红唇薄鳅2个野生群体的遗传多样性研究

采用9个微卫星DNA标记对长江支流岷江下游厥溪和长江上游干流朱杨溪红唇薄鳅的2个野生群体遗传多样性及遗传分化情况进行了研究。共检测出73条等位基因,其中厥溪群体中有55条等位基因,朱杨溪群体中有69条等位基因,两群体共有等位基因数为51条。厥溪群体和朱杨溪群体的平均等位基因数分别为6.111和7.667,平均观测杂合度分别为0.665和0.668;平均期望杂合度分别0.684和0.712,平均多态性信息指数分别为0.621和0.656,从各参数结果来看,朱杨溪群体的遗传多样性水平高于厥溪。AMOVA结果显示,大多数遗传变异存在于红唇薄鳅群体内(98.68%),群体间的遗传变异为1.32%,固定系数不显著。基因流为9.42,表明两群体间基因交流频繁。UPGMA聚类显示,厥溪和朱杨溪群体中的个体相互混杂。这些结果表明长江上游厥溪和朱杨溪群体未出现遗传分化。     

应用RAPD标记对东方(鱼屯)属进行种类鉴别及其聚类分析

利用RAPD技术对红鳍东方、假睛东方、暗纹东方和从日本引进的红鳍东方4个种进行了遗传标记鉴别研究.在事先优化的条件下,20个随机引物共扩增出134条谱带清晰、重复性高的DNA片段,其中多态性片段77条.结果证实每一种均有其特异性扩增图谱,可作为种鉴定的依据;用UPGMA和NJ等方法进行聚类,构建的系统树与借助形态学和生化特征进行的传统分类结果一致.研究表明,RAPD作为一种新的分子标记,在海洋动物遗传鉴定方面具有巨大的潜力.     

基于微卫星标记建立翘嘴鳜亲子鉴定技术

利用9个多态性较高的微卫星标记对翘嘴鳜(Siniperca chuatsi)进行亲子鉴定分析。结果显示,22个家系翘嘴鳜个体中共观测到95个等位基因,其观测杂合度和期望杂合度的平均值(范围)分别为0.578(0.219~0.800)和0.607(0.200~0.806),多态信息含量(范围)为0.552(0.187~0.787)。通过软件Cervus统计分析得到9个微卫星座位累计排除率为99.9658%,在27个可能的父母对条件下,混养养殖家系后代个体鉴定准确率为91%,研究结果表明筛选的这些多态微卫星分子标记可以用于翘嘴鳜优势家系的鉴定和分离,通过验证的微卫星标记建立的亲子鉴定技术为基础选育翘嘴鳜生长速度快的优势家系,为培育出生长速度快、抗病力强的翘嘴鳜新品种奠定基础。     

鲤IGF-Ⅰ基因2个高度多态微卫星位点的鉴定及其与生长相关性状的关联分析

利用PCR结合测序方法,在鲤(Cyprinus carpio)类胰岛素生长因子-Ⅰ(insulin-like growth factor-Ⅰ,IGF-Ⅰ)基因内含子1和内含子2中各鉴定1个微卫星多态性位点,分别命名为intron1189和intron2310,这两个位点均以4碱基为重复单元.以黑龙江鲤(Cyprinus cario haematopterus,YL)(n=263)、德国镜鲤选育系(Cyprinus carpio L.mirror,JL)(n=229),及荷包红鲤抗寒品系(Cyprinus carpio var.wuyuanensis,HL)(n=255)为研究对象,评估了这两个位点不同基因型(频率＞3％)与鲤4个生长时段(135 d、325 d、335 d和445 d)生长表型的关联.结果显示,2个位点在3个鲤群体中均表现为高度多态(PIC＞0.5).intron1189位点多态性主要对YL的135 d、325 d体长和325 d、385 d体质量有显著影响(P＜0.05),而intron2 310位点多态性对JL各检测时段的体长和体质量均有显著影响(P＜0.05).对不同基因型个体的体长和体质量性状进行多重比较,结果显示,在intron 1189位点,185/229基因型YL的135 d、325 d体长和325 d、385 d体质量最低,而205/221基因型YL的135 d、325 d体长和325 d体质量最高.在mtron2310位点,290/350基因型JL在各检测时段的体长及135 d、325 d、385 d体质量最低,而318/350基因型JL的135 d、325 d、385 d体长和体质量均为最高.上述结果表明,鲤IGF-Ⅰ基因内含子中的这两个高度多态微卫星位点潜在影响鲤的生长性能.     

Microsatellite marker isolation and cultured strain identification in <Emphasis Type="Italic">Carassius auratus gibelio</Emphasis>

Microsatellites have become the preferred molecular markers for strain selection and genetic breeding in fish. In this study a total of 105 microsatellites were isolated and identified in gibel carp (Carassius auratus gibelio) by microsatellite sequence searches in GenBank and other databases and by screening and sequencing of positive clones from the genomic library enriched for AG and GATA repeats. Moreover, nineteen microsatellites were randomly selected to design locus-specific primer pairs, and these were successfully used to identify and discriminate different cultured strains of gibel carp including strains A, D, L, and F. Three different types of microsatellite pattern were distinguished by the number and length of fragments amplified from the 19 primer pairs, and some microsatellite primer pairs were found to produce different microsatellite patterns among strains and strain-specific fragments. In addition, some duplicated alleles were also detected in two microsatellite patterns. Therefore, the current study provides direct molecular markers to discriminate among different cultured strains for selective breeding and aquaculture practice of gibel carp.     

A method to determine protein digestibility of microdiets for larval and early juvenile fish

A method to evaluate protein quality using in vivo methods was developed for larval fish. FluoSpheres^® fluorescent microspheres (10 μm) were incorporated into two test diets, our standard zein microdiet (ZMD) and a microdiet with identical ingredients except for the replacement of high quality fish meal with the same product cooked for 24 h at 80 °C (ZMD-CF). Several trials were performed to design a reliable method to test digestibility using FluoSpheres^® as a marker. The developed in vivo technique was tested on 35 days posthatch (dph) larval Atlantic cod ( Gadus morhua L.) and two tropical fish species in the early juvenile stage. The method took into account loss of total protein to the faecal pellet and water column. Apparent digestibility of protein in larval cod fed ZMD was significantly higher than that of larvae fed ZMD-CF ( P  < 0.05). A growth study to validate differences between the two diets showed significant differences in growth and survival of larvae fed ZMD versus ZMD-CF ( P  < 0.05). Further validation of our results was indicated through the use of a pH-stat method using enzymes extracted from 35 dph larval cod guts. This novel technique will be advantageous for researchers to evaluate feed ingredients for larval marine fish and is adaptable to many different areas of larval fish nutrition.     

Genetic variability in meiotic gynogenetic muskellunge,Esox masquinongy (Mitchell), estimated from segregation of microsatellite alleles

Muskellunge, Esox masquinongy, is an important recreational freshwater fish native to North America. Since muskellunge populations are often maintained through stocking efforts, advances in muskellunge reproductive technologies are of direct relevance to fishery enhancement. We evaluated the efficiency of inbreeding through induced meiotic diploid gynogenesis. Eggs from six female muskellunge were manually stripped and activated using ultra violet‐irradiated yellow perch, Perca flavescens, sperm. Hydrostatic pressure shocking regimes (48 263 kPa) were then applied to the eggs to prevent second polar body expulsion producing unambiguous meiotic gynogens. Six female dams and samples of 12–20 of their gynogenetic progeny were genotyped at seven polymorphic microsatellite loci. Chromosomal recombination frequencies of microsatellite loci based on retention of heterozygosity among gynogens ranged from 0.043 to 0.839 (0.576 ± 0.237). There were no statistical differences in recombination frequency among females at any of the loci. The average inbreeding coefficient (F‐value) ranged from 0.581 to 0.979, equivalent to three to fourteen generations of full‐sibling crosses respectively. The average F‐value overall was 0.712, equivalent to between five and six generations of full‐sibling crosses. Centromere map distances of the seven microsatellite loci ranged from 2.15 to 41.95 cM and meiotic gynogenesis was useful in eliminating heterozygosity at loci proximal to the centromere, but not distal. Since the age at maturity of female muskellunge is approximately 5 years, gynogenesis may pose an expeditious alternative to traditional breeding strategies for creation of homozygous pedigrees for some loci that may be outcrossed to introduce positive heterozygosity effects in the offspring.     

异源精子诱导犬齿牙鲆的雌核发育

用冷冻保存的花鲈精子作为异源精子,采用紫外线(UV)对精子进行照射使其遗传物质失活,然后与卵子进行"授精",可以刺激犬齿牙鲆鱼卵进行雌核发育,在受精后一定时间采用冷休克处理"授精"卵,抑制第二极体排出成功获得了犬齿牙鲆雌核发育二倍体鱼苗.实验表明:犬齿牙鲆同源精子经80 mJ/cm2的紫外线照射可以完全失活,冻存花鲈精子经紫外线照射后也同样具有诱导犬齿牙鲆雌核发育的能力.无论同源精子还是异源精子,最佳诱导条件为在18℃条件下,精子经80 mJ/cm2的紫外线照射,受精后4～5 min将受精卵放在3℃海水中进行冷休克处理,持续时间为45 min,同源精子和异源精子二倍体诱导分别为32.66%±7.03%和28.00%±6.48%.采用形态学、流式细胞仪DNA含量分析和微卫星标记技术对雌核发育鱼苗进行了分析,证明了雌核发育鱼苗为雌核发育二倍体.     

中华绒螯蟹37个多态性微卫星标记在亲子遗传中的分离方式分析

为了评估基因组扫描方法获得的中华绒螯蟹微卫星标记的遗传方式,随机选择60个候选三核苷酸微卫星标记,首先利用中华绒螯蟹F1家系双亲及其6个F1子代共8个样品进行PCR扩增验证和多态性检测,随后对多态性标记位点在80子代个体中的亲子遗传分离类型及连锁关系进行了分析。结果显示,42个（70.00%）位点得到清晰扩增产物,其中有5个单态微卫星位点和37个多态微卫星位点。多态位点中23个位点子代基因基因型为1：1：1：1分离类型,11个位点属1：1分离类型,余下3个位点为1：2：1分离类型。37个多态位点中35个位点（94.59%）的分离符合孟德尔分离比（P>0.05）,scaffold430598_213690和scaffold21303_16865位点显著偏离1：1：1：1分离比。35个分离比符合孟德尔分离比的位点中,scaffold240262_150253、scaffold216209_138892、scaffold293154_172768三个标记发生连锁关系,scaffold285640_169721和scaffold427534_212914发生连锁关系,scaffold507500_231891和scaffold92860_68250标记发生连锁关系。以上结果表明开发的候选微卫星标记适用于中华绒螯蟹亲子鉴定和遗传图谱构建。     

尼罗罗非鱼(♀)×萨罗罗非鱼(♂)杂交F_2与F_3群体遗传特征的微卫星分析

利用罗非鱼第二代遗传连锁图谱中微卫星标记对尼罗罗非鱼(Oreochromis niloticus)(♀)×萨罗罗非鱼(Sarotherodon melanotheron)(♂)杂交后代F_2、F_3群体遗传特征进行了初步比较分析。结果显示,28对引物中有22对引物能有效扩增,未观察到杂交后代F_2、F_3中有多倍体个体现象。筛选出7个在尼萨罗非鱼杂交后代F_2、F_3群体中存在差异的位点。杂交F_2群体平均等位基因(Na)为2.71,平均多态信息含量(PIC)为0.466,平均观测杂合度(Ho)为0.632;杂交F_3群体平均Na为2.14,平均PIC为0.370,平均Ho为0.432,杂交F_3遗传杂合性较杂交F_2降低。F_2自繁F_3过程中,F_3群体4个位点的等位基因与F_2完全相同,3个位点的等位基因少于F_2,且F_3群体在2个位点出现完全纯合,杂交F_3群体位点等位基因呈现纯合趋势。研究结果为尼萨罗非鱼杂交世代遗传变异与杂交利用积累基础资料。