基于微卫星标记的三疣梭子蟹家系系谱认证

用6个微卫星标记对三疣梭子蟹(Portunus trituberculatus)的6个家系进行系谱鉴别和遗传多样性研究。6个微卫星标记在6个家系中显示了高度的遗传差异,6个位点的多态信息含量(PIC)分别为Pot09位点0.6045,Pot14位点0.6072,Pot17位点0.8130,Pot18位点0.6870,Pot25位点0.7839,Pot42位点0.6330。6个多态性位点共发现了32个等位基因,每个位点的等位基因数在4～8个之间。不同位点共发现7个家系特异性等位基因,2#和3#家系中各发现2个,1#、5#、6#家系中各发现1个,4#家系未发现特异性等位基因。根据已知亲本及子代基因型,可推断出6个家系中全部亲本的基因型,据此鉴别各家系。在Pot18位点可将1#家系和6#家系与其他家系相区别;Pot14位点和Pot17位点可将3#家系与其他家系相区别;Pot42位点可将5#与其他家系相区别;Pot17位点和Pot25可将2#家系与其他家系相区别。因此,Pot18位点、Pot14位点和Pot17位点、Pot42位点、Pot17位点和Pot25位点可分别用于鉴别1#和6#家系、3#、5#、2#家系的特异性标记。研究表明,在选用的6个微卫星标记中,最少选用3个标记可鉴别6个三疣梭子蟹家系。     

大菱鲆亲子鉴定的微卫星多重PCR技术建立及应用

用8个微卫星标记组合建立了2个微卫星多重PCR体系,对大菱鲆7个人工选育家系进行了系谱认证、亲子鉴定和遗传多样性研究。2个多重PCR体系中8个微卫星位点共检测到等位基因49个,每个位点等位基因数为3~8个。根据已知亲本及子代基因型,成功推断出了3个缺失亲本的基因型。在双亲未知的情况下2个多重PCR的8个微卫星位点累积排除概率是96.58%,已知1个亲本时累积排除率为99.71%,亲子鉴定准确率为96.42%。采用70个个体进行双盲验证,利用UPGMA法对7个家系的70个体进行了聚类分析,同一家系95.71%的个体聚类分析结果与系谱来源一致。Cervus 2.0软件亲子鉴定结果表明亲子鉴定准确率为92.86%。2个多重PCR体系的建立为大菱鲆不同家系混养后的亲子鉴定、系谱分析和分子辅助家系管理提供了技术手段。     

长牡蛎(Crassostrea gigas)微卫星多重PCR 体系构建及其在家系鉴定中的应用

筛选多态性高、特异性好、片段大小适中的10 个长牡蛎微卫星位点进行优化组合, 根据扩 增片段大小及同一荧光不重叠原则构建了两组五重PCR 体系。运用CERVUS 3.0 软件对0527 组27 个长牡蛎全同胞家系的643 个子代和0612 组27 个全同胞家系382 个子代分别进行亲权鉴定。结果 发现, 用两组微卫星五重PCR 鉴别时, 在0527 组和0612 组的鉴定成功率均为100%; 只用第一组微 卫星五重PCR, 可以将0527 组96%的子代和0612 组96%的子代鉴定到亲本; 只用第二组微卫星五 重PCR, 可以将0527 组97%的子代和0612 组95%的子代鉴定到亲本。本研究中筛选出的两组微卫 星五重PCR 体系在两组家系中的鉴定效率均较高, 可以快速有效地将子代个体鉴定至所属父母本, 在长牡蛎家系鉴定中具有很好的应用价值。     

Assessing multiple mating and reproductive skew in three species of clinid fishes (Blenniiformes: Clinidae: Clinini), in reference to multiple mating in viviparous teleosts

This study investigated multiple mating in three species of intertidal klipfishes (family Clinidae): super klipfish Clinus superciliosus, bluntnose klipfish Clinus cottoides, and nosestripe klipfish Muraenoclinus dorsalis. These species display the rare reproductive mode of female vivipary with superfetation, a phenomenon where offspring at various stages of development are found within the female. Three or four microsatellite loci were used to genotype 25–30 adults of each species, as well as embryos of 131 C. superciliosus from six broods, 103 C. cottoides from six broods, and 63 M. dorsalis from five broods. The presence of multiple mating by females was assessed by maximum-likelihood sibship reconstruction implemented in the program COLONY, and the non-random distribution of reproductive success among individuals (reproductive skew) within broods was tested using the binomial skew index. Multiple mating by females was pervasive and observed in 83%, 100% and 80% of the broods of C. superciliosus, C. cottoides and M. dorsalis, respectively. The mean number of sires per brood was 4.3, 3.0 and 3.2, and, correspondingly, 5/5, 5/6 and 1/4 of multiply-sired broods showed significant reproductive skew in C. superciliosus, C. cottoides and M. dorsalis, respectively. The presence of pronounced reproductive skew may indicate post-copulatory processes taking place that bias paternity. We compared our results on multiple mating within the klipfish family, and with four other fish families that have vivipary with superfetation, and found the klipfish patterns were among those of live-bearing vertebrate groups with the highest average numbers of sires per brood.     

Establishment of microsatellite-based triplex PCR for parentage analysis of Chinese shrimp Fenneropenaeus chinensis

Through exploring the microsatellite primers from the random genome sequences of Chinese shrimp (Fenneropenaeus chinensis), some microsatellite primers were obtained with rich polymorphic genetic information, and a triplex PCR was established using three primers (RS1101, RS0683 and H081 primers). By adjusting the final concentration of Mg2 , dNTP and primers, and using a touch-town PCR program, the optimum amplification parameters of PCR system were obtained, which could successfully amplify the three primers in a PCR reaction. In the denatured PAGE gel, the amplified DNA fragments of three primers RS1101, RS0683 and H081 could be easily identified each other. For the triplex PCR system, the PPE (probabilities of paternity exclusion) is 0.967 9, and the DP (discrimination power) is 0.999 327. Using the triplex PCR to test ten individuals of a parentage and their parents, an individual was excluded from the parentage in all of the three microsatellite loci, which might be mixed into the parentage for some unknown reason such as factitious misplay. The triplex PCR will be of great practical value in identifying the parentages of F. chinensis.     

微卫星标记在刺参(Apostichopus japonicus)人工繁育中亲本识别的应用

选取8个高多态性的微卫星位点, 对240只刺参(Apostichopus japonicus)幼体和14只疑似亲本进行了亲缘关系的鉴定。通过检测, 8个微卫星位点共得到53个等位基因, 平均等位基因数为6.63; 观察杂合度在0.730—0.902; 各位点的多态信息含量为0.696—0.836。通过亲缘关系分析软件CERVUS 3.0分析, 微卫星位点累积排除概率分别为0.9934、0.9997、0.99999。基于排除法个体基因型判定, 有37个子代有1个候选亲本, 194个子代有2个及以上候选亲本; 基于似然法判定, 置信度为80%时, 有198个子代个体找到最似亲本。综合排除法和似然法的亲权鉴定, 成功为229个子代个体找到它们的亲本, 鉴定成功率达95%以上。本研究结果可为刺参育种工作中亲本识别及家系分析提供技术支持和理论依据。     

Multiplex PCR Sets of Novel Microsatellite Loci for Iwagaki Oyster Crassostrea nippona and Their Application in Parentage Assignment

Iwagaki oyster,Crassostrea nippona,widely distributes along the seashore of Eastern Asia,and has been considered to be a potential breeding species due to its delicious taste and high commercial value.In order to study its genetic background and population structure,we developed 46 novel polymorphic microsatellite markers using next-generation sequencing technique and characterized them in 30 individuals.The number of alleles ranged from 3 to 22,while the observed and expected heterozygosities varied from 0.133 to 1.000 and 0.455 to 0.949,respectively.Fifteen microsatellite markers were selected and grouped into five highly informative multiplex PCRs for C.nippona.We evaluated and validated these multiplex PCRs in a cultured population including 173 candidate parents and 486 offspring.In actual parentage analysis,80%of the offspring were correctly assigned to their parental pairs using three multiplex PCRs.Furthermore,the success rate of parentage assignment reached 96%when the other two multiplex PCRs were added.These 46 microsatellite loci with high variability and the five multiplex PCRs described here provide a powerful tool for pedigree reconstruction,resource conservation and selective breeding program of C.nippona.     

长毛对虾(Penaeus penicillatus)SNP标记开发及亲子鉴定技术研究

长毛对虾是我国南方沿海地区的重要经济虾类。近年来,由于过度捕捞、病害频发以及海洋环境恶化,长毛对虾的自然资源量大幅减少。为补充自然资源,改善种群结构,1980年我国开始对长毛对虾开展增殖放流工作。然而,增殖放流的效果如何,目前尚缺乏有效的评估手段。以长毛对虾为实验材料,通过对其基因组进行de novo测序和重测序开发SNP (single nucleotide polymorphism)标记,最终建立长毛对虾的亲子鉴定技术。具体研究结果如下:长毛对虾基因组大小为1 335.76 Mb GC (guanine cytosine)含量为40.86%,N50为1 221 bp;以组装的长毛对虾基因组为参考基因组通过重测序进行SNP挖掘,共获得12 579 780个原始SNP位点,经筛选,优化及模型选择,最终建立了基于192个SNP标记的长毛对虾亲子鉴定技术,亲子鉴定成功率为100%(95%的置信度)。研究结果可为下一步长毛对虾增殖放流效果评估提供参考。     

基于微卫星标记的长江江苏段鲢(Hypophthalmichthys molitrix)增殖放流资源贡献率的评估

近年来,长江下游进行了大规模鲢(Hypophthalmichthys molitrix)增殖放流活动,而增殖放流对鲢资源的贡献如何,成为亟待探究的科学问题.本研究基于已开发的11对微卫星引物,标记8个主要原良种场(为江苏省各地政府放流工作提供苗种的单位)鲢繁殖亲本群体,利用微卫星亲子鉴定技术,评估2016-2017年长江江苏段鲢增殖放流对鲢在江群体的资源贡献率.研究结果显示,621尾繁殖亲本群体和475尾长江捕捞鲢群体共检测出191种等位基因,每个座位的等位基因种类数、观测杂合度、期望杂合度范围分别为9～36、0.536～0.793、0.597～0.941;对应平均值分别为17.36、0.656、0.794.11个座位均表现出高度的多态性,每个座位的多态信息含量范围为0.560～0.938,平均值为0.771,证明选用的11对微卫星引物可作为亲子鉴定的有效工具.亲子鉴定结果表明,在亲本性别未知的情况下,非亲排除率(NEP)范围为2.4%～42.4%,累积非亲权排除率(CEP)在99.99%以上; 475尾长江鲢群体中,鉴定出39尾鲢个体来自于原良种场鲢亲本群体所繁殖的后代,即回捕率为8.21%.综合分析可见,2016-2017年,长江江苏段增殖放流对鲢资源量有较好的补充作用.