Cortical reaction and solicitation mechanism in Hemibarbus labeo ovum

There are 1 to 4 rows and five types of cortical alveoli in the cortex of the pallas (Hemibarbus labeo) egg. From the outer to the inner of the cortex, the diameter of the cortical alveoli decreases gradually. We found a new structure named solicitation speckle at the low latitude of the animal pole and near the micropylar apparatus between the ovum envelope and cell membrane in the zygote of fish. The solicitation speckle similar to type I cortical alveoli was very purple in H.E. chromosome, and it had no obvious boundary with the ovum envelope and membrane. Moreover, no membrane around the solicitation speckle in TEM was found. In SEM, the solicitation speckle looked flocculent. During cortical reaction, the solicitation speckle played a very important function in arousing cortical reaction. Thirty-five seconds after fertilization, cortical alveoli began to break down near the low latitude of the animal pole. At the same time, the same thing happened near the micropylar apparatus before cortical reaction. Both starting points encountered and healed up at the vestibule of the micropylar apparatus. The cortical reaction that happened near the low latitude of the animal pole was another new pattern. The cortical reaction was divided into four parts that included latent period, developmental period, climactic period and declining period. In the latent period, no cortical alveoli were released. In the developmental period, a few cortical alveoli were released outside the cortex. In the climactic period, several cortical alveoli were inosculated into a big vesicle and released intensely. In the declining period, the type V cortical alveoli and the other remnant cortical alveoli were released. Five minutes after fertilization, cortical alveoli were released entirely in the animal pole. Five minutes after fertilization, all of the remnant cortical alveoli were released. This leads us to conclude that cortical reaction is induced by type I cortical alveoli, and the solicitation speckle is a volcanic chain reaction under water or the other lower osmotic pressure of fluids. The outer cortical reaction can accelerate the inner cortical reaction. While cortical alveoli releases in batches, the cell plasma membrane is reorganized over and over. No cortical alveoli were found below the micropylar tube where sperm enters the ovum, which suggests that the cortical reaction prevents polyspermy. __________ Translated from Acta Hydrobiological Sinica, 2005, 29(5): 479–487 [译自: 水生生物学报, 2005, 29(5): 479–487]     

唇(鱼骨)受精卵的皮层反应及其引发机制

唇[鱼骨]皮层小泡1-4层,在光镜和透射电镜下均具5种形态,由外及内,小泡内颗粒直径逐渐减少。在H．E染色中,动物极低纬度区和精孔器附近的卵膜和质膜之间,具少量均匀的着色非常深的紫色斑点,与Ⅰ型皮层小泡内容物形态结构相似,在透射电镜下,这些斑点和卵膜、质膜有明显的界限,其外没有包被膜相结构,我们称之皮层反应引发斑,这是在鱼类受精卵中发现的一个新的结构。扫描电镜下,引发斑成絮状。引发斑对皮层反应的引发具有重要作用。皮层反应可分为潜伏期、始发期、高潮期、衰退期四个时期,潜伏期没有皮层反应发生,始发期只是位于受精卵外围的少量皮层小泡释放,高潮期为多个皮层小泡相互融合形成一个大的泡状体,泡状体再与质膜接触、融合后,随后破裂,释放内容物,可分为两个阶段,衰退期释放Ⅴ型皮层小泡和其他残存的皮层小泡以及未完全降解卵黄颗粒碎屑;皮层反应是由Ⅰ型皮层小泡和引发斑诱导的爆发性的链式反应,卵子外侧的皮层反应可以诱导内侧皮层反应。皮层反应有两个起始区域,在受精后35s开始于动物极低纬度区,稍后出现在精孔器前庭附近,随后在这两个始发区向四周扩散,并在前庭以外的区域愈合、打通。皮层小泡分批多次释放,质膜多次重组。精子人卵位点附近没有皮层小泡,不发生皮层反应,这提示皮层反应对鱼类多精受精的抑制效应有限。     

唇受精卵的皮层反应及其引发机制

唇皮层小泡1-4层,在光镜和透射电镜下均具5种形态,由外及内,小泡内颗粒直径逐渐减少。在H．E染 色中,动物极低纬度区和精孔器附近的卵膜和质膜之间,具少量均匀的着色非常深的紫色斑点,与Ⅰ型皮层小泡内 容物形态结构相似,在透射电镜下,这些斑点和卵膜、质膜有明显的界限,其外没有包被膜相结构,我们称之皮层反 应引发斑,这是在鱼类受精卵中发现的一个新的结构。扫描电镜下,引发斑成絮状。引发斑对皮层反应的引发具 有重要作用。皮层反应可分为潜伏期、始发期、高潮期、衰退期四个时期,潜伏期没有皮层反应发生,始发期只是位 于受精卵外围的少量皮层小泡释放,高潮期为多个皮层小泡相互融合形成一个大的泡状体,泡状体再与质膜接触、 融合后,随后破裂,释放内容物,可分为两个阶段,衰退期释放Ⅴ型皮层小泡和其他残存的皮层小泡以及未完全降 解卵黄颗粒碎屑;皮层反应是由Ⅰ型皮层小泡和引发斑诱导的爆发性的链式反应,卵子外侧的皮层反应可以诱导 内侧皮层反应。皮层反应有两个起始区域,在受精后35s开始于动物极低纬度区,稍后出现在精孔器前庭附近,随 后在这两个始发区向四周扩散,并在前庭以外的区域愈合、打通。皮层小泡分批多次释放,质膜多次重组。精子入 卵位点附近没有皮层小泡,不发生皮层反应,这提示皮层反应对鱼类多精受精的抑制效应有限。     

乌苏里江唇(鱼骨)的鳞片和生长特征

依据238尾鱼的测量数值,研究了乌苏里江野生唇钱(鱼骨)(Hemibarbus labeo)的鳞片及生长特征,并调查了乌苏里江抓吉镇江段唇(鱼骨)的捕捞资源情况.结果表明,唇(鱼骨)的鳞片较大,为规则圆鳞,年轮特征清晰,易于分辨,鳞径(R鳞径)与生长时间(年龄t)的回归方程为R鳞径=0.858 3t 2.275(=238,r=0.986 8),体长与鳞径的回归方程为L=4.332 6R鳞径 0.029 3(n=238,r=0.990 3).乌苏里江唇(鱼骨)体重与体长的回归方程为W=0.011 5L3.0868(N=238,r=0.996 2),其生长特征适合Von Bertalanffy生长方程,体重的生长拐点t=4.59龄,W=340.90 g.在乌苏里江抓吉镇江段主要捕捞唇(鱼骨)的时间从每年开冰期4月20日到封冰期11月15日左右,其捕捞量随季节的变化而不同,4～5月、10～11月数量最多,为100～150 kg/d,6～7月为50～100 kg/d,8～9月较少,为30～40 kg/d.     

花和唇的含肉率及肌肉营养成分分析

利用国内外通用的营养测试方法测定了花(Hemibarbus maculates)和唇(Hemibarbu labeo)的含肉率和肌肉营养成分。结果表明:花和唇含肉率分别是70.61%7、1.52%;花肌肉(鲜样)中蛋白质(18.41%)和脂肪含量(2.46%)显著高于唇的,而花的灰分含量要显著低于唇;水分含量分别是78.35%、78.51%,两者无显著差异。花和唇肌肉中脂肪酸种类丰富,饱和脂肪酸(SFA)4种,不饱和脂肪酸(UFA)7种;其中单不饱和脂肪酸(MUFA)4种,多不饱和脂肪酸(PUFA)3种;其中DHA含量高达5.00%和14.32%。花和唇肌肉中的氨基酸总量分别是63.07%和67.63%,呈味氨基酸分别为25.96%和26.30%。缬氨酸、蛋氨酸和胱氨酸为限制性氨基酸。     

基于COI和ND5序列的中国南部唇鱼骨和间鱼骨群体遗传结构

唇鱼骨和间鱼骨均为分布较广的初级淡水鱼类,是理想的亲缘地理研究材料;且两者形态特征较为相似,不易鉴别,故两者的分布记述和物种有效性存在争议.为了解我国南部唇鱼骨和间鱼骨的群体遗传结构并探讨两者的物种有效性,本研究对8条水系的唇鱼骨和9条水系的间鱼骨共130尾个体的COI和ND5基因序列片段进行了测定,并对这两个基因的组合序列(2151 bp)进行了分析.结果表明: 在130尾个体的COI和ND5基因组合序列中,共有196个核苷酸变异位点,共检测出50个单倍型,单倍型多样性为0.964,核苷酸多样性为0.019,遗传多样性较高.基于COI和ND5基因组合序列构建的 NJ 树显示,所有种群可分为两支,支系Ⅰ包含了韩江和九龙江的全部单倍型以及瓯江的部分单倍型,余下的单倍型组成了支系Ⅱ.两支系间的遗传距离为0.036,而唇鱼骨与间鱼骨之间的遗传距离为0.027.单倍型网络图表明,韩江、九龙江种群和其他水系种群分化较大;漠阳江种群由海南岛种群扩散而来;海南岛各种群及漠阳江种群的单倍型分支与珠江水系单倍型的分支之间的亲缘关系较近,与长江水系单倍型分支之间的亲缘关系则较远;湘江、桂江和柳江之间的亲缘关系较近.AMOVA分析结果显示,地理区之间的变异约占71.2%,地理区内种群间变异约占16.6%,种群内的变异占12.2%,表明其遗传分化主要来自地理区之间.错配分析及中性检验结果显示,全部种群、唇鱼骨种群、间鱼骨种群、支系Ⅰ和支系Ⅱ在历史上均没有发生过明显的扩张.     

唇鱼骨受精的细胞学研究

唇精孔器属深凹陷、短孔径型。精子在受精后2s到达精孔管、5s进入卵子。受精后8—15min,卵子进入第二次减数分裂后期。受精后10min,开始形成雄性原核。受精后20min,进入第二次减数分裂末期。受精后25min,雌性原核形成。受精后30—35min,雌性原核向雄性原核移动。受精后40min,雌雄原核接近。受精后50min,雌雄原核结合。受精后70min,受精卵进入第一次有丝分裂中期,受精后80min,进入第一次有丝分裂后期,受精后120min,进入末期。卵黄降解与其内部或外周小泡的泡状缺口紧密相关。雌雄原核结合是精子星光扩张、牵引和细胞质流动的共同结果。有多精入卵的现象。     

唇精子早期入卵观察

用扫描电镜对唇成熟卵子及早期精子入卵过程进行观察.结果 显示,唇成熟卵子在动物极中央有一深凹陷的表面光滑的精孔器,其外径2.512 μm,内径2.330 μm,精子直径1.567 μm.混匀的精卵刚遇水时,没有精子进入精孔器.受精后1 s,精孔器内出现精子.受精后5 s,组织切片显示,精子已经进入卵子内,并形成具有强烈抑制多精入卵作用的受精锥.受精后10 s,精子在精孔器前庭集结,尚未形成受精塞.受精后20 s,在精孔器内形成受精塞.受精塞没有阻塞精孔管,经分析它不是来源于皮层反应产物.受精塞形成后,可以吸附入卵的精子,这对多精入卵有积极的抑制作用;精子尾部在入卵过程中相互缠绕,这也是减少多精入卵的重要机制.受精后30 s, 受精塞和吸附的精子向精孔器外移动.受精后50 s, 受精塞和吸附的精子堵塞精孔器.受精后60 s, 受精塞吸附的精子开始解体,但是由于精孔管未封闭,还有精子通过精孔管进入到质膜.在人工受精过程中,卵子的单精受精屏障会因其周围精子密度大、精子与卵子距离短、精子运动速度快而被打破,从而导致这些卵子出现多精入卵的现象.受精后80 s, 精孔管仍然没有封闭,精孔器附近的精子明显出现活动能力的差异:精孔器外面的精子活动能力最强,精孔管旁边的精子活动能力较弱;精孔管外堆积的精子活性消失,受精塞吸附的精子已开始解体,经初步分析,这可能是进入其内的精子耗能有所差异的结果.受精后100 s,受精塞吸附的精子解体.     

Sperm penetration in vitro into ovarian and tubal oocytes from mice of the inbred KE and C57 strains

The method of in vitro fertilization was applied to test a previous suggestion that the lowered fertilizability of the tubal oocytes of female KE strain mice and the high resistance of their zona pellucida to proteolytic enzymes, are due to the premature cortical reaction taking place near the time of ovulation. Therefore higher fertilizability of ovarian oocytes is expected. The effectiveness of F₁ hybrid sperm penetration into ovarian and tubal KE oocytes confirmed these assumptions. The ovarian KE oocytes recovered 9–10 hours after administration of human chorionic gonadotropin (HCG) showed significantly higher penetrability (70–83%) than did the tubal oocytes recovered 12 hours after HCG (about 50%) and 14–16 hours after HCG (20%). Similar results were obtained with C57 oocytes. Sperm penetration into ovarian oocytes (10 hours after HCG) was much more effective (67%) than into tubal oocytes (18%); this finding correlated with more rapid zona dissolution by chymotrypsin. On the basis of these results one might speculate that premature cortical reaction takes place also in the C57 strain.     

Cortical modifications in Paracentrotus lividus eggs after ammonia activation

We have shown by electron microscopy that ammonia activation of Paracentrotus lividus eggs alters the inner ultrastructure of cortical granules. If activated eggs are inseminated, they fail to undergo a typical cortical reaction.     

Fertilization in a crab. II. Cytological aspects of the cortical reaction and fertilization envelope elaboration

At fertilization, the egg of Carcinus maenas undergoes cortical vesicle exocytosis, in response to the first contacts between the spermatozoon and the egg plasma membrane. This process was observed in vitro and may be connected with a cortical reaction. Carcinus maenas eggs display two populations of cortical vesicles which, during the reaction, successively release two different exudates: a fine granular material and a mass of ring-shaped granules. During the first steps of exocytosis, the two superimposed vitelline envelopes are detached from the egg surface, and the inner one gradually changes. Thus a new coating, derived from the coalescence of the secreted ring-shaped granules, is progressively elaborated under the vitelline envelopes. These events occur over a 7–8 hr period. The morphological uniqueness of the cortical vesicle exudates and the complexity of the related events are discussed in terms of the cortical reaction and of the formation of the fertilization envelope in Carcinus maenas.     

Fertilization in a Crab. III. Cytodifferentiation of vesicles enclosing ring-shaped elements involved in the cortical reaction

During the cortical reaction, Carcinus maenas eggs successively released a fine granular material and a massive amount of ring-shaped elements that subsequently formed most of the fertilization envelope. The ring-shaped elements came from egg cortical vesicles and, owing to their striking morphology, acted as naturally occurring markers in ultrathin sections, which permitted us to understand the pathway of their intracellular transport. In this respect it was established that the ring-shaped elements and their enclosing vesicles originated in the endoplasmic reticulum both in ripe oocytes and early fertilized eggs maintained under in vitro conditions. The intracellular transport pathway of the endoplasmic reticulum-derived vesicles seemed to bypass the Golgi apparatus. Accordingly, the ring-shaped elements appeared to be released by direct exocytosis from the endoplasmic reticulum system. Finally, a tentative scheme of oocytes functioning is suggested for crustacean decapods, based on the remarkable similarities between the structure and ER origin of the ring-shaped elements involved in the cortical reaction and the disc-shaped granules traditionally considered as endogenous yolk precursors. The scheme implies that the oocyte ER system might produce a precursor common to the cortical reaction exudate and to the endogenous yolk, in the form of the ring- or disc-shaped elements.     

Absence of furrowing activity following regional cortical tension reduction in sand dollar blastomere and fertilized egg fragment surfaces

The purpose of the present investigation was to test experimentally the possibility that division mechanism establishment at the equator of sand dollar eggs may be a consequence of cortical tension gradients between the equator and the poles. Cytochalasin has been shown to decrease tension at the sea urchin egg surface. The concave ends of cytochalasin D-containing agarose cylinders were held against regions of the surface of Echinarachnius parma blastomeres and enucleated fertilized egg fragments. The ability to interfere with normal furrowing activity was used as a biological indicator of the effectiveness of cytochalasin. When agarose containing 2 microg/mL cytochalasin contacted the equatorial region of the blastomeres resulting from the first cleavage, or the equatorial surfaces of nucleated fertilized egg halves, furrowing was blocked, stalled or delayed, indicating that the concentration of cytochalasin was effective. When the same concentration of cytochalasin was applied to the poles, the cells and nucleated fertilized egg fragments divided in the same way as the controls, indicating that the effectiveness of the cytochalasin did not spread from the poles to the equator and that bisection did not interfere with the division of nucleated fertilized egg fragments. When the same concentration of cytochalasin was applied to diametrically opposed surfaces of enucleated, spherical egg fragments, there was no evidence of furrowing activity between the areas that contacted the cytochalasin or in any other part of the surface. Because of the tension-reducing effect of cytochalasin, a tension gradient existed between the regions affected and unaffected by cytochalasin. The results strongly suggest that establishment of the division mechanism by simple gradients of tension at the surface is unlikely.     

A complex cortical reaction leads to formation of the fertilization envelope in the lobster,Homarus

We have examined the formation of the fertilization envelope in the lobsters Homarus americanus and H gammarus. Oocytes were fixed for electron microscopy either in the ovary or following extrusion from the gonopore. Mature ovarian oocytes are surrounded by a coat (envelope 1), which is comprised of small electron-dense granules and structures resembling “bottlebrushes.” At least part of this coat is synthesized by the follicle cells of the ovary. The cortex of ovarian oocytes contains four types of vesicles that we refer to as high-density vesicles (HDV), low-density vesicles (LDV), moderately dense vesicles (MDV), and ring vesicles (RV). Oocytes that were electrically extruded from the gonopore and fixed immediately had an envelope identical to that of ovarian oocytes. The cortex of gonopore oocytes contained the four types of vesicles found in ovarian oocytes. When unfertilized gonopore oocytes were allowed to incubate in sea water, the oocyte cortex appeared unaltered, but envelope 1 swelled and the bottlebrushes dispersed. When recently fertilized oocytes were fixed during natural spawning or following in-vitro fertilization, each type of vesicle was released in sequence from the cortex of the oocyte. The contents of the HDV and LDV appeared first in the perivitelline space, but their fate could not be determined at later times. The ring-shaped elements of the RV and the moderately electron-dense material of the MDV were released exocytotically somewhat later; these materials coalesced in the perivitelline space to form a new coat (envelope 2). Envelope 1 subsequently condensed to its original thickness and appeared firmly attached to envelope 2. Our results show that the fertilized lobster egg is surrounded by two discrete coats. The outer coat, which is formed in the ovary, undergoes a swelling/condensation cycle at spawning. The inner coat originates from a complex cortical reaction. Together these coats comprise the fertilization envelope of the lobster egg.     

Identification of cystatin as a component of carp chorion

An ovary-specific cystatin is immunocytochemically demonstrated to be localized in the chorions, cortical granules, and yolk granules of carp oocytes, as well as in the follicle cells surrounding oocytes. During cortical reaction, cystatin is exocytosed from cortical granules into the perivitelline space. In situ hybridization confirms that cystatin is synthesized by oocytes and follicle cells. Western blotting reveals that chorion cystatin appears in multiple bands of high molecular weight (from 65 kDa to larger than 200 kDa). No cystatin monomer of 14 kDa is found. These results indicate that chorion cystatin is conjugated with other chorion components. Two forms of conjugates are found. In one form, cystatin, ZP2, fibroin-like substance (FLS), and cathepsin-like substance (CLS) are conjugated, which is extracted by sodium dodecyl sulfate. In the other form, cystatin, FLS, and CLS are conjugated, which is extracted by guanidine thiocyanate (GTC). Most chorion cystatin of oocytes and ovulated eggs is solubilized by GTC, while a large amount of cystatin remains in the fertilization envelope of cortical reacted eggs after extraction by GTC. Mol. Reprod. Dev. 51:430–435, 1998. © 1998 Wiley-Liss, Inc.