EST-SSR标记对我国斑点叉尾鮰种质资源的研究

采用EST-SSRs对福建和湖北的1984年群体（P1984）、福建与辽宁的1997年群体（P1997）、湖南的2004年群体（P2004）和福建的1984年与1997年群体杂交的F。代群体（P8497）等4个斑点叉尾鮰（Ictalurus punctatus）养殖群体的遗传多样性进行了研究。结果表明,有10对引物可扩增出清晰条带,其中9对引物具有多态性,共获得32个等位基因,4个群体的平均等位基因数（A）为3．00-3．40,平均有效等位基因数（Ac）为1．95～2．30,平均观察杂合度（Ho）为O．4768-0．5982,平均期望杂合度（Ho）为004913-0．5695,平均多态信息含量（PIC）为0．4113-0．4829,群体间的多态性差异不显著,且各群体的遗传多样性处于中等水平。根据群体间遗传相似性系数、遗传距离及UPGMA聚类分析发现,P1997和P2004群体之间的遗传距离最近,P1984和P2004群体之间的遗传距离最远。4个群体有18．75％的位点偏离了Hardy-Weinberg平衡,表明群体各位点的基因频率和基因型频率稳定性较好。F-统计检验发现,P2004和P8497处于不同程度的杂合子过剩状态,P1984和P1997处于杂合子缺失状态。群体间分化程度很弱,遗传变异主要来自群体内个体之间。     

EST-SSR标记对我国斑点叉尾(鲴)种质资源的研究

采用EST-SSRs对福建和湖北的1984年群体(P1984)、福建与辽宁的1997年群体(P1997)、湖南的2004年群体(P2004)和福建的1984年与1997年群体杂交的F.代群体(P8497)等4个斑点叉尾鲴(Ictalurus punctatus)养殖群体的遗传多样性进行了研究.结果表明,有10对引物可扩增出清晰条带,其中9对引物具有多态性,共获得32个等位基因,4个群体的平均等位基因数(A)为3.00～3.40,平均有效等位基因数(Ae)为1.95～2.30,平均观察杂合度(Ho)为0.4768～0.5982,平均期望杂合度(He)为0.4913～0.5695,平均多态信息含量(PIC)为0.4113～0.4829,群体间的多态性差异不显著,且各群体的遗传多样性处于中等水平.根据群体间遗传相似性系数、遗传距离及UPGMA聚类分析发现,P1997和P2004群体之间的遗传距离最近,P1984和P2004群体之间的遗传距离最远.4个群体有18.75%的位点偏离了Hardy-Weinberg平衡,表明群体各位点的基因频率和基因型频率稳定性较好.F-统计检验发现,P2004和P8497处于不同程度的杂合子过剩状态,P1984和P1997处于杂合子缺失状态.群体间分化程度很弱,遗传变异主要来自群体内个体之间.     

吉富罗非鱼雌雄群体遗传差异的SSR分析

为探讨吉富罗非鱼（genetic improvement of farmed tilapia,GIFT）雌、雄群体间的遗传差异,本研究对国家级广西南宁罗非鱼良种场雌、雄吉富罗非鱼进行了遗传差异分析。研究结果表明,选取的11对SSR引物中有10对能获得稳定的目的条带;每个SSR基因座的等位基因数在2～4个之间,雌性罗非鱼的平均等位基因（Na）2.9个,稍高于雄性的2.8个;雌、雄吉富罗非鱼平均观察杂合度（HO）分别为0.4183和0.4154,多态信息含量（PIC）分别为0.4048和0.3932,属中度多态;雌雄个体间的遗传距离和相似性指数分别为0.0908和0.9132。此外,SSR基因座PRL-SO2在雄鱼中偏离Hardy Weinberg平衡（P〈0.005）。上述结果表明,吉富罗非鱼雌、雄群体的SSR多态性基本相同,推测这两者基因组间的差异较小。     

斑点叉尾鮰趋化因子基因SCYA113内含子1的多态性分析

运用变性聚丙烯酰胺凝胶电泳和PCR产物测序技术检测斑点叉尾鮰CC趋化因子基因SCYA113 内含子1的序列长度和多态性。在3个群体的60个个体中,斑点叉尾鮰CC趋化SCYA113 内含子1存在15种单元型和8种长度类型,长度类型分别为A、B、C、D、E、F、G和H型。对这8种序列进行比对分析发现,斑点叉尾鮰SCYA113 内含子1长度为395~443 bp, 8种长度类型中A、G、T、C的平均百分比为30.01%、15.43%、38.37%、16.19%,而且G+C（31.62%）含量明显小于A+T（68.38%）含量,内含子1与外显子1和2的连接处存在真核基因中mRNA剪接的识别信号GT/AG;引起长度变化的主要原因是短串联重复序列（微卫星序列）TTC和TTA引起的;除了微卫星序列以外,共检测到6个突变位点,其中3个转换位点为118（C→T）,209（G→A）,250（T→C）,3个颠换位点为266（T→A）,289（G→T）,387（G→C）,核苷酸多样性指数(π)为0.004,平均核苷酸差异(K)为1.576;在变异水平上,3个群体表现出一定的遗传差异,84群体中检测到8种长度类型和14种基因型,97群体中检测到8种长度类型和10种基因型,04群体中6种长度类型和10种基因型（缺少A、B等位基因）。从3个群体60个个体拥有22种频率较低(0.017~0.150)的基因型可以看出,斑点叉尾鮰的遗传基因资源较为丰富。     

AFLP分析江西省4个斑点叉尾鮰养殖群体遗传多样性

本文运用AFLP分子标记技术,对江西省4个斑点叉尾鮰(Ictalurus punctatus)养殖群体(GZ、XJ、PYA和PYB)进行遗传多样性分析。结果表明,在64对引物组合中,E3/M2、E4/M7、E3/M8和E5/M5引物从4个群体72个体中共扩增出179个位点,其中多态位点为109,占60.89%。其中,PYA、GZ、XJ和PYB群体的多态位点比例(P)分别为56.54%、56.47%、56.32%和56.14%。Shannon多样性指数(I)分别为0.2890、0.3003、0.2896和0.2852,平均杂合度(H)分别为0.1935、0.2027、0.1938和0.1898。4个群体间的遗传分化系数(Gst)为0.1314,说明群体间发生了一定程度的遗传分化,但分子方差分析(AMOVA)显示,群体的遗传变异90.98%来源于群体内的个体间,9.02%来源于群体间。聚类分析也表明,4个群体所产生的遗传分化主要也来源于群体内。本研究为斑点叉尾鮰种质资源的调查和保护提供参考,为斑点叉尾鮰优良品种的选育提供科学依据。     

鳜原种群体和养殖群体遗传多样性的微卫星分析

本研究利用20对微卫星引物对鳜（Sinipelrca chuatsi）原种群体和养殖群体进行遗传多样性分析。结果表明,在鳜原种群体中检测到多态性位点14个,养殖群体11个。在两个群体中共检测到等位基因数96个,其中原种群体检测到等位基因数53个,每个位点的等位基因数在1～7之间,平均有效等位基因数为2．7390;养殖群体检测到等位基因数43个,每个位点的等位基因数在1-6之间,平均有效等位基因数为2．1284。原种群体的平均观察杂合度0．5708,Nei氏期望杂合度0．5295,平均多态信息含量PIC0．5353;养殖群体的平均观察杂合度0．3839,Nei氏期望杂合度0．4011,平均多态信息含量PIC0．5043。因此,与养殖群体相比,鳜原种群体仍有丰富的遗传多样性。本研究可为鳜种质资源的保护、监测和遗传育种提供分子水平上的数据。     

微卫星标记分析广西水牛遗传多样性

为研究广西沼泽型水牛(Bubalus bubalis)核基因组的多态性,采用23对荧光标记微卫星引物,对随机抽取的60个广西本地水牛样本进行了PCR检测。结果表明,23对引物中,有19对可以获得特异性产物且存在多态,平均有效等位基因数为4.0189,基因座ILSTS086含有13个等位基因;各微卫星基因座的平均杂合度变化范围为0.1852~0.4722,ILSTS019基因座平均杂合度最高(0.4722),而ILSTS017平均杂合度最低(0.1852);群体基因平均多态信息含量(PIC)为0.6639,19个标记中有18个PIC大于0.5,属高度多态位点。     

江西青岚湖五种淡水蚌遗传多样性的微卫星DNA分析

利用北美Epioblasma capsaeformis（蚌科）和中欧Margaritifera margaritifera L.（珍珠蚌科）两种淡水双壳类的20对微卫星引物对江西青岚湖五种淡水蚌群体进行了PCR扩增，筛选出8对多态性较高的引物，并用这8个微卫星座位分别对三角帆蚌、褶纹冠蚌、洞穴丽蚌、射线裂脊蚌和中国尖嵴蚌五种蚌类群体进行了遗传多样性分析。结果表明：不同蚌类群体的平均等位基因数为2.8750～4.000，平均观测杂合度（HO）为0.4417～0.6333，平均期望杂合度（HE）为0.4430～0.5706，平均多态信息含量（PIC）为0.368～0.498，五个群体表现出较高的遗传多样性。有多个座位在不同蚌类群体中偏离哈代－温伯格平衡。五种蚌类群体间的遗传距离在0.6228与1.4724之间，三角帆蚌和褶纹冠蚌之间的遗传距离最大，射线裂脊蚌和洞穴丽蚌之间的遗传距离最小。     

浅析二氢吡啶对斑点叉尾鮰生长性能的影响

采用单因子试验设计,在蛋白质含量为31.99%和11.27 MJ/kg的基础饲料中分别添加0、50、100、150、200 mg/kg和250 mg/kg二氢吡啶制成6种试验饲料。试验选用平均初始体重为(5.53±0.11)g的斑点叉尾鮰360尾,随机分为6组,每组设置2个平行实验,每个平行30尾试验鱼。结果表明:饲料中二氢吡啶量为192.33 mg/kg时,斑点叉尾鮰的特定生长率最高,为2.65%/d;二氢吡啶含量为133.33 mg/kg时,斑点叉尾鮰的饵料系数最低,为1.61;二氢吡啶含量为137.93 mg/kg时,斑点叉尾鮰的饲料蛋白质效率最优(饲料蛋白质效率为1.94%)。     

利用微卫星标记分析马氏珠母贝4个养殖群体遗传结构

2007年4月,从马氏珠母贝基础群体选取2、4、32和158个亲本分别繁殖4个子代群体,分别命名为P1、P2、P3和P4。2009年7月,从这4个子代群体随机取样30个个体,利用7对微卫星引物分析其遗传结构。结果表明,7对微卫星引物共检测到22个等位基因,每个座位的等位基因数目为2~4个,平均等位基因数为3个,平均有效等位基因数为2.3193。P1、P2、P3和P4群体平均观测杂合度分别为0.4737、0.5489、0.6767和0.7143;P1、P2、P3和P4群体平均期望杂合度分别为0.4737、0.5489、0.6767和0.7143;P1、P2、P3和P4群体的多态信息含量分别为0.4472、0.4224、0.4726和0.4930。本结果表明4个养殖群体均具有较高的遗传多样性,而且有效亲本数目对子代遗传结构有较大的影响,这为马氏珠母贝的遗传育种提供依据。     

江西野生毛花猕猴桃群体SSR遗传多样性研究

为分析江西野生毛花猕猴桃群体遗传多样性,以江西省境内的5个野生毛花猕猴桃雄性群体(72个个体)为试验材料,采用SSR分子标记技术,选取15对多态性引物,利用聚丙烯酰胺电泳对PCR产物进行检测。结果表明,15对SSR引物共检测到86个位点,多态性位点百分率为100.0%;观察到的平均等位基因数为5.733,有效等位基因数为3.002,Shannon信息指数为1.046。表观杂合度介于0.111~0.819之间,预期杂合度介于0.041~0.876之间,遗传分化系数为2.01,野生毛花猕猴桃雄性群体间存在较大的遗传分化。5个毛花猕猴桃雄性群体遗传距离范围为0.102~0.409,遗传相似度范围为0.665~0.903,群体间遗传距离与地理距离无相关性。群体的遗传多样性丰富度依次为庐山>井冈山>南源山>武功山>麻姑山,江西地区供试的野生毛花猕猴桃雄性群体在分子水平上具有丰富的多态性。本研究结果为毛花猕猴桃雄性品种选育、种质创新与利用提供了一定的理论基础。     

Genetic Diversity in Tunisian Ceratonia siliqua L. (Caesalpinioideae) Natural Populations

The last two centuries witnessed the human-caused fragmentation of Tunisian Ceratonia siliqua L. (Caesalpinoideae) populations which were often represented by scattered individuals. Seventeen populations growing in four bioclimatic zones: sub-humid, upper semi-arid, mean semi-arid and lower semi-arid zones, were sampled for allozyme diversity to assess their genetic diversity and structuration using eight isozymes revealed by starch gel electrophoresis. The species showed high diversity within populations. The average number of alleles per polymorphic locus was 1.98, the percentage of polymorphic loci was 83.4% and the mean observed heterozygosity (Ho) and expected heterozygosity (He) under Hardy–Weinberg equilibrium were respectively 0.247 and 0.316. A substantial level of inbreeding within populations induced by Wahlund effect, was observed (F_IS = 0.231). High diversity resulted from the great number of genotypes in the ancestral population before fragmentation, favoured by the outbreeding of the species. High differentiation and low gene flow were detected among populations (F_ST = 0.200) and among pairs of ecological zones (0.113< F_ST <0.198). However, the differentiation coefficient of the four zones was low (F_ST = 0.085) and similar to the average F_ST for forest trees. Population structuration depends on geographic distance between sites rather than bioclimate, indicating that structuration has occurred slowly and that climatic conditions have had little effect. Nei's genetic distances (D) between populations were low and ranged from 0.004 to 0.201. Mean D value for all population was 0.087. The UPGMA clustering established for all populations through Nei's genetic distances did not clearly show that, for the majority of populations, grouping had resulted from ecological factors or geographic location. The substantial differentiation and the high genetic similarities between populations indicate that populations have been recently isolated as a result of anthropic pressure. In-situ conservation strategies must first focus on populations with a high level of genetic diversity and rare alleles. Appropriate conservation action should take account of bioclimatic zones. Ex-situ preservation should be based on a maximum number of individuals collected within populations in each ecological group and their propagation in different bioclimates by means of cuttings.     

桂林地区蜈蚣蕨群体遗传多样性及与南宁地区群体的对比分析

采用等位酶电泳技术,研究了桂林地区的桂林市、雁山镇、永福县的野生蜈蚣蕨群体的遗传多样性,并与南宁地区群体进行比较。所测定的酶系统包括：氨基肽酶（AMP）、还原型辅酶Ⅰ心肌黄酶（DIA）、异柠檬酸脱氧酶（IDH）、苹果酸脱氨酶（MDH）、6-磷酸葡萄糖酸脱氢酶（PGD）、磷酸葡萄糖异构酶（PGI）、磷酸葡萄糖变位酶（PGM）和莽草酸脱氧酶（SKD共8个酶系统,15个酶位点。分析结果表明：桂林地区蜈蚣蕨群体内遗传多样性水平中等偏上,每个位点的等位基因平均为1．7,多态位点百分数为60％,平均期望杂合度为0．251,略高于南宁地区。     

白孔雀微卫星DNA遗传多样性及其分类地位

利用14对蓝孔雀(Pavo cristatus)和绿孔雀(P.muticus)的微卫星标记对白孔雀基因组DNA进行扩增,发现都能扩增出特异性条带,每对引物扩增的平均等位基因数为1.71,有7对引物具有较丰富的多态性,其中MCW0080和MCW0098标记期望杂合度分别为0.7207和0.7571,多态信息含量分别为0.658和0.695,表现出丰富的遗传多样性和较高的选择潜力。白孔雀×蓝孔雀和绿孔雀群体的遗传多样性分析结果表明,白孔雀、绿孔雀和蓝孔雀3个群体的杂合度和遗传多样性水平都很低,期望杂合度分别为0.2579、0.2482和0.2744,群体间的遗传分化系数为9.7%,群体间分化极显著(P<0.001),白孔雀与蓝孔雀的亲缘关系最近,Reynolds'遗传距离和基因流分别为0.0295和8.6112,表明白孔雀不是蓝孔雀一个亚种。     

Investigation of recent population bottlenecks in Kenyan wild sorghum populations (<Emphasis Type="Italic">Sorghum bicolor</Emphasis> (L.) Moench ssp. <Emphasis Type="Italic">verticilliflorum</Emphasis> (Steud.) De Wet) based on microsatellite diversity and genetic disequilibria

Identifying populations that have recently suffered a severe reduction in size is particularly important for their conservation as they are likely to suffer an increased risk of genetic erosion. We investigated the presence of recent bottlenecks in two wild sorghum populations from different eco-geographical conditions in Kenya employing 18 microsatellite markers. Microsatellite analysis showed high allelic diversity in the two populations, with a mean of 4.11 and 6.94 alleles per locus in the North-West wild sorghum population (NWWSP) and the South-East wild sorghum population (SEWSP), respectively. The mean observed heterozygosity was 0.34 and 0.56 in NWWSP and SEWSP, respectively. A large long-term effective populations size for both populations was observed assuming either an infinite allele model or a stepwise mutation model. There was no apparent loss of genetic variability for either of the populations. Test of heterozygosity excess indicated that a recent bottleneck in the two populations is highly unlikely. Furthermore, analysis of the allele frequency distribution revealed an L-shaped distribution which would not have been observed in case a recent bottleneck had reduced genetic variability in the two populations. The fact that most loci displayed a significant heterozygosity deficiency could be explained by population subdivision and the mixed mating system exhibited by wild sorghum populations. Furthermore, the possibility of a historical expansion of wild sorghum populations and presence of null alleles could not be ruled out.     

Population structure and phylogenetic relationship of Peach [Prunus persica (L.) Batsch] and Nectarine [Prunus persica var. nucipersica (L.) C.K. Schneid.] based on retrotransposon markers

For effective varietal improvement of horticultural crops peach (Prunus persica) and nectarine (Prunus persica var. nucipersica), information about their population structure and genetic relatedness plays an important role. In this study we used retrotransposon-based markers (iPBS) to estimate the genetic diversity and population structure of 48 peach and nectarine genotypes from various distinct geographical regions of Punjab and Khyber Pakhtunkhwa, Pakistan. A total of 461 alleles were identified from PCR amplicons derived from nine iPBS primer pairs with an average of 8.5 alleles/locus. Among all four groups the genotypes collected from Swat and Hunza had the highest and the lowest expected heterozygosity, unbiased expected heterozygosity and Shannon’s information index, respectively. We constructed a Neighbour-Joining dendrogram and performed principal coordinate analysis based on the distance matrices, and both forms of analysis grouped the 48 genotypes into two distinct clusters. The STRUCTURE software distributed the forty-eight genotypes into two main populations (k?=?2) indicating a low diversity between genotypes collected from Chakwal, Swat, Mansehra and Hunza.

     

Genetic diversity and population structure of Guinea yams and their wild relatives in South and South West Ethiopia as revealed by microsatellite markers

Genetic diversity and population structure of Guinea yams and their wild relatives collected from south and south west Ethiopia were assessed using microsatellite markers. The total number of alleles amplified for the 7 loci studied was found to be 60, with an average of 8.6 alleles per locus. The average expected heterozygosity for the entire population was found to be 64 % indicating that Guinea yams and their wild relatives in the study area display a high level of genetic diversity. Using allelic richness as a measure of genetic diversity the wild forms exhibited greater allelic diversity than the cultigens. Contrary to what is expected in vegetatively propagated crops, none of the seven loci studied showed a significant excess of heterozygotes. In all the comparisons made, a low mean F_ST (but significant) has been observed, indicating that the majority of microsatellite diversity in the populations under study was found within rather than between populations.