马氏珠母贝(Pinctada martensii)黑壳色养殖群体SSR遗传多样性分析

本研究利用微卫星分子标记技术,对马氏珠母贝(Pinctada martensii)F8代黑壳色普通养殖群体和黑壳色选育群体2个群体共78个个体的遗传多样性进行分析.结果显示,10个SSR位点共扩增出34个等位基因,各位点的等位基因数为2～6个,平均等位基因数为3.4个,黑壳色普通养殖群体和黑壳色选育群体等位基因数(Na...     

合浦珠母贝三个养殖群体微卫星遗传多样性

以广东徐闻金碧公司养殖场、广西北海营盘镇养殖场和南海水产研究所海南实验基地3个合浦珠母贝养殖群体为对象,利用8个微卫星位点M1、M2、M3、M4、M5、M6、M7、M8的引物进行了遗传多样性分析.结果表明:8个微卫星标记位点在3个养殖群体中共检测到58个等位基因,观测等位基因数为2～9个,平均有效等位基因数3.72～5.06,平均观察杂合度0.41～0.56,平均期望杂合度0.67～0.75,3个群体的平均多态信息含量PIC值为0.62～0.70,全部为高度多态(PIC≥0.5),表明这几个合浦珠母贝养殖群体目前仍具有较高的遗传多样性,遗传信息丰富,遗传变异大,可以作为良好的育种材料;在这3个养殖群体中,南海水产研究所海南实验基地的养殖群体的遗传多样性最高,广西北海营盘镇养殖群体遗传多样性最低,这一结果可以为今后选择育种、种质保护提供可资借鉴的资料.

Abstract：

By using eight mierosatellite loci (M1, M2, M3, M4, M5, M6, M7 and MS), the genetic diversity of three Pinctada fucata populations from the pearl farms in Xuwen of Guang-dong and Beihai of Guangxi, and from the experimental base of South China Sea Fisheries Re-search Institute in Hainan was studied. A total of fifty eight alleles of these eight microsatellite lo-ci were detected, among which, the observed allele number was 2-9, average effective allele number was 3.72-5.06, average observed population heterozygosity was 0. 41-0. 56, and aver-age observed expected heterozygosity was 0. 67-0. 75. All the three populations had a polymor-phie information content (PIC) of 0. 62-0.70, suggesting their high polymorphism (PIC > 0. 5). Among the three populations, the cultured population from the experimental base of South China Sea Fisheries Institute had the highest polymorphism, and that from Beihai of Guangxi had the lowest one. These results provided useful information for the selective breeding and germplast conservation of P. Fucata.     

野生马氏珠母贝子一代的遗传多样性

分析了海南省三亚与广西省北海两地野生贝群体内交配所得子代两群体 (SS、BB)和群体间交配(SS♀ ×BB♂ →BS)所得子代群体 (BS)各 8个个体的遗传多样性。筛选的 2 0个含 1 0碱基的随机引物中 ,其中 1 4个产生稳定的可重复的多态扩增结果 ,共检测出 1 2 4个位点。用修正的Shannon表型多态性指数量化三个群体的遗传多态度 ,SS、BB、BS三群体的多态度分别为 0 2 47,0 2 3 7,0 2 61。SS与BB ,SS与BS ,BB与BS三群体间的遗传相似度分别为 87 2 4% ,80 3 9% ,83 90 %。讨论了不同地域之间进行马氏珠母贝育种及遗传多样性保护工作的可行性     

马氏珠母贝4个壳色选育系F_1遗传结构的AFLP分析

本研究从湛江流沙港马氏珠母贝养殖群体中挑选不同壳色个体为亲本,共构建了黑(BS)、红(RS)、黄(YS)和白壳色(WS)4个壳色选系F1,然后分别在4个壳色选育系F1中随机取样,利用3对AFLP引物分析其遗传结构与遗传分化。结果表明,每对引物的扩增位点数在104～109之间,共得到331个扩增位点;BS、RS、YS和WS壳色选系F1的多态位点比例分别为49.2%、49.5%、51.6%和63.4%,Shannon's多样性指数分别为0.1884、0.1886、0.1896和0.1954,4个壳色选育系F1的遗传分化系数(Fst)为0.1972。本研究说明经过一代壳色纯化4个壳色选育系F1出现显著遗传分化,也为马氏珠母贝壳色系选育或选育系间杂交提供了参考依据。     

马氏珠母贝F8代黑壳色选育系群体与普通养殖群体遗传多样性分析

利用9个SSR分子标记研究马氏珠母贝F_8代黑壳色选育群体与普通养殖群体的遗传多样性。结果显示:9个位点共检测出30个等位基因,各位点的等位基因数(Na)为2～5,平均等位基因数为3.333 3个。F_8代黑壳色选育系群体和普通养殖群体的平均等位基因数(Na)分别为2.777 8、3.222 2;平均有效等位基因数(Ne)分别为2.162 5、2.031 9;平均多态信息含量PIC值范围为0.129 1～0.730 0,平均期望杂合度(He)范围为0.223 1～0.857 7,平均观测杂合度(Ho)范围为0～0.950 0。F_8代黑壳色选育系群体有3个位点观测杂合度为0,说明这3个位点已被纯化。哈迪-温伯格平衡(HWE)检验发现,F_8代黑壳色选育系群体中有7个位点、普通养殖群体中有5个位点极显著偏离平衡(p0.01)。两群体遗传分化系数(Fst)为0.146 3。各项遗传参数表明,经8代群体继代选育,马氏珠母贝黑壳色选育系群体部分位点已被纯化,遗传多样性较普通养殖群体有所降低,但仍保持在较高水平。     

大亚湾核电站邻近水域马氏珠母贝的种群生态

１９９３年７月－１９９４年１２月,在大亚湾东山珍珠养殖场进行马氏珠母贝的生长和死亡率研究,结果表明：中、小贝种群个体大小组成呈正态分布,进入中贝以后,正态分布不明显。小贝生长快,壳高增幅大,死亡率较低,中贝以后,生长较慢,死亡率较高。     

马氏珠母贝雌雄同体和自体受精的研究

对马氏珠母贝(Pinctada martensiiDunker)成体的性腺进行外观和切片观察,可把马氏珠母贝雌雄同体的个体分为2种类型,其中A类型可以从性腺外观特征上辨别,而B类型需性腺穿刺或组织切片来确认。对试验群体的性腺的类型进行的初步统计表明,雌雄同体个体比例A类型为4.6%,B类型为3.4%,其中雌雄生殖细胞均接近成熟的个体分别约为1.8%和2.1%。通过解剖、0.07‰的氨海水处理,对雌雄同体个体的自体授精及其早期胚胎发育进行了研究,发现自体授精的受精率低于异体授精,同时在发育过程中有较多的卵裂球解体,但仍有部分胚胎可以发育成D型幼虫。     

马氏珠母贝galectin-4基因cDNA的克隆及表达分析

半乳糖凝集素(Galectins)属于一种多功能凝集素家族,在机体抵抗微生物的感染中起重要作用。本研究利用cDNA末端快速扩增(rapid-amplification of cDNA ends,RACE)技术克隆获得马氏珠母贝galectin-4(PmGal-4)基因cDNA的全长,并对其序列进行分析。PmGal-4基因cDNA全长1 071 bp,5′非翻译区(5′UTR)长75 bp,3′非翻译区(3′UTR)长72 bp;其开放阅读框(open reading frame,ORF)长度为924 bp,编码307个氨基酸组成的前体肽,理论分子量约为34.6 kD,理论等电点为8.80。多序列比对结果显示各物种间galectin-4具有高保守性。序列分析结果显示PmGal-4的氨基酸序列具有典型富含半胱氨酸(cysteine-rich domain,CRD)的结构域。实时荧光定量PCR分析表明,PmGal-4基因在马氏珠母贝所检测的组织中呈组成型表达特征,但在闭壳肌和外套膜中表达量最高。上述结果表明PmGal-4基因可能参与了马氏珠母贝多种生理功能,特别是在免疫防御反应中具有重要的作用。     

马氏珠母贝Caspase-3基因克隆和组织表达分析

半胱氨酸蛋白酶3 (Caspase-3)作为细胞凋亡通路中重要的效应蛋白,在细胞凋亡过程中发挥着重要作用.为初步探究马氏珠母贝Caspase-3(PmCaspase-3)的生物学功能,本研究利用cDNA末端快速扩增(RACE)技术克隆获得PmCaspase-3基因cDNA的全长序列并对其序列特征进行分析;同时利用实时荧光定量PCR (RT-qPCR)方法分析了PmCaspase-3基因mRNA在马氏珠母贝不同组织和不同发育时期的表达差异.结果 显示,PmCaspase-3基因cDNA全长为2233 bp,其中5'端非编码区长度为80 bp,3'端非编码长度为31 bp,开放阅读框长度为2088 bp,共编码695个氨基酸;生物信息学分析显示,PmCaspase-3含有Caspase家族特有的CASc结构域和半胱氨酸蛋白酶家族p20、p10活性位点以及多种磷酸化位点,经进化分析以及多序列比对可知与其他物种Caspase-3蛋白同源性较高.RT-qPCR结果表明,PmCaspase-3在肝胰腺中的表达量最高,在闭壳肌中的表达量最低;在发育过程中D型幼虫期和眼点期的表达量较高.     

Microsatellite Markers and Genetic Diversity of Four Scleractinian Corals

Russian Journal of Marine Biology - Eighteen microsatellite sequences were isolated from Platygyra acuta through magnetic bead hybridization enrichment method, and the site primers were used to...     

用4个微卫星标记分析7个绵羊群体之间的遗传关系

分析了4个微卫星基因座BM143、OarHH35、OarAE101、BMS2508在7个绵羊群体(小尾寒羊、湖羊、乌珠穆沁羊、萨福克羊、多赛特羊、夏洛来羊、多赛特公羊×小尾寒羊母羊F1代杂种羊)286只绵羊中的遗传多态性。结果表明,这4个微卫星标记在7个绵羊群体中的等位基因数分别为9、11、14和9,其多态信息含量/有效等位基因数/杂合度分别为0 7073/3 7231/0 7314、0 8267/6 4399/0 8447、0 5743/2 5178/0 6028、0 6172/3 0712/0 6744,其中OarHH35的遗传变异最大,OarAE101最小。7个绵羊群体中小尾寒羊的遗传变异最大,湖羊的最小。基于Nei氏DA距离和DS标准遗传距离,采用UPGMA方法构建了系统发生树。该发生树将中国地方品种(小尾寒羊、乌珠穆沁羊、湖羊)和法国的夏洛来羊归为一类,将F1杂种羊、英国品种(萨福克羊和多赛特羊)归为另一类。绵羊微卫星基因分型技术为检查品种(群体)之间的遗传关系提供了一个有用的工具。     

用4个微卫星标记分析7个绵羊群体之间的遗传关系

分析了4个微卫星基因座BM143、OarHH35、OarAE101、BMS2508在7个绵羊群体（小尾寒羊、湖羊、乌珠穆沁羊、萨福克羊、多赛特羊、夏洛来羊、多赛特公羊×小尾寒羊母羊F1代杂种羊）286只绵羊中的遗传多态性。结果表明,这4个微卫星标记在7个绵羊群体中的等位基因数分别为9、11、14和9,其多态信息含量/有效等位基因数/杂合度分别为0.7073/3.7231/0.7314、0.8267/6.4399/0.8447、0.5743/2.5178/0.6028、0.6172/3.0712/0.6744,其中OarHH35的遗传变异最大,OarAE101最小。7个绵羊群体中小尾寒羊的遗传变异最大,湖羊的最小。基于Nei氏DA距离和DS标准遗传距离,采用UPGMA方法构建了系统发生树。该发生树将中国地方品种（小尾寒羊、乌珠穆沁羊、湖羊）和法国的夏洛来羊归为一类,将F1杂种羊、英国品种（萨福克羊和多赛特羊）归为另一类。绵羊微卫星基因分型技术为检查品种（群体）之间的遗传关系提供了一个有用的工具。 Abstract：The genetic polymorphisms of four microsatellite loci BM143,OarHH35,OarAE101,and BMS2508 were analyzed in 286 sheep of seven sheep populations (Small Tail Han sheep, Hu sheep, Ujumqin sheep, Suffolk sheep, Dorset sheep, Charolais sheep, F1 of Dorset♂ × Small Tail Han sheep♀). The numbers of alleles for BM143,OarHH35,OarAE101,and BMS2508 are 9, 11, 14 and 9 in seven sheep populations, respectively. The polymorphism information content/number of effective alleles/ heterozygosity of BM143,OarHH35,OarAE101 and BMS2508 were 0.7073/3.7231/0.7314, 0.8267/6.4399/0.8447,0.5743/2.5178/0.6028,0.6172/3.0712/0.6744 in 286 sheep, respectively. The results revealed the greatest genetic variation at OarHH35 locus and the lowest at OarAE101, the greatest genetic variation in Small Tail Han sheep and the lowest in Hu sheep among seven sheep populations. In the unweighted pair group method with arithmetic mean (UPGMA) dendrograms based on Nei's DA distance and Nei's DS standard genetic distance, the Chinese native breeds (Small Tail Han sheep, Ujumqin sheep, Hu sheep) were grouped together, then with Charolais sheep. The F1 crossbred sheep, and the two British native sheep (Suffolk sheep, Dorset sheep) also clustered together. Microsatellite genotyping in sheep provided a useful tool for examining the genetic relationships among breeds(populations).     

Analysis of Genetic Diversity and Structure of Guanzhong Horse Using Microsatellite Markers

To determine the genetic diversity and validate the pedigree record of Chinese Guanzhong horse, 67 individuals were genotyped with eight microsatellite markers. In our study, the mean observed and expected heterozygosities were 0.51 and 0.66, respectively. The mean observed number of alleles for the Guanzhong horse was 3.88. Nonetheless, the total value of F_ST multiloci clearly indicates that about 0.5% of overall genetic variation is due to line founder differences, while differences among individuals are responsible for the remaining 99.5%. In addition, the polymorphic information content (PIC) result showed that five loci (HTG7, HMS7, HMS2, AHT4, and HMS6) were highly polymorphic (PIC?>?0.5) and three loci (HMS3, HTG6, and COR071) were moderate polymorphic (PIC?>?0.25). Genetic distances and cluster analysis showed that the genetic relationship among 67 Guanzhong horse was generally consistent with pedigree recorded. Our results not only evaluated the genetic diversity of Chinese Guanzhong horse, but also suggested that the eight microsatellite markers might be used as subservient markers for parentage verification and individual identification in the Guanzhong horse.     

Genetic Diversity and Conservation Implications of Four Cupressus Species in China as Revealed by Microsatellite Markers

Understanding the extent and distribution of genetic diversity is crucial for the conservation and management of endangered species. Cupressus chengiana, C. duclouxiana, C. gigantea, and C. funebris are four ecologically and economically important species in China. We investigated their genetic diversity, population structure, and extant effective population size (35 populations, 484 individuals) employing six pairs of nuclear microsatellite markers (selected from 53). Their genetic diversity is moderate among conifers, and genetic differentiation among populations is much lower in C. gigantea than in the other three species; the estimated effective population size was largest for C. chengiana, at 1.70, 2.91, and 3.91 times the estimates for C. duclouxiana, C. funebris, and C. gigantea, respectively. According to Bayesian clustering analysis, the most plausible population subdivision scheme within species is two groups in C. chengiana, three groups in C. duclouxiana, and a single group for both C. funebris and C. gigantea. We propose a conservation strategy for these cypress species.     

Study on Population Genetic Structure in Castanopsis fargesii with Microsatellite Markers

Genetic structure of four populations in Castanopsis fargesii Franch. in Fujian Province was studied with microsatellite (SSR) markers. A high level of genetic variation was detected in the populations of C. fargesii by using SSR with A=9.0, Ne=4.8, He=0.65 and the population differentiation coefficient ( Fst ) was only 0.031. The distributions of alleles of all loci were significantly different among the populations of C. fargesii , and the population differentiation could be found according to the distributions of SSR alleles. Some rare alleles in the populations of C. fargesii were revealed by SSR: Fifteen of 54 alleles appeared in one or two populations with lower frequencies; conservation of these rare alleles is of great importance.     

Microsatellite Markers Reveal Strong Genetic Structure in the Endemic Chilean Dolphin

Understanding genetic differentiation and speciation processes in marine species with high dispersal capabilities is challenging. The Chilean dolphin, Cephalorhynchus eutropia, is the only endemic cetacean of Chile and is found in two different coastal habitats: a northern habitat with exposed coastlines, bays and estuaries from Valparaíso (33°02′S) to Chiloé (42°00′S), and a southern habitat with highly fragmented inshore coastline, channels and fjords between Chiloé and Navarino Island (55°14′S). With the aim of evaluating the potential existence of conservation units for this species, we analyzed the genetic diversity and population structure of the Chilean dolphin along its entire range. We genotyped 21 dinucleotide microsatellites for 53 skin samples collected between 1998 and 2012 (swab: n = 8, biopsy: n = 38, entanglement n = 7). Bayesian clustering and spatial model analyses identified two genetically distinct populations corresponding to the northern and southern habitats. Genetic diversity levels were similar in the two populations (He: 0.42 v/s 0.45 for southern and northern populations, respectively), while effective size population was higher in the southern area (Ne: 101 v/s 39). Genetic differentiation between these two populations was high and significant (F_ST = 0.15 and R_ST = 0.19), indicating little or no current gene flow. Because of the absence of evident geographical barriers between the northern and southern populations, we propose that genetic differentiation may reflect ecological adaptation to the different habitat conditions and resource uses. Therefore, the two genetic populations of this endemic and Near Threatened species should be considered as different conservation units with independent management strategies.     

用SSR研究栲树群体遗传结构

利用微卫星（SSR）分子标记对福建省内4个栲树（Castanopsis fargesii Franch.）群体遗传结构进行了研究。SSR标记揭示了栲树群体丰富的遗传变异：平均等位基因数A＝9.0,平均有效等位基因数Ne=4.8,平均期望杂合度He=0.65,而群 具有较低的Fst值（Fst=0.031）。SSR每个位点的等位基因频率分布在栲树群体间都存在显或极显差异,表明根据SSR等位基因频率分布亦能了解各体的分化。SSR标记使栲树群体中一些稀有等位基因得以表现,54个SSR等位基因中有15个等位基因仅出现在1个或2个群体中,且频率较低,在遗传多样性保护中更应注重保护这些稀有的等位变异。