两种发育型鱼类卵母细胞成熟过程中促精核发育现象的研究

采用实验细胞学技术,比较研究了红鲤精核在雌核发育鱼类(银鲫)和两性融合发育鱼类(红鲤、彩鲫)卵母细胞成熟各阶段中的发育状况,结果表明:在两性融合发育鱼类中,当卵母细胞发育到胚泡破裂期吋,精核开始解凝发育,及至第一次成熟分裂中期后阶段,高度解凝的精核才开始原核化,相应地,在雌核发育银鲫中,精核也只有在与胚泡物质接触后,才能开始解凝,并且在三极纺锤体形成后期初步原核化,但与两性融合发育鱼类相比,精核的原核化程度明显降低。这些实验结果初步揭示,在两性融合和雌核发育鱼类卵中均可产生促精核解凝和原核化的两类因子(SNDFs和SPDFs),其中SNDFs的活性表达起始于卵母细胞胚泡破裂时期,而SPDFs活性则产生于第一次成熟分裂中期后或三极纺锤体形成后阶段,并且两性融合发育鱼类卵中的SPDFs活性远远高于雌核发育鱼类卵母细胞。     

银鲫精子在两性融合生殖鱼类卵质中的受精特征

红鲤(♀)×银鲫(♂)的杂种胚胎均不能成活。受精细胞学研究结果表明,雌核发育银鲫的精核在两性融合生殖的鲤鱼卵质中能转化为雄性原核,并和雌性原核融合成合子核。但在卵裂开始后,可观察到某些异常现象,如染色体丢失,多极纺锤体形成,以及第二次卵裂时受精卵的两分裂球的非同步性分裂等。我们初步认为,雌核发育银鲫的染色体和两性融合生殖的鱼类染色体之间存在某种不相容性,表现为彼此间的互相排斥。出现这种现象可能和银鲫染色体组的雌核发育遗传背景有关。     

蓖麻蚕卵受精的研究

我们从细胞形态上的研究, 证明:蓖麻蚕卵在成熟期分裂的中期(同一横剖面), 基组数染色体是14;分作两圈, 内层4个, 外层10个。成熟卵停止在第一次中期分裂, 纺锤体与卵膜垂直, 待精子入卵后继续向前分裂, 并发现有染色质消散的现象。第二次成熟期分裂结果获得3个极体和1个雌性原核。正常的卵平均能接受2-3条精子, 它们入卵后起收缩、囊化成雄性原核;其中一个与雌性原核合并为“双组核”。剩余的过数精核分裂缓慢, 终于中心体离纺锤体作异形的分裂。     

银鲫雌核发育的细胞学观察

在受精卵内,精子核呈凝缩状态,不形成雄性原核,没有看到两性原核融合。在刚产出的成熟卵子中没有看到极体,直到受精后10分钟(在水温19°—21℃)才有唯一的一个极体排出。在同一尾银鲫产出的同批卵子中,绝大多数具有成熟分裂中期的卵核,并在精子入卵后继续进行发育(雌核发育),接着排出唯一的一个极体;授精7分钟的少数卵子具有三极纺锤体状的核。根据现在的观察,双凤水库的银鲫是以雌核发育方式繁殖的种群。       

复合四倍体异育银鲫两种不同生殖方式的细胞学观察

在复合四倍体异育银鲫（）×银鲫（）的受精过程中,精子入卵后经过解凝、核化,最终形成雄性原核,并可与卵子的雌性原核融合,证明了复合四倍体异育银鲫卵子具有与两性融合生殖极为相似的拟两性融合生殖的能力;而在复合四倍体异育银鲫（）×兴国红鲤（）的组合中,精子入卵后以固缩状态存在,又表现出典型的雌核发育型生殖行为。因此我们认为复合四倍体异育银鲫具有两种不同的生殖发育机制。此外,我们还观察到在第一次有丝分裂中期有核物质被排斥到纺锤体之外的现象。本文就复合四倍体异育银鲫生殖发育的机制进行了初步的探讨。     

鲫鲤杂种一代(F_1)自交二代(F_2)的受精细胞学研究

荷包红鲫 (♀ )×湘江野鲤 (♂ )杂交产生的杂种一代 ( F1)成熟卵的直径为1 .0～ 1 .2 5mm;为单受精孔卵 ,一般只允许单个精子入卵 ;成熟卵在受精前处于第二次减数分裂中期 ;鲫鲤杂种一代的雄性部分可育 ,能产生正常的精子 ;杂种一代的受精方式为单精受精 ,具有正常的受精细胞学程序 .受精 30 s后 ,精子通过受精孔进入卵质 ;5min后 ,精子产生明显星光 ;1 5min后 ,精子头部膨大核化 ,最后形成雄性原核 ,与此同时 ,雌性原核也开始形成 ;2 5min后 ,雌、雄原核向胚盘中央靠近 ,然后彼此接触 ,最后融合为合子核 ;40 min后 ,开始第一次卵裂 ,在一个受精卵第一次卵裂中期的切片上看到了一个三极纺锤体 .     

雌核发育银鲫和两性融合彩鲫卵母细胞体外诱导成熟过程中周期蛋白合成和MPF活性变化的比较研究

采用体外诱导卵母细胞成熟技术 ,比较研究了雌核发育银鲫和两性融合发育彩鲫卵母细胞成熟过程中周期蛋白合成和MPF活性变化情况。结果表明 :1 7α ,2 0 β 二氢孕酮(简称DP)浓度为 0 5μg/ml,温度为 2 4℃ ,光照时间 2 0小时为最适诱导条件。在相同条件下 ,两性生殖彩鲫卵母细胞体外诱导成熟速度明显快于银鲫。相应的细胞学研究表明 ,在体外诱导时 ,银鲫和彩鲫卵母细胞的发育成熟是正常的。银鲫卵母细胞生发泡破裂 (GVBD)时已有周期蛋白的合成 ,但生发泡破裂开始后则呈现合成速度下降直至没有合成的现象。尽管如此 ,卵母细胞中MPF活性却仍保持继续增强之势 ,至GVBD达1 0 0 %时 ,活性最强。而在两性融合发育彩鲫卵母细胞成熟过程中 ,周期蛋白的合成呈现出由较多到无 ,再逐渐到多的变化。GVBD开始时 ,周期蛋白合成较多 ,此后则急剧下降至几无周期蛋白的合成 ,以后随着成熟诱导的进行 ,周期蛋白的合成速度又缓慢回升至GVBD开始时的状态。与此相对应 ,MPF活性也出现从较强变无 ,再逐渐增至最强的变迁。这些结果初步揭示 ,鱼类卵母细胞中周期蛋白的合成和MPF活性的出现与卵母细胞的成熟分裂密切相关 ,雌核发育银鲫卵母细胞生发泡破裂开始以后 ,周期蛋白合成的消失可能与其特殊的三极纺锤体形成及其后的动力     

中国对虾受精过程中精卵核的细胞学变化

中国对虾精子以其棘部顶端随机附着在卵上,精子在凝胶膜形成后,第一极体排出前入卵,精子入卵后,絮状的精核经过重建形成雄原核,中国对虾卵子排放时处于第一次成熟分裂的中期,卵子入海水时,纺锤体的长轴与质膜平行,卵子激活后,纺锤体的长轴开始旋转,旋转至纺鲑体长轴与质膜垂直时,由纺锤丝牵引着染色体向两极移动,外侧的染色体由质膜包裹形成第一极体,受膜举起后,由次级卵母细胞排放出第二极体,此后,单倍雌核重建形成雌原核,雄原核形成早于雌原核,雌雄原核于卵子中央联会形成联合核,受精后的50分钟纺锤丝牵关染色体称向两极,质膜内缢断裂形成两个细胞的胚胎。     

文蛤受精及早期胚胎发育过程的细胞学观察

用普通光镜、荧光显微镜技术和石蜡切片技术三种方法,对文蛤卵在受精及早期胚胎发育过程中的外形和核相变化进行了详细观察。结果表明:文蛤成熟未受精卵呈圆球形,直径90.06μm±5.59μm,核相处于第一次成熟分裂中期;精子为鞭毛型,全长48.05μm±1.60μm,头部呈狭茧形,长度为3.06μm±0.17μm;精卵混合后,精子迅速附着于卵子表面,受精后5min-10min,精子进入卵内并明显膨胀,激活卵子启动两次成熟分裂;分别在受精后20min、30min,受精卵完成第一次和第二次成熟分裂,先后排出第一、第二极体;成熟分裂完成之后,精、卵核体积迅速膨胀到最大,核膜重新出现,形成弥散状的雌、雄原核;受精后35min左右,雌、雄原核在卵子中央发生染色体联合,共同排列在纺锤体的赤道板上,形成第一次有丝分裂的中期分裂相;受精后40min-45min,在纺锤丝的牵引下染色体被拉向两极,结果形成2个大小不等的卵裂球;受精后55min-60min,第二次卵裂结束,形成1大3小4个卵裂球,卵裂过程中的核相变化与第一次卵裂基本相同,只是卵裂方向是与第一次卵裂的卵裂沟呈基本垂直的纵裂;受精后80min-90min,第三次卵裂完成,仍为不等全裂,但自此次起开始进行螺旋分裂。此外,实验中也发现了少量的多精入卵、多极分离和天然三倍体等异常现象。     

正常培养条件下绵羊卵母细胞减数分裂从中期Ⅰ至中期Ⅲ的动态变化过程

以绵羊卵母细胞为研究对象,通过免疫组织化学的方法研究其染色体和纺锤体微管及微丝在体外成熟、孤雌激活过程中的动态变化。结果表明:(1)纺锤体的形态由中期的桶形,变成早后期的圆柱形及后期和末期细长而扁平的三角锥形,与椎体底面连接的染色质将来进入极体并最终被排出。(2)染色体形态从中期单个的清晰可见的状态,变为后期和末期凝缩的染色质状态,随后在下一个中期再次呈现出清晰可见的形态。(3)第一次减数分裂中期(MI)纺锤体比第二次减数分裂中期(MII)和第三次减数分裂中期(MIII)大,但MII期纺锤体形态比MI期更接近桶形。(4)几乎所有组成纺锤体的微管和微丝都被分配到极体中。     

Comparative investigation on spindle behavior and MPF activity changes during oocyte maturation between gynogenetic and amphimictic crucian carp

The spindle behavior and MPF activity changes in the progression of oocyte maturation were investigated and compared with cytological observation and kinase assay between gynogenetic silver crucian carp and amphimictic colored crucian carp.MPF activity was measured by using histone H1 as phosphorylation substrate.There were two similar oscillatory MPF kinase activity changes during oocyte maturation in two kinds of fishes with different reproductive modes,but there existed some subtle difference between them.The subtle difference was that the first peak of MPF kinase activity was kept to a longerlasting time in the gynogenetic silver crucian carp than in the amphimictic colored crucian carp.It was suggested that the difference may be related to the spindle behavior changes,such as tripolar spindle formation and spindle rearrangement in the gynogenetic crucian carp.     

A Tripolar Spindle Formed at Meiosis I Assures the Retention of the Original Ploidy in the Gynogenetic Triploid Crucian Carp, Ginbuna Carassius auratus langsdorfii

A triploid crucian carp, ginbuna ( Carassius auratus langsdorfii ), reproduces by gynogenesis, in which sperm of diploid ginbuna or of other species triggers the development of the triploid eggs, but a male genome makes no contribution to the zygotic genome. Gynogenesis is maintained by two mechanisms: exclusion of male genome during fertilization and retention of somatic ploidy levels during oogenesis. We examined the mechanisms responsible for producing unreduced eggs. Microfluorometry with a DNA staining dye showed that DNA content in the ginbuna oocytes was not reduced in half during meiosis I. Cytological observations revealed that a tripolar spindle was formed at meiosis I and the first polar body was not extruded, whereas an ordinary bipolar spindle was formed and the second polar body was extruded at meiosis II. Activity of histone H1 kinase (as an indicator of maturation-promoting factor) decreased transiently between meiosis I and II, strongly suggesting a "normal" meiotic cycle progression in the ginbuna oocytes. These results have indicated that in the gynogenetic ginbuna the somatic ploidy levels are maintained by inhibiting the first polar body extrusion via the formation of the tripolar spindle at meiosis I.     

Continuous exposure to bisphenol A during in vitro follicular development induces meiotic abnormalities

Bisphenol A (BPA), a widely used environmental contaminant, may exert weak estrogenic, anti-androgenic and anti-thyroidic activities. BPA is suspected to possess aneugenic properties that may affect somatic cells and mammalian oocytes. Oocyte growth and maturation depend upon a complex bi-directional signaling between the oocyte and its companion somatic cells. Consequently, disturbances in oocyte maturation may originate either from direct effects of BPA at the level of the oocyte or from indirect influences at the follicular level, such as alterations in hormonal homeostasis. This study aimed to analyze the effects of chronic BPA exposure (3 nM to 30 microM) on follicle-enclosed growth and maturation of mouse oocytes in vitro. Oocytes were cultured and their spindle and chromosomes were stained by alpha-tubulin immunofluorescence and ethidium homodimer-2, respectively. Confocal microscopy was utilized for subsequent analysis. Only follicles that were exposed to 30 microM BPA during follicular development showed a slightly reduced granulosa cell proliferation and a lower total estrogen production, but they still developed and formed antral-like cavities. However, 18% of oocytes were unable to resume meiosis after stimulation of oocyte maturation, and 37% arrested after germinal vesicle breakdown, significantly different from controls (p<0.05). Only 45% of the oocytes extruded a first polar body (p < 0.05). 30 microM BPA led also to a significant increase in meiosis I-arrested oocytes with unaligned chromosomes and spindle aberrations. Oocytes that were able to progress beyond meiosis I, frequently arrested at an abnormal telophase I. Additionally, in many oocytes exposed to low chronic BPA that matured to meiosis II chromosomes failed to congress at the spindle equator. In conclusion, mouse follicle culture reveals non-linear dose-dependent effects of BPA on the meiotic spindle in mouse oocytes when exposure was chronic throughout oocyte growth and maturation.     

银鲫与彩鲫卵母细胞cDNA文库构建及周期蛋白A1的cDNA克隆

分别取行天然雌核发育繁殖的银鲫和两性生殖的彩鲫的卵母细胞为材料,提取总RNA,分离mRNA,进而反转录合成cDNA并定向插入λgtll Sfi-Not克隆载体,经体外包装构建了银鲫与彩鲫卵母细胞的表达型cDNA文库。测试结果表明库容量分别达到3.1×106(银鲫)和1.6×106(彩鲫)。进一步人工合成Cyclin A1保守引物,采用PCR扩增文库的方法,克隆了银鲫(1616bp)与彩鲫(1626bp)的Cyclin A1全长cDNA。序列分析结果表明:两种鱼编码区长度均为1173bp,起始于一个包含在脊椎动物起始密码子ANNATG基元内ATG的单一开放读码框,编码391个氨基酸;5'-端非编码区长度也同为70bp,3-'端非编码区长度略有不同,银鲫为373bp,而彩鲫则为383bp;二者3'-端均带有AATAAA的Poly(A)加尾信号以及24bp(银鲫)和27bp(彩鲫)的Poly(A)尾巴。比较银鲫、彩鲫和金鱼与人、爪蟾Cyclin A1氨基酸序列同源性的结果表明,Cyclin A1在人、爪蟾与鱼类之间具有较高同源性;而在银鲫、彩鲫和金鱼之间,Cyclin A1仅在周期蛋白框外存在5个氨基酸的差异,且这些差异均是由个别碱基的变异造成的。       

人工复合三倍体鲤与亲本相对DNA含量及倍性分析

本文通过显微荧光光度术测量了人工复合三倍体鲤的红细胞及亲本红鲤、红鲫与散鳞镜鲤个体的红细胞和精子的相对DNA含量。结果表明：每一种亲本的精子DNA含量是其红细胞DNA含量的二分之一,人工复合三倍体鲤DNA含量等于三个亲本精子DNA含量之和,为三个亲本血液红细胞DNA含量之和的二分之一。以外周血淋巴细胞制备染色体标本,人工复合三倍体鲤染色体数为150,其亲本红鲤、红鲫和散鳞镜鲤的二倍体染色体数均为100。研究进一步证明人工复合三倍体鲤与二倍体亲本的染色体倍性和相对DNA含量存在着明显的相关性。     

Transformation of sperm nuclei to metaphase chromosomes in the cytoplasm of maturing oocytes of the mouse

Zona-free oocytes of the mouse were inseminated at prometaphase I or metaphase I of meiotic maturation in vitro, and the behavior of the sperm nuclei within the oocyte cytoplasm was examined. If the oocytes were penetrated by up to three sperm, maturation continued during subsequent incubation and became arrested at metaphase II. Meanwhile, each sperm nucleus underwent the following changes. First, the chromatin became slightly dispersed. By 6 h after insemination, this dispersed chromatin had become coalesced into a small mass, from which short chromosomal arms later became projected. Between 12 and 18 h after insemination, each mass of chromatin became resolved into 20 discrete metaphase chromosomes. In contrast, if oocytes were penetrated by four to six sperm, oocyte meiosis was arrested at metaphase I, and each sperm nucleus was transformed into a small mass of chromatin rather than into metaphase chromosomes. If oocytes were penetrated by more than six sperm, the maternal chromosomes became either decondensed or pycnotic, and the sperm nuclei were transformed into larger masses of chromatin. As control experiments, immature and fully mature metaphase II oocytes were inseminated. In the immature oocytes, which were kept immature by exposure to dibutyryl cyclic AMP, no morphological changes in the sperm nucleus were observed. On the other hand, in the fully mature oocytes, which were activated by sperm penetration, the sperm nucleus was transformed into the male pronucleus. Therefore, the cytoplasm of the maturing oocyte develops an activity that can transform the highly condensed chromatin of the sperm into metaphase chromosomes. However, the capacity of an oocyte is limited, such that it can transform a maximum of three sperm nuclei into metaphase chromosomes. Furthermore, the presence of more than six sperm causes a loss of the ability of the oocyte to maintain the maternal chromosomes in a metaphase state.