用高碘酸盐活化葡聚糖凝胶制备亲和吸附剂的研究

 <正> 用高碘酸盐活化的Sephadex与鸡卵类粘蛋白偶合制备分离纯化胰蛋白酶的亲和吸附剂。该方法比CNBr活化Sepharose 4B制备亲和吸附剂的方法具有操作安全,价格低廉等优点。活化载体在4℃保存较长时间不失去键合能力。该亲和吸附剂可制备得比活力为11228.8u/mgBAEE单位电泳单带纯胰蛋白酶,并能反复使用十余次,仍具有较强亲和吸附能力。酶     

改性与修饰壳聚糖固定化酶纯化抑肽酶研究

采用化学改性与修饰微珠壳聚糖为载体,共价法偶联牛胰蛋白酶,制成抑肽酶亲和吸附剂,单位活力5 190 KIU/g（湿）,蛋白质偶联率60.5％,酶活性回收率55％;将其直接亲和层析牛肺提取液,分离纯化高比活抑肽酶.方法过程简单,样品比活力5 700 KIU/mg,质量稳定,成本较低;该吸附剂机械强度高,抗污染能力较强,非特异性吸附较小,可以反复使用,价格低廉,适合工业化生产.     

用壳聚糖替代Sepharse 4B固定相关配体纯化酶的研究

采用壳聚糖固定酶作用的特定底物（菌体细胞）,并用戊二醛交联制备成酶的亲和吸附剂。采用该吸附剂纯化溶葡球菌的研究表明,经一步纯化可提高纯度4倍,酶活性回收大于70％。SDS－PAGE的电泳结果显示,产品基本上达到了标准酶的纯度。同时表明该吸附剂没有非特异性吸附。由载体壳聚糖替代Sepharose 4B制备的吸附剂具有简单、快速、较高收得率和操作安全等优点,适用于特定酶或基因工程产品的分离纯化。     

固定化胰蛋白酶的快速制备

目的：快速制备高活力的固定化胰蛋白酶,用于转肽反应。方法：将壳聚糖与硅胶搅拌均匀,同时用戊二醛进行活化制成活化载体,再通过交联反应将胰蛋白酶固定至载体制备固定化胰蛋白酶。用正交法进行优化。结果：用快速工艺制得的固定化胰蛋白酶的活力单位为5990．5U/g,活力回收为16．7％,整个制备过程耗时21h。结论：快速工艺的制备过程较之改进前更为快捷简便,制备的固定化胰蛋白酶活力单位显著提高,利于工业应用。     

壳聚糖固定化酶一步纯化抑肽酶研究

采用化学改性与修饰微珠壳聚糖为载体,共价法偶联牛胰蛋白酶,制成抑肽酶亲和吸附剂,单位活力５１９０ＫＩＵ／ｇ（湿）,蛋白偶联率６０．５％,酶活性回收率５５％;将其直接亲和层析牛肺提取液,分离纯化高比活抑肽酶。方法过程简单,样品比活力５７００ＫＩＵ／ｍｇ,质量稳定,成本较低;该吸附剂机械强度高,抗污染能力较强,非特异性吸附较小,可以反复使用,价格低廉,适合工业化生产。     

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     

以壳聚糖为亲和层析载体提纯胰蛋白酶

以自制的壳聚糖为亲和层析载体,鸡蛋粘蛋白作配基,通过戊二醛交联构建成亲和吸附剂,对胰蛋白酶的亲和层析提纯进行了研究。结果表明,胰蛋白酶活性回收率达70％,纯度经聚丙烯酰胺凝胶电泳鉴定为一条带,实验有操作安全、简单、快速和收率高等优点。     

不同载体固定化胰蛋白酶的条件研究

试验分别选用壳聚糖、复合硅胶、阴离子交换树脂为载体制备固定化胰蛋白酶,通过正交试验优化确定不同载体的酶固定条件。研究表明,三种载体固定胰蛋白酶时的酶活回收率依次为81.9%、80.1%、44.8%。     

不同载体固定化胰蛋白酶酶学特性的研究

目的:研究以壳聚糖、复合硅胶、阴离子交换树脂为载体固定化胰蛋白酶的酶学特性。方法:通过测定不同载体固定化胰蛋白酶的活力得其最适反应温度值、最适反应pH值和米氏常数(Km)值。结果:以壳聚糖、复合硅胶、阴离子交换树脂为载体制备固定化胰蛋白酶的最适反应温度分别为70℃、60℃、60℃;最适反应pH值分别为7.5、8.0、8.0;表观米氏常数K’m分别为22.72mg/ml、25.12mg/ml、29.04mg/ml。结论:与游离酶相比,固定化胰蛋白酶均表现出一定的热稳定性、酸碱稳定性,利于工业化生产。     

果胶酶亲和吸附剂的制备及其性能比较

以甜菜渣、果胶、海藻酸钠为原料 ,与表氯醇在碱性条件下交联 ,制备了果胶酶亲和吸附剂并应用这几种亲和吸附剂对草酸青霉果胶酶和黑曲霉果胶酶进行亲和层析实验。结果表明 :用小于 60目的甜菜渣粉末和海藻酸钠制备的果胶酶亲和吸附剂 (分别简写为SBP吸附剂和SA吸附剂 )具有较好的纯化果胶酶性能 ,其中SBP吸附剂性能稳定 ,而SA吸附剂膨胀系数较大 ,在流动相改变时引起流速不稳。     

Separation and purification of enzymes by continuous pH-parametric pumping

Trypsin and chymotrypsin were separated from porcine pancreas extract by continuous pH-parametric pumping. CHOM (chicken ovomucoid) was convalently bound to laboratory-prepared crab chitin with glutaraldehyde to form an affinity adsorbent of trypsin. The pH levels of top and bottom feeds were 8.0 and 2.5, respectively. Similar inhibitor, DKOM (duck ovomucoid), and pH levels 8.0 and 2.0 for top and bottom feeds, respectively, were used for separation and purification of chymotrypsin. epsilon-Amino caproyl-D-tryptophan methyl ester was coupled to chitosan to form an affinity adsorbent for stem bromelain. The pH levels were 8.7 and 3.0. Separation continued fairly well with high yield, e.g., 95% recovery of trypsin after continuous pumping of 10 cycles. Optimum operational conditions for concentration and purification of these enzymes were investigated. The results showed that the continuous pH-parametric pumping coupled with affinity chromatography is effective for concentration and purification of enzymes.     

Blocking effect of trypsin associated with ovomucoid on the antibody binding to ovomucoid

Ovomucoid-trypsin association complex was prepared by incubating chicken egg white ovomucoid with bovine trypsin. The reactivity of ovomucoid-trypsin complex was investigated by immunodiffusion, quantitative precipitation and enzyme-linked immunosorbent assay (ELISA). It was demonstrated that the association of trypsin with ovomucoid hindered the binding of the specific antibody at some antigenic sites of ovomucoid by lowering the antibody-binding affinity of these sites. The anti-ovomucoid antiserum was absorbed with ovomucoid-trypsin complex, and non-absorbed antibody was collected by immunoaffinity chromatography of ovomucoid-coupled Sepharose 4B. The antibody blocked the trypsin-inhibitory activity of ovomucoid in a molar ratio (antibody/ovomucoid) of about 1.2:1. The findings suggested that at least one antigenic site is located near the reactive site of trypsin inhibition (Arg89 decreases Ala90) of ovomucoid.     

Purification and characterization of Locusta migratoria chymotrypsin

A chymotrypsin-like enzyme (CTLE) was isolated from the digestive tract of the African migratory locust Locusta migratoria migratorioides by ion-exchange chromatography on diethylaminoethyl (DEAE) cellulose followed by affinity chromatography on phenylbutylamine (PBA) Sepharose. The purity and homogeneity of CTLE have been shown by SDS-PAGE and on cellulose acetate strips. The enzyme has a molecular weight of 24,000, determined by SDS-PAGE and on a Sephadex G-75 calibrated column. It has an isoelectric point of 10.1 and contains 0-1 half cystine residues. Sequence analysis of the first 20 N-terminal amino acids has shown 25% homology with bovine chymotrypsin and 40% homology with Vespa crabo and Vespa orientalis chymotrypsins and with Hypoderma lineatum trypsin. The optimal pH for enzyme activity and stability was in the range of 8.5-9.0. The Km and kcat values, determined on substrates for proteolytic, esterolytic and amidolytic activity, similar to those for bovine chymotrypsin. CTLE was inactivated by PMSF and TPCK indicating the involvement of serine and histidine in its active site. The enzyme was fully inhibited by the proteinaceous, double-headed, chymotrypsin-trypsin inhibitors BBI from soybeans and CI from chickpeas, by chicken ovomucoid (COM) and turkey ovomucoid (TOM), as well as by the Kunitz soybean trypsin inhibitor (STI) which hardly inhibits bovine chymotrypsin. Inhibition studies of CTLE with amino acid and peptide-chloromethylketones point towards the existence of an extended binding site.     

Immunochemical studies on thermal denaturation of ovomucoid

The thermal denaturation of ovomucoid was investigated by immunochemical methods, namely immunoprecipitation analyses and antibody-Sepharose 4B column chromatography. In the immunoprecipitation analyses, heated ovomucoid (90 degrees C, 90 min, pH 7.2) required about twice the antigen addition of the native protein to approach maximal precipitation with specific antibody, and the maximal immunoprecipitation was decreased to 80% of that by native ovomucoid. However, heated protein inhibited the binding of antibody with native ovomucoid, and 100% inhibition was attained at about 4-times the antigen addition necessary for the native protein. Heated ovomucoid (100 degrees C, 120 min) showed little immunoprecipitation and inhibition. To ovomucoid antigenicity was diminished more slowly than the trypsin inhibitory activity by heating, e.g., heated ovomucoid (90 degrees C, 120 min) retained more than 30% of the antigenicity but little trypsin inhibitory activity. By passing through the immunoaffinity column, heated ovomucoid (90 degrees C, 90 min) was separated into two fractions, either with (fraction II) or without (fraction I) antigenicity. Fraction II contained smaller fractions of ordered secondary structure than native ovomucoid, and trypsin inhibitory activity of fraction II was only 24% of the native one. These results indicated that thermally denatured ovomucoid was heterogeneous regarding the conformational damage caused by heating, and the structure around some antigenic sites in an ovomucoid molecule was retained even after the backbone conformation was partially destroyed and trypsin inhibitory activity was lost.     

Turtle-dove ovomucoid, a glycoprotein proteinase inhibitor with P1-blood-group antigen activity.

Ovomucoid from the egg white of turtle-dove (Streptopelia risoria) was purified and shown to be a glycoprotein of mol. wt. 29 400, with valine as N-terminal residue. It is an inhibitor of both trypsin and chymotrypsin, but has a lower affinity for trypsin than has hen ovomucoid. Turtle-dove ovomucoid contains antigenic activity cross-reacting with the blood-group-P1 antigen of human erythrocytes. Hen ovomucoid has no detectable blood group-P1 activity. The carbohydrate composition of turtle-dove ovomucoid differs from hen ovomucoid in having substantially higher galactose content. The possible relationship between carbohydrate composition and antigenic activity is discussed.     

Monoclonal antibodies against hen's egg ovomucoid

Two monoclonal antibodies (mAb 23E5 and 32A8) to hen's egg ovomucoid (OM), which causes hen's egg allergy and has trypsin inhibitory activity, were prepared and purified. Their affinity to the three separate domains of the ovomucoid, which are homologous in primary structure and are designated as DI, DII, and DIII, was studied by a competitive radioimmunoassay. MAb 23E5 bound to OM more efficiently than to DI, DII, or DIII-2 (with carbohydrate), but reacted with DIII-1 (free from carbohydrate) more efficiently than with OM. Except for the binding to OM, mAb 32A8 bound to DIII-2 most efficiently and to DIII-1 least efficiently, suggesting that this antibody recognized the carbohydrate moiety of DIII. MAb 32A8 inhibited the trypsin inhibitory activity of OM, whereas mAb 23E5 had no effect on it. These monoclonal antibodies should be useful for analyzing the antigenic determinants and trypsin inhibitory activity of ovomucoid.     

壳聚糖锌离子固定化亲和层析填料的制备与性质

目的:制备了壳聚糖Zn2+固定化亲和层析填料,并对其性能进行了研究。方法:采用反相悬浮法制备了交联壳聚糖;再以环氧氯丙烷为活化剂,乙二胺为螯合配基,制备了固定化亲和层析填料;表征了其有效粒径以及均匀系数、含水量、失重率、氨基含量、骨架密度、堆积密度以及孔度值。从时间、加入ZnCl2的浓度、温度、pH方面对Zn2+固定化条件进行了优选,并确定了Zn2+的固定化量。含组氨酸标签的乙醛脱氢酶粗酶液,经硫酸铵盐析后,考察了壳聚糖Zn2+固定化亲和层析填料的亲和性能。结果:制备的填料有效粒径为105μm;均匀系数为1.46;含水量为58.03%;失重率为85.43%;氨基含量为9.20mmol/g;骨架密度为1.217 8g/ml;堆积密度为0.843 2g/ml;孔度值为36.40%。固定化Zn2+的最佳条件是:时间3 h、加入ZnCl2溶液浓度0.1mol/L、温度28℃、pH 5.5;且此条件下,亲和层析填料中Zn2+固定化量为3.35mmol/g。壳聚糖Zn2+固定化亲和层析填料对乙醛脱氢酶的亲和性能为4.14IU/g(干重)。结论:制备了壳聚糖Zn2+固定化亲和层析填料,可用于带有组氨酸标签重组蛋白的快速分离与纯化。     

Design and study of peptide-ligand affinity chromatography adsorbents: application to the case of trypsin purification from bovine pancreas

The purification of trypsin from bovine pancreas was employed in a case study concerning the design and optimization of peptide-ligand adsorbents for affinity chromatography. Four purpose-designed tripeptide-ligands were chemically synthesized (>95% pure), exhibiting an Arg residue as their C-terminal (site P(1)) for trypsin bio-recognition, a Pro or Ala in site P(2), and a Thr or Val in site P(3). Each tripeptide-ligand was immobilized via its N-terminal amino group on Ultrogel A6R agarose gel, which was previously activated with low concentrations of cyanuric chloride (10.5 to 42.5 mumol/g gel). Well over 90% of the peptide used was immobilized. Three different concentrations were investigated for every immobilized tripeptide-ligand, 3.5, 7.0, and 14 mumol/g gel. The K(D) values of immobilized tripeptide-trypsin complexes were determined as well as the purifying performance and the trypsin-binding capacity of the affinity adsorbents. The K(D) values determined were in good agreement with the trypsin purification performance of the respective affinity adsorbents. The tripeptide sequence H-TPR-OH displayed the highest affinity for trypsin (K(D) 8.7 muM), whereas the sequence H-TAR-OH displayed the lowest (K(D) 38 muM). Dipeptide-ligands have failed to bind trypsin. When the ligand H-TPR-OH was immobilized via its N-terminal on agarose, at a concentration of 14 mumol/g gel, it produced the most effective affinity chromatography adsorbent. This adsorbent exhibited high trypsin-binding capacity (approximately 310,000 BAEE units/mL of adsorbent); furthermore, it purified trypsin from pancreatic crude extract to a specific activity of 15,200 BAEE units/mg (tenfold purification), and 82% yield. (c) 1997 John Wiley & Sons, Inc.