用South-Western blot mapping方法观察锥虫VSG基因转录酶与基因组核酸片段的结合

应用South—Western blot mapping方法观察了初步提纯的锥虫转录变异抗原基因的聚合酶与其基因组DNA片段的结合情况.在选定的试验条件下,初步纯化的RNA聚合酶既能与变异抗原基因结合,也能与一些待鉴定的非特异性核酸片段结合.本文对存在的问题进行了讨论.

South-Western blot mapping方法的建立及其应用于锥虫细胞核中DNA结合蛋白的观察

South-Westerm blot mapping是一种结合Western blotting和Southern blotting某些特点的方法.本文介绍用其成功地观察到锥虫核蛋白中DNA结合蛋白的情况,并对一个分子量在40000左右、于较严谨条件下与DNA结合的核蛋白进行了特性鉴定.该蛋白等量地存在于锥虫的前循环期和血液期,对双链DNA有较大的亲和力,并能与酵母菌复制起始片段结合.本文还介绍了锥虫细胞核的提取技术和核蛋白的制备技术.

In Search of Regulators of <i>LeSPL-CNR</i>by South-Western Blotting and Yeast One-Hybrid Library Screening System

LeSPL-CNR is a crucial transcription factor for fruit ripening of Solanum lycopersicum. The cnr (colorless non-ripening) epimutation resulted from hypermethylation in a 286 bp region of LeSPL-CNR promoter inhibits normal fruit ripening. In present study, potential regulators of LeSPL-CNR, which could bind to the specific 286 bp region, were screened via south-western blotting and yeast one-hybrid (Y1H) library screening system. Results indicated that a total of 13 and 19 candidate proteins were acquired respectively, and both ribulose-1,5-bisphosphate carboxylase/oxygenase and 40S ribosomal protein were identified by two methods. These would provide some information for revealing roles of DNA methylation and the regulatory mechanism for LeSPL-CNR.

大鼠慢性间歇性低氧后氧自由基/JNK信号通路介导神经损伤的机制

目的探讨氧自由基/JNK信号通路在慢性间歇性低氧大鼠神经损伤中的作用。方法160只雄性SD大鼠随机分成对照组(n=40)、轻度间歇低氧组(n=40)、中度间歇低氧组(n=40)、重度间歇低氧组(n=40)。对照组暴露于空气中,间歇低氧组分别暴露于不同低氧条件下(100 ml/L、75 ml/L和50ml/L,暴露时间每天8 h,持续时间2、4、6、8周),电镜观察海马区神经细胞超微结构,采用硫代巴比妥酸法检测大脑组织丙二醛(MDA)水平;免疫印迹和免疫组化法检海马区磷酸化JNK和c-fos蛋白表达水平,原位缺口末端标记法(TUNEL)检测凋亡细胞。结果与对照组比较,随低氧时间的延长,三组间歇性低氧组大鼠海马神经元结构损伤;MDA水平、磷酸化JNK及c-fos表达增多,TUNEL阳性细胞增多(P<0.05);上述变化在重度间歇性低氧组最为显著(P<0.05);轻中度间歇性低氧组中MDA水平、磷酸化JNK及c-fos和TUNEL阳性细胞6周达高峰,两组比较二者差异无统计学意义;重度间歇性低氧组MDA水平、磷酸化JNK及c-fos和TUNEL阳性细胞8周达高峰,与轻中度间歇性低氧组比较,差异显著。结论慢性间歇性低氧后氧自由基激活的JNK信号通路,通过调控c-fos表达介导神经细胞凋亡。

机械应力下成骨细胞外信号调节激酶ERK1/2的早期变化

目的:观察体外培养的成骨样细胞在不同机械应力下细胞外信号调节激酶ERK1/2的表达变化.方法:采用四点弯曲细胞力学加载装置系统,对人成骨样细胞进行加力:频率0.5Hz,加力板变形量4000μstrain,按5,15,30min和1h不同时间段,使细胞发生单轴牵张和压缩应变.运用West-ernBlot检测不同方向、不同作用时间的应力应变下细胞外信号调节激酶ERK1/2所产生的变化.结果:在4000μstrain的周期性应力作用时,细胞外信号调节激酶ERK1/2在5min内被迅速激活,磷酸化程度大幅升高,牵张及压缩应力均有类似表现;1h左右恢复至基态水平.牵张应力所引发的ERK磷酸化较压缩应力更强,其差异有统计学意义(P<0.05).结论:较大的应力应变可以在早期激活成骨细胞内的MAPK/ERK信号转导通路,牵张应力所产生的效应较压缩应力更为明显,机械应力参与了细胞外信号调节激酶的活化.

重组真核质粒pEGFP-C2-hG3BP-Domain(1～5)的构建及表达

目的:将人类G3BP(Ras-GTPase activating protein SH3 domain binding protein)蛋白Domain(1～5)基因片段分别定向连入pEGFP-C2质粒,使G3BP蛋白各功能片段与绿色荧光蛋白在HeLa细胞内融合表达。方法:以重组质粒pEGFP-C1-G3BP为模板,PCR法扩增出目的基因,利用EcoRⅠ和BamHⅠ双酶切法将目的片段连接到pEGFP-C2载体上,再将构建成功的pEGFP-C2-hG3BP-Domain(1～5)重组质粒转染入HeLa细胞内,以荧光显微镜及Western印迹法检测绿色荧光蛋白与目的蛋白的融合表达情况。结果:以单/双酶切及基因测序法鉴定构建的重组质粒均无误,荧光显微镜及Western印迹结果均检测到绿色融合蛋白的表达。结论:重组pEGFP-C2-hG3BP-Domain(1～5)质粒成功构建并表达。

鹅源腺病毒基因组DNA物理图谱的构建

将鹅源腺病毒Y81G4 株全基因组DNA的HindⅢ酶切片段分别插入质粒 pUC18,成功构建了全基因组DNA文库。在此基础上 ,将重组质粒携带的插入片段切出、回收并分别用地高辛标记后作为探针 ,与经限制酶BamHI、EcoRI、PstI、EcoRV消化的病毒基因组DNA进行SouthernBlotting ,杂交结果经比较综合后获得了该病毒基因组DNA的HindⅢ、BamHI、EcoRI、PstI、EcoRV限制性内切酶的物理图谱。利用已发表的含有鸡EDS76病毒AA 2株基因组DNA右末端的重组质粒pBE4 2作为探针 ,与本病毒两末端重组质粒进行SouthernBlotting ,根据同源性杂交结果确定了本病毒基因组DNA物理图谱与EDSVAA 2株相应的方向。本病毒基础因组DNA物理图谱的精确构建 ,为进行基因组结构分析 ,筛选复制非必需区 。

混合血清孵育的肺腺癌组织双向蛋白印迹图谱的建立

目的:建立混合血清孵育的肺腺癌组织双向蛋白印迹图谱。方法:收集2例肺腺癌患者的手术标本,提取癌组织可溶性总蛋白并双向凝胶电泳分离,将蛋白转移到硝酸纤维素膜上,然后分别与4例肺腺癌患者的混合血清和4例良性肺部疾病患者(对照)的混合血清孵育2 h,再加入二抗羊抗人IgG反应2 h,DAB显色。结果:分别建立了肺腺癌混合血清和对照混合血清孵育的肺腺癌组织双向蛋白印迹图谱,两个图谱之间存在明显差异。结论:利用混合血清孵育的肺腺癌组织总蛋白能建立良好的双向蛋白印迹图谱,这为进一步鉴定肺腺癌肿瘤相关抗原奠定了基础。

玉米DNA限制性片段长度多态(RFLPs)的研究

文章简要介绍了10余年来有关玉米DNA限制性片段长度多态(RFLPs)的研究,说明RFLP的分析原理和特点,构建玉米RFLP连锁图的方法,以及玉米RFLPs在遗传育种中的主要应用。

电压门控快钾通道蛋白Kv4.3的抗体制备及检测

Kv4(voltagegatedK+channel4)是在哺乳动物心脏和脑组织中广泛表达的一类钾离子通道蛋白.它主要介导心肌细胞和神经细胞中的A-型(快速失活型)K+电流,是构成中枢神经系统和心肌细胞中的快速失活外向型电流的基础.Kv4.3是电压门控钾离子通道3种α亚基之一.通道中含有许多具有调节作用的辅助亚基,它们通过与Kv4.3互作实现对通道的调节.本研究根据人类氨基酸序列以MAPs法制备抗Kv4.3抗体.MAP由4条相同的17肽段连接成锥形结构分子.以MAP或MAP与佐剂免疫新西兰白兔,抽提了免疫前血清和免疫后血清,并对抗体的滴度进行评价.MAPs在白兔体内诱导出了效价比为1:1000的抗Kv4.3特异性抗体.

Overexpression of heme oxygenase-1 protects smooth muscle cells against oxidative injury and inhibits cell proliferation

To investigate whether the expression of exogenous heme oxygenase-1 (HO-1) gene within vascular smooth muscle cells (VSMC) could protect the cells from free radical attack and inhibit cell proliferation, we established an in vitro transfection of human HO-1 gene into rat VSMC mediated by a retroviral vector. The results showed that the profound expression of HO-1 protein as well as HO activity was 1.8- and 2.0-fold increased respectively in the transfected cells compared to the non-transfected ones. The treatment of VSMC with different concentrations of H2O2 led to the remarkable cell damage as indicated by survival rate and LDH leakage. However, the resistance of the HO-1 transfected VSMC against H2O2 was significantly raised. This protective effect was dramatically diminished when the transfected VSMC were pretreated with ZnPP-IX, a specific inhibitor of HO, for 24 h. In addition, we found that the growth potential of the transfected cells was significantly inhibited directly by increased activity of HO-1, and this effect might be related to decreased phosphorylation of MAPK. These results suggest that the overexpression of introduced hHO-1 is potentially able to reduce the risk factors of atherosclerosis, partially due to its cellular protection against oxidative injury and to its inhibitory effect on cellular proliferation.

Prokaryotical expression of structural and non-structural proteins of hepatitis G virus

AIM: To study the epitope distribution of hepatitis G virus (HGV) and to seek for the potential recombinant antigens for the development of HGV diagnostic reagents. METHODS: Fourteen clones encompassing HGV gene fragments from core to NS3 and NS5 were constructed using prokaryotic expression vector pRSET and (or) pGEX, and expressed in E.coli. Western blotting and ELISA were used to detect the immunoreactivity of these recombinant proteins. RESULTS: One clone with HGV fragment from core to E1 (G1), one from E2 (G31), three from NS3 (G6, G61, G7), one from NS5B (G821) and one chimeric fragment from NS3 and NS5B (G61-821) could be expressed well and showed obvious immunoreactivity by Western blotting. One clone with HGV framment from NS5B (G82) was also well expressed, but could not show immunoreactivity by Western blotting. No obvious expression was found in the other six clones. All the expressed recombinant proteins were in inclusion body form, except the protein G61 which could be expressed in soluble form. Further purified recombinant proteins G1, G31, G61, G821 and G61-821 were detected in indirected ELISA as coating antigen respectively. Only recombinant G1 could still show immunoreactivity, and the other four recombinant proteins failed to react to the HGV antibody positive sera. Western blotting results indicated that the immunoactivity of these four recombinant proteins were lost during purification. CONCLUSION: Core to E1, E2, NS3 and NS5 fragment of HGV contain antigenic epitopes, which could be produced in prokaryotically expressed recombinant proteins. A high-yield recombinant protein (G1) located in HGV core to E1 could remain its epitope after purification, which showed the potential that G1 could be used as a coating antigen to develop an ELISA kit for HGV specific antibody diagnosis.

Southwestern印迹图谱分析

Southwestern印迹图谱分折是近来研究DNA结合蛋白的理想方法,它可快速鉴定出DNA结合蛋白的分子量,还可确定基因组与蛋白质相结合的特异位置。 本文比较详细地介绍和讨论了核蛋白经SDS-聚丙烯酰胺凝胶电泳后,再转至硝酸纤维素膜上,利用不同的DNA探针与其结合,最后通过分析结合的复合物,确定DNA结合蛋白及其结合位置等操作步骤及关键问题。

赖型钩端螺旋体重组DNApCX7的特异性鉴定和限制性内切酶谱分析

本实验将赖型钩端螺旋体（简称钩体）ＤＮＡ基因库的克隆ｐＣＸ７制备成￣（３２）Ｐ－重组ＤＮＡ探针，对８个不同血清群的１７株问号状钩体、双曲钩体ＰａｔｏｃⅠ株以及细螺旋体３０５５株ＤＮＡ进行打点杂交；同时用１５种ＤＮＡ片断进行限制性内切酶谱分析。结果表明，该重组ＤＮＡ具有问号状钩体种（Ｓｐｅｃｉｅｓ）特异性，但与不同问号状钩体之间的同源性程度有差别；限制性内切酶谱分析发现ｐＣＸ７重组ＤＮＡ片段长约１．７ｋｂ，具有１个Ｂｇ１Ⅱ识别位点和３个ＢｓｔＢ１识别位点。

咖啡酸苯乙酯靶向调控人结肠癌HT-29细胞FAK-ERK信号通路的研究

目的探讨咖啡酸苯乙酯(caffeic acid phenethyl ester,CAPE)对结肠癌HT-29细胞FAK-ERK信号转导通路中相关蛋白表达的作用,寻找其作用靶点,试图阐明CAPE抗肿瘤作用的分子机制。方法用不同浓度CAPE处理HT-29细胞,利用Hoechst33258染色法和流式细胞术,检测细胞凋亡的发生。应用Western印迹法分析不同浓度CAPE对HT-29细胞中黏着斑激酶(focal adhesion kinase,FAK)和细胞外信号调节激酶(extracellular signal-regulatedkinase,ERK)蛋白表达的影响。结果 Hoechst33258染色发现CAPE作用后凋亡细胞数量增加。流式细胞仪细胞凋亡率分析显示,0,2.55,.0,7.5和10μg/ml处理HT-29细胞24 h后,细胞凋亡率上升,呈剂量依赖性。Western印迹结果显示,在0～10μg/ml范围内不同浓度CAPE作用于HT-29细胞24 h后,FAK、ERK蛋白表达随CAPE浓度的增加而下调。结论 CAPE可诱导人结肠癌HT-29细胞凋亡,其作用机制可能与CAPE抑制FAK-ERK信号转导通路的激活有关。