Inhibition of poly(ADP-ribose) polymerase activity by Bcl-2 in association with the ribosomal protein S3a.

We screened a human lymphocyte cDNA library using the yeast two-hybrid system and an automodification domain of PARP as a probe. The DNA sequence of an isolated clone (clone 3-9) was identical to the partial cDNA sequence of the human ribosomal protein S3a. We confirmed that PARP interacts with clone 3-9 by performing binding studies using a GST-3-9 fusion protein as bait. We also demonstrated that native S3a in nuclear extracts of HL-60 cells interacts with the automodification domain of PARP and that PARP from nuclear extracts is coprecipitated with the GST-3-9 fusion protein. Furthermore, we demonstrated that Bcl-2 interacts with PARP in association with S3a and that the interaction of S3a and Bcl-2 with PARP causes a significant decrease in PARP activity. Since Bcl-2 failed to inhibit PARP activity in the absence of S3a, we suggest that Bcl-2 together with S3a prevents apoptosis probably by inhibiting PARP activity.     

SUMO化修饰对NF-kB信号通路的调控

小泛素相关修饰物(small ubiquitin-related modifier,SUMO)经由一系列酶介导的生化级联反应共价结合于靶蛋白的赖氨酸残基上,稳定靶蛋白免受降解的过程称为SUMO化修饰(SUMOylation).核转录因子kB(nuclear factors kB,NF-kB)是公认的炎症和免疫反应的重要调节因子,并与糖尿病的发生发展密切相关.近年来研究发现,不仅NF-kB抑制蛋白(inhibitor of NF-kB,IkB)的SUMO化修饰参与NF-kB信号通路的调节,而且SUMO酶可以直接调节NF-kB对靶基因的转录.现就SUMO亚型及结构,SUMO化修饰与去SUMO化修饰过程,SUMO、SUMO酶对NF-kB的转录调控及其与糖尿病相关性的最新研究进展作以综述.     

外电场诱导叶肉原生质体融合

应用一交变电场(正弦波,500KHz,175—225V/cm),分别将裸大麦(正常或正常与黄化)、蚕豆、烟草的叶肉原生质体在一定间隔、平行的两电极间排列成串。再附加单个的方波脉冲(10—40μs,800V/cm,因不同的材料而异),以诱导相邻原生质体局部接触区发生质膜的可逆击穿而形成融合。上述正弦波和方波脉冲均由自制的细胞融合仪发生。在本实验条件下,融合率可达50%以上,并探讨了方波脉冲讯号以及其它有关的条件对于融合率的影响。     

禽病原性大肠杆菌iro和tsh基因缺失株的构建

通过SSH和SCOTS研究, 铁系统(Iro)和温度敏感性血凝素(Tsh)在禽病原性大肠杆菌(APEC)的感染中可能发挥重要作用。基因检测发现, 在243个禽源大肠杆菌分离株中, 有205株为iro+菌株, 其中高、中度和低致病株分别为89.8%(184/205)、8.8%(18/205)和1.5%(3/205); 有167株为tsh+菌株, 高、中度、低致病株分别为87.4%(146/167)、12.6%(21/167)和0%(0/167), 结果显示iro+或tsh+株大多数为高致病株。为了确定iro和tsh基因在APEC致病力中的作用, 以APEC E037株为基础, 通过自杀性载体分别构建了iro和tsh基因缺失突变株E037(Δiro)、E037(Δtsh)和E037(ΔiroΔtsh)。动物感染性试验表明, 突变株在鸡体内的繁殖能力和致病性均明显下降, 但两个基因的协同致病作用不显著。进一步证实Iro和Tsh为APEC重要的致病因子。     

绿洲农业生态经济系统的结构与功能分析以张掖绿洲为例

通过分析张掖绿洲农业生态经济系统的结构与功能,发现其种群结构单一、产业结构不甚合理、空间结构脆弱,决定了绿洲功能较差,产投比低下的特点,并据此从可持续发展的角度提出了改善绿洲农业生态经济系统结构、提高其功能的对策与建议     

Mouse-rabbit germinal vesicle transfer reveals that factors regulating oocyte meiotic progression are not species-specific in mammals

A series of experiments were designed to evaluate the meiotic competence of mouse oocyte germinal vesicle (GV) in rabbit ooplasm. In experiment 1, an isolated mouse GV was transferred into rabbit GV-stage cytoplast by electrofusion. It was shown that 71.8% and 63.3% of the reconstructed oocytes completed the first meiosis as indicated by the first polar body (PB1) emission when cultured in M199 and M199 + PMSG, respectively. Chromosomal analysis showed that 75% of matured oocytes contained the normal 20 mouse chromosomes. When mouse spermatozoa were microinjected into the cytoplasm of oocytes matured in M199 + PMSG and M199, as many as 59.4% and 48% finished the second meiosis as revealed by the second polar body (PB2) emission and a few fertilized eggs developed to the eight-cell stage. In experiment 2, a mouse GV was transferred into rabbit MII-stage cytoplast. Only 13.0-14.3% of the reconstructed oocytes underwent germinal vesicle breakdown (GVBD) and none proceeded past the MI stage. When two mouse GVs were transferred into an enucleated rabbit oocyte, only 8.7% went through GVBD. In experiment 3, a whole zona-free mouse GV oocyte was fused with a rabbit MII cytoplast. The GVBD rates were increased to 51.2% and 49.4% when cultured in M199 + PMSG and M199, respectively, but none reached the MII stage. In experiment 4, a mouse GV was transferred into a partial cytoplasm-removed rabbit MII oocyte in which the second meiotic apparatus was still present. GVBD occurred in nearly all the reconstructed oocytes when one or two GVs were transferred and two or three metaphase plates were observed in ooplasm after culturing in M199 + PMSG for 8 hr. These data suggest that cytoplasmic factors regulating the progression of the first and the second meioses are not species-specific in mammalian oocytes and that these factors are located in the meiotic apparatus and/or its surrounding cytoplasm at MII stage.     

猴免疫缺陷病毒特异性免疫复合物沉着与猴AIDS多系统病变关系的探讨

目的观察猴免疫缺陷病毒(SIV)感染后,病毒特异性免疫复合物(IC)在不同时间、不同组织的沉着情况,初步研究其与AIDS多系统病变的联系。方法对8只不同时间感染SIV的恒河猴及1只未感染SIV的猴进行尸检以获取多系统组织标本,进行连续切片和IgG、C3、SIV p27免疫荧光染色,并对结果进行比较分析。结果IgG、C3、p27在多个猴、多种组织的相同位置出现相同模式的荧光表达,证明存在IC的沉着;其中脑血管周(8/8),心肌间微血管(6/8)、和淋巴结副皮质(6/8)及生发中心(5/8)是阳性率最高的部位,肾小球及肾间质、肠黏膜固有层也有较多IC的沉着,且在感染中、晚期IC出现的比例更高。结论SIV感染后出现广泛的SIV-IC沉积,且随病情的进展而加重;IC可能是SIV导致AIDS多系统病变的主要形式。针对此过程进行研究,可帮助了解AIDS并发多系统器官病变的机制及研究新的治疗方法。     

Apelin-13 induces ERK1/2 but not p38 MAPK activation through coupling of the human apelin receptor to the Gi2 pathway

Apelin signaling to the family of mitogen-activated protein kinases (MAPKs), such as extracellular-regulated kinases 1/2 (ERK1/2) and p38 MAPK, through the coupling of apelin receptor (APJ) to G-protein, mediates important pathophysiological responses. Although apelin fragments have been reported to induce ERK1/2 activation through G_i-protein, the intracellular pathways by which APJ activates these MAPKs are only partially understood. Here, using stably transfected human embryonic kidney 293 (HEK293) cells overexpressing human APJ (HEK293-apelinR), we showed that apelin-13 signaling leads to ERK1/2 and p38 MAPK pathways through APJ activation. It was found in HEK293-apelinR cells that ERK1/2 activation was initiated by apelin-13 at 5 min, with the peak of activation occurring at 15 min, and a return to the basal level within 60 min. The activation of ERK1/2 appeared to be dose-dependent with a significant activation being observed at 10 nM apelin-13 and maximal activation at 100 nM. However, phosphorylated-p38 MAPK was not detected in HEK293-apelinR cells treated with apelin-13. We also shown that the apelin-13-induced ERK1/2 activation requires a coupling with pertussis toxin-sensitive G-protein, and that overexpression of dominant-negative G_i2 completely inhibits the apelin-13-induced ERK1/2 activation. In addition, treatment with apelin-13 resulted in a concentration-dependent reduction of forskolin-stimulated cAMP production. It is therefore suggested that apelin-13 activates ERK1/2 but not p38 MAPK, which involves the coupling of APJ to the G_i2 cascade. In conclusion, the ERK1/ 2, but not p38 MAPKpathway is activated by apelin-13 through coupling of human APJ to G_i2-protein, which contributes to cellular responses.