era因的高表达

为了高表达产生Era蛋白,借助计算机从Gene Bank中寻找N端几个氨基酸序列与Era相同的蛋白质,选其中能在大肠杆菌内高表达的λEa8．5蛋白,以其基因5’端序列替代天然ern基因5’端序列,从而赋予era基因转录物以强的翻译起始信号,而不改变其编码的氨基酸序列。将此重组era基因置于PL启动子下游、构建得质粒pCE3l,引入大肠杆菌TAPl06,经诱导后大量合成Era蛋白,且其他蛋白质的合成显著被抑制,从而使Era的含量能超过菌体总蛋白量的80％。经简单裂菌、洗涤步骤,就获得具有能特异结合鸟苷酸活性的、电泳单带纯的：Era蛋白。     

利用内蛋白子剪切功能一步纯化重组人神经营养因子-3

将人神经营养因子 - 3(h NT3)基因插入含内蛋白子 -几丁质结合区 (Intein- CBD)片段的质粒p TXB1的多克隆位点 ,构建成重组子 p TXB- h NT3,随后转化入 E.coli 2 566并进行融合表达 .表达产物包涵体经 8mol/ L脲变性 ,并在 GSH,GSSG存在下复性 .复性后的融合蛋白经几丁质珠亲和柱吸附 .待洗涤杂蛋白后 ,加入 50 mmol/ L DTT在 4℃或 2 5℃进行剪切反应 48h,再用缓冲液洗脱 ,即得 h NT3.SDS- PAGE分析表明 ,h NT3达电泳纯 .其分子量约为 1 4 k D     

PCR法检测水稻中存在Ras类蛋白基因家族(简报)

Ras类蛋白家族是普遍存在于动物及低等真核生物细胞中的一类单亚基GTP结合蛋白(20—29kDa),它们在一系列细胞过程中起重要作用。它们有GTP结合蛋白共有的作用机制。在刺激物诱导下,结合GTP成为活化状态,与效应子作用产生一定效应;GTP水解成GDP后恢复GDP结合状态,即非活化状态。它们通过GTPase驱动的构象变化的循环,作为“分子开关”起调控作用。目前已有40多种Ras类蛋白被发现,按结构可分为Ras、     

探索不同培养条件对大肠杆菌表达蛋白的影响

应用基因工程技术,在获得表达脱落酸受体蛋白PYL10的重组大肠杆菌菌株后,研究了表达时长、表达温度和诱导剂浓度对蛋白PYL10表达的影响。在22℃时加入200μmol/L IPTG时,设置变量诱导时间分别为0h、1h、2h、4h、8h、16h,结果发现诱导时长为16h时PYL10的表达量最高;其他条件相同时,探索诱导温度为4℃、15℃、22℃、37℃后发现在22℃下PYL10的表达量最高;同样,保持其他条件相同,改变IPTG浓度(0μmol/L、50μmol/L、100μmol/L、200μmol/L和400μmol/L)发现,在加入200μmol/L IPTG时PYL10的表达量是最高的。     

重组人MASP2蛋白在大肠杆菌中的表达和纯化

目的:获得酶原形式的重组人甘露聚糖结合凝集素相关丝氨酸蛋白酶2(MASP2)。方法:在大肠杆菌中诱导表达重组人MASP2全长蛋白,包涵体裂解后,经复性、透析、浓缩、考马斯亮蓝染色、SDS-PAGE及Western印迹,鉴定纯化结果及酶活性。结果:复性后的MASP2蛋白经考马斯亮蓝染色未见杂带。自激活实验表明,当MASP2浓度在1μmool/L以下时,无论在4℃还是37℃,都能较稳定地保持酶原形式;蛋白浓度为3.5μmool/L时只能在4℃保持稳定,37℃发生自激活;蛋白浓度达到12μmool/L后,在4℃时已不能稳定存在。结论:获得了较纯的重组人MASP2蛋白,且具有自激活活性。     

生物体内形形色色的G蛋白

G蛋白是一类可与GTP和GDP结合的蛋白,结合GTP时具有活性,结合GDP时为非活性状态,通过G蛋白活性和非活性状态的变化来打开或关闭细胞内某一过程,因此G蛋白也被称为分子开关。对存在于生物体内的一些G蛋白进行了简要的介绍。     

利用双启动子表达载体pDH2-YggG-Ptac-Era研究E. coli Era和YggG 蛋白间的相互关系

yggG是从大肠杆菌全基因组文库中钓取并克隆的Era结合蛋白基因,研究表明该基因表达的YggG294(amino acids 1-294)蛋白对宿主菌的生长具有强烈的抑制作用。为了阐明YggG与Era间的相互关系,构建可同时可控性表达Era和YggG294蛋白的双启动子表达载体。利用所构建的双启动子表达载体在同一细胞中同时可控性地表达YggG294与Era蛋白。结果显示,在不表达和少量表达YggG294的细菌细胞内,Era 的表达量与总蛋白量的比值随着诱导时间增加而增高,而YggG294大量表达的细菌内Era 的表达量与总蛋白量的比值基本保持不变;Era 蛋白的预表达对YggG294表达所引起的细菌生长率下降无影响。由此可以推论,YggG294的过表达引起宿主菌生长抑制进而影响了Era蛋白的进一步表达,而YggG294的过表达引起宿主菌生长抑制与YggG和Era蛋白间的相互作用无关     

铜胁迫下海州香薷根中铜诱导蛋白的鉴定

以铜耐性植物海州香薷为材料,在水培条件下对其幼苗进行不同浓度的CuSO4处理,通过铜结合蛋白分析和双向电泳(2D-AGE)分析,研究铜胁迫条件下海州香薷根中铜诱导蛋白的结合方式及表达情况.结果表明(1)100μmol/L CuSO4处理海州香薷幼苗6 d,可使其根中蛋白巯基的含量显著升高.(2)将其蛋白提取液通过SephadexG-50后,发现洗脱液中铜诱导物的增加与铜分布显著相关,表明铜诱导蛋白可能为铜结合蛋白.(3)通过2D-PAGE和质谱分析发现,铜胁迫下类抗性蛋白、S-腺苷甲硫氨酸合成酶和脂肪酸羟化酶的表达升高,而抗坏血酸过氧化物酶和半胱氨酸合成酶表达则降低.     

血管紧张素Ⅱ和阿片肽对Fos蛋白表达的影响

利用抗体免疫沉淀技术研究了血管紧张素Ⅱ(AⅡ),δ受体激动剂(DPDPE)和к受体激动剂(NDAP)对大鼠脑组织c-fos原癌基因表达的影响.结果表明,0.1μmol/LAⅡ可显著刺激脑组织中Fos蛋白的表达,0.1μmol/L DPDPE和0.1μmol/L NDAP对Fos蛋白的表达亦有一定的诱导作用.AⅡ与DPDPE或NDAP共同处理组织,Fos蛋白表达水平低于AⅡ单独诱导的水平.结果表明阿片肽可抑制AⅡ对Fos蛋白表达的作用.     

体外化学诱导人骨髓间充质干细胞分化为心肌样细胞

为了探讨人骨髓间充质干细胞(MSCs)的体外培养及化学诱导向心肌细胞分化的过程及条件,我们用1.073g/mL密度梯度离心法分离健康人骨髓单个核细胞,经骨髓间充质干细胞培养基传代培养后用流式细胞仪检测细胞表面抗原,在完全培养基中分别加入3、5、10μmol/L的5氮胞苷(每组n=5)进行化学诱导分化,阴性对照组采用完全培养基培养,诱导后21天细胞爬片免疫荧光法鉴定,透射电镜观察细胞超微结构。结果显示人MSCs为形态均一的梭形细胞,生长旺盛时呈旋涡样分布,流式细胞仪检测细胞表面CD44阳性,CD34、CD45阴性;5、10μmol/L的5氮胞苷进行化学诱导后细胞形态变长,诱导后14天时20%-30%细胞融合形成多核肌管样结构,3μmol/L组MSCs未出现肌管结构,诱导后21天5、10μmol/L组MSCs中desmin、心肌早期转录因子GATA4、心肌特异性cTnI及闰盘蛋白connexin43的表达阳性,10μmol/L组cTnI阳性染色细胞数目(65.3±4.7%)高于5μmol/L诱导组(48.2±5.4%)(p<0.05);3μmol/L组及阴性对照组无心肌特异性蛋白的表达。细胞诱导后28天透射电镜下可见肌丝形成。本实验说明,人MSCs在体外经化学诱导可分化为心肌样细胞,而且5-氮胞苷对于心肌相关蛋白的表达呈浓度依赖性正相关。     

Membrane-dependent guanine nucleotide binding and GTPase activities of soluble protein from bovine rod cell outer segments.

Soluble proteins can be extracted by osmotic shock of purified rod (photoreceptor cell) outer segments that have intact plasma membranes. The soluble proteins include a component that contains tightly bound GDP-Exchange of this GDP with exogenous nucleotide is catalyzed by (and requires) the membranes from the outer segments. ATP does not participate in these reactions. Approximately one-half of the binding sites in the soluble component require GTP as the source of exogenous nucleotide; the remainder accept GTP or GDP with equal facility. When exogenous GTP is the source of bound nucleotide, it is found in the complex in the form of GDP. Exchange of bound nucleotide with GTP is stoichiometrically related to GTPase activity; this activity is highly dependent upon the presence of both membranes and soluble protein. The soluble nucleotide binding protein was purified by making use of the fact that it binds tightly to the membranes (under conditions of moderate ionic strength) in the absence of GTP and can be eluted by solutions containing low concentrations of GTP (but not GDP or ATP, nor can it be eluted by GTP-free solutions of low ionic strength). The purified protein contains two polypeptide chains of molecular weights 41,000 and 37,000; these are the major species that can be extracted from the outer segments by osmotic shock, and they constitute approximately 7% of the total protein of the isolated organelle.     

Characterization of the autophosphorylation of Era, an essential Escherichia coli GTPase

Era is an essential protein in Escherichia coli which binds both GTP and GDP and has an intrinsic GTPase activity. Studies on the role of GTP/GDP binding and GTPase activity in an attempt to understand its function lead to the observation that Era is autophosphorylated. The autophosphorylated reaction is specific for GTP and cannot use ATP as a phosphoryl group donor. The reaction velocity is of first order with respect to protein concentration, suggesting an intramolecular mechanism. Autophosphorylation occurs at serine and threonine residues. The major phosphorylated tryptic peptide isolated after autophosphorylation has been identified as ISITSR, from residue 33 to 38. The peptide contains the site of phosphorylation and two potential sites for serine and threonine phosphorylation. Subsequently, both the threonine residue at position 36 and the serine residue at position 37 were altered to alanine. The double mutant Era, but not individual single mutants, was unable to functionally complement the growth of an E. coli strain which cannot produce wild-type Era protein at high temperature. This suggests that either threonine 36 or serine 37 has to exist for the function of Era In vivo. phosphorylation of Era was also examined by two-dimensional gel electrophoresis. Era has been previously assigned two distinct positions having two different X-Y co-ordinates: one of the spots (H032.0) was identified as phosphorylated Era, indicating that a substantial portion of Era in the cell is indeed phosphorylated. Therefore, Era autophosphorylation is likely to play an important physiological role in the cell. The sequence encoding the C-terminus previously published had a missing C between A900 and GgO1. As a resuit of the frameshift, Era consists of 301 residues, 15 fewer than originaiiy reported.     

Dephosphorylation of tubulin-bound guanosine triphosphate during microtubule assembly.

1. Tubulin purified from porcine brain in the presence of GTP contained 0.16 mole of GDP and 0.73 mole of GTP per 60,000 g of protein. 2. Microtubules reconstituted from the purified tubulin contained 0.43 mole of GDP and 0.41 mole of GTP per 60,000 g of protein. Guanine nucleotide bound to the exchangeable site of tubulin was converted to GDP during microtubule assembly, while GTP at the non-exchangeable site remained intact. 3. Guanine nucleotide which had been bound to the exchangeable site of tubulin before microtubule assembly was also exchangeable during disassembly.     

神经节苷脂GM_3对人单核样白血病J6-2细胞中磷脂代谢的影响

用50μmol/L GM_3处理J6-2细胞6天,经组化与细胞学检查,证实细胞沿单核巨噬细胞途径分化。以[~(32)P]Pi或[CH_3-~(14)C]胆碱冲激(Pulse)后,将洗净的细胞进行Folch分配。取下相进行薄层层析,再做放射自显影。结果表明:GM_3的处理能促进[~(32)P]Pi或[CH_3-~(14)C]胆碱向磷脂酰胆碱的参入,而抑制向其他磷脂组分的参入。用[CH_3-~(14)C]胆碱冲激的Folch分配上相含水溶性胆碱代谢物,经TLC,结果表明CM_3的处理使[CH_3-~(14)C]胆碱向CDP-胆碱的参入减少。本研究证实,GM_3能调节J6-2细胞的磷脂代谢,其调节机制值得研究。     

Era, an essential Escherichia coli small G-protein, binds to the 30S ribosomal subunit.

Era is an essential G-protein in Escherichia coli identified originally as a homologue protein to Ras (E. coli Ras-like protein). It binds to GTP/GDP and contains a low intrinsic GTPase activity. Its function remains elusive, although it has been suggested that Era is associated with the cytoplasmic membrane, cell division, energy metabolism, and cell-cycle check point. Recently, a cold-sensitive phenotype was found to be suppressed by the overexpression of 16S rRNA methyltransferase, suggesting Era association with the ribosome. Here we demonstrate that Era specifically binds to 16S rRNA and the 30S ribosomal subunit. Both GTP and GDP, but not GMP, inhibit Era binding to ribosomal component. Involvement of Era in protein synthesis is suggested by the fact that Era depletion results in the translation defect both in vitro and in vivo.     

Solubilization of receptors for thyrotropin-releasing hormone from GH4C1 rat pituitary cells: demonstration of guanyl nucleotide sensitivity

TRH receptors have been solubilized from GH4C1 cells using the plant glycoside digitonin. Solubilized receptors retain the principal binding characteristics exhibited by the TRH receptor in intact pituitary cells and their membranes. The binding of the methylhistidyl derivative of TRH [( 3H]MeTRH) attained equilibrium within 2-3 h at 4 C, and it was reversible, dissociating with a t1/2 of 7 h. Analysis of [3H]MeTRH binding to soluble receptors at 4 C yielded a dissociation constant (Kd) of 3.8 nM and a total binding capacity (Bmax) of 3.9 pmol/mg protein. Peptides known to interact with non-TRH receptors on GH cells failed to interfere with the binding of [3H]MeTRH, indicating that the TRH binding was specific. Chlordiazepoxide, a competitive antagonist for TRH action in GH cells, inhibited TRH binding to soluble receptors with an IC50 of 11 microM. When [3H]MeTRH was bound to membranes and the membrane proteins were then solubilized, we found enhanced dissociation of the prebound [3H]MeTRH from its solubilized receptor by guanyl nucleotides. Maximal enhancement of [3H]MeTRH dissociation by 10 microM GTP gamma S occurred within about 45 min at 22 C. GTP gamma S, GTP, GDP beta S, and GDP were all effectors of [3H]MeTRH dissociation, exhibiting EC50s in the range of 14-450 nM. The rank order of potency of the tested nucleotides was GTP gamma S greater than GTP congruent to GDP beta S greater than GDP much greater than ATP gamma S greater than GMP. We conclude that TRH receptors have been solubilized from GH cells with digitonin and retain the binding characteristics of TRH receptors in intact pituitary cells. Furthermore, prebinding [3H]MeTRH to GH4C1 cell membranes results in the solubilization of a complex in which the TRH receptor is linked functionally to a GTP binding protein.     

Guanosine 5''-[gamma-thio]triphosphate-stimulated hydrolysis of phosphatidylinositol 4,5-bisphosphate in HL-60 granulocytes. Evidence that the guanine nucleotide acts by relieving phospholipase C from an inhibitory constraint.

Myeloid differentiated human leukaemia (HL-60) cells contain a soluble phospholipase C that hydrolysed phosphatidylinositol 4.5-bisphosphate and was markedly stimulated by the metabolically stable GTP analogue guanosine 5'-[gamma-thio]triphosphate (GTP[S]). Half-maximal and maximal (up to 5-fold) stimulation of inositol phosphate formation by GTP[S] occurred at 1.5 microM and 30 microM respectively. Other nucleotides (GTP, GDP, GMP, guanosine 5'-[beta-thio]diphosphate. ATP, adenosine 5'-[gamma-thio]triphosphate, UTP) did not affect phospholipase C activity, GTP[S] stimulation of inositol phosphate accumulation was inhibited by excess GDP, but not by ADP. The effect of GTP[S] on inositol phosphate formation was absolutely dependent on and markedly stimulated by free Ca2+ (median effective concn. approximately 100 nM). Analysis of inositol phosphates by anion-exchange chromatography revealed InsP3 as the major product of GTP[S]-stimulated phospholipase C activity. In the absence of GTP[S], specific phospholipase C activity was markedly decreased when tested at high protein concentrations, whereas GTP[S] stimulation of the enzyme was markedly enhanced under these conditions. As both basal and GTP[S]-stimulated inositol phosphate formation were linear with time whether studied at low or high protein concentration, these results suggest that (a) phospholipase C is under an inhibitory constraint and (b) GTP[S] relieves this inhibition, most likely by activating a soluble GTP-binding protein.     

Expression of p21 proteins in Escherichia coli and stereochemistry of the nucleotide-binding site.

v-Ha-ras encoded p21 protein (p21V), the cellular c-Ha-ras encoded protein (p21C) and its T24 mutant form p21T were produced in Escherichia coli under the control of the tac promoter. Large amounts of the authentic proteins in a soluble form can be extracted and purified without the use of denaturants or detergents. All three proteins are highly active in GDP binding, GTPase and, for p21V, autokinase activity. Inhibition of [3H]GDP binding to p21C by regio- and stereospecific phosphorothioate analogs of GDP and GTP was investigated to obtain a measure of the relative affinities of the three diphosphate and five triphosphate analogs of guanosine. p21 has a preference for the Sp isomers of GDP alpha S and GTP alpha S. It has low specificity for the Sp isomer of GTP beta S. Together with the data for GDP beta S and GTP gamma S these results are compared with those obtained for elongation factor (EF)Tu and transducin. This has enabled us to probe the structural relatedness of these proteins. We conclude that p21 seems to be more closely related to EF-Tu than to transducin.     

Purification of the 22 kDa protein substrate of botulinum ADP-ribosyltransferase C3 from porcine brain cytosol and its characterization as a GTP-binding protein highly homologous to the rho gene product

The 22 kDa protein substrate of botulinum ADP-ribosyltransferase C3 was purified from porcine brain cytosol by acetone precipitation, CM-Sephadex, octyl-Sepharose and TSK phenyl-5PW HPLC chromatography to apparent homogeneity. ADP-ribosylation of the protein was increased by guanine nucleotides (GTP, GDP, GTP gamma S, each 100 microM) but not by GMP, ATP or ATP gamma S. The purified 22 kDa protein bound maximally 0.9 mol [35S]GTP gamma S and hydrolyzed GTP with the rate 0.007 mol per mol protein. Amino acid sequences were obtained from two tryptic peptides, selected from an in situ digestion of Immobilon electrotransferred, gel purified ADP-ribosylated substrate. The two sequences obtained, cover 23 residues from the corresponding sequences in human rho.