五唇兰未受精胚珠离体培养及雌配子体发育的研究

五唇兰(Doritispulcherrima Lindl.)的胚珠属于倒生型,具薄珠心,两层珠被.胚囊发育类型为双孢子葱型,授粉后约45 d形成七细胞八核的成熟胚囊.五唇兰未受精胚珠在离体培养初期对外源激素的依赖性很小,在没有外源激素的培养基上,大孢子母细胞也能经过减数分裂发育为二核胚囊.在培养后期,外源激素对胚囊发育的影响很大.在培养基无外源激素或仅含生长素或细胞分裂素时,雌配子体的发生过程不能顺利完成;在改良VW培养基上添加0.5 mg/L BA和0.1 mg/LNAA时,形成成熟胚囊.     

五唇兰雌配子体发育和胚胎发生的研究

五唇兰的胚珠倒生型,具薄珠心,两层珠被。胚囊发育为双孢子葱型,成熟胚囊８核。从传粉到受精约５０ｄ,正常双受精。胚具５－６细胞的胚柄,种子成熟时胚柄及胚乳核消失,成熟种子只具单层细胞的种皮和一个未分化的珠珠形胚。     

刺五加大、小孢子发生和雌、雄配子体发育的观察

刺五加Eleutherococcus senticosus(Rupr．et Maxim．)Maxim．雄株的小孢子发生和雄配子体发育过 程正常,大孢子发生和雌配子体发育过程多不正常。雄花具5个花药,花药4室,药壁发育属双子叶型, 腺质绒毡层,绒毡层细胞多具2核。小孢子母细胞经减数分裂形成四面体形四分体,其胞质分裂为同时 型。成熟花粉为3细胞型。子房下位,5室;每室有上胚珠和下胚珠,上胚珠退化,下胚珠倒生、具单珠 被、厚珠心;大孢子母细胞经减数分裂形成线形或“T”形四分体,偶尔有2个并列或串联的四分体或在 四分体之上又出现孢原细胞。其功能大孢子位置不确定。雌配子体发育中异常现象较多。开花时,雌 配子体主要为反足细胞退化后的四细胞胚囊。刺五加雌株的小孢子母细胞不能进行减数分裂或减数分 裂不正常,不能形成四分体。开花时,药室空瘪,无花粉形成。其大孢子发生和雌配子体发育过程正常, 大孢子母细胞减数分裂形成线形或“T”形四分体,合点端大孢子为功能大孢子,胚囊发育属蓼型。开花 时,雌配子体主要为七细胞八核或七细胞七核胚囊,其卵器尚未发育成熟。刺五加两性株的小孢子发生 过程无异常,但雄配子体发育过程有部分异常;开花时,药室内有或多或少的空花粉,且花粉粒大小悬 殊,大的直径达35μm,小的仅15～18 μm。两性株的雌蕊发育大部分正常,也有一些异常胚囊形成。开 花时,雌配子体主要是七细胞八核胚囊、七细胞七核胚囊和反足细胞退化后的四细胞胚囊,其卵器也未发育成熟。     

小叶兜兰的果实生长和雌配子体发育

为了解濒危兰科植物小叶兜兰(Paphiopedilum barbigerum Tang et Wang)胚珠和雌配子体的发育过程,采用常规石蜡切片技术对其果实的生长动态进行了研究。结果表明,授粉后60~75 d的蒴果内种子数量迅速增加,到授粉后120 d时种子充满整个蒴果。授粉后40 d的胎座上分化形成多数由1层表皮细胞包被1列细胞的胚珠原基;授粉后60 d时位于胎座指状结构末端处紧靠表皮细胞下方的孢原细胞分化为大孢子母细胞。之后,大孢子母细胞经过减数分裂和有丝分裂最终形成成熟胚囊;授粉后135 d胚囊发育成熟,附着在胎座上的种子个体分化明显。小叶兜兰胚囊的发育类型为双孢子葱型,胚珠为倒生胚珠,薄珠心,单珠被,成熟胚囊为8核。这为小叶兜兰的生殖生物学及繁殖体系的建立提供理论依据。     

延龄草(Trillium tschonoskii Maxim.)的胚胎学研究初报Ⅰ.——大孢子的发生及雌配子体的形成

本文描述延龄草(Trillium tschonoskii Maxim.)的大孢子发生,雌配子体的形成和雄配子体的形态。胚珠为倒生型,双珠被,厚珠心型。胎座为侧膜胎座向中轴胎座的过渡类型,胶囊发育为葱型的变异型。孢原细胞直接发生于幼胚珠的珠心表皮细胞之下,孢原细胞平周分裂,形成初生周缘细胞及初生造孢细胞。初生周缘细胞分裂先于初生造孢细胞,分裂结果与珠心表皮细胞共同形成了珠心组织。初生造孢细胞进一步发育,形成大孢子母细胞。大孢子母细胞经减数第一次分裂后,即出现壁,形成二分体。一般是珠孔端二分体细胞小于合点端二分体细胞,但偶尔也见到前者大于后者的情况。在二分体形成后珠孔端二分体细胞立即退化、或经减数第二次分裂后再退化(该次分裂多为斜向的)。合点端二分体细胞发育,经二核胚囊,四核胚囊,六核胚囊阶段至成熟胚囊。一般在珠孔端的周围淀粉粒丰富,并先于合点端的核进行分裂。珠孔端由二个助细胞,一个卵细胞构成卵器,助细胞具钩突,并具丝状器,两个极核。合点端常见多核仁的大核,成熟胚囊未见八核。成熟花粉粒为二细胞的,花药壁具变形绒毡层,花粉中充满淀粉粒。沼生目型胚乳。     

花叶开唇兰（兰科）大小孢子发生和雌雄配子体发育

花叶开唇兰的胚珠倒生,双珠被,薄珠心．雌配子体发育属蓼型,成熟胚囊７细胞．大小孢子发生过程中壁上都有胼胝质出现．小孢子四分体为四面体形,左右对称形,交叉形,Ｔ形,它们聚集成花粉小块．花粉散出时为２细胞型．药室壁４层,绒毡层底分泌型．     

兜兰胚胎学的研究

云南兜兰花药壁有五层细胞,绒毡层细胞具双核,属分泌型。小孢子母细胞减数分裂为同时型。四分体中四个小孢子呈四面体或左右对称式排列。成熟花粉为二细胞型。单粒分散的花粉包裹于黄色粘性物质中。生殖细胞最初形成的壁为胼胝质的,待游离到营养细胞质中时,具一层很薄的 PAS 正反应的壁,直到花药开裂时这层壁仍存在。成熟花粉无特化的萌发孔,只具薄壁区。胚珠为薄珠心,具一层珠被,胚囊发育为葱型,成熟胚囊为6—8核,胚发育过程中,具2—4细胞胚柄。胚乳具二核。种子成熟时胚柄及胚乳核都消失。成熟种子只具单层细胞的种皮和一个未分化的球形胚。     

车桑子大孢子发生与雌配子体发育

采用常规石蜡切片法,对车桑子大孢子的发生和雌配子体的发育进行观察,探讨车桑子自然结籽率低的原因和明确其胚胎发育特征。结果表明:(1)车桑子花柱有花柱道,子房3室,中轴胎座,横生胚珠,每心室两枚胚珠,双珠被,厚珠心,无承珠盘。(2)位于珠心表皮细胞下的孢原细胞经平周分裂产生造孢细胞,造孢细胞发育为大孢子母细胞,大孢子母细胞经减数分裂形成线性四分体,靠近珠孔端3个大孢子退化消失,靠合点端大孢子发育为功能大孢子,大孢子发生类型为单孢子发生型。(3)单核胚囊经3次有丝分裂形成7细胞8核的成熟胚囊,胚囊发育类型为蓼型。(4)花器官形态的变化和大孢子发育过程有一定联系,可根据雌花形态特征大致判断大孢子发育时期。研究认为,车桑子雌配子体发育过程中出现的胚囊不中空、游离核不进一步细胞化等异常现象,可能是导致车桑子自然结籽率低的原因之一。     

四倍体双穗雀稗兼性无孢子生殖的研究

研究了四倍体双穗雀稗(Paspalum distichum L)无孢子生殖胚囊、胚胎发育以及假受精特点。当其大孢子母细胞发育至四分体阶段时,大多数情况下会发生四分体退化,同时有多个特化珠心细胞发育为1—3个无孢子生殖胚囊的现象。成熟无孢子生殖胚囊一般3核,包括1个卵细胞和2个极核。卵细胞在抽穗前就能自发分裂形成原胚团,而极核则在抽穗和传粉后参与假受精形成胚乳。当胚珠内存在多个无孢子生殖胚囊时,只是靠近珠孔端的1个无孢子生殖胚囊内的极核与精核结合,而其它的并不参与。种子成熟后出现很低频率的二胚苗。此外,还能观察到少量的有性生殖胚囊的发育以及有性生殖胚囊和无孢子生殖胚囊在同一胚珠中的发育现象,因此判断该类群为兼性无孢子生殖体。     

白桦雌花发育、大孢子发生及胚胎发育的解剖学观察

白桦雌花从开花到雌性器官的成熟需经历1个月左右的时间,解剖学观察表明：四月下旬越冬的雌蕊原基开始了活跃的分裂和分化。子房和柱头开始生长。四月末开花,五月初授粉。此后胚珠开始长大。五月中旬即分化形成珠被,珠心,珠被为单层珠被,胚珠为厚珠心胚珠,胚珠倒生,五月中下旬,珠心内产生大孢子母细胞,一周左右发育为成熟胚囊-七细胞八核胚囊,五月末完成双受精,白桦胚胎发育经过合子,原胚,球形胚,心形胚和鱼雷形胚等时期最后发育成熟,胚乳发育与胚胎同步,即受精的极核进行几次分裂后形成核型胚乳,胚乳核不断增多,在形成心形胚后胚乳细胞形成细胞壁。     

Protoplast Culture and Plant Regeneration of Malus pumila

Calli were induced and suspension cell lines were set up from ovule of Malus pumila Mill. Protoplasts (5.40 × 106/g fr. wt) were isolated from suspension cell lines in enzyme mixture solution containing 2.0% Onozuka R-10, 0.5% pectinase, 0. 65 mol/L mannital, 0.01 mol/L CaC12, 0.7 mmol/L KH2 PO4, 0.3% dextran sulfate potassium salt, at pH 5.8 for 6 h at 26℃. The cell clumps were formed from protoplasts cultured in modified MS, K8p, D2 media. Calli were formed on MS solid medium containing 2.0 mg/L IAA, 2.0 mg/L NAA, 0.1 mg/L BA. Shoots were differentiated on differentiated medium after several changes of the medium. Eventually, shoots rooted and developed into whole plantlets on a rooting medium.     

Micropropagation of sweet orange, Citrus sinensis Osbeck. for the development of nucellar seedlings

Protocol for micropropagation of elite plants of sweet orange (Citrus sinensis) through nucellar embryo culture has been standardized. Three to four nucellar embryos and a zygotic embryo could be excised from a single mature seed and successfully generated as healthy plants in basal MS medium. MS medium supplemented with NAA (1 mg/L) or 2, 4.D (1 mg/L) promoted callus development in both nucellar and zygotic embryos. GA3 (1 mg/L) enriched medium induced plantlets initiation but their growth was very poor. No significant differences were observed between initial growth patterns of nucellar and zygotic seedlings developing from the same ovule. Five to six shoots were obtained from collar region of both category of embryos in MS medium supplemented with BAP (1 mg/L) within 60 days of inoculation. The number of plantlets were almost doubled after their transfer in the same medium and culture for another 30 days. Higher doses of BAP resulted in initiation of callus directly from the embryos. The regenerated shoots (2-3 cm) could be rooted in MS medium supplemented with either only NAA (0.75 mg/L) or NAA (0.50 mg/L) and IBA (2.0 mg/L). A number of plantlets could be obtained from a nucellar embryo grown shoot within a limited time period.     

Cytological Observation on Megasporogenesis and Embryo Sac Development of Regenerated Ovule in Hyacinth

The morphogenesis of regenerated ovule and cytological changes of its megasporogenesis and embryo sac development were studied. Results showed as follows: 1. the differentiation of the regenerated ovule had followed a normal process in the order of inner integument , outer integument and then funiculus. But the form of the regenerated ovules in vitro was quite different from that of ovule in vivo. Most of the regenerated ovules were orthotropous and hemianatropous , only a few were anatropous which are the same with that in vivo. 2. the megasporogenesis and the embryo sac development also had normal cytological process ,and the Polygonum type-embryo sac consisted of one egg, two synergids , one central cell and three antipodals could be seen in mature regenerated ovule. These ex-perimental results make clear that the regenerated ovule differentiated directly from explant could accomplish the complex processes of megasporogenesis and embryo sac development. By this fact ,authors infer that once the differentiation of ovule primordium, the complex biochemical programs for the megasorogenesis and embryo sac development can be controlled by the ovule itself and need no more information from flower bud and /or plant.     

无核白葡萄胚挽救育种技术研究

无核白葡萄在授粉后20－50d,将胚珠接种在含不同激素的Nitsch培养基上,培养80－90d后转入胚荫发培养基中,待胚萌发20d左右,再转入成苗培养基中使其发育成正常幼苗。结果表明,胚萌发适宜的培养基是附加0．5mg/L IAA,1.5mg/L BA和0.5mg/LGA3的Nitsh培养基,在所试10个接种时期中,无授粉后39d胚的发育率最高。     

山茱英的组织培养与植株再生

目的：建立山茱萸的组织培养及植株再生体系。方法：分别以山茱萸的叶片、花柄和花托为材料,进行山茱萸不同外植体的离体培养研究,筛选最佳培养基组成。结果：适宜山茱萸叶片愈伤组织诱导的培养基组合为1／2MS,附加BA2．0mg/L、IBA0,5—1．0mg／L;适宜山茱萸花柄、花托愈伤组织诱导的培养基组合为1／2MS,附加BA1．0mg／L、2,4-D0．5mg／L;在1／2MS附加BA2．0mg／L、IBA0．05mg／L的培养基上,可诱导不定芽的产生;1／2MS附加IBA2．0mg／L的培养基有利于山茱萸试管苗生根。讨论：山茱萸的花托是进行组织培养的最适外植体,白色或翠绿色、结构致密的愈伤组织较易分化产生不定芽。     

Guidance in vitro of the pollen tube to the naked embryo sac of torenia fournieri

The precise guidance of the pollen tube to the embryo sac is critical to the successful sexual reproduction of flowering plants. We demonstrate here the guidance of the pollen tube to the embryo sac in vitro by using the naked embryo sac of Torenia fournieri, which protrudes from the micropyle of the ovule. We developed a medium for culture of both the ovule and the pollen tube of T. fournieri and cocultivated them in a thin layer of solid medium. Although pollen tubes that had germinated in vitro passed naked embryo sacs, some pollen tubes that grew semi-in vitro through a cut style arrived precisely at the site of entry into the embryo sac, namely, the filiform apparatus of the synergids. When pollen tubes were unable to enter the embryo sac, they continuously grew toward the same filiform apparatus, forming narrow coils. Pollen tubes selectively arrived at complete, unfertilized embryo sacs but did not arrive at those of heat-treated ovules or those with disrupted synergids. These results convincingly demonstrate that pollen tubes are specifically attracted to the region of the filiform apparatus of living synergids in vitro.     

红花胚珠和雌配子体发育

用石蜡切片法研究了红花的大孢子发生和雌配子体发育过程,得到以下结果：（１）胚珠发育为薄珠心类型,倒生胚珠,具单珠被。（２）胚囊发育蓼型。（３）有珠被绒毛层,珠被绒毡层起始于大孢子母细胞时期,单核胚囊阶段高度发育,受精后从合点端逐渐退化。珠孔塞细胞呈毛状。     

The effect of medium composition on ovary-slice culture and ovule culture in intraspecific Tulipa gesneriana crosses

The effect of several media components on the germination percentage of ovules in intraspecific T. gesneriana L. crosses was studied by using two embryo rescue techniques, viz. ovary-slice culture followed by ovule culture and direct ovule culture. The addition of 9% sucrose to medium for ovary-slice culture, started at 3 or at 5 weeks after pollination (WAP), significantly improved the germination percentage as compared to 5% sucrose. The germination percentage did not differ between both sucrose concentrations (3% and 5%) used in ovule culture started 4 weeks later with ovules excised from the ovary-slices (at 9 WAP). Similar germination percentages were obtained with media containing the full or half of the concentrations of micronutrients and macronutrients of the MS-medium during ovary-slice culture and ovule culture. For direct ovule culture, started at 4, at 6, and at 8 WAP, the germination percentages did not differ between ovules cultured on media with 3%, 6% or 9% sucrose. The addition of the cytokinin BAP (0.01 or 0.1 mg l^-1) had no effect on the germination percentage. The use of liquid-shaken culture resulted in germination percentages which were similar to those on agar-solidified media. Analysis of the carbohydrate concentration of the media revealed that, in both media for ovary-slice culture and for ovule culture, ultimately all sucrose is converted into glucose and fructose. The total concentration of carbohydrates decreased with 19%–48% in the media for ovary-slice culture, whereas the total concentration of carbohydrates did not decrease remarkably in media for ovule culture.