甘蓝型油菜细胞质雄性不育系301A线粒体不育基因片段分析

提取细胞质雄性不育系301A、212A和'陕3A'及其共同保持系'中双2号'线粒体DNA,根据已报道的Polima油菜细胞质雄性不育相关基因orf224序列设计引物,对3种不同来源的线粒体DNA PCR产物进行分析.结果显示,这3种甘蓝型油菜细胞质雄性不育材料所获得片段序列完全一致,且与已报道的Polima油菜线粒体中细胞质雄性不育相关基因orf224序列完全相同.研究表明,不育材料301A从分子角度讲属于Polima系统,不育系301A、212A和'陕3A'线粒体中与细胞质雄性不育相关线粒体基因片段orf224具有高度同源性.     

不结球白菜新种质P70-203雄性不育细胞质类型的鉴定

本研究根据OguraCMS、PolimaCMS的不育性状相关的线粒体基因序列设计特异引物,对不结球白菜雄性不育系新种质P70-203及其保持系P60-27-1进行PCR分析.研究结果表明,Polima引物P3/P4,P5/P6在不育系与可育系中均无扩增条带;Ogura引物P1/P2在不育系中扩增出750 bp的特异片段,但可育系中无扩增条带.将扩增的特异条带回收并测序,将得到的测序结果在NCBI中进行Blastn同源性比较,结果与青花菜Ogura(登录号:EU604643)和萝卜Ogura(登录号:AB055438)细胞质雄性不育同源性均达到99%.从分子角度初步推测:该雄性不育系新种质P70-203具有Ogura细胞质.     

大白菜雄性不育系RC7育性相关基因克隆与特性分析

根据orf138的保守序列设计引物,以大白菜萝卜胞质雄性不育系RC7的mtDNA为模板进行PCR扩增,扩增出大小为588 bp的特异条带,该片段在叶片和花蕾中均有表达,没有转录后加工,可编码75个氨基酸,定名为orf75。同源性分析结果表明:orf75推导的氨基酸序列N末端与萝卜Ogu CMS所具有的ORF138一致性为100%,有28个氨基酸完全相同,C末端与钾依赖钠钙交换蛋白-1一致性为54%。初步认为,orf75可能是orf138与钾依赖钠钙交换蛋白-1的编码基因发生重排产生的新的开放阅读框。RC7的不育性与Ogu CMS具有相似性。该588 bp片段还可编码1个含有1个疏水基团和1个跨膜区的67aa的蛋白片段,定名为orf67,属可溶性蛋白。     

复合PCR扩增人mtDNA HVR方法的初探

目的:建立一种高效的扩增线粒体DNA高可变区(mtDNA HVR)的方法.方法:本研究选取5例健康成人静脉血,用人血全基因组DNA试剂盒,提取全基因组DNA,设计引物,用复合PCR方式,对线粒体DNA中的高可变区进行扩增.复合扩增的方式为:用6对套叠引物分开进行两次独立的PCR,扩增mtDNA HVR.第一次扩增用3对引物,目标DNA片段基本涵盖整个线粒体DNA的高可变区,扩增后得到互不重叠的3个短片段,分别为113 bp,126 bp和131bp.第二次复合扩增用其余的3对引物,目标片段基本重叠在第一次扩增所得的目标片段的区域内,扩增得到3个互不重叠的片段为124 bp,133 bp和93bp.所有扩增产物经过纯化后测序.结果:复合PCR方式获得的mtDNA HVR基因序列完整,5个样本均出现特异性条带,电泳结果条带单一、清晰.结论:复合扩增PCR方法对mtDNA HVR区的扩增效率高,测序结果稳定,结合6对套叠引物,不但保证了序列的完整性,另外,两次独立的PCR也减少了PCR反应过程中错配的发生,此法也适用于保存时间较久的古代线粒体DNA短片段的研究.复合扩增PCR还展示出了潜在的高产量的特点,相对传统PCR显示了其更多的优势.     

青花菜Ogu不育胞质分子鉴定和序列分析

雄性不育是农作物利用杂种优势、进行轮回选择和群体改良的重要手段,在农作物生产中具有巨大的利用价值。该研究为了鉴定青花菜细胞质雄性不育材料的不育胞质类型,以期今后为青花菜种质资源的收集、利用及分子标记辅助育种提供新的不育标记。根据Gen Bank中orf138基因保守序列设计特异引物,对20个青花菜种质资源基因组DNA进行PCR扩增。结果表明:特异引物P1/P2在12个青花菜雄性不育基因型中均扩增出392 bp的片段,在8个可育基因型中未扩增出条带,与田间育性鉴定结果相符。获得青花菜Ogu胞质雄性不育的特异基因orf138序列,Gen Bank中的登录号为HQ149728;用Blastn在Gen Bank中进行同源性比对分析,发现12个不育材料的特异片段与已报道的萝卜Ogu CMS所具有的Ogu orf138基因(Genbank登录号:Z18896.1)同源度高达100%。序列同源比对发现orf138基因存在变异位点。研究结果可为青花菜雄性不育细胞质的分子鉴定、进一步阐明胞质雄性不育败育机理,以及指导青花菜新型不育系的创建和杂种优势高效利用提供理论依据。     

花椰菜细胞质雄性不育基因特异PCR标记的筛选

基于同源序列的候选基因法(homology-based candidate gene method),通过检索NCBI核酸及蛋白数据库,获得细胞质雄性不育（cytoplasmic male sterility CMS）相关的基因或开放读码框。生物学软件分析,根据保守区设计5对特异引物,PCR扩增,其中引物P9/P10在花椰菜细胞质雄性不育系knxd612中特异扩增出313 bp的片段。单株检测,RT-PCR分析,斑点杂交鉴定,确定此片段为花椰菜细胞质雄性不育系knxd612所特有。序列分析表明该片段与Ogura型胞质不育萝卜,不育相关开放读码框orf138的同源性高达98％。初步结果显示实验所用不育花椰菜胞质亦可能为Ogura型。该结果为进一步从分子水平研究花椰菜细胞质雄性不育打下了坚实的基础。Abstract: The homology-based candidate gene method was used to identified the specific PCR markers linked to cytoplasmic male sterility (CMS) in cauliflower( Brassica oleracea var botrytis.).Searching the DNA and protein data-base of NCBI , correlative genes or open reading frames were indentified .Analysis of biosoft, based on the conservative regions ,five primers were designed . Among them, only primer P9/P10 produced a 313- bp specific fragment. Identified by individual plant testing , analysis of RT-PCR and dot blot ,this fragment was only existed in CMS cauliflower knxd612.Analysis of the sequence indicated it was high homologous(98%) with orf138 of Ogura CMS radish. Primary result suggested that the cytoplasmic type of CMS cauliflower knxd612 may belong to Ogura type. This research offered a good foundation to further investigate the CMS mechanism of cauliflower in molecular level.     

杨树木质素合成酶c3h基因的克隆及其序列分析

根据CYP98A3(GenBank登录号为AY064170)cDNA序列保守区设计引物,从正在分化的2年生‘欧美杨107’次生木质部提取的总RNA经RT-PCR扩增出一基因片段,然后与pMD20-T载体连接。重组质粒经限制性内切酶酶切、特异引物PCR扩增和测序鉴定。结果表明,扩增片段长度为994bp,其中包含一个长为495bp的开放阅读框,编码的氨基酸序列(登录号为CAP47423)与NCBI中AY064170的CYP98A3编码氨基酸序列的相似性为91%,初步断定其为CYP98A3家族中的一员,其cNDA序列GenBank登录号为AM920690。参照国内外已发表的部分植物的c3h基因序列,构建了c3h的遗传进化树,分析了不同植物c3h的遗传进化关系。     

不同产地中华鳖的线粒体控制区序列分析及结构比较

采用PCR特异引物,扩增了两产地中华鳖（Pelodiscus sinensis）个体的mtDNA控制区（CR）及其邻近片段,测序获得了长度分别为1830bp和1630bp的序列。结合GenBank中已发表的韩国产中华鳖mtDNA的CR区序列,比较了3个产地中华鳖的CR区结构。分析显示：中华鳖不同产地mtDNA CR区DNA中的A＋T含量分别为60.5%、63.6%和64.8%,它们的5′、3′末端以及CSB1-CSB2之间均存在丰富的可变数目串联重复序列（variable numbers oftandem repeats,VNTR）。基于mtDNA CR区序列和结构分析,显示中华鳖不同产地的野生个体中存在丰富的遗传多样性。     

BT型细胞质雄性不育水稻及其三系的线粒体DNA研究

用RAPD技术对BT型水稻胞质雄性不育系秀A及其保持系秀B、恢复系湘晴以及杂种F1代的线粒体DNA进行了比较分析。结果表明不育系与其保持系间存在显著差异;不育系与其F1之间mtDNA也存在差异。在引物OPJ－08的扩增产物中,秀A扩增出一条分子量为800bp的多态性片段,在引物OPK－10的扩增产物中,杂种F1扩增出一条分子量为900bp的片段。把这两片段回收、克隆并制备探针,OPJ－08800的Southern杂交结果显示不育系与其F1杂交图谱存在多态性;OPK－10900的Suthern杂交结果显示不育系与其保持系同存在差异。推测这两片段与育性可能有一定的联系。     

草鱼CYP1A和ACT基因cDNA片段的克隆与鉴定

以Trizol法分别提取BNF诱导和对照处理草鱼的肝组织总RNA并合成cDNA第一链,以此为模板利用1对ACT特异性引物和(8条)6对CYP1A简并引物进行扩增。结果显示,引物对F0-R0在对照和诱导草鱼中均扩增得到预期ACTcDNA片段,而引物对F4-R4在诱导草鱼中获得预期CYP1A cDNA产物。这两个cDNA片段分别进行克隆、测序和比对,BLAST结果表明草鱼ACTcDNA片段(800 bp)与GenBank中ACT基因(登录号M25013)同源性为99.1%,推导氨基酸序列同源性为99.2%;草鱼CYP1A cDNA片段(439 bp)与鲤鱼同源性最高,为92.5%,推导氨基酸同源性为96.6%。上述序列提交GenBank,获得登录号分别为DQ211096和DQ211095。通过Mega 3.1软件的Neighbor-joining程序对CYP基因的部分cDNA序列和氨基酸序列进行比对分析并绘制进化树,根据CYP1A部分蛋白的系统发育关系,在进化上可以将参与比对的真骨鱼划分为4个主要的分支。     

Investigation of the mechanism of temperature sensitivity of the electroreceptors of ampullae of lorenzini

In experiments on Black Sea skates (Raja clavata), the potential of the receptor epithelium of the ampullae of Lorenzini and spike activity of single nerve fibers connected to them were investigated during electrical and temperature stimulation. Usually the potential within the canal was between 0 and –2 mV, and the input resistance of the ampulla 250–400 k. Heating of the region of the receptor epithelium was accompanied by a negative wave of potential, an increase in input resistance, and inhibition of spike activity. With worsening of the animal's condition the transepithelial potential became positive (up to +10 mV) but the input resistance of the ampulla during stimulation with a positive current was nonlinear in some cases: a regenerative spike of positive polarity appeared in the channel. During heating, the spike response was sometimes reversed in sign. It is suggested that fluctuations of the transepithelial potential and spike responses to temperature stimulation reflect changes in the potential difference on the basal membrane of the receptor cells, which is described by a relationship of the Nernst's or Goldman's equation type.I. P. Pavlov Institute of Physiology, Academy of Sciences of the USSR, Leningrad. I. M. Sechenov, Institute of Evolutionary Physiology and Biochemistry, Academy of Sciences of the USSR, Leningrad. Pacific Institute of Oceanology, Far Eastern Scientific Center, Academy of Sciences of the USSR, Vladivostok. Translated from Neirofiziologiya, Vol. 12, No. 1, pp. 67–74, January–February, 1980.     

Principles of organization and evolution of systems of regulation of functions

Evolution of living organisms is closely connected with evolution of structure of the system of regulations and its mechanisms. The functional ground of regulations is chemical signalization. As early as in unicellular organisms there is a set of signal mechanisms providing their life activity and orientation in space and time. Subsequent evolution of ways of chemical signalization followed the way of development of delivery pathways of chemical signal and development of mechanisms of its regulation. The mechanism of chemical regulation of the signal interaction is discussed by the example of the specialized system of transduction of signal from neuron to neuron, of effect of hormone on the epithelial cell and modulation of this effect. These mechanisms are considered as the most important ways of the fine and precise adaptation of chemical signalization underlying functioning of physiological systems and organs of the living organism