鸡免疫球蛋白(GIgG)轻链的分离纯化及其抗血清的制备

经硫酸铵盐析、柱色谱分离得到纯化的鸡血清IgG。继用2-巯基乙醇还原、碘乙酰胶烷化拆开IgG的轻、重链,再经Sephadex G100凝胶过滤柱色谱分离得到IgG轻链。以IgG轻链免疫家兔制得兔抗鸡IgG轻链抗血清。     

莆田黑猪精液中NAGase酶学特性研究

试验对以莆田黑猪精液为材料分离纯化得到的N-乙酰-β-D-氨基葡萄糖苷酶(NAGase)进行了理化特性研究。经硫酸铵分级沉淀、DEAE Sepharose Fast Flow离子交换层析和Sephadex G100分子筛层析获得PAGE电泳纯化的NAGase酶制剂。以对硝基苯-N-乙酰-β-D-氨基葡萄糖苷(pNP-GlcNAc)为底物,研究酶催化水解的相关性质。分离纯化获得的酶制剂比活力为1561.42 U/mg,分子质量为58 ku,只有1个亚基,等电点pI为9.13。酶的最适pH为5.6,最适温度为45 ℃,酶在pH 3.6～7.8之间稳定,当pH>8时迅速失活,在50 ℃以下处理30 min酶活力保存稳定,高于50 ℃时,酶活力迅速降低。酶促反应动力学符合米氏双曲线方程,米氏常数K_m为0.82 mmol/L,最大反应速度V_m为39.23 μmol/(L·min)。催化pNP-GlcNAc反应的活化能为27.30 kJ/mol。金属离子中Na⁺、K⁺、Mg²⁺、Ca²⁺对酶活力无明显影响,Zn²⁺、Cu²⁺、Pb²⁺对酶有抑制作用。     

鸡肠道抗菌肽的提取及活性研究

取新鲜鸡肠黏膜超声波破碎,乙酸浸提,经Sephadex G-50层析后,收集具有抑菌活性的组分进行超滤离心,抑菌实验表明滤过物具有抑菌活性.滤过物经SDS-PAGE分析为一个条带,分子量约为6.078KD,得到电泳纯的鸡肠道抗微生物肽.该肽具有一定的耐热性,但经90℃以上热处理后活性下降较大;pH值对其活性影响较大,在pH6～8时活性最强.     

蛹虫草多糖纯化工艺研究

为优化蛹虫草多糖的纯化工艺,以蛋白去除率和多糖保留率为指标,比较Sevage法、改良的Sevage法、澄清剂法三种方法对粗多糖中蛋白杂质的去除效果。本试验依次采用DEAE－52、Sephdex G －100葡聚糖凝胶柱层析进一步分离纯化蛹虫草多糖,再经Sephdex G－200柱色谱及高效液相凝胶色谱进行纯度检验。结果显示：澄清剂法蛋白去除率为93．4％,多糖保存率为90．7％;DEAE －52柱层析得到一个洗脱峰CP ,再经Sephdex G －100柱层析后得到两个洗脱峰CP－1和CP－2。对CP－1和CP－2进行纯度检验,发现两者皆为均一性多糖。     

The characterisation of equine interleukin-1

Equine interleukin-1 has been produced from peripheral blood monocytes by stimulation with E. coli lipopolysaccharide. Sephacryl S200 gel filtration revealed a molecular weight of 17-18 kD. Chromatofocusing of the 17-18 kD peak identified four active fractions. Two major peaks were detected at pH 6.7 and pH 7, with smaller peaks at pH 6.3 and pH 5.9. The pI 7 molecule is probably the equine form of IL-1 beta.     

Parameters of production and partial characterization of feline interleukin 2

The conditions for the production of feline interleukin 2 (IL-2) from peripheral blood leukocytes (PBL) and splenocytes by concanavalin A (Con A) stimulation are described. Feline IL-2 was quantitated by measuring DNA synthesis in the murine IL-2-dependent cell line, CTLL-20. In addition, feline IL-2 was generated for the maintenance of long-term cultures of Con A-stimulated feline PBL and for biochemical characterization. Finally, IL-2 production was evaluated from the PBL of feline leukemia virus (FeLV)-infected cats. Con A at 9.6 micrograms/ml produced a plateau of peak IL-2 activity from 24 to 48 h following stimulation. The tumor promoter, phorbol myristic acetate, stimulated feline IL-2 production and enhanced Con A-stimulated feline IL-2 production. Fetal calf serum (FCS) was not required for IL-2 production; however, FCS at 5% (v/v) allowed for maximal Con A-stimulated IL-2 production. Feline IL-2 generated from Con A-stimulated splenocytes migrated with an apparent molecular size of 13.7 to 23 kD by gel filtration chromatography and supported the proliferation of Con A-activated feline PBL at a final concentration of 0.3 to 0.9 units/ml.     

不同生理时期梅花鹿血液GSH-Px含量测定及其纯化

研究不同生理时期梅花鹿全血中GSH-Px含量变化及其纯化技术,为开发鹿血抗衰老资源奠定理论基础.用DINB法测定梅花鹿的溶血液、血细胞内容物、血浆和血细胞细胞膜中GSH-Px含量并计算全血GSH-Px含量；利用10％～100％饱和度的(NH4)2SO4盐析和柱层析技术纯化GSH-Px;用SDS-聚丙烯酰胺凝胶电泳测定其亚基相对分子质量.试验结果表明:全血GSH-Px含量以生茸期最高为(1 973.07士25.43)U·mL-1,与配种期的(1 727.74士12.46)U·mL-1差异极显著(P＜0.01),与生茸前期的(1 961.83士16.54)U·mL-1差异不显著(P＞0.05)；GSH-Px的初始比活力为24.9 U·mg-1,经纯化后得到GSH-Px 0.37 mg· mL-1,最终比活力1 347.7U·mg-1,纯化倍数为54.1倍,回收率25.00％；鹿血GSH-Px亚基的相对分子质量为17.2 ku.结果提示生茸期鹿血的GSH-Px含量最高,开发利用价值最大,GSH-Px含量与生理特性相关；鹿血GSH-Px盐析条件为40％～80％饱和度的(NH4)2SO4,此时所得GSH-Px纯化倍数较高.     

Retinol transport system in cattle and purification of retinol-binding protein from bovine serum

Retinol transport system in cattle was investigated, followed by the purification and characterization of bovine serum retinol-binding protein (RBP). Gel filtration of serum from cow produced two retinol peaks, peak 1 and 2. The major, peak 1 having higher molecular weight corresponded to the retinol peak from human serum which consisted of RBP and prealbumin (PA). The peak 2 which was not presented in the human serum had lower molecular weight (about 20,000). In the presence of 3.0 M urea, the peak 1 was almost disappeared and peak 2 was increased. On the other hand, in the serum from calf, major retinol peak was corresponded to the peak 2 from cow. These results suggested that, in cow, retinol was transported by the complex of RBP and another protein, presumably PA, but in calf, mainly by RBP alone. Purification of bovine RBP was carried out by using four chromatographic steps as follows; 1. DEAE-cellulose (pH 6.0), 2. Sephadex G-100 (using the buffer containing 3.0 M urea), 3. DEAE-cellulose (pH 8.3), 4. Sephadex G-100. From 1,100 ml of serum, 14.1 mg of bovine RBP was finally obtained and the overall recovery was estimated to be about 32%. Its molecular weight, ultraviolet absorption and fluorescence spectra, electrophoretic mobility, and amino acid composition were similar to those of other species.     

Purification of an acid-stable bovine leukocyte interferon

Bovine leukocyte interferon (BoL-IFN), produced in bovine peripheral blood leukocytes after priming and induction with Sendai virus, was concentrated by precipitation with KSCN (pH 3.5) and purified by gel column chromatography. Recovery of BoL-IFN from precipitation was higher when crude BoL-IFN containing more fetal bovine serum (FBS) was used. However, purity of BoL-IFN recovered from the gel filtration column was highest when crude BoL-IFN with no FBS was used. The use of 25% ethylene glycol in the column elution buffer resulted in over 93% recovery of the applied IFN activity, versus only 25% when buffer contained no ethylene glycol. Column-purified BoL-IFN was further concentrated by ultrafiltration and analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) in denaturing buffer. When crude BoL-IFN containing no FBS was used for purification, BoL-IFN from a selected column fraction applied to SDS-PAGE resulted in a single narrow band with an apparent molecular weight (MW) of 19,000 Da. Extraction of the SDS-PAGE gel resulted in a single peak of IFN activity indicating identity of the activity and the polypeptide. This proved to be a practical method for obtaining sufficient quantities of purified natural BoL-IFN for use in the production of monoclonal antibodies to BoL-IFN and other biological experiments.     

桑枝中氧化白藜芦醇的分离与鉴定

氧化白藜芦醇具有抑制酪氨酸酶活性的作用。为了从桑枝中有效提取这一生物活性物质,采用乙醇提取法获得桑枝粗提液,通过硅胶柱、葡聚糖柱柱层析法分离制备桑枝氧化白藜芦醇样品。运用核磁共振、HPLC-MS等方法鉴定样品的化学结构和分子质量,证实制备样品为氧化白藜芦醇,通过高效液相色谱检测其质量分数大于99%。研究结果为从桑枝中分离提取氧化白藜芦醇提供了一种简便有效的方法。     

圆孢芽孢杆菌A95抗菌蛋白的分离纯化及性质研究

对圆孢芽孢杆菌(Bacillus globisporus)A95产生的抗菌蛋白进行了分离纯化,并研究了其部分性质。菌株摇瓶发酵液离心后的上清液经硫酸铵40%~60%分级盐析获得粗提物。粗提物溶液经Sephadex G-100柱层析、DEAE-Sepharose Fast F low离子交换层析、Sephadex G-50脱盐纯化获得的抗菌蛋白,通过性质检测、电泳及MALDL-TOF-MS质谱检测,表明为分子量1.464~1.529 kD的一组环肽类抗菌蛋白。该抗菌蛋白对多种家蚕病原真菌具有较好的抗菌活性,参照美国国家临床试验标准化委员会(NCCLS)提出的标准,用微量液基稀释法分别测定了对绿僵菌、白僵菌和黄曲霉的最小抑菌浓度(MIC)和最小杀菌浓度(MFC)。该抗菌蛋白对热稳定,对胰蛋白酶、蛋白酶K、氯仿有一定的耐受性,对酸部分敏感,对碱稳定。     

The antigenic activity of chromatographic fractions of a saline extract of Taenia saginata (Goeze, 1782) proglottides

A saline extract of a homogenate of Taenia saginata proglottides was partially purified by gel filtration chromatography on Sephadex G200 or Sepharose 4B and by ion exchange chromatography on DEAE cellulose. Gel filtration produced two distinct fractions with different antigenic properties. The first was of molecular weight of approximately 1,000,000 and contained a high level of activity in the haemagglutination inhibition test. The second fraction of molecular weigh of approximately 100,000 contained most of the immuno-precipitin activity. Other fractions had little or no antigenic activity. Eight fractions were obtained by DEAE cellulose chromatography, of which 4 had detectable antigenic activity. Subsequent rechromatography of fractions obtained by gel filtration on DEAE cellulose produced relatively pure fractions of high antigenic activity, from which small molecular weight contaminants had been removed.     

A protective antigen for Turkeys purified from a type 1 strain of Pasteurella multocida

A protective antigen was purified from a saline extract of a Type 1 strain of Pasteurella multocida by chromatographic methods, and its chemical and immunological ccharacteristics were studied. Three protein peaks were obtained from crude extract by gel filtration with Sephadex G-200. A bacteria-specific antigen was detected only in the first peak fraction, which, after passing through an immunoadsorbent column to remove any components originating from the growth medium, was adsorbed onto DEAE-cellulose followed by elution with a gradient of NaCl. From the first peak fraction of the gel filtration, 4 protein peaks were obtained, the second and third peaks being the major ones. Carbohydrate/protein ratios of the peak fractions varied from 0.06 to 1.0. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis showed that 2 proteins of molecular weights 44 000 and 25 000 were present in all the fractions. The 4 DEAE-cellulose fractions (DP-1 to DP-4) contained a single antigenically identical material, and induced protective immunity in turkeys against challenge exposure. The second peak fraction from DEAE-cellulose (DP-2) protected turkeys when subcutaneously injected as 2 doses of 10 μg protein with a 14-day interval between doses. The DP-2 fraction induced antibodies in rabbits which formed a single precipitin line against the crude extract. The purified antigen (DP-2) from a Type 1 strain was antigenically distinct from a similar antigen purified from a Type 3 strain; there was no significant cross protection in turkeys between the 2 antigens. These results indicate that protective antigens purified from soluble extracts of a Type 1 or Type 3 strain possess similar physicochemical properties, but that they are immunologically distinct from each other.     

鸡和猪分泌型免疫球蛋白A结构蛋白的比较

通过SephadexG 2 0 0凝胶过滤和DEAE纤维素柱 ,分别从胆汁和初乳中提纯鸡和猪的分泌型免疫球蛋白A (SIgA)。SDS PAGE结果显示 ,鸡SIgA的轻链分子量约为 2 6 0 0 0～ 2 80 0 0 ,与鸡IgG的轻链分子量相似 ,而重链分子量约为 670 0 0～ 70 0 0 0 ,比鸡IgG的分子量要大。猪的SIgA与猪IgG的轻链和重链的分子量均相同。轻链的分子量约为 2 6 0 0 0～ 2 80 0 0 ;重链的分子量约为 53 0 0 0～ 570 0 0。猪SIgA中J链的分子量为 1 6 0 0 0～ 1 70 0 0。本实验证明鸡SIgA轻链的分子量与猪的SIgA的轻链相似 ,而鸡SIgA重链的分子量则高于猪的SIgA的重链     

Isolation of exfoliative toxin from Staphylococcus hyicus subsp. hyicus and its exfoliative activity in the piglet

Exfoliative toxin was isolated from the sterile cell-free filtrate of 24 h culture of Staphylococcus hyicus subsp. hyicus strain P-1. The partial purification of exfoliative toxin produced by S. hyicus (shET) was performed by precipitation with 50-80% saturated ammonium sulfate, gel filtration on a Sephadex G-75 column and column chromatography on DEAE-cellulose. Partially purified shET (pp-shET) caused exfoliation in piglets at 8 to 12 h after intradermal or subcutaneous injection. However, heat-treated pp-shET did not cause exfoliation in piglets for up to 24 h after injection. On histopathological examination of the skin at 12 h after injection of pp-shET, an intraepidermal cleavage plane was shown between the stratum corneum and stratum granulosum and at the stratum granulosum.     

铜缺乏对奶牛肝脏金属硫蛋白代谢的影响

为阐明金属硫蛋白在铜缺乏奶牛肝脏中的代谢特征 ,选择铜缺乏区有明显临床症状的奶牛 6头 ,采集肝脏样品后用差速离心法分离肝脏金属硫蛋白 ,以Sephadex G75进行层析纯化 ,测定各部分洗脱液中金属元素铜、锌、铁、镁的含量。将 6头健康奶牛的肝脏样品作为对照。试验结果表明 ,发病奶牛肝细胞浆Sephadex G75柱层析洗脱液中铜、铁含量峰值显著高于健康奶牛 ,且在后面部分层析液中出现小峰 ;发病奶牛肝细胞浆金属硫蛋白 (MT)层析液锌、镁含量曲线峰值宽阔且高于对照组 ,第 2峰形宽大且有前移现象。结论 :铜缺乏能够改变奶牛肝脏中金属硫蛋白的代谢     

Studies on Aspergillus Fumigatus; Hydrolysis of Polyamino Acids by Mycelial Filtrate and Chromatographic Fractionation of the Filtrate

Mycelial filtrates from Aspergillus fumigatus (AF), shown to possess haemolytic, toxic, casein precipitating, and protein hydrolyzing activity, hydrolyzed poly-L-lysine and poly-L-glutamine in the pH range 4.6—5.3. Incipient activity against poly-L-lysin was observed at pH 9. Owing to spontaneous hydrolysis of the polyamino acid at pH > 10, no activity optimum could be traced.Gel filtration of mycelial filtrate on Sephadex G-75 or G-100 columns offered no definite information whether the protein hydrolyzing activity, using haemoglobin as substrate, at the optimum pH values, 2.9, 4.6 and 10, shows the activity of a single enzyme with more than 1 pH optimum or of more than 1 enzyme active at different pH values. Certain results of the investigations seem to indicate that the protein hydrolyzing activity at pH 2.9 was not caused by enzymes identical with the enzyme (s) causing the protein hydrolyzing activity at pH 4.6 or pH 10.Casein precipitating and protein hydrolyzing activity occurred, following gel filtration on a Sephadex G-100 column, in identical fractions whereas neither haemolysin nor toxin could be found in samples of 0.5 ml fraction solution from any of the fractions after filtration on Sephadex G-75 or G-100 columns.By using antiserum to a crude filtrate from a homologous AF strain it could be shown, applying immuno-electrophoresis, that dialyzed mycelial filtrate contained 8 precipitating antigens whereas proteinase purified by gel filtration and displaying protein hydrolyzing activity at pH 2.9, pH 4.6 and pH 10 contained 4 such antigens.     

Bovine interleukin 2: biochemical and biological characterization

Interleukin 2 (IL-2), secreted by bovine peripheral blood mononuclear cells (PBL) on stimulation with concanavalin A (Con A), was purified and characterized by different chromatographic and electrophoretic techniques. The ability of IL-2 to support proliferation of Con A-stimulated bovine lymphoblasts was used to assay and quantitate IL-2 activity. Bovine IL-2 having an apparent MW of 27,000 eluted from a gel-filtration column; from an anion exchange column peak activity was detected at 190 mM NaCl. Binding of bovine IL-2 to phenyl-Sepharose gel and elution with 35-60% ethanediol indicated its hydrophobic nature. Studies on cross-species reactivity revealed that both buffalo and goat lymphocytes respond to cattle IL-2 and detected 35% of activity from a standard cattle IL-2 preparation. Sheep lymphocyte response to cattle IL-2 was negligible.     

禽源多杀性巴氏杆菌(A:1)荚膜保护性抗原提纯及单克隆抗体细胞系建立

用Sep(?)adex G-200分之筛层析、DEAE-cellulose离子交换层析相结合,将禽源多杀性巴氏杆菌(A:1)荚膜抗原粗提物(CE)分为P1.P2两种成分,并经免疫保护试验证明,荚膜中含有保护性蛋白成份P1。P2分子量为129 100,且至少含有分子量分别为46700、42600和39800的3种蛋白亚基。用CE免疫BALB/c小鼠,建立了抗P1的单克隆抗体细胞系1B1和2B7,它们只与多杀性巴氏杆菌反应,而不与其他细菌交叉。     

鸡免疫球蛋白G Fc(IgG Fc)片段的分离纯化及其抗血清的制备 Ⅱ.豚鼠抗鸡IgG Fc片段血清的制备

经硫酸铵盐析、DEAE 32-纤维素和Sephadex G 200柱色谱法分离得到纯化的鸡血清IgG。然后用木瓜蛋白酶水解IgG,再经DEAE 32-纤维素柱色谱纯化制得IgG Fc片段,并以IgG Fc片段免疫豚鼠制备豚鼠抗鸡IgG Fc血清。