草鱼生长激素单抗免疫亲和柱的制备及初步应用

用纯化的草鱼生长激素单克隆抗体偶联到CNBr活化的Sepharose4B凝胶上,制成约10ml的亲和层析柱．用该柱一步纯化了重组鲤鱼生长激素基因的表达产物．偶联有13．65mg单克隆抗体的亲和柱一次可纯化得到约0．7mg重组鲤鱼生长激素．酶联免疫受体测定表明它具有强烈的生物学活性,SDS－PAGE表明它为单一蛋白带,分子量约为22000．     

舟山眼镜蛇毒神经生长因子的亲和层析分离

用层析和制备SDS-PAGE法纯化舟山眼镜蛇(Najanajaatra Cantor)毒神经生长因子(NGF),免疫家兔获得抗血清。用辛酸-硫酸铵沉淀法初步纯化IgG,蛋白A-Sepharose亲和层析进一步纯化IgG,并与CNBr活化的Sepharose4B偶联,采用亲和层析法对舟山眼镜蛇毒神经生长因子进行分离纯化。产物经过SDS-PAGE检测呈一条带,并显示了良好的生物学活性。纯化NGF最大比活性为5.0×104U/mg蛋白,亲和常数为4.35×108L/mol,亲和层析分离NGF得率比传统分离方法得率提高35.2%,该方法为NGF的大量提取提供了技术支持。     

草鱼生长激素单抗免疫亲和柱的制备及初步应用

用纯化的草鱼生长激素单克隆抗体联剂ＣＮＢｒ活化的Ｓｅｐｈａｒｏｓｅ ４Ｂ凝胶上制成约１０ｍｌ的亲和层析柱,用该柱一步纯化了重组鲤鱼生长激素基因的表达产物。偶联有１３．６５ｍｇ单克隆抗体的亲和柱一次强纯化得到约０．７ｍｇ重组鲤鱼生长激素。酶联免疫受体测定表明它具有强烈的生物学活性,ＳＤＳ－ＰＡＧＥ表明它为一蛋白带,分子量约为２２０００。     

免疫亲和层析法纯化苦瓜几丁酶

用扁豆几丁酶免疫家兔,获得抗扁豆几丁酶的抗体,将此抗体与Ｓｅｐｈａｒｏｓｅ ４Ｂ偶联,制备免疫亲和吸附剂,用以纯化苦瓜几丁酶．苦瓜叶片的粗提液经过免疫亲和吸附柱后,可获得电泳纯的几丁酶,其分子量为３５ ｋＤ,与用几丁质凝胶为亲和吸附剂的纯化结果一致．表明利用植物几丁酶在结构上的保守性,用免疫亲和法可纯化不同植物的同类几丁酶．与几丁质凝胶亲和柱相比,免疫亲和法纯化植物几丁酶具有快速、亲和柱可重复使用等的优点．利用免疫亲和层析获得的纯化样品,研究了苦瓜几丁酶对真菌的抑制试验,研究结果表明,苦瓜几丁酶能分解棉花枯萎病菌的菌丝体细胞壁制备物,并对其孢子芽管的伸长有一定抑制作用．     

抗牛生长激素单克隆抗体及其免疫亲和吸附柱的制备

我们用杂交瘤技术获得了分秘抗牛生长激素单克隆抗体的细胞系(4B-2)。接种此细胞于小鼠所产生腹水的抗体含量达10mg／ml。经免疫亲和层析方法纯化的单克隆抗体,属1BG1型。将单克隆抗体偶联到Sepharose 4B上,创成了免疫亲和吸附柱,可以从牛垂体匀浆中一步纯化牛生长激素。偶联有50mg单克隆抗体的亲和柱一次可结合3mg牛生长激素。经单克隆抗体亲和层析纯化的牛生长激豢,保持了与兔肝细胞膜受体结合的能力,及在去垂体大白鼠中促进胫骨生长板生长的功能。     

用免疫亲和层析法纯化细菌铁蛋白

用细菌铁蛋白免疫家兔,制备抗铁蛋白血清,用进一步纯化的抗铁蛋白抗体作为配基与溴化氰活化的Sepharose4B偶联,得到亲和免疫吸附剂。以此法纯化的铁蛋白为聚丙烯酰胺凝胶电泳纯,相对复合抗体作双向免疫电泳显示单峰,并具有较高的免疫活性。     

一种新型免疫亲和层析介质的研究

以国产琼脂糖介质为原料,合成了含肼琼脂糖介质。抗体Fc段的糖基经氧化后,可与此种含肼琼脂糖介质偶联,制成高亲和率的免疫亲和层析介质。与溴化氰法相比,这种对抗体上的糖特异的偶联方法制成的免疫亲和层析介质,容量高、稳定性强。用这种含肼琼脂糖介质分别与肿瘤坏死因子和γ-干扰素等的抗体偶联,制成的免疫亲和层析介质可用于分离纯化相应的基因工程产物抗原。     

改性甲壳素固定化胰蛋白酶直接纯化牛肺Kunitz抑制剂的研究

通过对天然甲壳素 (或壳聚糖 )进行化学改性并修饰作为载体 ,再经氯代环氧丙烷活化偶联 ,制成固定化胰蛋白酶亲和吸附剂 (蛋白酶偶联率为 6 2 1% ,酶活性回收率为 5 7 8% ) ,直接亲和层析牛肺提取液中Kunitz抑制剂。纯化的产品每毫克蛋白酶抑制剂活力相当于 5 82 0BAEETTU/mg蛋白质 ,纯化率为 40 7。提高了Kunitz抑制剂的稳定性能和回收率 ,简化了工业化生产程序 ,具开发前景     

单克隆抗体亲和层析纯化长叶车前花叶病毒

长叶车前花叶病毒上海分离株(HRVsh)单克隆抗体1H2,经纯化后以溴化氰活化法偶联于Sepharose 4B上制成亲和层析柱。HRVsh感染的三生烟提取液,经一次聚乙二醇沉淀初步纯化,悬浮液上亲和层析柱,于磷酸缓冲液中吸附,蒸馏水洗脱。收集的病毒制剂接种心叶烟有感染性,电镜观察见典型的HRVsh粒子,紫外吸收光谱与常规方法提纯的病毒相似,SDS-聚丙烯酰胺凝胶电泳呈一条带。结果表明单克隆抗体亲和层忻得到高度纯化的HRVsh。最后讨论了单克隆抗体亲和层析方法的优点。     

拟南芥MnSOD的原核表达、纯化及抗体制备

PCR扩增拟南芥MnSOD cDNA的保守区段,构建pET-SOD重组质粒,转化大肠杆菌JM109(DE3),IPTG诱导融合蛋白高效表达;经检测表达产物占菌体总蛋白的69％,且以不溶的包涵体形式存在;表达产物变性后经Ni—NTA Superflow亲和柱分离纯化,得到相对分子质量约为29000的PAGE纯蛋白。融合蛋白经还原复性处理后,比活达到200U／mg;免疫家兔制备MnSOD融合蛋白抗体,抗体效价为1：10000。以上结果为进一步大规模制备MnSOD及其功能研究奠定基础。     

虎血清免疫球蛋白（IgG）的纯化及纯度、活性鉴定

目的 建立高纯度、高活性的虎血清IgG纯化方法。方法 用饱和硫酸铵沉淀虎血清得到IgG粗品;结合Hitrap Protein A亲和层析预装柱及阴离子交换层析法对粗品IgG进一步分离纯化,采用PAGE电泳和Western-Blot免疫印迹法鉴定IgG纯度和免疫活性。结果 80 mL虎血清亲和纯化得到84 mg IgG,阴离子交换层析纯化得到30 mg虎的IgG纯品。结论 建立了简便快速、纯度高、活性好的虎血清IgG的分离纯化方法,为虎血清IgG二级抗体的制备提供了高纯度、活性好的一级抗体免疫原。     

Variation in epitopes of the B subunit of Vibrio cholerae non-O1 and Vibrio mimicus cholera toxins.

Monoclonal antibodies reacting with the B subunit of Vibrio cholerae O1 strain 569B cholera toxin (CT-B) were used to identify unique and common epitopes of V. cholerae non-O1 and Vibrio mimicus CT-B. Vibrio cholerae non-O1 strains produced CT-B showing three monoclonal antibody reaction patterns (epitypes), which corresponded with epitypes described previously for V. cholerae O1 classical biotype CT-B (CT1), El Tor biotype CT-B (CT2), and a unique V. cholerae non-O1 CT-B (CT3), which lacked an epitope located in or near the GM1 ganglioside binding site of 569B CT-B. Vibrio mimicus CT-B was immunologically indistinguishable from 569B CT-B. These and previous results define six epitopes on 569B CT-B, and a fourth epitope in or near the GM1 ganglioside binding site.     

貉血清IgG纯化及抗血清的制备

目的 制备高纯度貉血清IgG和兔抗貉IgG抗血清,作为建立多种动物抗体检测技术的储备。方法 采用Hitrap Protein A亲和层析及盐析再沉淀法纯化貉血清IgG,通过PAGE电泳和Western-Blot免疫印迹法对IgG作纯度及免疫活性检测;常规免疫法制备兔抗貉IgG血清。结果 貉血清IgG与Protein G虽有较强的结合力,但同时也结合血清中其他杂蛋白;用二步纯化法可从5 mL貉血清中纯化IgG约7 mg,电泳和免疫印迹测定显示,IgG纯度大于95%,常规免疫法制备抗血清免疫双扩散效价达1∶32。结论 建立了可行的貉血清IgG的纯化方法和高效价的兔抗貉血清IgG抗血清,为貉血清IgG二级抗体酶联物的制备储备了资源。     

Binding of cholera toxin B-subunits to derivatives of the natural ganglioside receptor, GM1.

In a previous paper we showed that the B-pentamer of cholera toxin (CT-B) binds with reduced binding strength to different C(1) derivatives of N-acetylneuraminic acid (NeuAc) of the natural receptor ganglioside, GM1. We have now extended these results to encompass two large amide derivatives, butylamide and cyclohexylmethylamide, using an assay in which the glycosphingolipids are adsorbed on hydrophobic PVDF membranes. The latter derivative showed an affinity approximately equal to that earlier found for benzylamide ( approximately 0.01 relative to native GM1) whereas the former revealed a approximately tenfold further reduction in affinity. Another derivative with a charged C(1)-amide group, aminopropylamide, was not bound by the toxin. Toxin binding to C(7) derivatives was reduced by about 50% compared with the native ganglioside. Molecular modeling of C(1) and C(7) derivatives in complex with CT-B gave a structural rationale for the observed differences in the relative affinities of the various derivatives. Loss of or altered hydrogen bond interactions involving the water molecules bridging the sialic acid to the protein was found to be the major cause for the observed drop in CT-B affinity in the smaller derivatives, while in the bulkier derivatives, hydrophobic interactions with the protein were found to partly compensate for these losses.     

Analysis of structure and function of the B subunit of cholera toxin by the use of site-directed mutagenesis

Oligonucleotide-directed mutagenesis of ctxB was used to produce mutants of cholera toxin B subunit (CT-B) altered at residues Cys-9, Gly-33, Lys-34, Arg-35, Cys-86 and Trp-88. Mutants were identified phenotypically by radial passive immune haemolysis assays and genotypically by colony hybridization with specific oligonucleotide probes. Mutant CT-B polypeptides were characterized for immunoreactivity, binding to ganglioside GM1, ability to associate with the A subunit, ability to form holotoxin, and biological activity. Amino acid substitutions that caused decreased binding of mutant CT-B to ganglioside GM1 and abolished toxicity included negatively charged or large hydrophobic residues for Gly-33 and negatively or positively charged residues for Trp-88. Substitution of lysine or arginine for Gly-33 did not affect immunoreactivity or GM1-binding activity of CT-B but abolished or reduced toxicity of the mutant holotoxins, respectively. Substitutions of Glu or Asp for Arg-35 interfered with formation of holotoxin, but none of the observed substitutions for Lys-34 or Arg-35 affected binding of CT-B to GM1. The Cys-9, Cys-86 and Trp-88 residues were important for establishing or maintaining the native conformation of CT-B or protecting the CT-B polypeptide from rapid degradation in vivo.     

兔抗金黄地鼠酶标抗体的制备及应用

目的 纯化金黄地鼠血清IgG,制备兔抗金黄地鼠酶标抗体(IgG-HRP),开展金黄地鼠仙台病毒的初步检测.方法 采用亲和层析纯化法纯化金黄地鼠IgG,用SDS- PAGE电泳测定IgG纯度并制备兔抗金黄地鼠IgG抗体(second antibody,Ab2);用免疫双扩散法检测抗血清效价后,再用亲和层析纯化抗血清IgG( Ab2);采用改良过碘酸钠标记法制备兔抗金黄地鼠酶标抗体( rabbit anti-hamster IgG-HRP);用直接ELISA和Western-blot法对兔抗金黄地鼠IgG酶标抗体进行工作浓度测定;应用金黄地鼠酶标抗体对金黄地鼠仙台病毒进行酶免检测(IEA).结果 金黄地鼠血清IgG纯度达95％;兔抗金黄地鼠IgG抗体(Ab2)免疫双扩散效价为1(:)64;兔抗金黄地鼠IgG -HRP经直接ELISA和Western-Blot测定工作浓度分别为1∶5000和1∶2000;酶免(IEA)效价为1:2000.结论 高效快速纯化了金黄地鼠IgG,制备了金黄地鼠IgG-HRP,为金黄地鼠病原微生物的血清学检测提供了条件.     

长爪沙鼠IgG的纯化及抗血清的制备

目的 纯化长爪沙鼠血清IgG,制备兔抗长爪沙鼠IgG抗血清。方法 采用Hitrap Protein G亲和层析预装柱来纯化长爪沙鼠血清IgG;通过SDS-PAGE电泳和Western-Blotting免疫印迹法对长爪沙鼠血清IgG进行纯度鉴定,免疫兔子制备抗血清。结果 7 mL长爪沙鼠血清纯化得到11 mg IgG;电泳和免疫印迹测定,IgG纯度大于95%;用纯化的IgG作抗原制备了兔抗血清,免疫双扩散测定效价达1∶32。结论 建立了长爪沙鼠血清IgG的纯化方法,制备了长爪沙鼠IgG抗血清,证实长爪沙鼠血清IgG和Protein G具有较高的亲和性。     

羊抗人IgG的纯化及其在抗—HCV检测中的应用

单独或联合应用辛酸沉淀、饱和硫酸铵沉淀、阴离子交换等方法对羊抗人IgG进行纯化,对纯化前后抗体的纯度和免疫学活性进行比较,并与辣根过氧化物酶连接,作为二抗用于抗－HCV的ELISA检测。结果表明,不同方法纯化的抗体其纯度和免疫学活性具有一定程度的差别,其中经辛酸＋饱和硫酸铵沉淀纯化的抗体为最佳,凝胶扫描纯度为98．05％,比活性近1800,为纯化前的6．8倍。用痞根过氧化物酶标记后,作为酶标二抗检测HCV阴性和阳性标准血清各40份,阴性符合率为97．5％,阳性符合率为95％,可用于抗－HCV的ELISA检测。     

Comparison of the glycolipid-binding specificities of cholera toxin and porcineEscherichia coli heat-labile enterotoxin: identification of a receptor-active non-ganglioside glycolipid for the heat-labile toxin in infant rabbit small intestine

The binding specificities of cholera toxin andEscherichia coli heat-labile enterotoxin were investigated by binding of¹²⁵I-labelled toxins to reference glycosphingolipids separated on thin-layer chromatograms and coated in microtitre wells. The binding of cholera toxin was restricted to the GM1 ganglioside. The heat-labile toxin showed the highest affinity for GM1 but also bound, though less strongly, to the GM2, GD2 and GD1b gangliosides and to the non-acid glycosphingolipids gangliotetraosylceramide and lactoneotetraosylceramide. The infant rabbit small intestine, a model system for diarrhoea induced by the toxins, was shown to contain two receptor-active glycosphingolipids for the heat-labile toxin, GM1 ganglioside and lactoneotetraosylceramide, whereas only the GM1 ganglioside was receptor-active for cholera toxin. Preliminary evidence was obtained, indicating that epithelial cells of human small intestine also contain lactoneotetraosylceramide and similar sequences. By computer-based molecular modelling, lactoneotetraosylceramide was docked into the active site of the heat-labile toxin, using the known crystal structure of the toxin in complex with lactose. Interactions which may explain the relatively high toxin affinity for this receptor were found.Abbreviations CT cholera toxin - CT-B B-subunits of cholera toxin - LT Escherichia coli heat-labile enterotoxin - hLT humanEscherichia coli heat-labile enterotoxin - pLT porcineEscherichia coli heat-labile enterotoxin - EI electron ionization     

蝙蝠血清IgG的纯化及兔抗蝙蝠IgG酶标抗体的制备

目的纯化蝙蝠血清IgG,制备兔抗蝙蝠IgG酶标抗体。方法采用亲和层析纯化法纯化蝙蝠血清IgG,SDS-PAGE电泳鉴定蝙蝠IgG纯度。免疫大白兔制备兔抗蝙蝠IgG抗血清,免疫双扩散法测定抗血清效价,亲和层析纯化法纯化抗血清IgG。用改良过碘酸钠标记法制备兔抗蝙蝠IgG酶标抗体,直接ELISA和Western blot法对兔抗蝙蝠IgG酶标抗体进行工作浓度测定。结果纯化的蝙蝠血清IgG,其SDS-PAGE测定纯度大于95%;免疫大白兔所制备的抗血清免疫双扩散效价为1∶64;用改良过碘酸钠标记法制备兔抗蝙蝠IgG酶标抗体,其直接ELISA和Western blot工作浓度分别为1∶12800和大于1∶2000。结论制备了蝙蝠血清IgG的抗血清和酶标抗体,为蝙蝠的血清学检测体系提供了技术和资源储备。