亲和层析纯化HepG2细胞分泌的PAI—1

本文报道用抗ＰＡＩ－１单克隆抗体（ＭｃＡｂ）亲和层析建立了纯化ＰＡＩ－１的简便方法。经免疫亲和层析,Ｓｅｐｈａｃｒｙｌ Ｓ２００凝胶过滤,从ＨｅｐＧ２细胞培液中分离到糖基化和非糖基化两种形式的ＰＡＩ－１,回收率为８４％,ＰＡＩ－１比活性为６．１×１０＾４ＩＵ／ｍｇ。糖基化ＰＡＩ－１分子量为５０ｋＤ,比活性５．８×１０＾４ＩＵ／ｍｇ。非糖基化ＰＡＩ－１分子量４３ｋＤ,占总ＰＡＩ－１３０％,仍具有ＰＡ     

Ⅰ型纤溶酶原激活物抑制剂cDNA在P.pastoris酵母菌中的表达和鉴定

将编码３７９个氨基酸残基的ＰＡＩ－１ｃＤＮＡ插入到含ＡＯＸ１启动子和ＰＨＯ１分泌信号肽序列的甲醇营养型酵母载体中,构建成表达质粒ｐＹＩＳ－１．表达质粒转化Ｐ．ｐａｓｔｏｒｉｓ甲醇营养型酵母细胞,筛选Ｈｉｓ＋Ｍｕｔ－表型的转化子,经低密度摇瓶培养,１％甲醇诱导表达７ｄ后,培液经ＳＤＳ－ＰＡＧＥ分析,ＰＡＩ－１生物活性测定和Ｗｅｓｔｅｒｎｂｌｏｔ证实表达出分子量为４３～５１ｋＤ的４条ＰＡＩ－１条带．表达的ＰＡＩ－１能有效地分泌到培液中,占培液总蛋白的２６％左右,达４ｍｇ／Ｌ培液;其比活性为１．１６×１０４ＡＵ／ｍｇ．不同分子量ＰＡＩ－１可能与其糖基化程度不同有关     

重组PAI－1在大肠杆菌中的高效表达

纤溶酶原激活物抑制因子－１（ＰＡＩ－１）在天然状态下含量很低。为了进行ＰＡＩ－１的结构与功能的研究,构建了表达重组ＰＡＩ－１的质粒ｐＢＶ２２０／ＰＡＩ－１,并在大肠杆菌中得到了高效表达。最高表达量为菌体总蛋白量的４９％以上,经Ｗｅｓｔｅｒｎ ｂｌｏｔｉｎｇ检测,得到了分子量为４３．０ｋＤａ的反应条带。对形成包涵体的表达产物进行变、复性处理及Ｓｅｐｈａｄｅｘ Ｇ－７５的初步纯化,得到了潜伏态的重组Ｐ     

用国产微孔玻璃珠初步纯化人u-PA

用国产微孔玻璃珠从ＣＤ－１工程细胞株培养上清中纯化ｕ－ＰＡ,摸索了微孔玻璃珠结合ｕ－ＰＡ的条件和洗脱方法,比较了硫酸铵线性梯度洗脱或２５％乙二醇洗脱ｕ－ＰＡ活性的结果,最后确定洗脱的条件为０．２５ｍｏｌ／ＬＴｒｉｓ、１～２ｍｏｌ／Ｌ（ＮＨ４）２ＳＯ４、ｐＨ９．３。经此一步纯化,ｕ－ＰＡ比活性达到１５３２９ＩＵ／ｍｇ,回收率７８％,还原条件下ＳＤＳ－ＰＡＧＥ分子量为５２×１０３的单链ｕ－ＰＡ占７４％。     

糖基化、非糖基化、重组PAI－1功能和性质的比较

对从ＨｅｐＧ２细胞培养液中分离得到植基化和非糖基化ＰＡＩ－１（１型纤溶酶原激活物抑制剂）,以及从ｐＹＺＨＢＩ－６６表达菌中纯化的非糖基化重组ＰＡＩ－１的某些性质和功能进行比较,结果显示,糖基化ＰＡＩ－１对ｔＰＡ（组织型纤溶酶原激活物）有较强的抑制,能较显著地被蛋白质变性剂所激活,对热有较强的稳定性,糖基化与非糖基化ＰＡＩ－１在ｐＨ２．５－９．０的范围内都相当稳定。纤维蛋白原和肝素能明显提高两者对ｔＰＡ的抑制作用。     

人胎肺细胞的条件化培养液中两种类型纤溶酶原活化物的分离

用正常人胎肺细胞体外培养,从其培养液中分离纤溶酶原活化物（ＰＡ）,通过ＣＭ－ＳｅｐｈａｄｅｘＣ－５０层析,硫酸铵沉淀和Ｆｉｂｒｉｎ－Ｓｅｐｈａｒｏｓｅ,Ｌｙｓｉｎｅ－Ｓｅｐｈａｒｏｓｅ亲和层析及ＳｅｐｈａｄｅｘＧ－５０凝胶过滤等步骤,从１０．５ｌ条件培养液中分离纯化得到两种类型的纤溶酶原活化物,ｔ－ＰＡ９０μｇ,ｕ－ＰＡ８００μｇ．在还原条件下ＳＤＳ－ＰＡＧＥ均显示单带,分子量ｔ－ＰＡ为７２ｋＤ,ｕ－ＰＡ为５４ｋＤ,纤溶比活分别为１５６０００ＩＵ／ｍｇ蛋白和１０６０００ＩＵ／ｍｇ蛋白．     

盐生杜氏藻生油—3—磷酸脱氢酶的分离化及其特性的研究

利用ＰＥＧ分级,ＤＥＡＥ离子交换层析,Ｂｈｕｅ Ｓｅｐｈａｒｏｓｅ拟亲和层析,ＭｏｎｏＱ离子交换层析等手段,分离纯化直二氏藻甘油三磷酸（Ｇ－３－Ｐ）脱氢酶（ＥＣ１．１．１．８）得到比活为１２．６ｕ／ｍｇ的电泳纯的酶,并对此酶的生化特性进行了研究。４－２０％非变性聚丙烯酰胺梯度凝胶电泳测得全酶分子量约为２７０ｋＤ,ＳＤＳ－ＰＡＧＥ表明该酶只有一种分子量约为６５ｋＤ的亚基,据此推测该酶应为同四聚体。酶     

猪C1q的分离纯化与鉴定

猪Ｃ１ｑ由猪血清通过ＰＥＧ沉淀优球蛋白、低离子强度透析沉淀、ＩｇＧ－Ｓｅｐｈａｒｏｓｅ４８亲和层析、ＳｅｐｈａｄｅｘＧ－２００凝胶层析等步骤分离纯化,每３００ｍｌ血清可制得９．８ｍｇＣ１ｑ,产率为４６．７％。纯化的猪Ｃ１ｑ在ＳＤＳ－ＰＡＧＥ上显示出三条染色带,分别在２９、２６、２２ｋＤ处,薄层扫描结果表明纯度达９１％;纯化的Ｃ１ｑ保持了较高活性,终浓度为４μｇ／ｍｌ时仍可使致敏的绵羊红细胞出现明显的凝集现象。猪Ｃ１ｑ－ＥＬＩＳＡ结果表明,动物Ｃ１ｑ代替人Ｃ１ｑ应用于临床检测是可行的。     

猪肺源肝素的分离纯化及其成分鉴定

本文报告了从猪肺中用改进后的碱性氯化钠盐解法萃取的粗肝素为原料,以新型分离材料ＤＥＡＥ－Ｓｅｐｈａｃｅｌ分离纯化,并与ＳｅｐｈａｄｅｘＧ－５０进行比较,前者使粗肝素比活由１３．９ＵＳＰ／ｍｇ提高到２０３．６４ＵＳＰ／ｍｇ（美国药典单位）,纯化系数达到１４．６５,回收率达８６．９３％,而通过ＳｅｐｈａｄｅｘＧ－５０分离纯化后的肺肝素其比活性提高到１０２．１０ＵＳＰ／ｍｇ,纯化系数为７．３５,回收率为７２．２２％,其比活性、总活性回收率及纯化系数等,ＤＥＡＥ－Ｓｅｐｈａｃｅｌ均优于ＳｅｐｈａｄｅｘＧ－５０。纯化相当量粗肝素所需时间、次数亦大大减少,并用醋酸纤维薄膜电泳,高效液相色谱进行性质和纯化鉴定,用红外光谱进行基团分析鉴定。     

Nm23-H1/NDPK-A基因在大肠杆菌中的高效表达及产物纯化的研究

利用聚合酶链反应（ＰＣＲ）技术扩增人二磷酸核苷激酶Ａ亚基（ＮＤＰＫ－Ａ）基因,即ｎｍ２３－Ｈ１／ＮＤＰＫ－Ｋ基因的编码序列,经序列分析后,定向克隆于表达质粒载体ｐＢＶ２２０,在大肠杆菌ＤＨ５α中高效表达出重组人ＮＤＰＫ－Ａ．表达产物为可溶性的非融合蛋白,占菌体总蛋白４２％．斑点ＥＬＩＳＡ法鉴定表明表达产物与ＮＤＰＫ－Ａ标准抗血清呈阳性反应．以ＤＥＡＥ纤维素弱阴离子交换层析、ＣｉｂａｃｒｏｎＢｌｕｅ染料亲和层析结合高效液相排阻色谱技术纯化ｒＮＤＰＫ－Ａ,得纯度为９６．７％的目标蛋白．以反相高效液相色谱法进行酶活性分析,表明纯化的ｒＮＤＰＫ－Ａ能催化ＡＴＰ＋ＵＤＰ＝ＡＤＰ＋ＵＴＰ的反应,比活性为８００Ｕ／ｍｇ蛋白．     

重组人组织型纤溶酶原激活剂(rht-PA)及其突变体的纯化

稳定高效表达重组人组织型纤溶酶原激活剂 (rht PA)的CHO细胞株和表达组合突变体的细胞株进行了 3L转瓶培养 .将培养上清分别进行了Lys Sepharose 4B亲和层析和Zn2 + Sepharose 4B层析两步纯化 ,rht PA纯度提高了 5 34倍 ,比活达 2 5× 10 5IU mg ,产率为 73% ;突变体纯度提高了1119倍 ,比活达 5 9× 10 5IU mg ,产率为 6 9% .纯化产物SDS PAGE分析显示 ,rht PA和突变体基本都呈单一条带 ,扫描分析均达到 98%以上纯度 .rht PA和突变体在纯化系统中的行为作对照分析发现 ,突变体的构建思想在Lys Sepharose 4B亲和层析过程中有充分体现 .这两步层析组合是很好的纯化t PA及其突变体的方法 ,尤其是Lys Sepharose 4B纯化突变体效果更好     

融合蛋白GST-Ulp1p在大肠杆菌中的高效可溶性表达及其活性鉴定

利用基因工程技术,体外重组小分子类泛素修饰蛋白酶1(Ulp1)的活性片段,获得高表达、高特异性重组蛋白酶。从酿酒酵母Saccharomyces cerevisia中提取Ulp1编码第403到621个氨基酸残基之间的DNA片段(Ulp1p),在其C端加入6×His并连接到大肠杆菌表达载体pGEX中,构建重组表达质粒pGEX-Ulp1p-his6。将重组质粒转化至大肠杆菌Rosetta(DE3)中,氨苄青霉素抗性筛选转化子。表达、纯化后,以SUMO融合蛋白检测其活性。经过优化,该蛋白可溶性表达,表达量占菌体总蛋白的40.12%。可通过谷胱甘肽琼脂糖凝胶柱或Ni-NTA凝胶亲和层析纯化得到纯度98%的蛋白。经酶切分析,比活力为1.375×104U/mg。融合蛋白GST-Ulp1p-His6无需切除谷胱甘肽S-转移酶(GST)标签,具有很高的活性,制备简易;6×His标签,有利于底物蛋白切割后纯化,减少蛋白损失。本研究为制备高活力的SUMO蛋白酶提供了一个新方法。     

高分子量和低分子量尿激酶的分离纯化及动力学性质研究

人尿激酶粗品经苯甲脒亲和柱纯化和Protein-PahSP柱分离后,得到两种分子量的尿激酶（UK）,即高分子量尿激酶（HUK）和低分子量尿激酶（LUK）．采用考马斯亮蓝法测定蛋白质浓度,纤维蛋白平板法测定活力,测得HUK比活为2.9×105IU／mg蛋白,LUK为3.5×105IU／mg蛋白,活力回收为70％以上．经SDS-PAGE鉴定,HUK和LUK均是单一条带,分子量分别为54kD和33kD．HUK和LUK水解显色底物S2444的动力学常数,分别测得HUK的Km为64μmol/L,Kcat为15s-1,LUK的Km为49μmol／L,kcat为13s-1,LUK的催化效率（Kcat／Km）稍高于HUK．     

Identification of determinants involved in binding of tissue-type plasminogen activator-plasminogen activator inhibitor type 1 complexes to HepG2 cells

Complexes between tissue-type plasminogen activator (t-PA) and its rapidly acting inhibitor plasminogen activator inhibitor type 1 (PAI-1) are bound, internalized, and degraded by HepG2 cells. The mechanism involves endocytosis mediated by a specific high-affinity receptor. However, the particular domains of the complex that are recognized by the receptor have not been elucidated. To identify the determinants involved in ligand binding to the receptor, several variants of t-PA were assessed for their ability to form complexes with PAI-1 and thereby to inhibit specific cellular binding of complexes between structurally unmodified 125I-t-PA and PAI-1. Catalytically active variants lacking selected structural domains form complexes with PAI-1 and inhibit 125I-t-PA.PAI-1 binding to HepG2 cells. In addition, several forms of the plasminogen activator urokinase (u-PA), which shares partial structural homology with t-PA, were evaluated as competitors of cellular binding. The catalytically active two-chain forms of u-PA, but not the inactive proenzyme single-chain form, complex with PAI-1 and inhibit specific binding of 125I-t-PA.PAI-1, suggesting that the serine protease domain, rather than other domains, may confer the determinants required for cellular binding. However, a mutant t-PA with markedly reduced catalytic activity, resulting from replacement of the active site serine with threonine, not only forms complexes with PAI-1 but also inhibits specific cellular binding of unmodified 125I-t-PA.PAI-1. These data indicate that specific binding of t-PA.PAI-1 to HepG2 cells does not require a serine-containing catalytic site in the protease domain. To determine whether binding of the complex is mediated through other components of t-PA or through structural elements of PAI-1, both t-PA and PAI-1 were examined separately for capacity to bind directly to HepG2 cells. To exclude potential interactions with components of the extracellular matrix which contains binding sites for PAI-1, ligand binding to HepG2 cells in suspension was assessed. Although neither t-PA nor PAI-1 alone binds specifically to HepG2 cells, the preformed t-PA.PAI-1 complexes do. These findings suggest that specific binding of t-PA.PAI-1 requires elements of the PAI-1 moiety and/or parts of the protease domain of t-PA.     

Molecularly imprinted cryogels for human interferon‐alpha purification from human gingival fibroblast culture

Interferons are important proteins for the immune system because of their antiviral, anti‐proliferating and immunomodulatory activities. Therapeutic value of these proteins against certain types of tumors caused interest and investigations aimed to obtain highly purified interferons. Molecular imprinting is an efficient method for purification with high selectivity, specificity and good reproducibility. In this study, we utilized advantages of molecular imprinting technique for the purification of interferon from human gingival fibroblast culture. For this purpose, interferon α‐2b imprinted poly(hydroxyethyl methacrylate) cryogel (hIFN‐α‐MIP) was prepared. Optimum adsorption conditions were determined, and maximum adsorption capacity of hIFN‐α‐MIP cryogel was found as 254.8 × 10⁴ IU/g from aqueous solution. All interferon measurements are expressed as International Unit (IU), which is a unit measurement used to quantify biologically active substances like interferon based on their biological activity or effect. Selectivity experiments were performed using competitive proteins and repeated adsorption–desorption studies showed that the adsorption capacity maintained almost at a constant value after ten cycles. For the purification of interferon from human gingival fibroblast culture, fast protein liquid chromatography was used and the specific activity of the purified interferon α‐2b on HeLa cell line was found between the values 3.45 × 10⁸ IU/mg and 3.75 × 10⁸ IU/mg. The results are promising, and the molecular imprinting technique is effective for the purification of interferon α‐2b. Copyright © 2013 John Wiley & Sons, Ltd.     

人尿激酶原cDNA在昆虫杆状病毒真核表达系统中的高效表达

人尿激酶原(pro-urokinase,pro-UK)是一种新型溶栓剂,优于尿激酶,具有血纤维蛋白特异性。为了在昆虫杆状病毒表达系统中高效表达pro-UK,我们在pAc373基础上,插入野生型AcMNPV polyhedrin启动子区-7～1碱基序列,构建了一个高表达转移载体pAcYT。分别经三次克隆将pro-UK cDNA正向插入到转移载体pAc373或PAcYT的BarnHI-KpnI位点上。用LiPofectin将pAcyT-UKDNA或pAc373-UK DNA与AcMNPV DNA共转染到昆虫Sf9细胞中,空斑法筛出重组病毒阳性克隆株。高效表达结果是:1.ELISA法确定重组病毒Sf9细胞分泌表达产物pro-UK为96mg/L培养基上清,平板法测定溶圈活性为1600IU/mL培养基上清;2.亲和层析一步法纯化表达产物,回收率选70％,以上,比活约为60000IU/mg;3.纯化的pro-UK,无论是否经还原处理,其SDS-PAGE图谱均为相同的单一条带,MR 50000;4.Western blot与SDS-PAGE图谱吻合。     

Identification and partial characterization by chemical cross-linking of a binding protein for tissue-type plasminogen activator (t-PA) on rat hepatoma cells. A plasminogen activator inhibitor type 1-independent t-PA receptor.

Plasma tissue-type plasminogen activator (t-PA) is cleared rapidly in vivo by the liver. Previous studies with the human hepatoma cell line HepG2 have identified a clearance system for t-PA modulated by plasminogen activator inhibitor type 1 (PAI-1). In the present study, a rat hepatoma cell line MH1C1 is shown to contain a PAI-1-independent t-PA clearance system. At 4 degrees C, binding of 125I-t-PA to MH1C1 cells was rapid, specific, and saturable. Scatchard analysis of the binding data yielded a mean estimate of 105,000 high affinity binding sites per cell (Kd = 4.1 nM). When the bound ligand was analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, the majority (about 90%) of the specific binding was in the form of uncomplexed 125I-t-PA. This is in contrast to HepG2 cells in which specific binding was mainly in the form of a sodium dodecyl sulfate-stable 125I-t-PA.PAI-1 complex. When availability of matrix-associated PAI-1 was blocked by preincubation with anti-PAI-1 antibody or removed by elastase treatment, specific 125I-t-PA binding to MH1C1 cells was unaffected, whereas most of the specific 125I-t-PA binding to HepG2 cells was abolished. Furthermore, when the active site of t-PA was inactivated with diisopropyl fluorophosphate, the diisopropyl fluorophosphate-t-PA specifically competed for binding of 125I-t-PA to MH1C1 cells, but failed to block specific 125I-t-PA binding to HepG2 cells. At 37 degrees C, PAI-1-independent t-PA binding to MH1C1 cells was followed by ligand uptake and degradation with kinetics similar to that seen in HepG2 cells. Chemical cross-linking of t-PA to MH1C1 cells revealed a specific t-PA binding protein with a molecular mass of about 500,000 daltons. Ligand-receptor complexes generated by chemical cross-linking were immunoprecipitable by anti-t-PA antibody but not by anti-PAI-1 antibody, further supporting the finding that binding of t-PA to MH1C1 cells is PAI-1-independent.     

重组人r干扰素的纯化及其N端氨基酸序列分析

本文对两个重组人γ干扰素高效表达株pIFN-γ及PBVIFN-γ的表达产物进行了纯化并对纯化的γ干扰素进行了活性鉴定及N端氨基酸序列分析。采用连续沉淀的方法对高表达菌株pBVIFN-γ及低表达菌株pIFN-γ,裂解液进行初步纯化,然后应用单克隆抗体亲和层析方法进行纯化,分别可纯化14倍与933倍,均达电泳纯,回收率分别为25％和30％,比活性达7.56×10~7U/mg蛋白。SDS-PAGE电泳上γ干扰素分子量约17.5kD。测定了纯化的γ干扰素N末端19个氨基酸序列,与由其DNA序列推导的氨基酸序列完全一致,确认了本研究所表达、纯化的γ干扰素达到了较高纯度。本方法为γ干扰素的批量生产奠定了基础。