甘蓝型黄籽油菜种皮色泽QTL作图

甘蓝型黄籽油菜具有低纤维、高蛋白及高含油量的优点,因而己成为广大油菜育种工作者研究的重点之一。利用甘蓝型黑籽品系油研2号作父本,计蓝型黄籽品系GH06为母本,获得132个单株的F2群体;以AFLP和SSR为主要分析方法,构建了包括164个标记的甘蓝型油菜遗传连锁图谱,其中包括125个AFLP标记、37个SSR标记及一个RAPD和一个SCAR标记,分布在19个连锁群上,覆盖油菜基因组2549．8cM,标记间平均距离15．55cM。利用多区间作图法,对种皮色泽QTL进行分析,在第5及第19连锁群上各检测到一个QTL位点,分别解释表型变异46％及30．9％。     

家蚕重要经济性状的QTL定位研究

利用AFLP技术, 对家蚕品系C₁₀₀和大造的回交一代BC₁群体进行了连锁图谱的构建. 在此基础上, 利用WinQTLCart2.0软件分析了影响家蚕全茧量、茧层量、茧层率和蛹体重等4个重要经济性状的QTL, 通过复合区间作图分析共检测到11个QTLs, 其中控制全茧量的QTLs有 2个, 分别定位在第6, 19两个连锁群上; 控制茧层量的QTLs有3个, 分别定位在第3, 14, 19三个连锁群上; 控制茧层率的QTLs有3个, 分别定位在第2, 11, 15三个连锁群上; 控制蛹体重的QTLs有3个, 分别定位在第2, 14, 19三个连锁群上. 利用紧密连锁的分子标记将不同的增效QTLs进行聚合, 为优质高产家蚕新品种的选育打下了极好的基础.     

金针菇单孢菌株菌丝生长速度QTL定位分析

本研究以已经完成基因组测序的单核菌株“6-3”与“6-21”为出发菌株,配对后获得有锁状联合的异核菌株并进行出菇,收集担孢子,单孢分离获得90个菌株构成作图群体,对作图群体的每个菌株进行二代测序并测定菌丝在PDA培养基的生长速度。分析“6-3”与“6-21”两单核菌株的SNP,获得68 914个高质量SNP标记用于遗传连锁群分析,构建了14个遗传连锁群,总长度744.32cM,平均长度为53.17cM,标记间平均遗传距离为1.88cM。QTL分析获得一个控制菌丝生长速度的基因座qMGRP1-LG7,该基因座包含134个基因,富集了与物质代谢有关的通路和基因。     

吴茱萸的AFLP指纹图谱的初步研究

首次报道中草药植物吴茱萸基因组DNA指纹图谱的研究。吴茱萸是贵州省内经济价值极高的中草药之一,采用扩增片段长度多态性（AFLP）技术来分析来自不同地区的石虎、疏毛、大花吴茱萸3个品种的DNA指纹图谱,从18对引物中筛选出3对引物对19份材料的DNA检测,共得到93条带,其中多态性片段57条（平均61.3%）。3对引物组合从DNA指纹图谱上将19份材料完全区分开,结果表明AFLP技术是鉴别吴茱萸相近品种的有效方法,是形态学鉴定方法的有益补充;UPGMA方法聚类分析显示19份种质材料间的相似系数为0.235～0.941,表明吴茱萸种质间的遗传多样性丰富;余庆地区种植基地的石虎和疏毛样本聚为一类,提示人工栽培影响到吴茱萸的遗传特性。     

大白菜部分形态性状的QTL定位与分析

应用352个标记位点的大白菜AFLP和RAPD图谱和一套栽培品种间杂交获得的重组自交系群体,采用复合区间作图的方法对大白菜9个形态性状进行QTL定位及遗传效应研究。在14个连锁群上检测到50个QTL:其中控制株型的QTL有5个;控制株高的QTL有6个;控制开展度的QTL有5个;控制最大叶长的QTL有7个;控制最大叶宽的QTL有4个;控制叶形指数的QTL有6个;控制中肋长的QTL有7个;控制中肋宽的QTL有4个;控制抽苔的QTL有6个。另外,估算了单个QTL的遗传贡献率和加性效应。这将为大白菜品种改良中形态性状的分子标记辅助选择提供理论依据。     

谷子SSR分子图谱的构建及主要农艺性状QTL定位

试验拟对谷子重要农艺性状进行数量性状位点QTL分析。以表型差异较大的沈3/晋谷20F2作图群体为材料,观测其株高、穗长等性状,选用SSR做分子标记,利用完备区间作图法(BASTEN C J)进行QTL分析。结果显示,表型数据在作图群体中呈现连续分布,表现为多基因控制的数量性状,被整合的54个SSR标记构建10个连锁群,LOD阈值设置为2.0,检测到与株高相关的主效QTL2个,联合贡献率45.9637%,穗长主效QTL1个,贡献率14.9647%,与穗重、粒重相关的主效QTL为同一位点,贡献率分别为11.9601%和10.1879%。有6组QTL位点之间存在基因互作效应,大小范围为-0.4986-16.6407,对性状的贡献率在2.2716％至6.7478％之间。谷子表型控制复杂,相关QTL的检测受环境影响较大,不同连锁群QTL间互作明显。     

7个烤烟产量相关性状的QTL定位分析

以烤烟Y3和K326为亲本,采用单粒传法(SSD)获得一个包含262个F6株系的重组自交系群体(RILs)。基于该群体构建了一张含有24个连锁群、626个SSR标记,总长为1 120.45cM的遗传图谱。通过两年一点3次重复的随机区组田间试验,测定了株高、节距、叶数、茎围、茎叶角度、腰叶长和腰叶宽7个与产量相关农艺性状,采用混合线性模型的严格复合区间作图法(rMQM)在烟草全基因组范围内进行QTL扫描分析。结果显示:(1)烤烟7个目标性状在RILs群体内各株系间存在较大范围的连续变异,具有显著的双向超亲分离,且各性状的平均值很接近中亲值;7个农艺性状的平均广义遗传率为73.33%,其中株高和节距的广义遗传率在80%以上,而茎围和茎叶角度的广义遗传率则低于60%,表明7个与烤烟产量相关的农艺性状是既受微效多基因控制又受环境条件影响的数量性状。(2)共检测到30个QTLs分布在9条连锁群上,其中与株高、节距、叶数、腰叶长和腰叶宽相关的5个主效QTLs在连续两年中均可检测到,且具有较大的效应值,可解释大于10%的表型变异。(3)7个目标性状之间存在一定程度的相关性,与之对应在基因组中也存在一些较小区域,每个区域包含2个或2个以上紧密连锁的不同性状的QTLs。烟草产量相关农艺性状的QTL分析和主效QTLs的获得,为进一步利用分子标记辅助选择培育烟草高产新品种奠定了理论基础。     

中国明对虾AFLP分子标记遗传连锁图谱的构建

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。     

利用RFLP标记定位水稻重要农艺性状的主效基因与微效基因

以一对籼粳交(圭630/02 428)经花药培养产生的双单倍体(DH)群体构建了含233个RFLP标记、覆盖基因组约2070cM的水稻分子图谱.利用QTL区间作图对水稻重要农艺性状如抽穗期、株高、有效穗、着粒数、实粒数、结实率和千粒重等7个性状的基因座位进行了定位分析,检测到8个主效基因和29个微效基因.双亲间性状差异较大有利于主效基因的鉴别.     

利用RFLP进行数量基因定位及效应分析的原理与方法

本文介绍了利用RFLP分子标记进行数量基因定位及效应分析的原理与方法,并讨论了其应用存在的问题．     

PERMANENT GENETIC RESOURCES: Twelve new microsatellite markers for the Chinese shrimp Fenneropenaeus chinensis

Twelve new microsatellite markers were isolated by sequencing random clones from a genomic library of Fenneropenaeus chinensis. The number of alleles per locus ranged from five to 15. The polymorphism information content ranged from 0.568 to 0.898, and observed and expected heterozygosities from 0.344 to 0.882 and from 0.691 to 0.915, respectively. All loci except one conformed to Hardy-Weinberg equilibrium. These markers, described here for Chinese shrimp, will be further used to analyse the species' population genetics.     

中国明对虾基因组小卫星重复序列分析

通过对中国明对虾基因组随机DNA片断的测序 ,我们获得了总长度约 6 4 10 0 0个碱基的基因组DNA序列 ,从中共找到 172 0个重复序列。其中 ,小卫星序列的数目为 398个 ,占重复序列总数目的 2 3 14 %。这些小卫星序列的重复单位长度为 7- 16 5个碱基 ,集中分布于 7- 2 1个碱基范围内 ,其中以重复单位长度为 12个碱基的重复序列数目最多 ,为 5 8个 ,占小卫星重复序列总数目的 14 5 7%。不同拷贝数目所对应的重复序列的数目情况为 :拷贝数目为 2的重复单位所组成的重复序列数目最多 ,为 137个 ;其次是拷贝数目为 3的重复序列 ,为12 2个 ,且随着拷贝数目的增加 ,由其所组成的重复序列的数目呈递减的趋势。其中一部分序列见GeneBank数据库 ,登录号为AY6 990 72 -AY6 990 76。 398个重复序列分别由 398种重复单位所组成 ,因而小卫星重复序列的类型很多 ,我们初步分成三类 :两种碱基组成类别、三种碱基组成类别和四种碱基组成类别 ,并进一步根据各个重复序列中所含有的碱基种类的数量从大到小排列这些碱基而分成若干小类。从这些分类中可以看出 ,中国明对虾基因组中的小卫星整体上是富含A T的重复序列 ,并具有一定的“等级制度” ,揭示了其与微卫星重复序列之间的关系 ,即一部分小卫星重复序列可能起源于微卫星     

Synaptonemal complex analysis in spermatocytes of diploid and triploid Chinese shrimp Fenneropenaeus chinensis

A modified surface spreading technique for synaptonemal complex (SC) analysis was tested to assess the process of chromosome synapsis in spermatocytes of diploid and induced triploid Fenneropenaeus chinensis. Spermatocytes of diploid shrimp showed typical morphological characteristics of eukaryote SC, with complete synapsis of bivalents. No recognizable bivalent associated with sex chromosomes was observed in spermatocytes of diploid shrimp. However, differences in morphology of SC, including unsynapsed univalents, bivalents, totally paired trivalents with non-homologous synapsis, partner switches and triple synapsis were identified at early pachytene stage of triploid spermatocytes. Triple synapsis was especially common at late pachytene stage in spermatocytes of triploid shrimp. The observed abnormal synapsis behavior of chromosomes in spermatocytes indicated that triploid male shrimp may find it difficult to develop normal haploid sperm.     

Molecular characterization and mRNA transcript profile of vitellogenin in Chinese shrimp, Fenneropenaeus chinensis

A full-length cDNA encoding vitellogenin (Vg) was cloned from Chinese shrimp, Fenneropenaeus chinensis using RACE method. The full-length cDNA consist of 7,942 nucleotides including a 7,761 bp open reading frame, which encodes 2,587 amino acid residues. The deduced amino acid sequence showed high (from 94% to 37%) identity with other known crustacean Vgs. In addition, a consensus cleavage site (R-X-K/R-R) recognized by an endopeptidase and a member of subtilisin family of serine protease were identified in the deduced Vg precursor. RT-PCR analysis shown that Vg mRNA can be detected in both ovary and hepatopancreas of vitellogenic females but not in other experimental tissues including muscle, heart, lymph organ, gill, haemocytes and intestine. These results suggest that the Vg gene may be expressed exclusively in mature females, and both ovary and hepatopancreas are the possible tissues for Vg synthesis in F. chinensis. In addition, Vg gene is detected in genomic DNA of both females and males.     

中国对虾精子顶体反应的超微结构和蛋白成分变化的研究

用卵水 (eggwater)对中国对虾纳精囊内精子进行人工诱导顶体反应 ,并分别用透射电镜和SDS—PAGE及复性单向电泳对顶体反应的超微结构变化和蛋白成分的变化进行了研究。结果表明 ,中国对虾精子在人工诱导条件下 3 0min内有 5 0 %以上完成反应。电镜观察证明 ,中国对虾精子的顶体反应可分为两个阶段 :(1 )棘突的收缩 ;(2 )顶体颗粒的释放和顶体帽的消失。在反应过程中许多蛋白被降解 ,且反应开始后精子本身释放出一些水解酶类 ,主要有 2 0 0kDa、1 3 0kDa、66kDa、5 3kDa、48kDa和 41kDa 6种。在对卵水成分的初步分析中发现两种分子量约 2 0 0kDa的蛋白。     

QTL mapping of economically important traits in Silkworm (<Emphasis Type="Italic">Bombyx mori</Emphasis>)

A backcrossed population(BC1)was derived from a cross between C1AFLP technique was employed for mapping the QTLs.The QTLs for the whole cocoon weight,cocoon shell weight,ratio of cocoon shell,weight of pupae etc.Were analyzed and 11 QTLs were detected based on the constructed linkage map.Two QTLs for whole cocoon weight were localized on linkage group 6 and 19; three QTLs for cocoon shell weight were localized on linkage group 3,14 and 19; three QTLs for ratio of cocoon shell were localized on the linkage group 2,11and 15,and three QTLs for the weight of pupae were localized on linkage 2,14 and 19.All these have laid an important base for the marker assisted breeding of the silkworm.     

Molecular characteristics and expression analysis of calreticulin in Chinese shrimp Fenneropenaeus chinensis

Calreticulin (CRT), as an endoplasmic reticulum luminal resident protein, plays important roles in Ca(2+) homeostasis and molecular chaperoning. CRT on the surface of the cell can modulate cell adhesion, phagocytosis and integrin-dependent Ca(2+) signaling. The full length cDNA of calreticulin (FcCRT) was cloned from Chinese shrimp Fenneropenaeus chinensis. It consists of 1672 bp with an open reading frame of 1221 bp, encoding 406 amino acids. This is the first reported cDNA sequence of calreticulin in Crustacea. The deduced amino acid sequence of FcCRT showed high identity with those of Bombyx mori (88%), Drosophila melanogaster (83%), Mus musculus (82%) and Homo sapiens (82%). Highest expression of FcCRT was detected in ovary by Northern blot and in situ hybridization. Different mRNA levels of FcCRT were detected at various molting stages. Expression of FcCRT was induced significantly after 3 h of heat shock treatment, reached the maximum at 4 h and dropped after that. Differential expression profiles of FcCRT were observed in hepatopancreas and haemocytes when shrimp were challenged by white spot syndrome virus (WSSV). From the above results, we inferred that FcCRT might play important roles in Ca(2+) homeostasis, chaperoning and immune function in shrimp.