四川省凉山州北部栽培苦荞麦的遗传多样性研究

用等位酶电泳技术测定了四川省凉山彝族自治州北部越西和甘洛２县的苦荞麦「Ｆａｇｏｐｙｒｕｍ ｔａｔａｑｒｉｃｕｍ（Ｌ．）Ｇａｅｒｔｎ．」１７个栽培居群的遗传多样性和分化,结合农业生物学性状进行了分析。对７个酶系统的１５个位点的检测表明,苦荞麦居群内的遗传多样性水平高于该州南部的苦荞麦和其他地区甜荞麦,每个位点的等位基因平均数为１．９,多态位点比率为５２．１％,平均实际杂合度和预期杂合度分别为０．１９     

天然红松林等位酶研究

利用红松种子的单倍体胚乳,采用水平切片淀粉凝胶电泳技术,对采自三个地区的天然红松林的材料进行了１０种酶系统的等位酶实验,共获得了１８个等位基因位点,对这１８个位点等位基因的统计分析表明：红松种群的多态位点百分数为Ｐ＝７７．７８％,等位基因平均数为Ａ＝２．０,预期杂合度为Ｈｅ＝０．１６４８。红松种群间遗传分化程度在松属于较低水平。在红松１８个等位基因位点的变异中,绝大部分变异９４．２％来自种群内部,     

柚品种的等位酶变异研究

研究了柚的48个品种的等位酶变异,利用等位酶分析技术对柚的酯酶（EST）,6－磷酸葡萄糖异的酶（PGI）,6－磷酸葡萄糖变位酶（PGM）,莽草酸脱氢酶（SKD）,超氧化物歧化酶（SOD）共5个酶系统的10个等位酶基因座进行了分析,除PGI－1,PGI－2两个基因座外,其它8个均为多态性基因座;10个等位酶基因座共观察到的等位基因25个,平均每个基因座的有效等位基因数目为1．55,基因多样度0．2805,柚的品种间具有较为丰富的等位酶标记遗传多样性,但柚类种质资源群体总的遗传多样性水平偏低。柚的较低的有效等位基因数目与基因多样度可能由于人工选择及资源流失造成。     

松毛虫属（Dendrolimus) 部分种类亲缘关系与遗传分化的等位酶分析

采用等位酶聚丙烯酰胺凝胶电泳技术对松毛虫属5个种和亚种的野生种群进行了亲缘关系和遗传变异的研究.8种等位酶系统(乳酸脱氢酶LDH、苹果酸脱氢酶MDH、苹果酸酶ME、乙醇脱氢酶ADH、甲酸脱氢酶FDH、谷氨酸脱氢酶GDH、过氧化物酶POD、过氧化氢酶CAT)共检测到12个基因位点,其中6个位点为多态位点,检测到15个等位基因.松毛虫属5个种和亚种的总体水平多态位点比率P＝50%,平均有效基因数A = 1.917,平均期望杂合度He =0.267,平均遗传距离为0.0730～0.5701.遗传参数表明松毛虫属昆虫种间存在较高程度的遗传变异,聚类图和遗传距离数据表明赤松毛虫与马尾松毛虫亲缘关系最近,落叶松毛虫与思茅松毛虫亲缘关系最远.     

毛乌素沙地根茎灌木羊柴的遗传多样性和克隆结构

采用淀粉凝胶电泳技术对毛乌素沙地根茎灌木羊柴（ＨｅｄｙｓａｒｕｍｌａｅｖｅＭａｘｉｍ．）８个群体的遗传多样性和克隆结构进行了初步研究。利用１０个酶系统１５个等位酶位点的检测表明,羊柴群体具有较高的遗传变异水平,多态位点百分率Ｐ＝３７．０,等位基因平均数Ａ＝１．４８,平均期望杂合度Ｈｅ＝０．１０１;但８个群体间的分化很小（Ｆｓｔ＝０．０６７）;固定沙丘群体和半固定沙丘群体在等位酶水平上的变异性无显著差异。通过７个多态位点的研究表明,羊柴群体中的克隆多样性很高（Ｄ＝０．９１５６）,但不同克隆在规模上相差很大。同时,群体间的克隆分化较大,广布基因型仅占３．２％。克隆空间结构的分析表明,羊柴的基株分布为游击型构型,克隆之间的镶嵌明显。     

湖北海棠的等位酶变异和遗传多样性研究

采用超薄平板微型聚丙烯酰胺等电聚焦电泳方法对湖北海棠（Malus hupehensis)的9个野生居群和2个人工栽培居群的等位酶变异和遗传多样性进行了初步研究。通过对12个酶系统29个酶位点的检测,结果表明湖北海棠有25个酶位点的等位基因频率分布差异,,有10个居群发现稀有等位基因,并有11个（37．9％）重复位点;湖北海棠的遗传多样性水平很高,等位基因平均数A＝2．127,多态位点百分率P＝74．927,平均预期杂合度He=0.376;居群间的基因分化系数GST＝0．224。与其他苹果属植物相比,湖北海棠具有中等丰富的遗传变异水平。居群间的基因流仅为Nm=0.866,表明遗传漂变是影响居群遗传变异和遗传结构的一个重要因素。     

黑斑蛙乳酸脱氢酶和酯酶同功酶的研究

用聚丙烯酰胺凝胶电泳技术,分析了黑斑蛙肝脏和眼球中的乳酸脱氢酶（LDH）和酯酶（EST）同功酶,乳酸脱氢酶有3个遗传位点,Ldh-2和Ldh-3在肝脏和眼球中均表达,而Ldh-1仅在眼球中表达,这3个位点均为单态。酯酶共有10个点,其中Est-2、Est-4和Est-8为多态位点,Est-1、Est-2和Est-3在肝脏中表达,且活力很高,而在眼球中不表达。     

苍术（Atractybeslancea（Thunb．）DC．）种内遗传多样性分析

分析了苍术（Ａｔｒａｃｔｙｌｏｄｅｓｌａｎｄｅａ（Ｔｈｕｎｂ．）ＤＣ．）５种等位酶（ＭＤＨ,ＧＤＨ,ＰＰＯ,ＳＯＤ,ＰＥＲ）１２个位点上２５个等位基因的分化特征。结果表明：群体内多态位点比例平均为０．６１,每个位点的平均杂合率为０．２６,每个位点发现的平均等位基因数为１．７８。苍术种内基因多样性的８６％产生在群体内,群体间分化的明显效果为１４％。所有配对组合,群体间的平均遗传距离是０．１１,遗传同一性是０．９０。说明苍术种内变异很大。同时探讨茅苍术的分类位置,认为茅苍术不是苍术和白术的杂交种。     

梭梭同工酶遗传多态性初步研究

采用不连续聚丙烯酰胺凝胶电泳技术对采自新蛹阜康绿洲荒漠过渡带的40个梭梭个体的同工酶遗传多态性进行了初步研究。从24个酶系统中筛选,得到了14个酶系统可用于该植物的遗传变异分析。共检测出30个位点、54个等位基因,其中18个位点表现出多态性。在物种水平上,多态位点比率为60％,而平均每个位点的等位基因数为1．8。本研究的方法和结果将为后续相关研究提供一定的参考。     

红原鸡与家鸡的亲缘关系研究

对中国红原鸡滇地亚种和海南亚种与我国茶花鸡,泰和鸡和寿光鸡等地方鸡种以及芦花鸡,洛岛红等外国鸡种进行了血型（３个位点,１３个等位基因）,蛋白质（酶）多态（５个位点,１１个等位基因）和ＤＮＡ指纹分析,结果表明,红原鸡与茶花鸡（原始型品种）的亲缘关系较近;与泰和鸡,寿光鸡,芦花鸡,洛岛红（进化型品种）的亲缘关系较远,呈红原鸡－茶花鸡－泰和鸡,寿光鸡或芦花鸡,洛岛红这样一个进化阶梯,以上结果与国外资料（     

Entwicklungsgeschichte und Ultrastruktur von Pollenkitt und Exine bei nahe verwandten entomophilen und anemophilen Angiospermensippen derAlismataceae,Liliaceae, Juncaceae,Cyperaceae, Poaceae undAraceae

Some closely related members of the monocotyledonous familiesAlismataceae, Liliaceae, Juncaceae, Cyperaceae, Poaceae andAraceae with variable modes of pollination (insect- and wind-pollination) were studied in relation to the ultrastructure of pollenkitt and exine (amount, consistency and distribution of pollenkitt on the surface of pollen grains). The character syndromes of pollen cementing in entomophilous, anemophilous and intermediate (ambophilous or amphiphilous) monocotyledons are the same in principal as in dicotyledons. Comparing present with former results one can summarize: 1) The pollenkitt is always produced in the same manner by the anther tapetum in all angiosperm sub-classes. 2) The variable stickiness of entomophilous and anemophilous pollen always depends on the particular distribution and consistency of the pollenkitt, but not its amount on the pollen surface. 3) The mostly dry and powdery pollen of anemophilous plants always contains a variable amount of inactive pollenkitt in its exine cavities. 4) A step-by step change of the pollen cementing syndrome can be observed from entomophily towards anemophily. 5) From the omnipresence of pollenkitt in all wind-pollinated angiosperms studied one can conclude that the ancestors of anemophilous angiosperms probably have been zoophilous (i.e. entomophilous) throughout.

     

Identification and Characterization of the First Equine Parainfluenza Virus 5

正Dear Editor,Parainfluenza virus 5 (PIV5), known as canine parainfluenza virus in the veterinary field, is a negative-sense,nonsegmented, single-stranded RNA virus belonging to the Paramyxoviridae family (Chen 2018). The virus was first reported in primary monkey kidney cells in 1954 (Hsiung1972), then it has been frequently discovered in various     

Pathogenic Characterization and Full Length Genome Sequence of a Reassortant Infectious Bursal Disease Virus Newly Isolated in Pakistan

<正>Dear Editor,Infectious bursal disease (IBD) is one of the most important diseases of the poultry. The IBD virus (IBDV), a nonenveloped virus belonging to the Birnaviridae family with a genome consisting of two segments of double-stranded RNA (segments A and B), targets B lymphocytes of bursa of Fabricious leading to immunosuppression. In Pakistan,poultry farming is the second biggest industry and IBD is the second biggest disease threating the poultry sector.However, there is limited genome information of IBDV     

Mink Circovirus Can Infect Minks,Foxes and Raccoon Dogs

正Dear Editor,Mink circovirus (MiCV), which is clustered in the genus Circovirus of the family Circoviridae, was first described in minks from farms in Dalian, China in 2013 (Lian et al.2014). The complete single-stranded circular genome of the virus is 1,753 nucleotides long and contains two major open reading frames (ORFs), designated ORF1 (Rep gene)and ORF2 (Cap gene)(Lian et al. 2014; Ge et al. 2018).Sequence analysis has shown that MiCV is most closely     

CypA Regulates AIP4-Mediated M1 Ubiquitination of Influenza A Virus

Cyclophilin A (CypA) is a peptidyl-prolyl cis/trans isomerase that interacts with the matrix protein (M1) of influenza A virus (IAV) and restricts virus replication by regulating the ubiquitin–proteasome-mediated degradation of M1. However,the mechanism by which CypA regulates M1 ubiquitination remains unknown. In this study, we reported that E3 ubiquitin ligase AIP4 promoted K48-linked ubiquitination of M1 at K102 and K104, and accelerated ubiquitin–proteasome-mediated degradation of M1. The recombinant IAV with mutant M1 (K102 R/K104 R) could not be rescued, suggesting that the ubiquitination of M1 at K102/K104 was essential for IAV replication. Furthermore, CypA inhibited AIP4-mediated M1 ubiquitination by impairing the interaction between AIP4 and M1. More importantly, both the mutations of M1 (K102 R/K104 R) and CypA inhibited the nuclear export of M1, indicating that CypA regulates the cellular localization of M1 via inhibition of AIP4-mediated M1 ubiquitination at K102 and K104, which results in the reduced replication of IAV.Collectively, our findings reveal a novel ubiquitination-based mechanism by which CypA regulates the replication of IAV.