兰州百合组培鳞茎发育研究

该研究以兰州百合商品种球鳞片为外植体材料,通过组织培养诱导丛生芽萌发及高频增殖,再以丛生芽为材料诱导其发育形成小鳞茎,调节培养基对小鳞茎进行膨大发育培养,最终形成促进兰州百合组培鳞茎膨大发育的“三步”组培培养技术路线;对发育过程中形成的丛生芽、小鳞茎及膨大鳞茎进行淀粉含量测定与生长特征参数统计,分析各步培养对鳞茎形成发育过程中淀粉含量与形态变化的影响。结果表明：所建立的“三步”培养方案培育出的组培鳞茎直径、重量与鳞片数分别为1.66 cm、2.48 g和26.33片,有效地促进了鳞茎的膨大,并能诱导鳞茎主茎杆的形成发育;在培养进程中其淀粉含量呈现逐步增加的趋势,这表明与鳞茎膨大发育正相关,同时鳞茎大小、重量及鳞片数三者也表现为正相关性;当鳞茎所含鳞片数在26片以上时,其生长点易发育形成主茎杆。该文研究了兰州百合组培鳞茎的形成与膨大发育技术,所研发的“三步”培养组成的鳞茎膨大发育组培技术有效地促进了鳞茎的膨大发育,而膨大发育的鳞茎能有效地缩短田间生长周期,从时间上提高百合生产量,同时为实现兰州百合膨大的鳞茎种球规模化生产提供技术支撑。     

茭白生育过程中地上各部位内源激素的含量变化

以两个茭白品种为试材,测定了植株茎蘖生育过程中地上各部位主要激素及肉质茎膨大过程中的干重变化。结果显示：茭白植株生育过程中各部位的激素以玉米素及玉米素核苷(Z ZR)的含量最高,生长素(IAA)其次,赤霉素(GA3)和脱落酸(ABA)含量很低;在各部位间总体以茎尖最高,叶鞘其次,叶片最低。其中Z ZR含量在肉质茎膨大前即已明显上升,膨大开始后显著下降;IAA含量在肉质茎膨大后期至末期才出现下降;叶片内ABA含量在肉质茎膨大前即开始上升,叶鞘内ABA．含量在肉质茎膨大后期上升,茎尖内则无明显变化;各部位GA2含量在整个生育期内无明显变化。肉质茎的干重增加也与其Z ZR含量下降密切相关。认为Z ZR是刺激肉质茎膨大的关键激素。品种间差异表现为各部位激素含量及其变化有一定差异,尤其是肉质茎膨大阶段差异比较明显。     

爬山虎属三种植物吸盘的解剖学研究

运用常规石蜡切片法,对3种爬山虎属(Parthenocissus)植物的吸盘结构进行了观察研究.结果表明:吸盘膨大部位、吸附方式、卷须长短及托叶可以作为种的分类依据;3种植物的吸盘均由表皮、皮层、维管柱组成,未吸附表皮细胞外弦壁增厚,具角质层;吸盘膨大主要是由维管柱扩大而非表皮细胞膨大引起;吸盘未吸附部位的皮层细胞含有较多晶体;吸盘膨大时维管柱转变成维管束,维管形成层活动期较短.3种植物的吸附结构由表皮及皮层细胞反分化分裂形成多层指状细胞构成.     

兰州百合组培鳞茎发育研究（英文）

该研究以兰州百合商品种球鳞片为外植体材料,通过组织培养诱导丛生芽萌发及高频增殖,再以丛生芽为材料诱导其发育形成小鳞茎,调节培养基对小鳞茎进行膨大发育培养,最终形成促进兰州百合组培鳞茎膨大发育的"三步"组培培养技术路线;对发育过程中形成的丛生芽、小鳞茎及膨大鳞茎进行淀粉含量测定与生长特征参数统计,分析各步培养对鳞茎形成发育过程中淀粉含量与形态变化的影响。结果表明:所建立的"三步"培养方案培育出的组培鳞茎直径、重量与鳞片数分别为1.66 cm、2.48 g和26.33片,有效地促进了鳞茎的膨大,并能诱导鳞茎主茎杆的形成发育;在培养进程中其淀粉含量呈现逐步增加的趋势,这表明与鳞茎膨大发育正相关,同时鳞茎大小、重量及鳞片数三者也表现为正相关性;当鳞茎所含鳞片数在26片以上时,其生长点易发育形成主茎杆。该文研究了兰州百合组培鳞茎的形成与膨大发育技术,所研发的"三步"培养组成的鳞茎膨大发育组培技术有效地促进了鳞茎的膨大发育,而膨大发育的鳞茎能有效地缩短田间生长周期,从时间上提高百合生产量,同时为实现兰州百合膨大的鳞茎种球规模化生产提供技术支撑。     

第24届国际生物学奥林匹克竞赛试题实验3·进化生态学

<正>总分:94分,时间:90 min本测试包括3项任务:任务1:定量攻击行为1.1实验设计1.2黄金燕尾鱼的攻击行为1.3撞击或撕咬的例子1.4量化黄金燕尾鱼的撞击和撕咬(30分)1.5其他重复1.6撞击和撕咬的统计分析(20分)任务2:喉部膨大行为2.1黄金燕尾鱼的喉部膨大行为2.2喉部膨大行为例子2.3量化喉部膨大行为(21分)     

光敏色素对黄化绿豆幼苗下胚轴原生质体膨大的调节作用

红光引起黄化绿豆（ＰｈａｓｅｏｌｕｓｒａｄｉｔｕｓＬ．）幼苗下胚轴原生质体膨大,远红光可逆转红光的作用。这种可逆现象至少能在两个红光－远红光循环中观察到;膨大反应与红光光照强度和时间呈正相关,表明黄化绿豆幼苗下胚轴原生质体膨大是由光敏色素诱导的。红光引起的膨大只是在培养液中有Ｃａ２＋ 存在时才能发生,Ｍｇ２＋ 、Ｂａ２＋ 、Ｚｎ２＋ 或Ｋ＋ 均不能替代Ｃａ２＋ 的作用。膨大与原生质体吸水有一定关系     

钙在IAA诱导绿豆下胚轴原生质体膨大过程中的作用

含钙培养液(对照)和仅用IAA处理的原生质体的体积和~(45)Ca~(2 )放射性强度均无变化。IAA处理含钙培养液中的原生质体,5min后~(45)Ca~(2 )积累明显增多,体积开始膨大。处理30min时~(45)Ca~(2 )积累最多,此时原生质体的膨大效应最好;随后~(45)Ca~(2 )积累和膨大效应逐渐下降。K~ 、Zn~(2 )、Ba~(2 )、Mg~(2 )等也可在一定程度上代替Ca~(2 )使原生质体体积膨大。原生质体的吸水在膨大中起着一定作用。EGTA、LaCl_3和verapamil均抑制IAA诱导的原生质体~(45)Ca~(2 )积累和体积膨大。说明Ca~(2 )可能在6-BA诱导原生质体膨大的过程中起着重要作用。     

甘薯块根膨大过程中ATP酶活性、ATP和ABA含量的变化

研究选用鲁薯7号和徐薯18号为材料,对甘薯块根膨大速率变化动态及其块根中可溶性碳水化合物含量、ATP含量、ATP酶活性和脱落酸（ABA）含量的变化进行了研究分析。结果表明：（1）块根膨大速率变化动态呈一双峰曲线,第一个高峰出现在栽秧后50－70d,第二个高峰出现在栽秧后120－165d;（2）块根膨大高峰期,块根中可溶性碳水化合物含量较高,ATP含量则较低;（3）块根中ATP酶活性和ABA含量变化动态与块根膨大速率变化动态相似。讨论了ATP酶和ABA在块根膨大过程中的可能作用。     

广西野牡丹科一新种,大明山异药花

详细描述了广西产的异药花属一新种——大明山异药花。该种与产于福建、广西等地的异药花近似,但不同在于本种叶基出脉较多,7-9条;多歧聚伞花序长2.5-3cm,宽6-7cm;长雄蕊花药线形,基部伸长,略膨大成囊状,分离,药隔膨大,伸长成短距,短雄蕊花药线形,药隔膨大,伸长成短距。     

MeJA对大蒜鳞茎膨大及内源激素含量的影响

于大蒜鳞茎开始膨大时叶片喷施茉莉酸甲酯（Methyl Jasmonate,MeJA)可明显促进鳞茎膨大;酶联免疫法（ELISA）测定结果显示外源MeJA影响内源植物激素的含量,10μmol/LM可明显提高大蒜鳞茎膨大过程中IAA（吲哚乙酸）的含量。降低GA1 3（赤霉素）、ABA（脱落酸）的含量,但对iPAs含量的影响不大,分析表明MeJA可能通过与其他植物激素的协调作用而促进大蒜鳞茎膨大。     

AcMNPV的囊膜形成与囊膜蛋白gp64在细胞内的定位

应用电镜观察了重组AcMNPV感染的Sf9细胞,结果表明该病毒的囊膜形成至少有两种形式：一是通过细胞质膜上出芽,二是在核内被膜结构包围而获得囊膜,此外通过核膜出芽也可能是病毒获得囊膜的一种方式。应用免疫荧光技术研究了该病毒在Sf9细胞内囊膜的形成及其与病毒囊膜蛋白gp64间的关系,结果表明gp64主要存在于细胞的质膜与核膜上。该存在方式使得通过出芽而获得囊膜的病毒粒子与核内包被产生的病毒粒子在囊膜成分上有很大差异。     

A cellular reaction to antibody in tissue culture studied with electron microscopy

The reaction of embryonic chick heart cells grown in tissue culture to specific guinea pig antiserum has been studied with electron microscopy. Heart fragments from chick embryos were cultured with a plasma clot. After being tested with antiserum or normal serum, they were fixed with buffered osmium tetroxide and embedded in butyl methacrylate before removal from the glass culture chamber. Thin cells found by phase microscopy to have reacted were sectioned in a plane parallel to the glass surface on which they had grown. The results confirm and extend observations made previously while the reactions were occurring. The plasma membrane, like that of the red cell, becomes disrupted or less resistant to trauma following the action of antiserum. The membranes of mitochondria and endoplasmic reticulum vesiculate and swell. Before nuclear shrinkage becomes prominent, the outer nuclear membrane separates over a large portion of the nuclear envelope and forms one or more large swollen blebs. Thus, the outer nuclear membrane shows a reactivity similar to endoplasmic reticulum. It is suggested that the various physical and chemical changes observed to follow the action of antibody and complement on fibroblasts may be explained by osmotic pressure differences between various cell components. Some basic similarities to the action of hemolytic agents on red cells are noted.     

A Cellular Reaction to Antibody in Tissue Culture Studied with Electron Microscopy

The reaction of embryonic chick heart cells grown in tissue culture to specific guinea pig antiserum has been studied with electron microscopy. Heart fragments from chick embryos were cultured with a plasma clot. After being tested with antiserum or normal serum, they were fixed with buffered osmium tetroxide and embedded in butyl methacrylate before removal from the glass culture chamber. Thin cells found by phase microscopy to have reacted were sectioned in a plane parallel to the glass surface on which they had grown. The results confirm and extend observations made previously while the reactions were occurring. The plasma membrane, like that of the red cell, becomes disrupted or less resistant to trauma following the action of antiserum. The membranes of mitochondria and endoplasmic reticulum vesiculate and swell. Before nuclear shrinkage becomes prominent, the outer nuclear membrane separates over a large portion of the nuclear envelope and forms one or more large swollen blebs. Thus, the outer nuclear membrane shows a reactivity similar to endoplasmic reticulum. It is suggested that the various physical and chemical changes observed to follow the action of antibody and complement on fibroblasts may be explained by osmotic pressure differences between various cell components. Some basic similarities to the action of hemolytic agents on red cells are noted.     

The subnuclear localization of tRNA ligase in yeast

Yeast tRNA ligase is an enzyme required for tRNA splicing. A study by indirect immune fluorescence shows that this enzyme is localized in the cell nucleus. At higher resolution, studies using indirect immune electron microscopy show this nuclear location to be primarily at the inner membrane of the nuclear envelope, most likely at the nuclear pore. There is a more diffuse, secondary location of ligase in a region of the nucleoplasm within 300 nm of the nuclear envelope. When the amount of ligase in the cell is increased, nuclear staining increases but staining of the nuclear envelope remains constant. This experiment indicates that there are a limited number of ligase sites at the nuclear envelope. Since the other tRNA splicing component, the endonuclease, has the characteristics of an integral membrane protein, we hypothesize that it constitutes the site for the interaction of ligase with the nuclear envelope.     

Role of the nuclear envelope in synthesis, processing, and transport of membrane glycoproteins

The outer nuclear membrane is morphologically similar to rough endoplasmic reticulum. The presence of ribosomes bound to its cytoplasmic surface suggests that it could be a site of synthesis of membrane glycoproteins. We have examined the biogenesis of the vesicular stomatitis virus G protein in the nuclear envelope as a model for the biogenesis of membrane glycoproteins. G protein was present in nuclear membranes of infected Friend erythroleukemia cells immediately following synthesis and was transported out of nuclear membranes to cytoplasmic membranes with a time course similar to transport from rough endoplasmic reticulum (t 1/2 = 5-7 min). Temperature-sensitive mutations in viral membrane proteins which block transport of G protein from endoplasmic reticulum also blocked transport of G protein from the nuclear envelope. Friend erythroleukemia cells and NIH 3T3 cells differed in the fraction of newly synthesized G protein found in nuclear membranes, apparently reflecting the relative amount of nuclear membrane compared to endoplasmic reticulum available for glycoprotein synthesis. Nuclear membranes from erythroleukemia cells appeared to have the enzymatic activities necessary for cleavage of the signal sequence and core glycosylation of newly synthesized G protein. Signal peptidase activity was detected by the ability of detergent-solubilized membranes of isolated nuclei to correctly remove the signal sequence of human preplacental lactogen. RNA isolated from the nuclear envelope was highly enriched for G protein mRNA, suggesting that G protein was synthesized on the outer nuclear membrane rather than redistributing to nuclear membranes from endoplasmic reticulum before or during cell fractionation. These results suggest a mechanism for incorporation of membrane glycoproteins into the nuclear envelope and suggest that in some cell types the nuclear envelope is a major source of newly synthesized membrane glycoproteins.     

The nuclear envelopathies and human diseases

The nuclear envelope (NE) consists of two membrane layers that segregate the nuclear from the cytoplasmic contents. Recent progress in our understanding of nuclear-lamina associated diseases has revealed intriguing connections between the envelope components and nuclear processes. Here, we review the functions of the nuclear envelope in chromosome organization, gene expression, DNA repair and cell cycle progression, and correlate deficiencies in envelope function with human pathologies.     

Comparative proteomic analyses of the nuclear envelope and pore complex suggests a wide range of heretofore unexpected functions

Since the discovery of several inherited diseases linked to the nuclear envelope the number of functions ascribed to this subcellular organelle has skyrocketed. However the molecular pathways underlying these functions are not clear in most cases, perhaps because of missing components. Several recent proteomic analyses of the nuclear envelope and nuclear pore complex proteomes have yielded not only enough missing components to potentially elucidate these pathways, but suggest an exponentially greater number of functions at the nuclear periphery than ever imagined. Many of these functions appear to derive from recapitulation of pathways utilized at the plasma membrane and from other membrane systems. Additionally, many proteins identified in the comparative nuclear envelope studies have sequence characteristics suggesting that they might also contribute to nuclear pore complex functions. In particular, the striking enrichment for proteins in the nuclear envelope fractions that carry phenylalanine-glycine (FG) repeats may be significant for the mechanism of nuclear transport. In retrospect, these findings are only surprising in context of the notion held for many years that the nuclear envelope was only a barrier protecting the genome. In fact, it is arguably the most complex membrane organelle in the cell.