嗜碱单胞菌的新型羧基转移酶α亚基基因Aa-accA及其抗盐碱性能

[目的]探讨解淀粉嗜碱单胞菌(Alkalimonas amylolytica)N10来源的羧基转移酶α亚基(Acetyl-coenzyme A carboxylase subunit alpha,AccA)基因Aa-accA对细菌及植物细胞耐盐碱性的作用.[方法]通过PCR方法从嗜碱菌N10基因组中扩增基因Aa-accA,并在大肠杆菌(Escherichia coli)K12中表达,通过测定工程菌及对照菌在不同盐浓度[0%,2%,4%,6%(W/V) NaCl]及不同碱性pH(8.0,8.5,9.0,9.5)的LB中生长12 h后的OD600值,以及二者在分别含6%(W/V) NaCl及pH 9的LB中的生长曲线,评价Aa-accA对大肠杆菌耐盐碱性的影响.同时以pPZP111为载体,构建了植物细胞重组表达载体,通过农杆菌介导方法将该基因转入烟草BY-2悬浮细胞表达,利用FDA染色方法测定经盐碱溶液处理后残存的活细胞数量评价该基因对植物细胞耐盐碱性的影响.[结果]PCR扩增得到基因Aa-accA,其ORF含957 bp,编码318个氨基酸的多肽,BLAST比对显示该基因为羧基转移酶α亚基(AccA)家族中的成员,其氨基酸序列与E.coli的AccA具有76%同源性;含有Aa-accA的E.coli K12相较于对照组在不同NaCl浓度及不同碱性pH的LB中表现出了明显的生长优势,特别是在6%(W/V) NaCl及pH 9的LB中培养12 h后,终OD600分别是对照菌的2.6倍和3.5倍;缺失体实验结果显示基因缺失的突变体E.coli K12△accA在6%(W/V) NaCl及pH 9的LB中不能正常生长,而含有Aa-accA基因的重组质粒使得E.coli K12△accA在同样条件下OD600值达到0.5和0.2;转入此基因的烟草BY-2细胞,经盐碱溶液处理后,其存活细胞比例高于野生型.[结论]本研究首次发现了Aa-accA基因与盐碱性的相关性,可提高大肠杆菌及烟草BY-2细胞的耐盐碱能力.     

Oct4基因在猪孤雌激活和体外受精早期胚胎中的表达特征

目的研究植入前胚胎发育重要基因Oct4在猪孤雌和体外受精胚胎中的表达特征。方法收集成熟卵母细胞、孤雌和体外受精2细胞、4细胞、8细胞胚胎和囊胚,做荧光即时定量PCR检测,以体外成熟的猪卵母细胞做对照分析相对表达量。结果孤雌组和体外受精组胚胎在8细胞期Oct4表达量均最高(P<0.05),在孤雌和体外受精组囊胚相对于其他时期Oct4表达量最低(P<0.05)。在同一时期孤雌和体外受精胚胎上Oct4表达并没有差异。结论多能性基因Oct4在卵裂发育时期表达量动态变化,孤雌胚胎在一定程度上可作为体外胚胎基因表达的模型,且不同的胚胎培养条件可能导致基因表达的差异。     

PP2A-A/在金鱼及斑马鱼发育中的分化表达模式

以金鱼和斑马鱼为研究对象,运用RT-PCR和Western Blot技术分析蛋白磷酸酶2A(PP2A)结构亚基A(PP2A-A/)在金鱼、斑马鱼成体9种组织和12个发育时期胚胎中mRNA和蛋白水平的表达情况,得到其分化表达模式为:(1)在mRNA水平上,PP2A-A/在金鱼、斑马鱼9种组织中具有较强表达;种属差异性和组织差异性均较大;结构亚基A的两亚型A和A的表达存在差异。(2)在蛋白水平上,PP2A-A/在金鱼、斑马鱼9种组织中均有表达;种属差异性不大但出现明显的组织差异性。(3)PP2A-A/mRNA在金鱼和斑马鱼卵裂期到囊胚期胚胎中大量存在,PP2A-AmRNA在金鱼眼色素期量剧增推测其对金鱼眼色素的形成至关重要。(4)PP2A-A/基因在金鱼、斑马鱼12个发育时期胚胎中均有较高水平的蛋白存在,提示其为维持胚胎的正常发育发挥重要作用。       

Caveolin-1在围植入期小鼠子宫内膜组织中的动态变化

目的检测caveolin-1在胚胎植入过程中小鼠子宫内膜组织中的表达,探讨其在胚胎植入过程中的作用。方法选择成年雌性昆明小白鼠42只,随机均分为7组(处于动情期的未孕组、妊娠3.5天组、妊娠4.5天组、妊娠5.5天组、妊娠6.5天组、妊娠7.5天组、妊娠9天组),采用免疫组织化学和RT-PCR方法检测子宫内膜组织中caveolin-1蛋白及mRNA水平在围植入期的变化。结果 (1)caveolin-1在胚胎植入前期(0d、3.5d)小鼠子宫内膜组织中的表达高于胚胎植入期(4.5d、5.5d、6.5d),差异有显著性(P<0.05)。(2)caveolin-1在胚胎植入后期(7.5d、9d)小鼠子宫内膜组织中的表达高于胚胎植入期(4.5d、5.5d、6.5d),差异有显著性(P<0.05)。(3)caveolin-1在胚胎植入后期小鼠子宫内膜组织中的表达略高于胚胎植入前期,但差异无显著性(P>0.05)。结论 Caveolin-1在胚胎植入前期和后期均高表达,植入期低表达。这种变化提示caveolin-1是影响胚胎植入的重要因素之一。     

IL-6促进小鼠胚胎干细胞多能性并以发育依赖的方式调控心肌分化（英文）

白细胞介素6 (interleukin 6, IL-6)是心脏微环境的重要组成部分。在不同模型中，IL-6通过促进心肌细胞再生帮助心脏修复。胚胎干细胞是心脏修复中心肌再生的良好来源。本研究旨在探讨IL-6对小鼠胚胎干细胞(mouse embryonic stem cells,mESCs)及其心肌分化的影响。IL-6处理mESCs两天，用CCK-8法检测mESCs增殖情况，用实时荧光定量PCR(quantitative real-time PCR, qPCR)检测干性和胚层分化基因mRNA表达水平，用Western blot检测干细胞相关信号通路的磷酸化水平，用siRNA干扰STAT3磷酸化功能。通过检测搏动拟胚体(embryoid bodies, EBs)比例和qPCR检测心脏前体细胞标记物和心肌细胞离子通道mRNA表达水平来评估mESCs的分化能力。从胚胎干细胞分化第1天(EB0)开始使用IL-6中和抗体阻断内源性IL-6的作用，分别在EB7、EB10和EB15检测心肌细胞分化；在EB15用免疫组织化学染色法示踪心肌细胞，并用Western blot检测干细胞相关信号通路的磷酸化情况...     

一氧化氮对小鼠胚胎围植入期子宫VEGF及其受体表达的调节

为研究NO在胚胎植入中的作用机理 ,本文采用子宫角注射、原位杂交及Westernblot方法研究了一氧化氮 (NO)在小鼠胚胎植入过程中对血管内皮生长因子 (VEGF)及其受体表达的调节。受试小鼠于妊娠第三天 (D3 )在一侧子宫角内注射一氧化氮合酶 (NOS)抑制剂N 硝基 L 精氨酸甲酯 (L NAME)或者L NAME与NO的供体硝普钠 (SNP)合用 ,另一侧子宫角为对照侧 ;收集并分别检测了D5,D6和D7天小鼠子宫中VEGF及其受体mRNA和蛋白的表达情况。结果显示 :与对照侧相比 ,L NAME处理后小鼠胚胎围植入期子宫中VEGF及其受体mRNA的表达有不同程度的下降 ;对VEGF及其受体蛋白表达水平检测表明 ,抑制的NO产生也使VEGF及其受体蛋白在小鼠围植入期子宫中的表达有不同程度的降低。当NOS抑制剂和NO的供体SNP同时注射小鼠时 ,VEGF及其受体mRNA和蛋白表达都恢复到正常水平。以上结果表明 ,在小鼠胚胎植入中NO可通过调节VEGF及其受体的表达参与血管新生 ,从而对胚胎植入起到调节作用     

利用斑马鱼胚胎快速鉴定真核质粒中目的基因表达的研究

目的建立利用斑马鱼胚胎快速鉴定真核质粒中目的基因表达的实验体系。方法选20枚斑马鱼受精卵,在显微镜下每隔1h记录胚胎的发育情况。另选250枚单细胞期斑马鱼胚胎,平均分成5组,一组胚胎作为对照,剩余4组分别向胚胎的单细胞内注射pEGFP-N1(真核表达质粒)、pCMV-DsRed-Express2(真核表达质粒)、pET28-GFP(原核表达质粒)、pET28-RFP(原核表达质粒)质粒,在不同时间点连续观察绿色荧光及红色荧光的表达情况。另选600枚单细胞期斑马鱼胚胎,平均分成3组,一组胚胎作为对照,一组向胚胎单细胞内注射pEGFP-N1质粒,另外一组向胚胎单细胞内注射pEGFP-N1-MUC1外源基因融合重组质粒,注射4h后在荧光显微镜下观察绿色荧光的表达情况,并用RT-PCR的方法检测目的基因MUC1mRNA的转录情况。结果注射pEGFP-N1、pCMV-DsRed-Express2真核表达质粒的胚胎,注射4h后分别观察到很强的绿色荧光及红色荧光;注射pET28-GFP、pET28-RFP原核表达质粒的胚胎,10h内都未观察到绿色荧光及红色荧光;注射pEGFP-N1-MUC1外源基因融合质粒,注射4h后同样...     

胃癌发展相关阶段中E-cadherin基因启动子甲基化及蛋白表达的研究

为了研究E cadherin基因启动子甲基化在胃癌发生及发展阶段中的作用 ,我们采用甲基化特异性PCR和免疫组化的方法对异型增生 (2 3例 )、早期胃癌 (2 0例 )和进展期胃癌 (2 0例 )石蜡标本进行启动子甲基化状态及蛋白表达的分析。结果表明E cadherin基因启动子在异型增生、早期胃癌和进展期胃癌中均有甲基化 ,其阳性率分别为78 3% ,80 %和 90 % ,经χ2 检验各病例组与正常组 (30 % )比较均有差异 (P <0 0 5 ) ,但各病例组间没有差异 (P >0 0 5 ) ;进展期胃癌E cadherin蛋白表达全部阴性 ,早期胃癌 70 %阴性 ,异型增生中无蛋白阴性 ,在早期胃癌和进展期胃癌 34例蛋白表达阴性的标本中 31例有启动子甲基化 (91 2 % ) ,蛋白表达与启动子甲基化呈明显负相关 (P <0 0 1)。表明E cadherin启动子甲基化是胃癌发生的早期事件 ,也是胃癌发生、进展的重要事件     

“EB-82灭蚜菌”制剂对蔷薇三节叶蜂和菜青虫毒力测定

利用“EB 82灭蚜菌”菌剂 ,通过设定不同方法处理蔷薇三节叶蜂 (Argegeei)和菜青虫 (Pierisrapae)幼虫 ,进行室内防治实验 ,分析“EB 82灭蚜菌”菌剂对蔷薇三节叶蜂和菜青虫幼虫的作用。结果表明 ,“EB 82灭蚜菌”菌剂不同浓度及不同时间与胃毒作用杀虫剂敌敌畏和对照处理 ,其死亡率和取食量均差异极显著。“EB 82灭蚜菌”菌剂不同浓度处理蔷薇三节叶蜂对死亡率和取食量比较 ,2 0 0倍和 4 0 0倍之间死亡率无差异 ,10 0倍和 2 0 0倍之间 ,2 0 0倍和 4 0 0倍之间取食量无差异 ,进一步确定“EB 82灭蚜菌”菌剂的最低施用浓度 ;“EB 82灭蚜菌”菌剂浸叶不同时间喂养菜青虫 ,死亡率和取食量比较表明 ,1min和 5min之间 ,10min、30min和 60min之间死亡率无差异 ,10min和 30min之间取食量无差异。     

慢病毒介导的牛生长素基因对小鼠胚胎发育的研究

生长素是促进动物生长发育所必需的激素之一。本研究探索牛生长激素(bovine growth hormone,bGH)对小鼠胚胎发育的影响。将牛生长激素基因连接到慢病毒载体(Lenti-CMV-EF1-eGFP)形成Lenti-CMV-bGH/EF1-eGFP,重组病毒经293T细胞包装后直接感染小鼠胚胎和G1胚胎干细胞(embryonicstemcells,ESCs)。阳性表达的胚胎经体外培养,发育到囊胚期的胚胎进行胚胎移植,为直接感染组。感染的小鼠G1胚胎干细胞注射到正常昆明白小鼠囊胚制作嵌合胚胎后进行胚胎移植,为嵌合体组。分别解剖3只妊娠15d的直接感染组和嵌合组的小鼠,观察受体小鼠妊娠情况。结果发现,在1-细胞期感染胚胎,感染效率可达(74.7±6.7)%,在2-细胞期连续感染,感染效率为(79.4±5.7)%,两组感染方法的效率没有显著差异(P>0.05)。1次和2次感染胚胎发育和正常胚胎之间没有显著差异((87.6±3.5)%,(85.4±6.3)%VS(83.0±5.5)%,P>0.05)。所有移植的胚胎没有发育到足月,解剖妊娠15d的小鼠,发现直接感染组没有妊娠,嵌合组胎盘发育正常,但胚胎部分已经死亡和被吸收。因此,本研究证明bGH对小鼠附着前胚胎发育没有影响,但影响小鼠胚胎附着后的发育。这为后期bGH的研究提供参考。     

Effets de divers facteurs de croissance (FGF,IGF-1) sur les ébauches des membres de l'embryon d'orvet (Anguis fragilis L.)

The present experiments were carried to investigate the effects of some growth factors (FGFs, IGF-1) on the development of limb buds in the slow-worm (Anguis fragilis L.). This serpentiform reptile is devoid of legs in adulthood; but anlagen of limbs appear during embryonic life; their existence is only temporary: their growth ceases, they regress and disappear before hatching. Treatment of embryos was performed either by injection of the drugs around the limb buds or by application of small fragments of cellulosic paper soaked in the growth factors. The embryos were treated (27 by injection, 24 by application of cellulosic paper) at the stage of the allantoic bud 0.2 mm to 0.5 mm long and at an older stage (allantoic bud 1.8 mm to 4 mm long) (21 embryos treated). The administered growth factors were FGF-2, FGF-4 and IGF-1. Dosages were around 1 000 to 3 900 ng. Anterior limb buds display only very weak sensitivity to the effect of the applied growth factors: only a small proportion of the treated embryos presented a weak hypertrophy of these buds; however, after application of a fragment of cellulosic paper soaked in FGF-2, two thickening of the somatopleure in a embryo and two salient buds in another developed in the territory of the limb, propably representing anlagen of supernumerary limbs. In 25% of the embryos treated at the stage of the allantoic bud 1.8 to 4 mm long, the anlagen of the posterior limbs were greatly stimulated under the action of FGFs and IGF-1: the volume of the treated limbs was several times greater than the one of control limbs; histological study showed in the hypertrophied buds, numerous mitoses in the mesoblast and an apical ridge which did not degenerate. These results are in agreement with previous experiments and they show that it is possible to check experimentally the evolutive regression of the limbs of Anguis embryos.     

Somatic embryogenesis in asparagus: the role of explants and growth regulators

Summary The explant used to initiate embryogenic callus and the growth regulators used in subsequent induction (IM) and embryo development media (EDM) both influenced rate of somatic embryo development and conversion to plantlets in asparagus. Embryogenic callus derived from spear-cross sections (SS), in vitro crowns (IVC) and lateral buds (LB) was cultured on IM of MS salts and vitamins with 2, 4-D or NAA at 0, 0.01, 0.1, 1.0 or 10 mg/l and kinetin at 0, 0.1, 1.0 or 10 mg/l. The auxin 2,4-D at 1–10 mg/l, in combination with kinetin at 0–1 mg/l, in IM induced the highest frequency of embryos after four weeks; callus derived from SS, IVC and LB had means of 394, 382, and 344 small globular embryos, and 4, 11 and 9 bipolar embryos per gram of callus, respectively. After 6 weeks on EDM, 128, 116 and 51 bipolar embryos (4–7 mm in length) occurred per gram callus and 4.5, 1.4 and 2.1 embryos converted for IVC, SS and LB, respectively. NAA at 1–10 mg/l, in combinations with kinetin 0–1 mg/l, yielded means of 64, 175 and 225 small globular embryos per gram callus on IM for SS, IVC and LB, respectively. NAA promoted a higher rate of embryo development: means of 27, 54 and 91 bipolar embryos per gram callus for SS, LB and IVC, respectively, on EDM. There were 0.5, 9.4 and 11.9 plantlets from these respective callus sources. There was no difference between kinetin levels of 0–1 mg/l on callus growth and embryogenesis, whereas, 10 mg/l in IM was inhibitory.Abbreviations 2,4-D 2,4 dichlorophenoxyacetic acid - EDM embryo development medium - IAA indole-3-acetic acid - IM induction media - IVC in vitro crowns - LB lateral bud - LS Linsmaier and Skoog (1965) - MS Murashige and Skoog (1962) - NAA naphthaleneacetic acid - SS spear-cross section     

Effects of 1,25(OH)2D3, 25OHD3, and EB1089 on cell growth and Vitamin D receptor mRNA and 1alpha-hydroxylase mRNA expression in primary cultures of the canine prostate

The aim of this study was to investigate effects of 1,25(OH)(2)D(3) (calcitriol), 25OHD(3), and EB1089 on cell growth and on Vitamin D receptor (VDR) mRNA and 1alpha-hydroxylase (1alpha-OHase) mRNA expression in normal canine prostatic primary cultures. Canine prostatic epithelial cells were isolated, cultured, and treated with vehicle (ethanol), calcitriol, 25OHD(3), and EB1089 at 10(-9) and 10(-7)M. The VDR was present in epithelial and stromal cells of the canine prostate gland. 1,25(OH)(2)D(3), 25OHD(3), and EB1089 inhibited epithelial cell growth at 10(-7)M compared to vehicle-treated controls [calcitriol (P < 0.01), EB1089 (P < 0.01), and 25OHD(3) (P < 0.05)]. Epithelial cells treated with calcitriol and EB1089 at 10(-7)M had slightly increased VDR mRNA expression (0.2-0.3-fold) at 6 and 12h compared to controls. There was no difference in 1alpha-OHase mRNA expression in epithelial cells treated with these three compounds. 1,25(OH)(2)D(3) and its analogs may be effective antiproliferative agents of epithelial cells in certain types of prostate cancer.     

A staging system for forelimb regeneration in the axolotl,Ambystoma mexicanum

A staging system has been devised for normal regeneration from the upper arm in the mature axolotl. It consists of seven externally definable stages: (1) Wound healing (WH); (2) Dedifferentiation (DD); (3) Early bud (EB); (4) Medium bud (MB); (5) Late bud (LB); (6) Palette (Pal), and (7) Digital outgrowth (DO). Serial histological sections of 38 regenerating limbs were used to correlate gross stages with microscopic events in the regenerative process.     

Initial stages in the course of adventitious bud formation on embryos of Picea abies

Adventitious buds on embryos of Picea abies (L.) Karst. developed after a pulse treatment with 250 μ M benzyladenine (BA) of pH 5.5 for 2 h. Light and temperature regimes were not critical during the initial stages. Adventitious buds developed faster after a pulse treatment and the variation among different experiments was lower compared to when the embryos were cultured on media supplemented with BA. Various stages of the differentiation of adventitious buds were identified: stage 1 - appearance of meristematic centres (approximately the first two weeks); stage 2 - development of adventitious bud primordia (approximately the third week); stage 3 - adventitious bud development (from approximately the 4th to the 8th week). This system may be used for further studies on bud differentiation.     

PGE2、PGF2α和Iloprost对小鼠2-细胞胚胎体外发育的影响

目的研究PGE2、PGF2。以及Hoprost（PGl2的稳定类似物）对小鼠2-细胞胚胎体外发育的影响。方法在含0．5％BSA的mCZB液中分别添加0、10^-4、10^-5和10^-6mol／L的PGE2,0、10^-4、10^-5和10^-6mol／L PGF2α以及0、1×10^-6、2×10^-6和4×10^-6mol/L Iloprost,观察小鼠2-细胞胚胎的体外发育,同时利用H33342染色进行囊胚和孵化囊胚的细胞核计数。结果添加PGE2、PGF2α以及Iloprost的各处理组2-细胞胚胎体外培养的囊胚率和孵化率均显著低于对照组（P〈0．05）,但各处理组与对照组之间在囊胚或孵化胚胎的细胞数上差异不显著（P〉0．05）。结论培养液中添加这三种前列腺素均不利于小鼠2-细胞胚胎的体外发育,但不影响囊胚或孵化胚胎的细胞数。     

Effect of different cryoprotectants and vitrificant solutions on the hatching rate of turbot embryos (Scophthalmus maximus)

Vitrification could provide a promising tool for the cryopreservation of fish embryos. However, in order to achieve a vitrifiable medium, a high concentration of permeable cryoprotectants must be employed, and the incorporation of high molecular weight compounds should also be considered. The toxicity of these permeable and non-permeable agents has to be assessed, particularly when high concentrations are required. In the present study, permeable and non-permeable cryoprotectant toxicity was determined in turbot embryos at two development stages (F stage-tail bud and G stage-tail bud free). Embryos treated with pronase (2mg/ml, 10 min at 22 degrees C) were incubated in dimethyl sulfoxide (Me2SO), methanol (Meth.) or ethylene glycol (EG) in concentrations ranging from 0.5 to 6M for periods of 10 or 30 min, and in 5, 10, and 15% polyvinylpyrrolidone (PVP), 10, 15, and 20% sucrose or 0.1, 1, and 2% X-1000 for 2 min. The embryos were then washed well and incubated in seawater until hatching. The toxicity of permeable cryoprotectants increased with concentration and exposure time. There were no significant differences between permeable cryoprotectants. However, embryos tolerated higher concentrations of Me2SO than other cryoprotectants. Exposure to permeable cryoprotectants did not affect the hatching rate except at G stage with X-1000 treatment and 20% sucrose. Taking into account the cryoprotectant toxicity and the vitrification ability of cryoprotectant mixtures, three vitrification solutions (V1, V2, and V3), and one protocol for stepwise incorporation were designed. The tested solutions contained 5M Me2SO+2M Meth+1M EG plus 5% PVP, 10% sucrose or 2% X-1000. The hatching rate of embryos that had been exposed to the the vitrification solutions was analyzed and no significant differences were noticed compared with the controls. Our results demonstrate that turbot embryos can be subject to this cryoprotectant protocol without deleterious effect on the hatching rate.     

Teratogenic effects of retinoic acid and dimethylsulfoxide on embryonic chick wing and somite

In order to document the stage(s) at which the embryonic chick wing bud is sensitive to vitamin A teratogenesis and the kinds of defects produced by vitamin A insult to the embryonic chick wing, 1-microgram doses of retinoic acid (1 microliter RA in 90% DMSO at a concentration of 1 microgram/microliter) were locally applied to the right wing bud of chick embryos at stages 17-23 (Hamburger and Hamilton: J. Morphol., 88:49-92, '51), and the resulting limb skeleton anatomy was observed at 10 days of incubation. Local application of RA at stages 17-20 resulted in distal wing skeleton defects. There were significantly more wing skeleton defects among embryos treated at these stages with RA solution than among solvent (DMSO)-treated control embryos and than among untreated control embryos. Wings of embryos treated with RA at stages 21-23 were always normal. Scapular and vertebral defects were seen at 10 days of incubation among embryos which had been treated prior to stage 21 with both the RA solution and the solvent control. Statistical analysis and histological data suggest that scapular and vertebral defects were caused by DMSO-induced damage to somites.     

Enhanced expression of bovine growth hormone gene by different culture conditions in Escherichia coli

To optimize the production of bovine growth hormone (bGH) in E. coli, the cells harboring pUBJ10 plasmid, which contains the modified 59-coding region of bGH cDNA under the control of trc promoter, was induced to express under various culture conditions such as medium (LB or M9CA), temperature, induction stage, expression time, IPTG concentration, and hosts. Induction stage was effective at early logarithmic phase. The expression levels of bGH were not largely affected by IPTG concentrations, slightly greater in LB medium than in M9CA medium, and efficient in 4 to 6 h of expression time. The highest level of bGH production was obtained in E. coli BL21 strain.