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利用RAPD和SSR分子标记结合拟测交策略,对中国对虾(Fenneropenaeus chinensis)“黄海1号”雌虾与野生雄虾作为亲本进行单对杂交产生的F1代,采用RAPD和SSR 两种分子标记技术初步构建了中国对虾雌、雄遗传连锁图谱。对460个RAPD引物和44对SSR引物进行筛选,共选出61个RAPD引物和20对SSR引物,用于对父母本和82个F1个体进行遗传分析。共得到母本分离标记146个(RAPD标记128个,微卫星标记18个)和父本分离标记127个(RAPD标记109个,微卫星标记18个)。雌性图谱包括8个连锁群、9个三联体和14个连锁对,标记间平均间隔为11.28 cM,图谱共覆盖1 173 cM,覆盖率为59.36%;雄性图谱包括10个连锁群、12个三联体和7个连锁对,标记间平均间隔为12.05 cM,图谱共覆盖1 144.6 cM,覆盖率为62.01%。中国对虾遗传图谱的构建为其分子标记辅助育种、比较基因组作图及数量性状位点的定位与克隆奠定了基础。 相似文献
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中国明对虾AFLP分子标记遗传连锁图谱的构建 总被引:26,自引:0,他引:26
以中国明对虾抗WSSV(白斑综合症病毒,WhiteSpotSyndromeVirus)选育群体第四代为母本,野生中国明对虾为父本,采用单对杂交方式产生F1代,F1代个体姊妹交产生F2代共42个个体为做图群体。62对AFLP选择性引物组合共产生529个分离位点,符合1∶1孟德尔分离类型位点共253个,3∶1孟德尔分离类型位点共276个。利用拟测交理论分别构建中国明对虾雌虾、雄虾的遗传连锁图谱,利用F2自交模型构建共同的AFLP分子标记连锁图谱。三张连锁图上分别有31、25和44个连锁群,图谱分辨率为分别为2.4cM、2.4cM和2.1cM。标记间隔距离分别为12.20cM、11.45cM和11.12cM图谱覆盖率分别达到50.21%、51.93%和48.08%。能够基本满足进行QTL(数量性状位点,QuantitativeTraitLocus)定位的需要。将该图谱和其他对虾类遗传连锁图谱进行了比较分析,探讨了利用相关分子标记将已有图谱进行整合的可能。 相似文献
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中国植物遗传连锁图谱构建研究进展 总被引:21,自引:0,他引:21
遗传连锁图谱构建是基因组研究中的重要环节,是基因定位与克隆乃至基因组结构与功能研究的基础上。近十几年来,分子生物学特别是分子标记技术的飞速发展,为构建高饱和的植物遗传连锁图谱和利用分子标记进行辅助育种奠定了基础。综述了我国在植物遗传连锁图谱构建研究方面的进展及发展动态,列举了我国利用DNA分子标记构建的34张植物遗传连锁图谱实例,且讨论了当前我国在该领域研究中存在的问题并提出了解决途径。 相似文献
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用AFLP的方法分析中国白桦×欧洲白桦的78个F1个体,并按照拟测交作图策略,建立了中国白桦和欧洲白桦遗传连锁图谱。从群体的45对引物组合中分离出343个分离位点,χ^2检验表明,其中有311个符合1:1拟测交分离位点。在这些位点中168个来自中国白桦,143个来自欧洲白桦。软件分析表日月,中国白桦的168个位点构成9个连锁群,11个三联体和14个连锁对,55个为非连锁位点,连锁标记覆盖的总距离为1909.2cM,平均图距为16.9cM;来自欧洲白桦的143个位点构成12个连锁群,4个三联体和9个连锁对,21个为非连锁位点,连锁标记覆盖的总距离为1857.3cM,平均图距为15.2cM。 相似文献
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利用RAPD标记构建美洲黑杨×欧美杨分子标记连锁图谱 总被引:5,自引:0,他引:5
本文利用RAPD标记和美洲黑杨(Populusdeltoides)×欧美杨(P.euramericana)的F1 群体 ,构建了美洲黑杨×欧美杨的分子标记连锁图谱。实验过程中对1040个寡核苷酸随机引物进行了重复筛选 ,共选出127个引物用于作图群体(包括双亲共92个无性系)的随机扩增 ,这127个引物产生229个多态基因座 ,其中符合“拟测交”1∶1分离的有214个。利用多点连锁分析 ,形成19个连锁群及6个三连体和14个连锁对。由19个连锁群构成的图谱含标记129个 ,总图距为1914 2cM ,覆盖杨树基因组约73 62 %。标记间的平均间距为14 84cM。本研究获得了中等密度的美洲黑杨×欧美杨的一个连锁框架。 相似文献
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利用RAPD标记构建美洲黑杨×欧美分子标记连锁图谱 总被引:22,自引:3,他引:22
张新叶 尹佟明 诸葛强 黄敏仁 朱立煌 翟文学 邬荣领 王明庥ZHANG Xin-ye YIN Tong-ming ZHUGE Qiang HUANG Min-ren ZHU Li-huang ZHAI Wen-xue WU Rong-ling WANG Ming-xiu 《遗传》2000,22(4):209-213
本文利用RAPD标记和美洲黑杨(Populus deltoides)×欧美杨(P.euramericana)的F1群体,构建了美洲黑杨×欧美杨的分子标记连锁图谱。实验过程中对1040个寡核苷酸随机引物进行了重复筛选,共选出127个引物用于作图群体(包括双亲共92个无性系)的随机扩增,这127个引物产生229个多态基因座,其中符合“拟测交”1∶1分离的有214个。利用多点连锁分析,形成19个连锁群及6个三连体和14个连锁对。由19个连锁群构成的图谱含标记129个,总图距为1914.2cM,覆盖杨树基因组约73.62%。标记间的平均间距为14.84cM。本研究获得了中等密度的美洲黑杨×欧美杨的一个连锁框架。
Abstract:A molecular linkage map was constructed for the parents of a P.deltoides × P.euramericana F1 family based on random amplified polymorphic DNA(RAPD)markers.A set of 1040 random oligonucleotide primers were screened and 127 primers were selected to generate RAPD markers within a sample of 90 F1 progenies.A total of 229 segregating loci were identified.Among the 229 loci,15 loci were found distorted from the normal 1∶1 ratio.Using multiple analysis,the 214 markers formed 19 main Linkage groups (including 129 markers)and b triples and 14 pairs.The resulting Linkage map of Populus deltoides × P.euramericana (including 129 markers)spanned 1914.2cM(73.62% coverage of genome length)with an average distance of 14.84cM between markers. 相似文献
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利用RAPD标记构建美洲黑杨×欧美分子标记连锁图谱 总被引:3,自引:0,他引:3
本文利用RAPD标记和美洲黑杨(Populus deltoides)×欧美杨(P.euramericana)的F1群体,构建了美洲黑杨×欧美杨的分子标记连锁图谱。实验过程中对1040个寡核苷酸随机引物进行了重复筛选,共选出127个引物用于作图群体(包括双亲共92个无性系)的随机扩增,这127个引物产生229个多态基因座,其中符合“拟测交”1∶1分离的有214个。利用多点连锁分析,形成19个连锁群及6个三连体和14个连锁对。由19个连锁群构成的图谱含标记129个,总图距为1914.2cM,覆盖杨树基因组约73.62%。标记间的平均间距为14.84cM。本研究获得了中等密度的美洲黑杨×欧美杨的一个连锁框架。
Abstract:A molecular linkage map was constructed for the parents of a P.deltoides × P.euramericana F1 family based on random amplified polymorphic DNA(RAPD)markers.A set of 1040 random oligonucleotide primers were screened and 127 primers were selected to generate RAPD markers within a sample of 90 F1 progenies.A total of 229 segregating loci were identified.Among the 229 loci,15 loci were found distorted from the normal 1∶1 ratio.Using multiple analysis,the 214 markers formed 19 main Linkage groups (including 129 markers)and b triples and 14 pairs.The resulting Linkage map of Populus deltoides × P.euramericana (including 129 markers)spanned 1914.2cM(73.62% coverage of genome length)with an average distance of 14.84cM between markers. 相似文献
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白桦RAPD遗传连锁图谱的构建 总被引:3,自引:1,他引:3
以80个来自欧洲白桦(Betula pendula Roth)×中国白桦(Betula platyphylla Suk)的F1个体为作图群体。利用2个亲本和10个F1个体对1,200个10 bp的随机寡核苷酸引物进行筛选, 确定了208个多态性引物。利用RAPD标记, 按照拟测交的作图策略, 分别构建了欧洲白桦和中国白桦的分子标记连锁图谱。对2个亲本和80个F1代作图群体进行随机扩增, 共获得了364个多态性位点。χ2检验结果表明有307个位点符合1∶1分离的拟测交分离, 26个位点符合3∶1分离, 31个位点属偏分离位点。拟测交位点中有145个位点来自欧洲白桦, 有162个位点来自中国白桦。利用2点连锁分析, 欧洲白桦中的145个连锁标记构成了14个不同的连锁群(4个以上标记), 6个三连体和6个连锁对, 37个为非连锁位点, 连锁标记覆盖的总图距为955.6 cM (centimorgan), 平均图距14.9 cM。而来自中国白桦的162个标记构成了15个连锁群(4个以上标记), 4个三连体和6个连锁对, 21个为非连锁位点, 连锁标记覆盖的总图距为1,545.8 cM (centimorgan), 平均图距15.2 cM。该图谱的建立为进一步将两个图谱整合为一个高密度图谱及重要基因的定位奠定了基础。 相似文献
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The primary genetic linkage maps of Fenneropenaeus
chinensis (Osbeck) were constructed by using the “two-way pseudo-testcross” strategy with RAPD and SSR markers. Parents and F1 progeny
were used as segregating populations. Sixty-one RAPD primers and 20 pairs of SSR primers were screened from 460 RAPD primers
and 44 pairs of SSR primers. These primers were used to analyze the parents and 82 progeny of the mapping family. About 146
primers (128 RAPDs, 18 microsatellites) in the female and 127 primers (109 RAPDs, 18 microsatellites) in the male were segregating
markers. The female linkage map included eight linkage groups, nine triplets and 14 doublets, spanning 1,173 cM with the average
marker density of 11.28 cM, and the observed coverage was 59.36%. The male linkage map included 10 linkage groups, 12 triplets
and seven doublets, spanning 1,144.6 cM with the average marker density of 12.05 cM, and the observed coverage was 62.01%.
The construction of the F. chinensis genetic linkage maps here opened a new prospect for marker-assisted selection program, comparative genomics and quantitative
trait loci (QTL) gene location and cloning. 相似文献
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梨遗传连锁图谱的构建及其与苹果图谱的比较 总被引:1,自引:0,他引:1
以‘丰水’为母本、‘砀山酥梨’为父本杂交所得的F1代104株单体为作图群体,利用SSR分子标记进行遗传连锁分析,应用Jionmap 3.0作图软件,构建了一张包含104个SSR分子标记,分属于18个连锁群的梨遗传连锁图谱,覆盖梨基因组总长831.8cM,平均图距为8.0cM。根据定位到该图谱上的SSR标记与苹果‘Fiesta’图谱进行比较,25个共有的SSR标记将该图谱和苹果图谱各连锁群连接起来,这些标记不仅呈现良好的共线性而且它们之间的相对遗传距离也很相近。研究认为,SSR标记作为锚定引物,可以与不同物种的遗传图谱相比较整合,为不同物种之间遗传信息的转移提供参考依据;同时该研究为梨树相关性状的基因定位、分离以及克隆奠定了基础。 相似文献
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为了系统性地开发和拓展柑桔SSR标记,通过对公布的柑桔BAC文库末端序列(BAC-End sequence,BES)进行SSR分析,选择1500个SSR位点设计合成并检测323对引物。结果表明:(1)从总长度为28.1 Mb的46 339条序列中共检测出22 403个SSR位点,约每2条序列就会出现一个SSR位点,发生频率为48%,相当于平均1.25kb的序列中就会出现1个SSR,频率约为柑桔EST的2倍,且不同核心重复序列的SSR发生特点与EST也不同。(2)所合成的323对引物中,有效扩增316对,扩增率约98%,173对表现多态性,总多态性比率约55%,多态性引物中单核苷酸重复类型15对,双核苷酸重复类型100对,三核苷酸及以上重复类型58对,表明柑桔BES中具有较为丰富的多态性SSR标记。(3)结合已发表的遗传作图数据,对总计349个多态性位点进行遗传连锁分析,获得的新遗传连锁图谱共含有9个连锁群、334个SSR标记、总长844.2cM、平均图距2.53cM,延长和加密了先前的图谱。该研究开发的新SSR标记为开展柑桔遗传鉴定分析和遗传图谱构建提供了新的标记来源,加密的遗传图谱为柑桔的基因定位、图位克隆和标记辅助育种等奠定了基础,SSR分析结果也为其他物种SSR标记的开发提供了参考。 相似文献
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苜蓿遗传多样性的取样数目——RAPD和SSR群体标记法 总被引:1,自引:0,他引:1
紫花苜蓿为异花授粉植物,其DNA多态性研究的取样策略与遗传多样性分析直接相关.选取了4个苜蓿品种陇东(地方品种)、中兰1号(育成品种)、牧歌(Graze)和金皇后(Queen)(引进品种),设置了取样数目分别为10、20、40和60个单株进行DNA混合,利用RAPD(random amplification polymorphic DNA,随机扩增长度多态性DNA)和SSR(simple sequence repeat,简单重复序列)标记分别进行了遗传多样性分析,结果发现40和60个单株DNA混合样的聚类结果一致,表明10和20个单株组成的群体太小,随着苜蓿群体取样数目的增加,遗传多样性分析的准确性也随之增加,但是分析成本也相应提高.鉴于此,利用RAPD和SSR标记分析苜蓿遗传多样性时采用40个单株的DNA混合样是较适宜的群体大小. 相似文献
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A set of 300 random ohgonucleotide primers was screened for random amplified polymorphic DNA (RAPD) fragments within a sample of 79 megagametophyte DNAs of a single masson pine ( Pinus massoniana Lamb. ) to generate RAPD markers and construct the molecular linkage map for masson pine. 64 repeatable RAPD markers segregated in a 1 present to 1 absent ratio. Through multipoint linkage analysis, 47 markers were assigned to 13 different linkage groups(pairs). It covered a tdtal genetic distance of over 692.5 cM (centimorgan). The average distance between markers was 14.7 cM. It supplied a linkage framework for a more saturated linkage map of masson pine. 相似文献
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An Integrated High-density Linkage Map of Soybean with RFLP, SSR, STS, and AFLP Markers Using A Single F2 Population 总被引:3,自引:0,他引:3
Xia Zhengjun; Tsubokura Yasutaka; Hoshi Masako; Hanawa Masayoshi; Yano Chizuru; Okamura Kayo; Ahmed Talaat A.; Anai Toyoaki; Watanabe Satoshi; Hayashi Masaki; Kawai Takashi; Hossain Khwaja G.; Masaki Hirokazu; Asai Kazumi; Yamanaka Naoki; Kubo Nakao; Kadowaki Koh-ichi; Nagamura Yoshiaki; Yano Masahiro; Sasaki Takuji; Harada Kyuya 《DNA research》2007,14(6):257-269
Soybean [Glycine max (L.) Merrill] is the most important leguminouscrop in the world due to its high contents of high-quality proteinand oil for human and animal consumption as well as for industrialuses. An accurate and saturated genetic linkage map of soybeanis an essential tool for studies on modern soybean genomics.In order to update the linkage map of a F2 population derivedfrom a cross between Misuzudaizu and Moshidou Gong 503 and tomake it more informative and useful to the soybean genome researchcommunity, a total of 318 AFLP, 121 SSR, 108 RFLP, and 126 STSmarkers were newly developed and integrated into the frameworkof the previously described linkage map. The updated geneticmap is composed of 509 RFLP, 318 SSR, 318 AFLP, 97 AFLP-derivedSTS, 29 BAC-end or EST-derived STS, 1 RAPD, and five morphologicalmarkers, covering a map distance of 3080 cM (Kosambi function)in 20 linkage groups (LGs). To our knowledge, this is presentlythe densest linkage map developed from a single F2 populationin soybean. The average intermarker distance was reduced to2.41 from 5.78 cM in the earlier version of the linkage map.Most SSR and RFLP markers were relatively evenly distributedamong different LGs in contrast to the moderately clusteredAFLP markers. The number of gaps of more than 25 cM was reducedto 6 from 19 in the earlier version of the linkage map. Thecoverage of the linkage map was extended since 17 markers weremapped beyond the distal ends of the previous linkage map. Inparticular, 17 markers were tagged in a 5.7 cM interval betweenCE47M5a and Satt100 on LG C2, where several important QTLs wereclustered. This newly updated soybean linkage map will enableto streamline positional cloning of agronomically importanttrait locus genes, and promote the development of physical maps,genome sequencing, and other genomic research activities. 相似文献
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A rice (Oryza sativa L. ) molecular linkage map has been constructed form over 52 random amplified polymorphic DNA (RAPD) markers with the double haploid (DH) population. It covered a total genetic distance of over 898.4 cM (centimorgan) with 17.3 cM between markers and was complemental with RFLP linkage map. 相似文献