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AIM:To explore the effect of annexin A2 (ANXA2) on the proliferation, migration and apoptosis abilities of human cervical cancer HeLa cells. METHODS:Overexpression vectors and siRNA of ANXA2 were constructed, and then transfected into HeLa cells. The HeLa cells were divided into 4 groups:control group, scramble group, ANXA2 overexpression group and ANXA2-siRNA group. The expression of ANXA2 at mRNA and protein levels was examined by real-time PCR and Western blotting. MTT assay, Boyden chamber and flow cytometry were used to determine the effect of ANXA2 on the proliferation, migration and apoptosis abilities of the HeLa cells. RESULTS:The proliferation and migration of HeLa cells were obviously promoted by ANXA2 overexpression. The proliferation and migration of HeLa cells were remarkably inhibited by the transfection of ANXA2-siRNA. ANXA2 had no effect on apoptosis of HeLa cells. CONCLUSION:Silencing of ANXA2 effectively inhibits the proliferation and migration of cervical cancer cells, but has little effect on apoptosis. ANXA2 may play a pivotal role in the occurrence and development of cervical cancer, and may be used as a molecular target for the treatment of cervical cancer. 相似文献
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根据一个从巴西橡树胶乳cDNA文库中获得的EST片段的序列设计引物,通过RACE的方法获得了橡胶树编码annexin的cDNA,命名为AnnHb1。序列分析表明,AnnHb1长为1 198 bp,含有945 bp的阅读框,62 bp的5'-UTR和191 bp的3'-UTR,编码314个氨基酸,分子量为35.99 ku,等电点为8.18。该氨基酸序列与蓖麻、麻疯树、棉花、苜蓿、烟草和拟南芥中的annexin的同源性分别为82%、72%、72%、64%、60%和60%。半定量RT-PCR分析结果表明AnnHb1基因在愈伤、花、树皮、叶、胶乳中均有表达,其中在愈伤组织中表达量最低,树皮中表达量最高。 相似文献
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膜联蛋白是一个多基因家族,在植物逆境胁迫应答和生长发育等方面起重要作用。本研究以已发表的膜联蛋白氨基酸序列为探针,对橡胶树和其他5种植物的转录组和基因组进行搜索,鉴定得到14个橡胶树膜联蛋白基因家族成员,命名为Ann Hb1-Ann Hb14。基因结构分析发现,14个家族成员的内含子数目为3~6个,结构域的数目为2~4个。在进化上,橡胶树、木薯和蓖麻共3种大戟科植物的膜联蛋白具有较近的亲缘关系。表达方面,Ann Hb1在各组织中普遍表达,而Ann Hb6和Ann Hb7主要在胶乳中表达,Ann Hb10、Ann Hb8和Ann Hb13分别在树叶、树皮和雄花中特异表达,其他成员在各组织中低丰度表达或不表达;部分家族成员的表达还与叶片发育、乙烯利刺激、真菌侵染和低温胁迫等具有一定相关性。 相似文献
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为挖掘花生抗逆境胁迫相关基因,克隆抗逆相关膜联蛋白Annexin基因,以花生品种花育25号为试验材料,从已知抑制消减杂交文库中获得花生膜联蛋白Annexin类似基因片段,通过RACE技术获得Annexin基因5'-RACE片段。对5'-RACE序列和抑制消减杂交文库中已知基因片段进行拼接,设计特异引物通过逆转录-聚合酶链式反应(RT-PCR)扩增得到该基因,命名为AhAnn1。结果表明,AhAnn1全长为1 277 bp,开放阅读框为951 bp。根据编码区预测AhAnn1编码一条316个氨基酸组成的多肽,预测分子量为36.10 k Da,等电点为7.07。预测该基因编码的蛋白含有膜联蛋白Annexin保守结构域,定位于细胞质中。蛋白序列多重比对和系统发育分析表明,花生与大豆、苜蓿、鹰嘴豆等豆科植物中的膜联蛋白相似性最高,亲缘关系最近。荧光实时定量PCR结果显示,AhAnn1在根系和叶片中的表达量随干旱胁迫程度的增加而增加。由此推测AhAnn1是一种干旱胁迫应答基因,在花生逆境调控中发挥作用。结果为进一步研究花生AhAnn1基因的功能和花生抗逆境胁迫相关分子机理提供了理论基础。 相似文献
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猪繁殖与呼吸综合征病毒(PRRSV)侵染Marc145过程中HSP27和Annexin A2蛋白可参与病毒粒子的组装过程,且HSP27可起到抑制侵染早期细胞凋亡,增加病毒复制时间的作用。本研究分别构建HSP27和Annexin A2下调的Marc145细胞系,经PRRSV感染后发现,与空白对照相比,两者子代病毒TCID50值有明显下降。这一结果为研究PRRSV侵染过程及HSP27和Annexin A2调控机制奠定了基础,也为疫苗的研制提供了新的思路。 相似文献
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将低分子量尿激酶与膜联蛋白 (AnnexinV)的融合基因重组到家蚕杆状病毒转移载体pBacPAK8中 ,获得重组转移载体pBacPAK UKAV ,并与线性化的病毒Bm PAK6DNA共转染家蚕细胞 ,获得重组病毒BacPAK UKAV。将重组病毒BacPAK UKAV感染家蚕培养细胞 (MOI=10 )和 5龄幼虫 (10 5pfu/头 ) ,Western印迹方法表明表达产物大小约为 6 9kD。用纤维蛋白平板溶圈法测定表达产物的纤溶活性 ,其融合蛋白具有明显的纤溶活性 ,约为 5× 10 -5U/个细胞。用APTT法测定表达产物的抗凝活性 ,比野生病毒Bm PAK6感染表达产物的APTT时间延长了 1倍以上 ,表现出明显的抗凝活性。体外实验表明 ,家蚕培养细胞和幼虫表达的重组低分子量尿激酶与AnnexinV融合蛋白具有溶栓与抗栓双功能。研究结果为今后进一步探索具有溶栓抗栓功能的血栓药物提供了新的方向。 相似文献
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从梅花鹿(Cervus nippon)鹿茸间充质中成功克隆出包括膜联蛋白A1(Anxa-1)基因全部编码区的c DNA序列,并结合生物学信息方法及实时荧光定量技术对该基因的氨基酸序列及不同生长时期的表达情况进行了分析。结果表明:Anxa-1基因编码346个氨基酸。经生物学信息分析,该基因编码蛋白为稳定蛋白,不具备信号肽,相对分子质量为38 830.4,理论等电点为6.17,一级结构中亮氨酸占最大比例(10.4%)。同源序列比对及系统进化树分析表明,梅花鹿Anxa-1氨基酸序列与藏羚羊(Pantholops hodgsonii)、绵羊(Ovis aries)、山羊(Capra hircus)和水牛(Bubalus bubalis)相似性较高。实时荧光定量RT-PCR分析表明,Anxa-1基因在不同生长时期鹿茸顶端间充质表达存在差异,生长前期的表达量高于中期与后期。 相似文献
18.
Comparison of established and novel methods for the detection and enumeration of microparticles in canine stored erythrocyte concentrates for transfusion 
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LIU Yuan-sheng FAN Hong-tao GUO Qiu-ye GUO Xiu-zhi TAN Guang-xiao CHEN Peng ZHOU Tao CHEN Xiao-yin 《园艺学报》2002,18(5):517-521
AIM:To study the effect of IL-12 on T lymphocytes apoptosis, the expression of Fas/FasL and TNFR/TNFα. METHODS:Terminal dUTP nick end labeling(TUNEL) and Annexin V assay were used. Anti-TNFR were labeled with FITC, anti-CD95 was labeled with PE and Anti-FasL with biotin. Three kinds of T cells (HTB176,TIB152 and human normal T cells) were analysed through flow cytometry. RESULTS:At 1st hour after being treated with IL-12, the expression of FasL protein and FasL mRNA in HTB176 and TIB152 began to increase and reached peak value in 24 hours. In the normal T cells, FasL just began to increase in 1 hour and maintained stability in 6, 12 and 24 hours through the later experiment period. All three kinds of T cells displayed no change in the expression of CD95 and TNFR/TNFα under the stimulation of IL-12. CONCLUSION:Expression of such apoptosis regulating factors were different in the apoptosis of T cells induced by IL-12. 相似文献
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AIM: IL-12 acts upon T lymphocytes and activates its receptor complexes of β1/β2 ,and so IL-12 can regulate TH1/TH2 balance. Our study is aimed at IL-12-inducing apoptosis of T cells and expression and signal conduction of Bcl-2 during T cell apoptosis. METHODS: The apoptosis of T cells was detected by Annexin V staining cytometry and the expression of Bcl-2 under different inhibitors were detected by the method of semi-quantitative PCR. RESULTS: IL-12 can induce the human leukemic T cell line(TIB-152) and the human lymphoma T cell line(HTB-176) and the normal human T cells to undergo apoptosis. The Bcl-2 expression at 6 hours of treatment with IL-12 increased aparently, and reached the max at 24 hours. But IL-12 did influence Bcl-2 expression. IL-12 can induce T cells to undergo apoptosis which is characterized by early membrane changes. CONCLUSION: The inducing effect is correlated with the concentration of IL-12 and the maturation of T cells. Bcl-2 takes part in the progression of T cells' apoptosis as a apoptosis mediator. 相似文献