ISSR fragments that were absent in other somaclones or the original maize line. On the basis of six specific fragments (five RAPD and one ISSR), SCAR (Sequence Characterized Amplified Region) markers were developed. Specific polymorphism revealed with random primers was completely confirmed using five SCAR markers. Polymorphism of one SCAR marker differed from that revealed with random primers. Five SCAR fragments were inherited as simple dominant traits. One SCAR fragment displayed codominant inheritance.  相似文献   

15.
The fungus Peronosclerospora sorghi [Weston and Uppal (Shaw)] infects both sorghum and maize and incites downy mildew disease. Pathogenic and molecular variability among isolates of P. sorghi from sorghum and maize has been reported. In the present study we developed a DNA sequence characterized amplified region (SCAR) marker for identification of isolates of P. sorghi from maize by using polymerase chain reaction (PCR). The random amplified polymorphic DNA (RAPD) primer OPB15 consistently amplified a 1,000 base pairs (bp) product in PCR only from DNA of P. sorghi isolates from maize and not from isolates of sorghum. The PCR-amplified 1,000-bp product was cloned and sequenced. The sequence of the SCAR marker was used for designing specific primers for identification of maize isolates of P. sorghi. The SCAR primers amplified a 800 bp fragment only from genomic DNA of maize isolates of P. sorghi. The SCAR primers developed in this study are highly specific and reproducible, and proved to be powerful tool for identification of P. sorghi isolates from maize.  相似文献   

16.
与葡萄抗霜霉病基因紧密连锁的分子遗传标记   总被引:18,自引:0,他引:18  
以种间杂交组合88-110[83-4-96(毛葡萄,抗霜霉病)×粉红玫瑰(欧洲葡萄,感霜霉病)]的F  相似文献   

17.
从常规鉴定、生化鉴定及分子标记技术鉴定等方面,阐述了玉米种子纯度鉴定的重要性。进一步对RAPD、RFLP、SSR和AFLP等分子标记技术在种子纯度鉴定和品种真实性分析中的应用潜力及存在问题进行比较,得出SSR分子标记技术是目前种子纯度和品种真实性鉴定中最适宜的技术。  相似文献   

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