Localization of An Exogenous GH Gene on Chromosomes of Transgenic Pig by in situ Hybridizaiton

近些年来随着原位杂交技术的不断改进,该技术已广泛用于染色体的基因定位。非放射性标记探针的应用使基因定位变得更加简单易行,从而有可能对动物的转基因进行定位研究。本文首次采用胶体金标记药盒（Ａｎｔｉｄｉｇｏｘｉｇｅｎｉｎｇｏｌｄ）和银加强试剂（Ｓｉｌｖｅｒｅｎｈａｎｃｅｍｅｎｔｒｅａｇｅｎｔｓ）的非同位素原位杂交技术对转基因猪外源基因进行了定位研究。如Ｆｉｇ．１所示：表达质粒ｐＳＭＴＰＧＨ含有载体ｐＵＣ１９,羊启动子ＭＴ０１１和猪生长激素ＰＧＨ基因。选５头带有ｐＳＭＴＰＧＨ的转基因猪,分别制备含有染色体ＤＮＡ的杂交膜。用ＢｇｌＩＩ和ＳｍａＩ对ｐＳＭＴＰＧＨ进行完全酶切,收集０．９Ｋｂ片段作为探针,以ｄｉｇ１１ｄＵＴＰ进行标记。探针与ＤＮＡ杂交后,用Ａｎｔｉｄｉｇｏｘｉｇｅｎｉｎｇｏｌｄ和Ｓｉｌｖｅｒｅｎｈａｎｃｅｍｅｎｔｒｅａｇｅｎｔｓ进行显色反应。胰酶法Ｇ—显带后,用光学显微镜检查。选择分散相良好、显影银颗粒清楚的玻片进行摄影记录（Ｆｉｇ．２）。对染色体上的显影银颗粒进行统计分析,参照家猪的染色体标准带型,确定外源ＰＧＨ基因整合位点。Ｆｉｇ．３为４１０４号转基因猪染色体上的银颗粒分布情况。对５头     

人乳头状瘤病毒诱导人胚食管上皮永生化细胞恶性转化

为了证实ＨＰＶ１８Ｅ６Ｅ７基因诱导的人胚食管上皮永生化细胞（ＳＨＥＥ）６１代（ＳＨＥＥ６１）部份细胞（ＳＨＥＥ６１Ａ）已经恶性转化,以寻找监控细胞早期恶性转化的方法。对培养的ＳＨＥＥ第１０代（ＳＨＥＥ１０）和６１代（ＳＨＥＥ６１）细胞,用光学是为微镜和电子显微镜观察细胞形态及生长形式;用流工细胞仪分析细胞周期;用染色体Ｇ带核型分析和间期核染色体１、７、８号着丝粒探针荧光原位杂交９ＦＩＳＨ）检测细胞     

重组人MCAF／GM－CSF融合蛋白表达及其生物学活性研究

利用ＰＣＲ技术和ＤＮＡ体外重组方法,把作为导向效应细胞到靶部位的单核细胞趋化激活因子（ＭＣＡＦ）和粒细胞巨噬细胞集落刺激因子（ＧＭ－ＣＳＦ）进行基因融合,置于ｐＢＶ２２０载体的λＰＲＰＬ串联启动子下游,构建了ＳＤ序列与ＡＴＧ之间含有不同核苷酸组成的重组质粒ｐＭＧ０１、ｐＭＧ０２和ｐＭＧ０３。ｐＭＧ０１、ｐＭＧ０２和ｐＭＧ０３的翻译起始区都不存在稳定的二级结构,但ＤＨ５α（ｐＭＧ０２、ＤＨ５α（ｐＭＧ０３）的表达水平远远高于ＤＨ５α（ｐＭＧ０１）,ＤＨ５α（ＰＭＧ０１）几乎没有表达。表达产物经Ｗｅｓｔｅｒｎｂｌｏｔ检测表明,它能分别与ＭＣＡＦ和ＧＭ－ＣＳＦ抗体发生特异反应。生物学活性测定表明,表达产物具有明显的单核细胞趋化活性和维持ｈＧＭ－ＣＳＦ依赖的ＴＦ１细胞生长的特性,说明ＭＣＡＦ和ＧＭ－ＣＳＦ的生物学功能是相容的．     

水稻亚铁胁迫诱导ADH的基因定位及其遗传分析

籼稻品种ＩＲ６４与粳稻品种Ａｚｕｃｅｎａ及其ＤＨ群体１３５个系用于进行Ｆｅ＾２＋胁迫（２５０ｍｇ／Ｌ,ｐＨ４．５）及对照实验,对处理及对照条件下的ＡＤＨ进行基因定位及遗传分析,结果表明,在Ｆｅ＾２＋胁迫条件下,ＡＤＨ酶的活性大大提高,群体在Ｆｅ＾２＋胁迫条件下,表现低值的超亲现象,分布偏向ＩＲ６４,单标记分析和最大似然区间作图结果表明,Ｆｅ＾２＋胁迫条件下,１１号染色体上紧密连锁的３个标记位点ＲＧ     

闭锁繁育乌骨鸡群体的RAPD指纹分析

随机抽样测定了一个长期闭锁繁育和一个开放繁育雪峰乌骨鸡群体的早期生长和成活率,并藉ＲＡＰＤ分析比较了２个乌骨鸡群体的遗传学特征,结果表明：闭锁繁育群体ＲＡＰＤ标记的平均共带系数和平均带纹频率显著高于开放群体．标记效应估计结果表明随机引物Ｓ１０２扩增的ｂ４（１８２０ｂｐ）和ｂ５（１９３０ｂｐ）片段和Ｓ１０５扩增的ｂ９（１８４９ｂｐ）和ｂ１０（４１０４ｂｐ）片段作为遗传标记对于体重（尤其是３５日龄和７０日龄体重）具有很高的负向相关效应,因此,该４个ＲＡＰＤ标记可以作为近交衰退候选指示标记加以深入研究,最终结论有待于在大样本、多群体、多世代资料中验证．     

转OMT／PGH基因猪外源基因整合及遗传特性研究

实验以转ＯＭＴ／ＰＧＨ基因猪的Ｇ０,Ｇ１,Ｇ２和Ｇ３代共８头猪为材料,应用同位素和非同位素标记的染色体原位杂交技术,对外源ＯＭＴ／ＰＧＨ基因在猪染色体上整合位点进行研究,结果表明：（１）外源基因可以整合在染色体上,整合的位点是随机的。（２）整合在染色体上的外源基因可以遗传给子代;（３）整合在染色体上的外源基因在转基因动物世代过程中整合的位点是相对稳定的。     

肝刺激因子对人肝癌细胞BEL—7402p21^ras表达的影响

从雄性初断乳ＳＤ大鼠肝匀浆中提取肝刺激因子（ＨＳＳ）并加以部分纯化,观察其促人肝癌细胞增殖活性及对ｐ２１＾ｒａｓ蛋白表达的影响。结果表明：⑴ＨＳＳ具有明显的促人肝癌细胞增殖活性,其分子量为１４－２０ｋＤ;⑵ＨＳＳ可提高ｐ２１＾ｒａｓ蛋白表达,具有时间－效应关系,并与ＥＧＦ呈协同作用;⑶ＨＳＳ调节ｐ２１＾ｒａｓ蛋白表达具有剂量－效应关系,且呈现出饱和性。鉴于我们已报道ＨＳＳ上调ＥＧＦ受体蛋白和基因表     

哺乳动物性别分化的调控

哺乳动物性别分化调控的分子机制的研究特别是性别分化的层次调控、剂量补偿和性染色体进化这三个领域,已取得快速进展。已经发现Ｙ染色体性别决定区基因（ＳＲＹ）、Ｘ染色体ＤＳＳ－ＡＨＣ决定区基因１（ＤＡＸ－１）、甾类生成因子１基因（ＳＦ１）和Ｗｉｌｍｓ瘤抑制基因（ＷＴ－１）等与哺乳动物性别决定有关。ＳＲＹ启动睾丸分化,但胚胎发育成雄性的其余步骤由事丸分泌的激素控制。ＤＡＸ－１且编码一种女性特异功能的蛋白质,它在男性中被ＳＲＹ所抑制。ＳＦ－１和ＷＴ－１在ＳＲＹ开启之前作用于性腺和肾上腺发育的启动。哺乳动物通过随机失活雌性两条Ｘ染色体中的一条来使Ｘ连锁的基因在两性间的表达水平达到平衡（剂量补偿）。Ｘ染色体失活由Ｘ染色体失活中心（ＸＩＣ）控制。失活的Ｘ染色体专一转录基因（ＸＩＳＴ）是ＸＩＣ的强烈候选者,它可能参与Ｘ失活的启动。对有袋目和单孔目动物性染色体的研究为我们提供了其进化的信息。有证据支持性染色体起源于一对同源常染色体,而ＳＲＹ的祖先基因可能是ＳＯＸ－３。     

表皮生长因子对培养的气道上皮细胞抗臭氧损伤的保护作用

本研究观察到臭氧（Ｏ３）对体外培养经３Ｈ－ＵｄＲ标记的免气道上皮细胞有明显细胞毒性作用,且损伤程度与Ｏ３作用时间呈正相关。Ｏ３暴露组细胞内丙二醛（ＭＤＡ）产生增多（Ｐ＜０．０１）,提示Ｏ３损伤细胞的机制与胞膜脂质过氧化有关。表皮生长因子（ＥＧＦ）可明显降低Ｏ３所致的３Ｈ释放率（Ｐ＜０．０１）、降低Ｏ３的细胞毒指数及细胞内ＭＤＡ含量（Ｐ＜０．０１）,证明ＥＧＦ对气道上皮细胞有保护作用。进一步还观察到浓度为５ｎｇ／ｍｌ的ＥＯＦ可以取消Ｏ３所引起的细胞内还原型谷胱甘肽（ＧＳＨ）含量降低（Ｐ＜０．０１）,并增加细胞内谷胱甘肽总含量（Ｐ＜０．０５）,但不能改变Ｏ３所致的氧化型谷胱甘肽（ＧＳＳＧ）含量的增加（Ｐ＞０．０５）,对ＧＳＨ／ＧＳＳＧ比值也无明显提高,这些都提示ＥＧＦ的细胞保护机理可能与其促进细胞内谷胱甘肽合成有关,而对ＧＳＳＧ转化为ＧＳＨ的还原过程影响不明显。     

乙型肝炎、肝硬变和肝癌中HBxAg的表达及其在肝癌发生中的作用

对３７９例良、恶性肝组织进行的免疫组织化学研究显示,３３％的慢性迁延性肝炎（６／１８）、７６％的慢性活动性肝炎（２６／３４）、９２％的肝硬变（５７／６２）和９７％的肝细胞性肝癌（ＨＣＣ）（５８／６０）中有ＨＢｘＡｇ表达,阳性率高于ＨＢｓＡｇ或ＨＢｃＡｇ。癌周肝中的ＨＢｘＡｇ阳性率显著高于非癌周肝。与其它２种ＨＢＶ抗原不同,ＨＢｘＡｇ表达在细胞类型上有较明显的选择性,在肝小多角细胞（ＳＰＬＣ）、小细胞性不典型增生（ＳＣＤ）及ＨＣＣ中较强。与ＩＧＦⅡ、ｃ－ｅｒｂＢ－２、ｃ－ｍｙｃ和ＥＧＦ－Ｒ表达进行的对照研究表明ＨＢｘＡｇ与ＩＧＦⅡ和ｃ－ｅｒｂＢ－２这２种ＨＣＣ发生相关基因的表达关系密切。ＰＣＮＡ染色结果显示ＨＢｘＡｇ阳性组织的细胞增殖活性显著高于ＨＢｘＡｇ阴性组织。我们的结果还表明ＨＢｘＡｇ表达与肝细胞不典型增生的发生和进展有关、提出ＨＢＶＸ基因可能通过其表达产物（ＨＢｘＡｇ）首先激活ＩＧＦⅡ、ｃ－ｅｒｂＢ－２基因,继而引起显著的ＳＰＬＣ增生和ＳＣＤ而参与ＨＣＣ发生的．     

Optimal marker-assisted selection to increase the effective size of small populations

An approach to the optimal utilization of marker and pedigree information in minimizing the rates of inbreeding and genetic drift at the average locus of the genome (not just the marked loci) in a small diploid population is proposed, and its efficiency is investigated by stochastic simulations. The approach is based on estimating the expected pedigree of each chromosome by using marker and individual pedigree information and minimizing the average coancestry of selected chromosomes by quadratic integer programming. It is shown that the approach is much more effective and much less computer demanding in implementation than previous ones. For pigs with 10 offspring per mother genotyped for two markers (each with four alleles at equal initial frequency) per chromosome of 100 cM, the approach can increase the average effective size for the whole genome by approximately 40 and 55% if mating ratios (the number of females mated with a male) are 3 and 12, respectively, compared with the corresponding values obtained by optimizing between-family selection using pedigree information only. The efficiency of the marker-assisted selection method increases with increasing amount of marker information (number of markers per chromosome, heterozygosity per marker) and family size, but decreases with increasing genome size. For less prolific species, the approach is still effective if the mating ratio is large so that a high marker-assisted selection pressure on the rarer sex can be maintained.     

HOMOEOLOGOUS CHROMOSOME PAIRING AND RESTRICTED SEGREGATION IN THE FERN CERATOPTERIS

The segregation of a marker characterized by pale green gametophytes was monitored within an inbreeding study of the polyploid fern Ceratopteris. Although all of the sporophytes showing segregation were derived from the self-fertilization of haploid gametophytes, a low overall frequency of 2.5% pale gametophytes was observed in the F₃–F₅ generations. A model based upon a duplicated locus and homoeologous chromosome pairing can explain the segregational behavior within the study. The overall level of homoeologous pairing was determined to be 10%. Occasionally, green gametophytes that were presumably heterozygous for the marker contained pale sectors. This behavior may involve mitotic crossing-over between homoeologous chromosomes.     

Mapping markers linked to porcine salmonellosis susceptibility

The goal of this study was to identify pig chromosomal regions associated with susceptibility to salmonellosis. Genomic DNA from pig reference populations with differences in susceptibility to Salmonella enterica serovar Choleraesuis as quantified by spleen and liver bacterial colonization at day 7 post-infection (dpi; Van Diemen et al. 2002 ) was used. These samples belonged to the offspring of a sire thought to be heterozygous for genes involved in susceptibility to salmonellosis. Amplified fragment length polymorphism (AFLP) markers were created and used to determine associations with spleen or bacterial counts at 7 dpi. To position linked markers, two mapping populations, the Roslin and Uppsala PiGMaP pedigrees were used to create an integrated map which included the AFLP markers associated with salmonellosis. Twenty-six AFLP markers located in 14 different chromosomal regions in the porcine genome were found to be significantly associated with susceptibility (Chi-square P  < 0.05). More than one linked marker was found on chromosomes 1, 7, 13, 14 and 18. It is likely that these regions contain genes involved in Salmonella susceptibility. Regions on chromosomes 1, 7 and 14 were significantly associated with Salmonella counts in the liver and regions on chromosomes 11, 13 and 18 with counts in spleen. The identification of these chromosomal regions highlights specific areas to search for candidate genes that may be involved in innate or adaptive immunity. Further investigation into these chromosomal regions would be useful to improve our understanding of host responses to infection with this widespread pathogen.     

The genetic conditions in heterozygous and homozygous populations ofDrosophila I. The fate of alien chromosomes

In experimental populations ofDrosophila melanogaster lethal chromosomes with dominant markers and inversions were introduced and the frequency changes of the markers studied during a period of several generations. The base populations of the various experiments differed from each other with respect to their degree of heterozygosity. Monochromosomal populations were isogenic for a quasinormal + chromosome, dichromosomal populations contained the genetic material of two different + chromosomes, trichromosomal of three, tetrachromosomal of four, hexachromosomal of six and polychromosomal populations of many normal chromosomes. Marker chromosomes with the dominant genesLCy, Cy, Pm orD respectively were added to the populations with an initial frequency of 16,6 per cent. The fate of the dominant markers was different in different populations. In some the marker chromosome reached equilibrium frequencies, in others they were eliminated with variable speed. As a rule the lethal marker chromosomes were accepted by monochromosomal populations; however, they were eliminated from populations with a higher degree of heterozygosity. Since in all populations one genotype, namely the homozygote for the marker chromosome, was lethal, the adaptive values c of the +/LCy, +/Cy, +/Pm or +/D heterozygotes could easily be calculated from the experimental data. This c value can be used as a measure for the combining ability of the marker chromosomes. It could be shown that c depends on the degree of heterozygosity of a population or in other words that the average degree of heterozygosity of the marker free individuals determines the selection processes. An equation can be arrived at which fits the experimental results very well if superiority of heterozygous +/+ individuals over +/+ homozygotes is assumed. From that it was concluded that heterosis is the determining variable in our experiments. An attempt was undertaken in order to decide if in our case the observed heterosis was due to dominance or to overdominance. It was postulated that in di-, tri-, tetra- or hexachromosomal populations the adaptive values of the marker free normals should progressively increase if recessive detrimental genes are the cause of heterosis but not if heterozygosity on many loci leads to overdominance. The a values of the +/+ individuals were ealeulated from the frequency changes of the marker chromosomes for each subsequent two-generation period. Unfortunately only two different dichromosomal populations were available. These showed increasing adaptive values for the normals. The tri-, tetra-, and hexachromosomal populations, however, gave different results, some with increasing, some with fluctuating adaptive values. From that it was concluded that heterosis can be due in one case to dominance and in the other to overdominance. In either case, the recessive genetic load may be rather important as a determinating factor in the dynamics of populations.Dedicated to Prof. Th. Dobzhansky on the occasion of his seventieth birthday in deepest gratitude.     

FEMALE FECUNDITY IN A HYBRID ZONE BETWEEN TWO CHROMOSOME RACES OF THE SCELOPORUS GRAMMICUS COMPLEX (SAURIA,PHRYNOSOMATIDAE)

Individuals of the F5 and FM2 cytotypes of the Sceloporus grammicus complex form a narrow zone of parapatric hybridization near Tulancingo, Hidalgo, Mexico. Reproductive parameters were examined among chromosomally parental and hybrid females to assess the degree to which reduced clutch size is correlated with the level of chromosomal heterozygosity. Although clutch size in the two parental groups was highly correlated with female body size, this was not the case for females with intermediate karyotypes. These females displayed increased levels of infertility manifested as smaller clutches and as inviable embryos. F₁ females produced the smallest average clutches and suffered the most precipitous fecundity loss (up to 75%). The number of heterozygous marker chromosomes and heterozygosity at chromosome 2 had significant effects on the number of viable embryos. Analysis of embryo karyotypes revealed the production of triploid offspring and an excess number of embryos heterozygous at chromosome 1. Differences in viability, among females heterozygous for the same number of chromosomes, suggest that genetic background of the female and/or sire may be an important factor in determining reproductive success.     

Chromosomal origin of small ring marker chromosomes in man: characterization by molecular genetics.

Ten cases of small ring chromosomes which did not stain with distamycinA/DAPI and did not possess satellite regions associated with nucleolus-organizing regions are described. In situ hybridization with a battery of biotinylated pericentric repeat probes specific either for individual chromosomes or for groups of chromosomes allowed the identification of the chromosomal origin of these marker chromosomes. There was one example of a marker derived from each of chromosomes 1, 3, 6, 14, 16, 18, 20, 13 or 21, and the X, and there were two examples of markers derived from chromosome 12. One case possessed two markers, one derived from chromosome 6, and one derived from the X. The mechanism of generation of ring marker chromosomes is discussed. Five of seven cases who could be phenotypically assessed were abnormal. Three of these--the first with a ring chromosome derived from chromosome 1; the second with two markers, one derived from chromosome 6 and the other from the X chromosome; and the third with a ring chromosome derived from chromosome 20--each possessed distinctive facies. Additional cases with identified rings may allow the delineation of new chromosomal syndromes.     

Allozyme variation in populations, full-sib families and selfed lines in Betula pendula Roth

Changes in genetic variability in populations (stand origins), full-sib (FS) families and three generations of selfed lines of Betula pendula were observed based on 15 allozyme loci. Growth vigour, measured as stem volume, and its relationship with heterozygosity was studied to determine the effect of inbreeding. Pooled FS families showed a higher percentage of polymorphic loci (P) and allelic numbers per locus (A) than those of natural populations, but no difference in heterozygosity. There was no difference in allozyme variability between fast-and slow-growing family groups, and heterozygosity was not correlated with stem volume among FS families. Allozyme variability was significantly decreased in advancing generations of selfing, and the further the selfing generation, the lower the heterozygosity and the slower the growth. Observed heterozygosity after advancing generations of inbreeding was increasingly higher than expected, indicating overdominance effects or, alternatively, selection against deleterious homozygotes.     

豫医无毛小鼠分离近交系的建立及其遗传纯度测定

采用强迫杂合性史妹酱方式培育携带无毛突变基因的分离近交系,然后用生化标记法,皮肤移植实验和毛色基因测试法对其进行遗传监测。并对其基本生物学特性进行了研究。结果育成了具有独特生物学特性的豫医无毛小鼠分离近交系,现已达30代,生化标记法测定的9条染色体上13个生化标记位点全部纯合;同系异体间皮肤移植100天后,未见排斥现象,为同系组织遗传性;与DBA/2交配进行的毛色基因测试,杂交的F1代相同,全部为野生色,基因型为AABBccDD ,表明豫医无毛小鼠已成为一个达到国际标准的新品系。     

SELECTION ON OVERDOMINANT GENES MAINTAINS HETEROZYGOSITY ALONG MULTIPLE CHROMOSOMES IN A CLONAL LINEAGE OF HONEY BEE

Correlations between fitness and genome‐wide heterozygosity (heterozygosity‐fitness correlations, HFCs) have been reported across a wide range of taxa. The genetic basis of these correlations is controversial: do they arise from genome‐wide inbreeding (“general effects”) or the “local effects” of overdominant loci acting in linkage disequilibrium with neutral loci? In an asexual thelytokous lineage of the Cape honey bee (Apis mellifera capensis), the effects of inbreeding have been homogenized across the population, making this an ideal system in which to detect overdominant loci, and to make inferences about the importance of overdominance on HFCs in general. Here we investigate the pattern of zygosity along two chromosomes in 42 workers from the clonal Cape honey bee population. On chromosome III (which contains the sex‐locus, a gene that is homozygous‐lethal) and chromosome IV we show that the pattern of zygosity is characterized by loss of heterozygosity in short regions followed by the telomeric restoration of heterozygosity. We infer that at least four selectively overdominant genes maintain heterozygosity on chromosome III and three on chromosome IV via local effects acting on neutral markers in linkage disequilibrium. We conclude that heterozygote advantage and local effects may be more common and evolutionarily significant than is generally appreciated.     

Microsatellite Analysis of Homozygosity Progression of Heterozygous Genotypes Segregating in the Rice Subspecies Cross Pei��ai64s/Nipponbare

Progression to homozygosity of heterozygous genotypes was studied in a cross of the rice subspecies Pei'ai64s and Nipponbare, using a set of 157 polymorphic microsatellite (SSR) markers. The segregation of heterozygous genotypes ranged from 49.13% in the F(2) population to 4.52% in the F(6) population (progression value 11.15%). The heterozygous genotypes were widely distributed in 180 F(2) plants, 330 F(6) lines, and 157 SSR markers. Homozygosity progression showed a wide distribution in plants and SSR markers but not in chromosomes. The segregation of heterozygous genotypes was not significant between populations but varied greatly in F(2) plants, F(6) lines, and SSR markers. The correlation between the progression to homozygosity and the heterozygosity of SSR markers was significant at the chromosome level. The segregation of heterozygous genotypes in plants, SSR markers, and chromosomes was not completely in accordance with Mendel's law. This information will help rice geneticists and breeders to understand heterozygous genotype segregation at the DNA level and to screen special markers for breeding.