NF-κB和存活蛋白抑制药物诱导的倍体化与衰老巨核细胞的死亡

目的:筛选诱导巨核细胞倍体化药物,研究倍体化细胞的抗死亡机制,探索促进倍体化细胞死亡的用药方法。方法:采用不同药物处理巨核细胞白血病细胞系Dami细胞,检测细胞倍性、衰老、死亡及相关分子的变化。结果:Nocodazole、SP600125与SU6668可阻断Dami细胞增殖,诱导倍体化,促进细胞衰老,短期诱导不影响细胞活力。分子水平表明,抗凋亡分子存活蛋白表达上调,衰老相关分泌表型调控因子NF-κB(p65)活性降低。持续的药物诱导可致细胞死亡。结论:诱导巨核细胞倍体化抑制恶性增殖,促进细胞衰老发生,存活蛋白与NF-κB(p65)共同抑制倍体化和衰老细胞的死亡,而持续的药物诱导可促进细胞死亡,可作为急性巨核细胞白血病的治疗策略。     

S6K1 C端自抑制假底物结构域磷酸化与Akt去磷酸化协同调节SP600125诱导巨核细胞系多倍体化

目的:探讨JNK抑制剂SP600125诱导巨核细胞白血病系多倍体化的调控机制。方法:用SP600125和3种抑制剂(PD184352、U0126和LY294002)处理Dami和CMK细胞,用点突变技术对核糖体蛋白S6激酶1(S6K1)C端自抑制假底物结构域和疏水基序突变构建的S6K1质粒转染细胞,流式细胞术分析细胞的DNA倍性,Western印迹检测S6K1、MAPK和Akt蛋白的表达及磷酸化修饰位点的变化。结果:当单独使用3种抑制剂时,对Dami和CMK细胞的倍性无影响。当SP600125与3种抑制剂联合时,尽管PD184352下调了p44/42 MAPK在Thr202/Tyr204位点的磷酸化,但其并不抑制SP600125诱导的Dami和CMK细胞的多倍体化;相反,U0126抑制SP600125诱导的Dami和CMK细胞的多倍体化,但并不下调p44/42 MAPK的磷酸化;而LY294002增加Akt的磷酸化,并阻断SP600125诱导的Dami和CMK细胞的多倍体化。这3种抑制剂均在SP600125诱导的多倍体Dami和CMK细胞中部分抑制S6K1的Thr421/Ser424磷酸化,但并不增加S6K1的Thr389磷酸化。转染S6K1突变质粒的Dami细胞,并没有对SP600125诱导的多倍体化产生影响,同时,无论是模拟磷酸化或去磷酸化的Thr389突变均对SP600125诱导的多倍体化无影响,且未显现出与LY294002的协同作用。C端自抑制假底物结构域突变质粒(S6K1-D3E)可以进一步阻断SP600125诱导的已经被LY294002部分阻断的Dami细胞多倍体化。结论:S6K1的C端自抑制假底物结构域磷酸化与Akt去磷酸化协同调节SP600125诱导巨核细胞白血病系的多倍体化。     

用流式细胞仪检测大黄鱼三倍体

通过对大黄鱼二倍体和三倍体的倍性分析,建立流式细胞仪检测三倍体的方法。大黄鱼受精卵经三倍体诱导处理后,胚胎期进行染色体滴片证实在处理组中有三倍体细胞存在。接着对该组胚胎进行育苗,获得1￣3cm的鱼苗,用流式细胞仪进行检测。以二倍体大黄鱼的肌肉组织或血液细胞DNA含量的峰值道数作为对照,用同样的方法取样处理、上机、测定处理组样本个体细胞的DNA含量的峰值道数。如果处理组个体细胞的DNA含量的峰值道数是二倍体组的1.5±0.1倍,则认为该个体为三倍体。实验结果经冷休克或静水压诱导处理的样本共检测182个,三倍体检出率为12.09%,其中有一组检出率高达55.56%。     

小鼠胚胎体外培养方法的优化及胚胎质量评估

实验采用输卵管收集获得的 2 细胞、原核受精卵和体外受精得到的胚胎。 2 细胞胚胎在所有培养浓度下均达到较高的囊胚发育率 ,而ISF和IVF受精卵在减低培养浓度后发育率显著降低 (p <0 .0 1 ) ,ISF受精卵从高密度 (1 /μl)下约 82 .5 %的发育率到低密度 (1 /1 0 0 0 μl)下 2 2 .3 %的发育率。而IVF胚胎的这两个值分别为 46 .3 %和5 .2 %。2 细胞胚胎与其他两种受精卵相比 ,每个囊胚所含的细胞数目差异显著 (p <0 .0 1 )。添加 1ng/ml(1 /1 0 μl)和 1 0ng/ml(1 /1 0 0 μl)的PAF显著增加了IVF胚胎的囊胚发育率 (p <0 .0 1 )。在胚胎密度为 1 /1 0 μl的培养密度下 ,添加 1 0ng/ml以上的IGF Ⅰ同样改善IVF受精卵的发育能力 (p <0 .0 1 )。培养液中添加EGF对囊胚的发育率没有影响。PAF和IGF Ⅰ协同作用的效果与IGF Ⅰ单独处理的结果并无差异 (p >0 .0 5) ,但高于PAF单独处理组 (p <0 .0 5)。结果表明 ,胚胎生长所需的生长因子在低密度培养条件下被稀释并影响胚胎的正常发育。PAF和IGF Ⅰ作为自分泌性胚胎营养因子在一定程度上补偿了由于低密度培养所带来的负效应。     

低温胁迫导致斑马鱼尾部发育畸形的分子机制

相比于恒温动物,环境温度对鱼类等变温动物的影响更加剧烈。为研究低温胁迫对鱼类胚胎发育时期的影响,我们将斑马鱼体节发生期的胚胎分成3组,其中两组分别在低温12℃处理12 h(12℃/12 h)和24 h(12℃/24 h),第三组作为对照在常温下孵育。我们发现经受低温胁迫的胚胎发育成幼鱼后体长均变短,并且这种体长变短的现象在12℃/24 h组中比12℃/12 h明显。在12℃/12 h处理组中大约5%的幼鱼尾部弯曲出现畸形状态,而经过12℃/24 h处理后大约有90%的幼鱼尾部出现畸形。为了探究低温胁迫导致尾部发育畸形的原因,我们用RT-qPCR的方法检测与凋亡相关的基因p53、c-Jun、gadd45αa和与肌肉发育相关的基因myod、mrf4、myf5,发现低温胁迫以后凋亡相关基因p53、c-Jun、gadd45αa的表达量显著上升,而肌肉发育相关基因myod、mrf4、myf5的表达量显著下降。并且利用TUNEL(TdT mediated dUTP nick end labeling)凋亡检测方法也发现低温胁迫后斑马鱼幼鱼的尾部出现细胞凋亡信号。证明低温胁迫可引起细胞凋亡和肌肉发育的阻滞,进而导致尾部发育畸形。     

放线菌素D对小麦花粉胚胎发生的影响

在小麦花药培养初期,用低浓度(10微克/毫升)的放线菌素D处理花药1—2天,可以显著地促进花粉胚胎的发生,花粉诱导物(愈伤组织和胚状体)的产量比对照增加1.13倍。细胞学的观察表明,花粉细胞的发育变慢,较长时间地滞留在单核时期,细胞分裂推迟,但分裂开始后,非配子体途径发育的细胞显著增多。     

鱼类体细胞移核胚胎发育影响因素的探讨

将脱膜后的泥鳅 (Misgurnusanguillicaudatus)受精卵置于不同孵化液中孵化 ,结果表明 ,孵化液 1×Holtfreter中正常鱼苗和总鱼苗的孵化率最高 ,分别为 5 4 8%和 5 9 2 %。 1/ 2×Holtfreter、 1/ 10×Holtfreter、曝气冷开水和改变孵化液处理 ,正常鱼苗的孵化率差别不大 ,分别为 48 0 %、 49 6 %、 5 0 0 %和 48 8%。曝气冷开水畸形率最高 ,为 8 8%。PBS不适合用作孵化液。机械损伤对胚胎的孵化率无明显影响 (73 39%vs 75 70 % ) ,但对胚胎发育有明显的致畸作用 (8 0 6 %vs 0 )。以雌核发育鳙 (Aristichthysnobilis)尾鳍培养细胞作供体 ,泥鳅未受精卵作受体 ,微卫星标记分析表明 ,移核胚胎的核来源于供体核 ,受体卵中未除去的核被排斥。供体细胞培养代数严重影响移核胚胎的发育率。随着培养代数的增加 ,移核胚胎的发育率逐渐降低。继代核移植可提高移核胚胎的发育率 ,尤其是第 1次体细胞继代核移植 ,晚期囊胚的发育率急剧上升 (4 3 84%vs 7 6 9% ) ,说明继代核移植可促进受体卵对供体核的再程序化。泥鳅和大鳞副泥鳅 (Paramisgurnusdabryanus)未受精卵作受体 ,其移核胚胎发育率无明显区别 (7 6 9%vs 7 0 2 % )。     

白细胞介素-1通过JNK信号通路调控Schlafen2基因的表达

目的：在多效生长因子（Ptn）基因稳定沉默的小鼠胚胎成纤维细胞Ptn-siRNA B/MEF241中,研究白细胞介素-1（IL-1）调控Schlafen2（Slfn2）基因表达的机制。方法：应用Northernblot检测Ptn沉默细胞Ptn-siRNAB/MEF241处于不同生长密度时Slfn2基因的表达变化,以确定Ptn沉默细胞中Slfn2基因的表达是否受到某种分泌性细胞因子的调控;用不同浓度的IL-1α中和抗体及IL-1受体拮抗剂处理Ptn沉默细胞,通过Northern blot检测细胞内Slfn2表达的抑制情况;用不同浓度的IL-1α中和抗体及IL-1受体拮抗剂处理Ptn沉默细胞不同时间,通过Western blot检测细胞中JNK磷酸化水平;Northern blot检测SP600125（JNK/MAPK通路抑制剂）对Ptn沉默细胞中Slfn2基因表达的影响。结果：Ptn沉默细胞中Slfn2基因的表达水平同细胞密度相关;用中和抗体和受体拮抗剂阻断IL-1通路,Slfn2表达受到显著抑制;IL-1受到抑制会影响JNK通路的活化;阻断JNK通路,Slfn2的表达受到显著抑制。结论：IL-1可以通过JNK通路诱导Slfn2的表达。     

人工诱导鱼类三倍体的试验

本试验利用大鳞副泥鳅的受精卵为材料,温度处理诱导大鳞副泥鳅同源三倍体,获得三倍体的胚胎和幼鱼。通过受精细胞学观察,初步提出了人工诱导鱼类三倍体过程中,染色体加倍的几种细胞学途径。     

人工诱导泥鳅雌核发育的细胞学研究和诱导参数优化

为培育泥鳅(Misgurnus anguillicaudatus)全雌品种,研究通过细胞荧光染色后进行细胞学观察确定人工诱导泥鳅雌核发育的热休克起始时间,并进一步利用核型和流式细胞分析等方法对人工诱导雌核发育泥鳅进行鉴定。结果显示,二倍体泥鳅受到灭活的鲤(Cyprinus carpio)精子刺激后,第二极体与卵核分开的时间在人工授精后3—5min;卵子在人工授精后3.5min后再热休克2min的诱导孵化率达到10.26%。通过分析野生型泥鳅胚胎、人工诱导雌核发育泥鳅胚胎、泥鳅×鲤杂交胚胎和单倍体泥鳅胚胎的发育,发现部分雌核发育的胚胎可以正常发育,而杂交胚胎和单倍体胚胎会出现明显的发育障碍。核型和流式细胞检测分析表明利用本研究获得的热休克参数进行处理可得到二倍体雌核发育子代,二倍率达64.71%。研究从细胞学层面获得泥鳅雌核发育的诱导参数,可为利用人工诱导雌核发育开展全雌泥鳅育种提供指导。     

激光微束在两种鱼受精卵上打孔技术研究

在埃及胡子鲶和苏氏芒鲶两种鱼受精卵上,用脉冲ＹＡＧ激光微束打孔技术,成功地导入了外源指示剂和用激光微束打过孔的受精卵孵化出了仔鱼,为今后激光微束打孔植入外源基因和针类转基因研究做了一些有意义的探索工作。     

Ligand-independent activation of the androgen receptor by insulin-like growth factor-i and the role of the MAPK pathway in skeletal muscle cells

In this study, the roles of the p38 MAPK, ERK1/2 and JNK signaling pathway in IGF-I-induced AR induction and activation were examined. C2C12 cells were treated with IGF-I in the absence or presence of various inhibitors of p38 MAPK (SB203580), ERK1/2 (PD98059), and JNK (SP600125). Inhibition of the MAPK pathway with SB203580, PD98059, or SP600125 significantly decreased IGF-I-induced AR phosphorylation and total AR protein expression. IGF-I-induced nuclear fraction of total AR and phosphorylated AR were significantly inhibited by SB203580, PD98059, or SP600125. Furthermore, IGF-I-induced AR mRNA and skeletal α-actin mRNA were blocked by those inhibitors in dose-dependent manner. Confocal images showed that IGF-I-induced AR nuclear translocation from cytosol was significantly blocked by SB203580, PD98059, or SP600125, suggesting that the MAPK pathway regulates IGF-I-induced AR nuclear localization in skeletal muscle cells. The present results suggest that the MAPK pathways are required for the ligand-independent activation of AR by IGF-I in C2C12 skeletal muscle cells.     

The carotenoids of eggs of wild and farmed Atlantic salmon, and their changes during development to the start of feeding

The only carotenoid detected in newly fertilized eggs of wild Atlantic salmon, Salmo salar, from western Scotland was astaxanthin at a concentration [μg carotenoid g^?1 wet wt of eggs, mean ±S.D. (number of parental females)] of 6.2±1.2(7) in 1982, 6.4±1.8(20) in 1983, and 7.6 ± 13(6) in 1984. In eggs of farmed Atlantic salmon the only carotenoid detected was canthaxanthin at concentrations which varied significantly between farms depending on the level of synthetic canthaxanthin in the broodstock diet. Thus on two farms using feed with 50 μgg^?1, the levels were 11.8 ± 3.4(7) and 12.3 ± 2.9(6), while on two farms using 75μgg^?1 the levels were 18.7 ± 5.0(9) and 21.2 ± 2.7(21). The levels in eggs of one-seawinter fish (grilse) did not differ from those of two-seawinter fish reared on the same farm and diet. During development from newly fertilized egg to fry at the end of yolk-sac absorption, the quantity of carotenoid present per individual decreased, presumably as a result of metabolism. Despite large differences in quantity present, the quantity so metabolized was fairly constant at 2–4 μg carotenoid g^?1 original egg weight for eggs from two-seawinter farmed and wild salmon, except that in eggs from farmed grilse it was 7 μg g^?1. In fry from wild eggs, 99.14% of the remaining carotenoid was present in the integument (skin and fins) as astaxanthin, astaxanthin monoester and astaxanthin diester. In fry from farmed salmon eggs, 47 ± 8% of the carotenoid present was found in the unused yolk oil droplets and in the liver, and 37 ± 6% was found in the integument as canthaxanthin and an unidentified metabolite of canthaxanthin. These findings explain visible colour differences between fry from wild parents and fry from canthaxanthin-fed farmed parents, particularly in the fins, liver and residual oil droplets. The canthaxanthin metabolite was also found, together with canthaxanthin, in the skin of farmed adults fed canthaxanthin. Preliminary tests showed it to be unchanged by saponification but reduced by sodium borohydride. For eggs from the three farms incubated under the same conditions in the same season, percentage mortality both to the eyed stage and between hatching and first feeding varied significantly between farms, but percentage mortality between the eyed stage and hatching did not do so. Results combined from two seasons for eggs from three farms and one wild source showed that egg mortality between fertilization and the eyed stage was not significantly different between wild and farmed salmon, but mortality between the eyed stage and hatching, and between hatching and first feeding, were both significantly higher in farmed salmon than in wild salmon. Such differences could not be explained simply by the large differences in egg carotenoid content, but were almost certainly due to factors such as broodstock nutrition, broodstock management, and stripping and fertilization procedures.     

燕鳐受精卵的孵化与仔幼鱼培育的初步研究

燕鳐是黄海沿岸重要鱼种之一。本文描述了燕鳐受精卵与仔幼鱼发育的形态特点和培育条件。 烟台崆蛔岛沿岸的燕鳐,5月底开始产卵,7月结束。人工受精在船上进行。受精卵和仔幼鱼在室内用静止水进行培育。 仔幼鱼的主要饵料是皱褶臂尾轮虫和卤虫幼体。幼体在室内水泥池(0.8立方米)进行培育。 受精卵和幼体在水温20.0—27.2℃,盐度31.28—31.74‰,pH8.32—8.52,溶氧(DO)1.52—8.32毫克/升的条件下进行培育。共育成幼鱼4801尾,到1981年9月20日,幼鱼最大全长92毫米。 1982年又进行了重复试验,共育出幼体6万余尾。     

Ablation of the spindle assembly checkpoint by a compound targeting Mps1

The spindle assembly checkpoint ensures accurate chromosome segregation by delaying anaphase initiation until all chromosomes are properly attached to the mitotic spindle. Here, we show that the previously reported c-Jun amino-terminal kinase (JNK) inhibitor SP600125 effectively disrupts spindle checkpoint function in a JNK-independent fashion. SP600125 potently inhibits activity of the mitotic checkpoint kinase monopolar spindle 1 (Mps1) in vitro and triggers efficient progression through a mitotic arrest imposed by spindle poisons. Importantly, expression of an Mps1 mutant protein refractory to SP600125-mediated inhibition restores spindle checkpoint function in the presence of SP600125, showing that its mitotic phenotype is induced by Mps1 inhibition in vivo. Remarkably, primary human cells are largely resistant to the checkpoint-inactivating action of SP600125, suggesting the existence of Mps1-independent checkpoint pathways that are compromised in tumour cells.     

池沼公鱼移殖放流试验研究

作者于1984—1986年进行了池沼公鱼移殖放流试验研究,移入水库的池沼公鱼已能自然产卵繁殖,形成了经济群体。本文论及了移殖放流的理论依据、移殖放流技术、移殖放流效果、移殖池沼公鱼的生态效益的分析和池沼公鱼的资源管理。     

鳜春季、夏季和秋季按季节人工繁育模式的研究

为满足不同地区、不同季节鳜(Sinierca chuatsi)养殖需要, 实现均衡上市的苗种供应要求, 研究通过对两批亲鱼在不同季节各进行4次交替人工催产, 按月建立苗种繁育模式。结果显示, 池塘中自然培育的亲鱼, 卵巢成熟系数出现2个峰值, 而网箱中培育的亲鱼, 经过4次人工催产, 出现4个成熟系数峰值, 产卵量和出苗量与成熟系数峰值正相关。以二繁的成熟系数、产卵量和出苗量最高, 显著高于其他三次(P<0.05), 二繁、三繁和四繁的受精率、孵化率和苗种培育成活率均较高, 显著高于一繁(P<0.05), 温度是影响一繁受精率、孵化率和苗种培育成活率的主要因素。产后亲鱼成活率随人工繁殖次数增加而下降, 其中以一繁的成活率最高, 达93.33%, 显著高于三繁和四繁(P<0.05)。综上结果表明, 通过按季节分梯次人工繁育模式解决鳜苗种生产的均衡供应是可行的。这为转变鳜的养殖方式提供了科学依据, 也为其他鱼类苗种的均衡生产提供了借鉴意义。     

酸性水对几种主要淡水鱼类的影响

在实验室条件下,研究了酸性水对几种主要淡水鱼类的毒性影响,结果表明,这几种淡水鱼的胚胎和鱼苗的死亡率与Ｈ的浓度呈现相关性,在低ｐＨ水平下,胚胎的发育进程明显地迟缓,要使鱼类受精卵正常孵化不受影响,水中的ｐＨ值应保持在６．５以上,在受试的几种鱼类中,没有发现对低ｐＨ敏感性有显著性差异,但在各自的发育过程中,其敏感性呈出现较大的差异,当ｐＨ〈６．０时,鱼的鳃组织就会受到损害,低ｐＨ加上铝,则对鱼类呈现     

黏性卵鱼类受精卵一种快速高效的显微注射方法

黏性卵鱼类受精卵遇水后产生的黏性和卵壳变硬的现象严重影响着大批量显微注射操作的速度和随后的取材。研究建立了一种高效的黏性受精卵快速脱黏显微注射方法, 并利用荧光标记葡聚糖Alex-Fluor488-dextran评估了消化脱黏、直接注射和脱壳注射三种方法的技术特点和适用范围。结果表明: 在23℃, 用0.25%胰蛋白酶(pH=7.1-7.4)消化4min可获得脱黏受精卵。与直接注射和脱壳注射方法相比, 研究建立的消化脱黏方法兼具二者的优点: 在受精后5min可以开始显微操作, 无黏性, 容易进针, 胚盘清晰便于观察、注射后容易培养和取材。实验方法适用于研究与黏性卵鱼类卵子发生、卵-胚转换和早期胚胎发育密切相关基因的功能, 亦可满足追踪受精过程中核质细微变化研究的需要。     

Swimming performance and morphology of juvenile sockeye salmon, <Emphasis Type="Italic">Oncorhynchus nerka</Emphasis>: comparison of inlet and outlet fry populations

We raised two populations of sockeye salmon fry from fertilized eggs in the laboratory and tested the hypothesis that outlet fry populations, fish which must migrate upstream to reach rearing lakes after yolk-sac absorption, have better swimming ability and morphological characteristics conducive to enhanced swimming performance than inlet fry populations, fish which migrate downstream to rearing lakes. Despite being of identical age, fry from the outlet population were larger (approx. 6.7% longer, ~5 mm on average) and more laterally compressed than inlet fry at the time of our initial experiments. Using an open-top box flume, we found that the burst-swimming performance (in cm s⁻¹) of the outlet population was 31% better. We found no differences between populations in prolonged-swimming performance. We were unable to find any direct relationships between measures of swimming performance and size or shape variables, suggesting that the larger, more robust morphology of outlet fry was not responsible for the superior burst ability. Recent biochemical studies indicate outlet fry may be metabolically better provisioned for burst swimming than inlet fry. It is possible that the morphological differences between the populations of fry reflect adaptations needed by adults during their migration and spawning.