生长激素和生长激素受体的分子生物学

1 .生长激素的结构生长激素 (ｇｒｏｗｔｈｈｏｒｍｏｎｅ ,ＧＨ)一般含有 1 91个氨基酸 ,约 2 2ｋＤ。猪与牛的ＧＨ氨基酸序列具有高度的同源性 (约 90 % ) [1] 。猪和牛的ＧＨ对人没有促进生长的作用 ,可能是猪和牛ＧＨ对人的生长激素受体(ｇｒｏｗｔｈｈｏｒｍｏｎｅｒｅｃｅｐｔｏｒ ,ＧＨＲ )的结合亲和性低于人ＧＨ对人ＧＨＲ的结合亲和性的缘故。ＧＨｍＲＮＡ翻译的初级产物是前生长激素 ,它比成熟ＧＨ在Ｎ端多出 2 6个氨基酸残基的疏水信号肽[2 ] 。通过Ｘ射线衍射技术等研究发现 ,ＧＨ由 4个螺旋组成 ,自Ｎ端至Ｃ端依次为螺旋 1～ …     

生长激素结合蛋白

动物的生长调控作用中垂体分泌的生长激素 (ＧＨ)起着重要的作用。ＧＨ的生理调控作用的发挥又与血液中的生长激素结合蛋白(ｇｒｏｗｔｈｈｏｒｍｏｎｅｂｉｎｄｉｎｇｐｒｏｔｅｉｎ ,ＧＨＢＰ)以及靶细胞膜上的生长激素受体 (ｇｒｏｗｔｈｈｏｒｍｏｎｅｒｅ ｃｅｐｔｏｒ,ＧＨＲ)的作用不可分割。这三者以及下丘脑的生长激素释放因子 (ＧＨｒｅｌｅａｓｅｆａｃ ｔｏｒ ,ＧＨＲＦ) ,还有垂体的生长抑素 (ｓｏｍａｔｏ ｓｔａｔｉｎ ,ＳＳ)等共同构成动物的内分泌生长轴(ｓｏｍａｔｏｔｒｏｐｉｃａｘｉｓ) ,对动物的生长发育起着决定性的…     

抗HBsAg二硫键稳定性Fv抗体（dsFv）基因的构建与表达

采用ＰＣＲ定点突变方法,成功地构建了抗ＨＢｓＡｇｄｓＦｖ抗体的轻、重链突变基因,ＮｄｅＩ和ＥｃｏＲＩ酶切后分别插入ｐＥＴ２０ｂ表达质粒,经测序证明在重链第４４位氨基酸和轻链第１００位氨基酸已突变形成半胱氨酸（Ｃｙｓ）。ＶＨ和ＶＬ重组质粒分别转化到大肠肝菌ＢＬ２１（ＤＥ３）中,ＩＰＴＧ诱导后,经ＳＤＳＰＡＧＥ电泳表明在１２ｋＤ处有包含体蛋白表达,表达蛋白含量分别为２８％和３５％。ＶＨ和ＶＬ包含体蛋白经ＧｕＨＣｌ变性后,等量混合在复性折叠液中结合,形成了一个约２４ｋＤ并有一定活性的ｄｓＦｖ蛋白。抗ＨＢｓＡｇｄｓＦｖ抗体表达及复性的成功,为今后基因工程抗体的研究及应用奠定了基础。     

白细胞介素—2—绿脓杆菌外毒素融合蛋白的分高纯化及其复性研究

表达的白细胞介素－２－绿脓杆菌外毒素（ＩＬ－２－ＰＥ）融合蛋白以包含体形式存在于宿主菌中,为分离纯化表达产物提供了方便,但因需进行复性,也增加了后处理的难度．我们采用４ｍｏｌ／Ｌ尿素、０．５％ＴｒｉｔｏｎＸ－１００的１×ＰＢＳ洗涤包含体两遍,再经ＳｅｐｈａｃｒｙｌＳ－３００分子筛及ＤＥＡＥ－ＳｅｐｈａｒｏｓｅＦＦ阴离子交换柱层析后,获得的融合蛋白纯度可达９０％～９５％。此外,我们从ＧＳＳＧ浓度、Ｌ－精氨酸浓度、复性蛋白质的起始浓度、复性液的ｐＨ值、复性温度及复性时间等参数入手,系统地研究了融合蛋白的复性条件,探索到了ＩＬ－２－ＭＥ４０和ＩＬ－２－ＰＥ６６４Ｇｌｕ融合蛋白复性的最适条件。     

猪生长激素基因表达质粒的构建及其转基因动物研究

将猪生长激素基因（ＰＧＨ）克隆到质粒ｐＵＣ１９上,经酶切分析,确定其酶切图谱．把ＰＧＨ转录起始位点以前的序列切掉,换上羊ＭＴ－１ａ基因的启动子,构建成可以调控的表达载体ｐＳＭＴＰＧＨ,用于转基因动物的研究．采用微注射法将线状ｐＳＭＴＰＧＨ导入猪、鼠和金鱼的受精卵中,得到了相应的转基因动物．对这些动物鉴定分析表明,外源基因整合率因动物不同而异,但该基因在这３种动物中的整合率均在９％以上,其生长速度都高于对照组．     

猪生长激素基因表达质粒的构建及其转基因动物研究

将猪生长激素基因（ＰＧＨ）克隆到质粒ｐＵＣ１９上,经酶切分析,确定其酶切图谱。把ＰＧＨ转录起始位点以前的序列切掉,换上羊ＭＴ－１ａ基因的启动子,构建成可以调控的表达载体ｐＳＭＴＰＧＨ,用于转基因动物的研究。采用微注射法将线状ｐＳＭＴＰＧＨ导入猪、鼠和金鱼的受精卵中,得到了相应的转基因动物。对这些动物鉴定分析表明,外源基因整合率因动物不同而异,但该基因在这３种动物中的整合率均在９％以上,其生长速度都     

雌性激素影响大鼠生长激素结合蛋白水平

雌性激素影响大鼠生长激素结合蛋白水平在正常大鼠中,雌性鼠循环血中的生长素结合蛋白（ＧＨＢＰ）水平比雄性鼠高,而在生长素缺乏的侏儒鼠,血浆中的ＧＨＢＰ没有性别差异。为了研究性激素和生长素在ＧＨＢＰ和生长素受体调节上的作用,作者用正常鼠、侏儒鼠、切除垂体...     

VISTA-Ig融合蛋白的表达及其包涵体复性研究

[目的]构建VISTA-Ig融合蛋白表达载体,进行诱导表达获得VISTA-Ig融合蛋白。[方法]以C57BL/6小鼠脾脏细胞c DNA为模板,扩增小鼠VISTA胞外段基因,利用重叠延伸PCR的方法合成VISTA-Ig融合基因,构建重组质粒p ET-22b-VISTA-Ig,在大肠杆菌表达菌株E.coli BL21(DE3)中诱导表达。[结果]VISTA-Ig融合蛋白主要以包涵体的形式存在。变性后,利用镍柱纯化,通过采用氧化型/还原型谷胱甘肽(GSH/GSSG)复性体系,复性效率达到80%以上,提高了复性效率。利用r Protein A柱对目标蛋白进一步纯化,Western Blot鉴定结果显示,能与Ig G Fc(HRP)抗体特异性结合。[结论]成功构建了重组质粒p ET-22b-VISTA-Ig,纯化的VISTA-Ig包涵体蛋白复性效率得到明显提高,为后续VISTA-Ig免疫学功能的研究奠定了基础。     

猪囊尾蚴CE18重组蛋白的复性纯化及抗原性鉴定

猪囊尾蚴CE18重组蛋白(rCE18)在大肠杆菌表达后形成包涵体, 为了获得高纯度的、有生物活性的rCE18, 本研究采用超声破碎菌体, 0.2%、2% DOC(脱氧胆酸钠)逐次洗涤包涵体及0.9% SKL(十二烷基肌氨酸钠)溶解包涵体后, 利用透析与凝胶过滤层析技术相结合对rCE18进行复性和纯化。同时, 采用GST-FF亲和柱层析及SDS-PAGE胶回收蛋白两种方法纯化rCE18, 比较三者的纯化效果。并通过间接ELISA检测复性蛋白的生物学活性。结果表明: 经透析与凝胶层析复性纯化后的rCE18蛋白的纯度可达到60%以上, 活性回收率为41.3%, 间接ELISA证实, 复性后的rCE18蛋白能特异性识别猪囊虫阳性血清, 检测敏感性高达97.2%, 与全囊虫抗原检测的符合率为100%。本试验初步建立了猪囊尾蚴rCE18包涵体纯化及复性的有效方法, 为猪囊尾蚴rCE18蛋白的诊断应用奠定了基础。     

重组蛋白ApSerpin-FA72的包涵体复性及活性研究

[目的]原核表达及制备重组光滑鳖甲丝氨酸蛋白酶抑制剂(Ap Serpin-FA72),探索包涵体最优复性条件与最适酶反应条件。[方法]采用超声破碎获得大量包涵体,通过包涵体的洗涤、包涵体的溶解方法对包涵体进行纯化,获得高纯度的包涵体进行复性液成分与复性方法的摸索。测定Trx A-Ap Serpin-FA72对胰蛋白酶的IC50、最适反应p H和最适反应温度。[结果]在32℃、180 r/min、0. 4 mmol/L IPTG浓度下以沉淀形式表达大量蛋白,通过包涵体复性在含有L-精氨酸复性液中获得有生物活性的Trx A-Ap Serpin-FA72,对胰蛋白酶的IC50为0. 48μmol/L,p H在7～9,温度在60℃时有较高的抑制活性。[结论]L-精氨酸是复性液中重要的组成部分,复性的重组蛋白Trx A-Ap SerpinFA72对胰蛋白酶有较强的抑制能力,是一种热稳定较好的弱碱性胰蛋白酶抑制剂。     

Human apolipoprotein E3 in aqueous solution. I. Evidence for two structural domains

The stability and structure of human apolipoprotein (apo) E3 in aqueous solution were investigated by guanidine HCl denaturation and limited proteolysis. The guanidine HCl denaturation curve, as monitored by circular dichroism spectroscopy, was biphasic; the two transition midpoints occurred at 0.7 and 2.5 M guanidine HCl, indicating that there are stable intermediate structures in the unfolding of apoE. Limited proteolysis of apoE with five enzymes demonstrated two proteolytically resistant regions, an amino-terminal domain (residues 20-165) and a carboxyl-terminal domain (residues 225-299). The region between them was highly susceptible to proteolytic cleavage. Because of their similarity to the proteolytically resistant regions, the amino-terminal (residues 1-191) and carboxyl-terminal (residues 216-299) thrombolytic fragments of apoE were used as models for the two domains. Guanidine HCl denaturation of the carboxyl- and amino-terminal fragments gave transition midpoints of 0.7 and 2.4 M guanidine HCl, respectively. The results establish that the two domains identified by limited proteolysis correspond to the two domains detected by protein denaturation experiments. Therefore, the thrombolytic fragments are useful models for the two domains. The free energies of denaturation calculated from the denaturation curves of intact apoE or the model domains were approximately 4 and 8-12 kcal/mol for the carboxyl- and amino-terminal domains, respectively. The value for the carboxyl-terminal domain is similar to those of previously characterized apolipoproteins, whereas the value for the amino-terminal domain is considerably higher and resembles those of soluble globular proteins. These studies suggest that, in aqueous solution, apoE is unlike other apolipoproteins in that it contains two independently folded structural domains of markedly different stabilities: an amino-terminal domain and a carboxyl-terminal domain, separated by residues that may act as a hinge region.     

A Comparative Investigation on Different Refolding Strategies of Recombinant Human Tissue-type Plasminogen Activator Derivative

Recombinant human tissue-type plasminogen activator derivative (r-PA), fused with thioredoxin (Trx), was expressed in Escherichia coli. The resultant fusion protein, Trx-r-PA, was almost completely in the form of inclusion bodies and without activity. Different refolding strategies were investigated including different post-treatment of solubilized Trx-r-PA inclusion bodies, on-column refolding by size-exclusion chromatography (SEC) using three gel types (Sephacryl S-200, S-300 and S-400), refolding by Sephacryl S-200 with a urea gradient and two-stage temperature control in refolding. An optimized on-column refolding process for Trx-r-PA inclusion bodies was established. The collected Trx-r-PA inclusion bodies were dissolved in 6 m guanidine hydrochloride (Gdm·HCl), and the denatured protein was separated from dithiothreitol (DTT) and Gdm·HCl with a G25 column and simultaneously dissolved in 8 m urea containing oxidized glutathione (GSSG). Finally a refolding of Trx-r-PA protein on Sephacryl S-200 column with a decreasing urea gradient combined with two-stage temperature control was employed, and the activity recovery of refolded protein was increased from 3.6 to 13.8% in comparison with the usual dilution refolding. Revisions requested 31 October 2005; Revisions received 20 December 2005     

一种丹参高质量总RNA的提取方法

高质量RNA的获得是开展丹参分子生物学研究的基础。采用异硫氰酸胍(Guanidine Thiocyanate,GT)法、尿素法、CTAB法、苯酚法和热硼酸改良法等五种方法．以丹参组织培养的幼苗为材料,进行丹参RNA的分离试验,发现所采用的几种方法获得的RNA都有不同程度的降解。分析可能是由于丹参中含有大量的多糖以及各种次生代谢成分造成的。在分析现有结果的基础上对GT法进行了改良,在第二次沉淀前附加低浓度乙醇(10％～20％)沉淀20min对于高质量总RNA的获得效果较好。琼脂糖凝胶电泳检测改良后的GT法无论对于组织培养中幼嫩的根、茎、叶还是大田两年生的丹参根、茎、叶和种子均具有很好的RNA分离效果。mRNA电泳检测发现所得mRNA集中分布在500b～3kb之间且质量较高,完全可以满足丹参各种RNA相关的分子生物学实验要求,为丹参RT—PCR、Northern杂交等分子生物学实验提供了良好的基础。     

Expression of recombinant human nerve growth factor in Escherichia coli.

Nerve growth factor (NGF) is a neurotrophic factor for basal forebrain cholinergic neurons and may be of benefit in neurodegenerative diseases of humans. A method is described to obtain significant amounts of biologically active recombinant human NGF (rhNGF) in one step. RhNGF was expressed in E. coli and the majority of the protein accumulated in inclusion bodies. It was immunoprecipitated by a serum against mouse NGF. Solubilization of the inclusion bodies was done in 3M guanidine HCl and renaturation was effected by dilution and air oxidation in the presence of 6 microM CuSO4. Recoveries were 10-12 micrograms of rhNGF per ml of bacterial suspension. Its biological activity was tested in a bioassay system employing sympathetic chick embryo ganglia and was inhibited by the monoclonal antibody 27/21 against mouse NGF.     

单纯疱疹病毒1型囊膜糖蛋白gD在大肠杆菌中的表达、纯化及其免疫活性的鉴定

目的:在大肠杆菌中表达1型单纯疱疹病毒(HSV-1)囊膜糖蛋白gD,纯化重组蛋白并对其免疫活性进行鉴定。方法:将HSV-1 gD 基因克隆入原核表达载体pET-28b,利用异丙基-B-D-硫代吡喃半乳糖苷(IPTG)诱导重组质粒转化的大肠杆菌,探讨IPTG浓度、诱导时间、诱导温度对重组蛋白表达的影响;盐酸胍裂解变性包涵体,镍柱亲和层析法纯化gD蛋白,并对纯化后的蛋白进行透析复性;Western blot和ELISA检测gD蛋白的免疫活性。结果:酶切和测序结果表明gD基因克隆入pET-28b载体。该重组质粒转化的大肠杆菌经IPTG诱导后重组蛋白主要以包涵体形式存在,大小约40kDa。gD蛋白诱导表达的最佳条件为0.5mmol/L IPTG于37℃诱导8h。镍柱亲和层析法纯化获得的gD蛋白总量为3.1mg/L,透析复性后获得的gD蛋白总量为1.3mg/L,复性率为41.37%。Western blot及ELISA检测表明表达的gD蛋白具有免疫活性。结论:在大肠杆菌中表达并纯化获得具有免疫活性的HSV-1 gD蛋白,为进一步制备HSV-1诊断试剂和预防疫苗奠定了基础。     

Effects of urea and guanidine · HCl on the folding and unfolding of pancreatic trypsin inhibitor

Concentrated solutions of urea and of guanidine · HCl produced a random spectrum of single-disulphide forms of the polypeptide chain of the pancreatic trypsin inhibitor. Guanidine · HCl also unfolded completely, with accompanying interchange of disulphide bonds, the two-disulphide form of this protein in the native-like conformation; urea produced an equilibrium mixture in which one-quarter of the molecules had the native-like conformation and disulphide bonds. The unfolded forms of the protein in the denaturants were very flexible polypeptide chains. The observations suggest that urea and guanidine · HCl are denaturants because they produce essentially equally favourable solvation of all portions of a polypeptide.The energetics of the conformational transitions involved in folding and unfolding of the inhibitor were determined in urea and compared with those observed in its absence. The denaturant lowers the stability of the native, folded inhibitor relative to that of the reduced, unfolded state by 6.5 kilocalories per mole; the greatest part of this apparent free-energy difference was expressed at the two-disulphide stage of folding. The results are consistent with other indications that most of the favourable interactions stabilizing the native conformation of this protein are not encountered until the final stage of folding, when all may occur simultaneously.The unfolded one- and two-disulphide species produced in guanidine · HCl were trapped, and their rearrangement to the normal intermediates followed after removal of the denaturant. The random single-disulphide species, with one exception, reverted very rapidly to the non-random spectrum of intermediates normally observed during folding; this confirms that these species are normally rapidly interconverted and that normal refolding of the reduced protein is not dependent kinetically upon residual stable conformation in the reduced protein. The unfolded two-disulphide species refolded to the native-like conformation more slowly, but appeared to pass through the same intermediates normally observed during refolding from the fully reduced state.     

Cloning, expression, and characterization of Mycobacterium tuberculosis dihydrofolate reductase

The gene for dihydrofolate reductase of Mycobacterium tuberculosis was amplified by polymerase chain reaction (PCR) from M. tuberculosis H37Rv strain genomic DNA. The protein was expressed in inclusion bodies in high yield in Escherichia coli under the control of the T7 promoter. Active enzyme was obtained by refolding from guanidine HCl and after a single chromatography step the sample was > 99% homogeneous with a specific activity of approximately 15.5 micromol min(-1) mg(-1). Mass spectrometry analysis confirmed the expected mass of 17.6 kDa. Gel filtration of the enzyme indicated that it was a monomer. Steady-state kinetic parameters were determined and the effect of pH and KCl on the enzyme examined. Methotrexate and trimethoprim inhibited the enzyme.     

Refolding of therapeutic proteins produced in Escherichia coli as inclusion bodies

Overexpression of cloned or synthetic genes in Escherichia coli often results in the formation of insoluble protein inclusion bodies. Within the last decade, specific methods and strategies have been developed for preparing active recombinant proteins from these inclusion bodies. Usually, the inclusion bodies can be separated easily from other cell components by centrifugation, solubilized by denaturants such as guanidine hydrochloride (Gdn-HCl) or urea, and then renatured through a refolding process such as dilution or dialysis. Recent improvements in renaturation procedures have included the inhibition of aggregation during refolding by application of low molecular weight additives and matrix-bound renaturation. These methods have made it possible to obtain high yields of biologically active proteins by taking into account process parameters such as protein concentration, redox conditions, temperature, pH, and ionic strength.     

重组PAI－1对u－PA抑制活性的研究

利用大肠杆菌表达的重组纤溶酶原激活物抑制因子－１（ｒＰＡＩ－１）具有许多与天然ＰＡＩ－１相同的性质,ｒＰＡＩ－１对ｕ－ＰＡ抑制活性研究的内容包括：几种化学物质（盐酸胍、尿素、硫氰酸钾、ＳＤＳ、氯化钠等）对ｒＰＡＩ－１的激活作用、盐酸胍激活ｒＰＡＩ－１的浓度与温度效应、显色底物法和ＳＤＳ－ＰＡＧＥ纤维蛋白自显影对ｒＰＡＩ－１活性的测定、活性态ｒＰＡＩ－１向潜状态的转变及其与盐浓度和ｐＨ值的关系。