Comparative Studies on the Changes of Microtubule Distribution and Reorganization During the Meiotic Stages of Development in Normal(IR36) and a Temperature/photoperiod Sensitive Male Sterile Line(Pei

水稻激荡IR36 及光温敏核雄性不育系培矮64S 小孢子母细胞减数分裂期间微管骨架的变化 徐是雄¹刘向东²冯九焕² 卢永根²     

胡杨小孢子发生及微管骨架变化与异常研究

利用压片法和间接免疫荧光结合DAPI(4′,6-diamidino-2-phenylindole)染色法,对胡杨小孢子母细胞减数分裂过程中微管骨架变化和染色体行为进行观察研究。结果表明:（1）胡杨小胞子母细胞减数分裂进程中染色体行为正常,其中:偶线期可观察到单价体,中期Ⅰ会出现落后染色体,末期Ⅰ和末期Ⅱ的核仁呈现动态变化。（2）胡杨小孢子发生过程中细胞内微管骨架呈动态变化过程,其中:中期Ⅱ形成平行纺锤体以及三极纺锤体;末期Ⅱ未观察到典型的成膜体结构,同时型胞质分裂受子核间辐射微管系统调节,通过胞质向心收缩而发生,胞质分裂后形成四边形和四面体型四分体。（3）胡杨小孢子母细胞减数分裂过程中还存在各种异常细胞学现象,其中:中期Ⅱ平行纺锤体发生融合;中期Ⅱ 和后期Ⅱ孢母细胞两个纺锤体间的胞质会出现裂沟;四分体时期存在三分体和二分体,并产生天然2n花粉和连体花粉。     

水稻雄性不育系珍汕97A小孢子发育过程中的微管骨架

水稻（Oryza sativaL.)雄性不育系珍汕97A,保持系珍汕97B和恢复系测64三系小孢子发生过程的研究表明;恢复系测64小孢子母细胞细胞质浓,有明显的微管荧光围绕着细胞核。小孢子母细胞经两次减数分裂形成四分体。四分体和小孢子的微管从细胞核表面向胞质周缘延伸,形成放射性排列格局,花粉发育正常。细胞质中有少量点状微管荧光,保持系珍汕97B小孢子发生过程的细胞形态和微管结构与恢复系测64相似。但细胞质中的点状微管荧光多一些。雄性不育系珍汕97A小孢子发生早期,小孢子母细胞内出现液泡,核中染色质凝集,微管荧光很弱,没有清晰的微管丝结构。细胞质中有许多点状微管荧光等不正常现象。小孢子母细胞经过减数分裂形成的四分体也没有清晰的丝状微管结构。随后,所有的小孢子迅速败育,雄性不育系珍汕97A在小孢子母细胞发生的很早时期,微管结构就明显不正常。     

水稻雄性不育系珍汕97A小孢子发育过程中的微管骨架

水稻(Oryza sativa L.)雄性不育系珍汕97A、保持系珍汕97B和恢复系测64三系小孢子发生过程的研究表明:恢复系测64小孢子母细胞细胞质浓,有明显的微管荧光围绕着细胞核.小孢子母细胞经两次减数分裂形成四分体.四分体和小孢子的微管从细胞核表面向胞质周缘延伸,形成放射性排列格局,花粉发育正常.细胞质中有少量点状微管荧光.保持系珍汕97B小孢子发生过程的细胞形态和微管结构与恢复系测64相似,但细胞质中的点状微管荧光多一些.雄性不育系珍汕97A小孢子发生早期,小孢子母细胞内出现液泡,核中染色质凝集,微管荧光很弱,没有清晰的微管丝结构,细胞质中有许多点状微管荧光等不正常现象.小孢子母细胞经过减数分裂形成的四分体也没有清晰的丝状微管结构.随后,所有的小孢子迅速败育.雄性不育系珍汕97A在小孢子母细胞发生的很早时期,微管结构就明显不正常.     

水稻小孢子发育过程中微管骨架的变化

对水稻（ＯｒｙｚａｓａｔｉｖａＬ．）小孢子发育过程中微管变化的研究表明,微管在小孢子不同发育阶段呈现多样性。在花粉母细胞内,微管形成许多粗束和分支,围绕着核分布形成一个网络。花粉母细胞经第一次减数分裂形成二分体。在每一个二分体细胞内,有许多微管束,从核周辐射至细胞质各部位;在细胞质存在一个疏松的微管束网络。二分体经第二次减数分裂形成四分体,在每一个四分体细胞内,微管束呈辐射状,从核膜辐射入细胞质内。四分体形成后不久,四分体的四个细胞便分开,每一个细胞变成一个独立的小孢子。在早期的小孢子细胞内,微管束呈疏松网状分布。其中有些微管束朝向胞质一个小突起聚集。当小孢子进入中期发育阶段,在胞质的小突起部位微管束密度增大。小突起最终形成为萌发孔。当小孢子发育至成熟期,细胞内的微管束变得纤细,而网络则变得紧密。之后的发育阶段（即花粉发育不同阶段）因荧光标记难以进入细胞,无法获得清晰的图像。     

同源四倍体水稻小孢子发生的超微结构

利用透射电子显微镜对同源四倍体水稻小孢子母细胞减数分裂前及期间的超微结构进行观察,结果发现:(1)减数分裂前及减数分裂早期,小孢子母细胞核糖体密度高,线粒体、质体等细胞器丰富;粗线期核糖体密度显著下降,线粒体、质体等细胞器数量减少;终变期核糖体密度逐渐恢复到减数分裂前状态,而其他细胞器的数量除在二分体时期出现短暂的回升,终变期以后的时期均较少.(2)小孢子母细胞间的连接在小孢子母细胞时期以典型的胞间连丝为主,进入细线期,胞间连丝数量显著减少,宽孔道的胞质通道逐渐增多,粗线期小孢子母细胞间基本通过胞质通道连接,终变期小孢子母细胞间完全分离.(3)随着减数分裂的进行,药壁四层细胞逐渐液泡化,绒毡层细胞中部分小液泡融合成大液泡,形成胞内"空腔";药室内壁细胞出现大量的具有叶绿体结构特征的质体,内含丰富的淀粉粒,到了四分体时期质体数量及内含的淀粉粒显著减少.     

小麦小孢子发生过程的超微结构

采用透镜电镜技术对小麦（Ｔｒｉｔｉｃｕｍ ａｅｓｔｉｖｕｍ）小孢子发生过程进行了超微结构观察。造孢细胞时期细胞质中含有丰富的核糖体,质体和线粒体。在小孢子母细胞减数分裂过程中,有核糖体数量存在逐渐减少的现象,质体和线袜体结构在双线期／终变期和中期１简化,二分体时期,质体和线粒体形态结构基本恢复正常。结果表明,啵麦小孢子母细胞减数分裂过程中存在质体和线粒体的脱人化与再分化过程,但该过程与核糖体数量增     

洋葱小孢子母细胞减数分裂过程中微管分布变化

应用间接免疫荧光标记技术和激光共聚焦扫描显微镜成像技术观察洋葱小孢子母细胞减数分裂过程中微管分布变化。减数分裂之前,小孢子母细胞中的微管较短,呈辐射状,由细胞核表面向四周扩散。减数分裂开始后,细胞质中的一部分微管蛋白聚集成纺锤体微管,控制染色体的分布。进入减数分裂I后期,纺锤体微管变为牵引染色体移向两极的着丝粒微管和连接纺锤体两极的极丝微管。之后,所有微管集中在两个核之间,构成成膜体。然后,微管解聚成微管蛋白弥散在细胞质中。减数分裂I完成后,二分体2个子细胞中的微管蛋白又聚集成2个纺锤体微管,开始减数分裂II过程。经过减数分裂II中期,2个二分体细胞中的微管再次集中在2个细胞核之间形成成膜体,隔离2个细胞核。此后,微管蛋白解聚,弥散分布在小孢子细胞质中。     

鹤顶兰胚囊发育过程中微管变化的共焦显微镜观察

光镜的观察确定了鹤顶兰（Ｐｈａｉｕｓ ｔａｎｋｅｒｖｉｌｌｉａｅ （Ａｉｔｏｎ） Ｂｌ．）胚囊发育属单孢子蓼型。应用免疫荧光标记技术及共焦镜观察了胚囊发育过程中微管分布的变化。当孢原细胞初形成时,细胞内的微管呈网状分布。之后,孢原细胞体积增大发育为大孢子母细胞。大孢子母细胞延长,进入减数分裂Ⅰ。微管由分裂前的网状分布变为辐射状排列。二分体的两个细胞内的微管分布一样,呈辐射状。四分体的近珠孔端的３ 个大孢子解体,细胞内的微管消失。靠合点端的功能大孢子内有许多微管呈网状分布。当功能大孢子进入第一次有丝分裂时,细胞内的微管由网状变为辐射状,从核膜伸展至周质。再经两次有丝分裂形成八核胚囊。在核分裂之前微管一般是呈网状分布并紧包围着核。在分裂期间二核和四核胚囊都呈极性现象,微管系统也呈极性分布。微管在八核胚囊内的分布变化情形特别复杂。首先,八核分别作不同程度的移动,其中两个核移向胚囊中央,珠孔端和合点端的３ 个核分别互相靠拢,形成３ 个区,即中央区、反足区和卵器区。胚囊未形成区时,８ 个核都被网状分布的微管包围着。当胚囊明显分成区时,反足区内的微管仍作网状分布。中央区的微管分布则趋疏松,形成篮形结构,包围着液泡和两个极核。在     

大葱小孢子母细胞至二孢早期花粉发育的超微结构观察

用电镜观察了章丘大葱（Ａｌｌｉｕｍ ｆｉｓｔｕｌｏｓｕｉｍ Ｌ．）从包子母细胞至二胞早期花粉发育的超微结构。终变期的花粉母细胞,胼胝壁外方的相邻初生壁 胞间隙内,存在胞间物质,四分体期,此物质上孢子母细胞减数分裂前,细胞质内含有脂滴,小孢子有丝分裂以后,商增多增大。小孢子分裂后期,质体已积累淀偻粒１至多个。二胞早期花粉之营养细胞质内,有些含淀粉质本亦含脂滴。各发育期,核糖体及多聚合糖体丰富。并有很     

天然型与非天然型脱落酸的生物活性比较

采用新方法精制脱落酸（ＡＢＡ）异构体试样,提高了（Ｓ）－（＋）－ＡＢＡ与（Ｒ）－（－）－ＡＢＡ两对映体纯度。抑制生长试验和残留量分析以及气孔闭合试验表明：天然型（Ｓ）－（＋）－ＡＢＡ活性显著高于非天然型（Ｒ）－（－）－ＡＢＡ或（ＳＲ）－（±）－ＡＢＡ。抑制莴苣种子发芽５０％的活性强度,（Ｓ）－（＋）－ＡＢＡ约是（Ｒ）－（－）－ＡＢＡ的５倍,（ＳＲ）－（±）－ＡＢＡ介于两者之间。抑制萝卜下胚轴生长试验,最显著有效期为２～６ｄ,生理作用期约为一周,（Ｓ）－（＋）－ＡＢＡ活性是（Ｒ）－（一）－ＡＢＡ的３．５倍。鸭跖革气孔闭合试验,（Ｓ）－（＋）－ＡＢＡ活性比（Ｒ）－（－）－ＡＢＡ高１倍。     

Obesity and variants of the GHRL (ghrelin) and BCHE (butyrylcholinesterase) genes

Ghrelin coded by the GHRL gene is related to weight-gain, its deactivation possibly depending on its hydrolyzation by butyrylcholinesterase (BChE) encoded by the BCHE gene, an enzyme already associated with the body mass index (BMI). The aim was to search for relationships between SNPs of the GHRL and BCHE genes with BChE activity, BMI and obesity in 144 obese and 153 nonobese Euro-Brazilian male blood donors. In the obese individuals, a significant association with higher BChE activity, in the 72LM+72MM; -116GG genotype class (GHRL and BCHE genes, respectively) was noted. No significant differences were found otherwise, through comparisons between obese and control individuals, of genotype and allele frequencies in SNPs of the GHRL gene (Arg51Gln and Leu72Met), or mean BMI between 72LL and 72LM+72MM genotypes. Although there appears to be no direct relationship between the examined GHRL SNPs and BMI, the association of the 72M SNP with higher BChE activity in obese subjects probably points to a regulatory mechanism, thereby implying the influence of the GHRL gene on BChE expression, and a consequential metabolic role in the complex process of fat utilization.     

The heart of the dugong (Dugong dugon) and the west indian manatee (Trichechus manatus) (Sirenia)

Thirty-eight dugong (Dugong dugon) hearts and 28 Florida manatee (Trichechus manatus) hearts were obtained from stranding programs in Australia and the United States. In addition to a double ventricular apex, a feature that has astonished scientists since the eighteenth century, the hearts of both animals have a double subvalvular conus and a dorsal left atrium. The heart lies in a vertical plane at right angles to that of the completely dorsal, symmetrical lungs. The dugong heart has a deeper interventricular cleft and a more conical left ventricle. The latter features may be part of a general morphological trend toward specialization for a more energetic aquatic existence. The presence of a bulbous ascending aorta in the manatee but not in the dugong is without explanation.     

Linkage between the loci for the Lp(a) lipoprotein (LP) and plasminogen (PLG)

Summary A locus, LP, that determines quantitative variation of Lp(a) lipoprotein phenotypes is linked to the plasminogen (PLG) locus (peak lod score =12.73). This linkage relationship assigns a locus with alleles that have an affect on risk for coronary artery disease to the long arm of chromosome 6.     

Characterization of divalent cation localization in the minor groove of the A(n)T(n) and T(n)A(n) DNA sequence elements by (1)H NMR spectroscopy and manganese(II)

The localization of Mn(2+) in A-tract DNA has been studied by (1)H NMR spectroscopy using a series of self-complementary dodecamer oligonucleotides that contain the sequence motifs A(n)(n) and T(n)A(n), where n = 2, 3, or 4. Mn(2+) localization in the minor groove is observed for all the sequences that have been studied, with the position and degree of localization being highly sequence-dependent. The site most favored for Mn(2+) localization in the minor groove is near the 5'-most ApA step for both the T(n)A(n) and the A(n)T(n) series. For the T(n)A(n) series, this results in two closely spaced symmetry-related Mn(2+) localization sites near the center of each duplex, while for the A(n)T(n) series, the two symmetry-related sites are separated by as much as one half-helical turn. The degree of Mn(2+) localization in the minor groove of the T(n)A(n) series decreases substantially as the AT sequence element is shortened from T(4)A(4) to T(2)A(2). The A(n)T(n) series also exhibits length-dependent Mn(2+) localization; however, the degree of minor groove occupancy by Mn(2+) is significantly less than that observed for the T(n)A(n) series. For both A(n)T(n) and T(n)A(n) sequences, the 3'-most AH2 resonance is the least broadened of the AH2 resonances. This is consistent with the observation that the minor groove of A-tract DNA narrows in the 5' to 3' direction, apparently becoming too narrow after two base pairs for the entry of a fully hydrated divalent cation. The results that are reported illustrate the delicate interplay that exists between DNA nucleotide sequence, minor groove width, and divalent cation localization. The proposed role of cation localization in helical axis bending by A-tracts is also discussed.     

Structural requirements of echistatin for the recognition of alpha(v)beta(3) and alpha(5)beta(1) integrins

There are key differences between the amino acid residues of the RGD loops and the C termini of echistatin, a potent antagonist of alpha(IIb)beta(3), alpha(v)beta(3) and alpha(5)beta(1), and eristostatin, a similar disintegrin selectively inhibiting alpha(IIb)beta(3). In order to identify echistatin motifs required for selective recognition of alpha(v)beta(3) and alpha(5)beta(1) integrins, we expressed recombinant echistatin, eristostatin, and 15 hybrid molecules. We tested them for their ability to inhibit adhesion of different cell lines to fibronectin and von Willebrand factor and to express ligand-induced binding site epitope. The results showed that Asp(27) and Met(28) support recognition of both alpha(v)beta(3) and alpha(5)beta(1). Replacement of Met(28) with Asn completely abolished echistatin's ability to recognize each of the integrins, while replacement of Met(28) with Leu selectively decreased echistatin's ability to recognize alpha(5)beta(1) only. Eristostatin in which C-terminal WNG sequence was substituted with HKGPAT exhibited new activity with alpha(5)beta(1), which was 10-20-fold higher than that of wild type eristostatin. A hypothesis is proposed that the C terminus of echistatin interacts with separate sites on beta(1) and beta(3) integrin molecules.