rBS-WC霍乱疫苗的动物免疫方案及免疫持久性

用小鼠、家兔观察了rBS-WS疫苗免疫的部分方案的效果。rBS与WC单独使用的免疫效果不如组合使用的效果好;小鼠或家兔的免疫间隔作适当缩短对免疫保护影响不大;小鼠一次大剂量口服疫苗后亦可获得良好保护。家兔肌肉注射免疫条件下rBS-WC与吸附霍乱类毒素菌苗(上海苗)及吸附霍乱菌苗(武汉苗)进行比较,武汉苗无抗CT反应,对CT攻击无保护,对Eltor(小川)攻击保护效果较差,上海苗则抗CT反应较低。家兔口服rBS-WC半年后,抗CT及杀弧菌抗体维持较高水平,显示其动物免疫的持久性。     

不同支持物对攀援植物--葎草雌雄株光合特性及生物量结构的影响

葎草[Humulus scandens(Lour.)Merr.]为草本雌雄异株攀援植物,采用野生种群人为控制的方法,设置分枝找到乔木支持物(高度(3±0.5)m)、灌木支持物(高度(1±0.5)m)和无支持物3种生长方式,测定雌(♀)、雄(♂)株分枝的叶面积参数、光合参数、叶绿素含量、可溶性糖含量及茎、叶、花在分枝、构件、单株水平下生物量分配比等指标,分析支持物对分枝光合特性和生物量结构的影响,探讨雌、雄分枝利用支持物的性别差异及响应支持物的生态适应差异。结果表明:(1)分枝的单叶面积、总叶面积、叶面积比率、比叶面积对支持物响应存在性别差异,♀株叶面积参数均大于♂株;支持物差异主要影响叶绿素a含量,对叶绿素b、叶绿素a/b影响不显著。(2)支持物差异对分枝叶片的光合参数均有显著的影响(P0.05),支持物对光合参数影响顺序为GsPnTrCi,性别差异影响顺序为GsTrPnCi;可溶性糖含量在性别间、支持物间均表现出极显著的差异(P0.01),♂株糖含量显著高于♀株。(3)在分枝水平下,♀株叶、茎及花生物量分配比都未受到支持物不同的影响(P≥0.05),而♂株在叶、茎的生物量分配比方面受影响显著(P0.05);在构件水平下,支持物差异显著影响了♂株分枝间的营养生长构件分配比,显著影响了♀株分枝间的生殖生长构件分配比;在单株水平下,叶分配比仅在支持物间差异显著(P0.05),而茎、花分配比在性别间、支持物间均有显著差异。(4)雌雄分枝的光合特性和生物量结构对不同支持物的响应差异明显,使葎草单株的生理整合性和适应性大幅度提高。研究以雌雄异株攀援植物为材料,从分枝水平分析支持物对雌雄株光合特性及生物量结构的影响,研究结果对探讨雌雄异株攀援植物的生态适应性具一定的价值。     

一种新的免疫吸附亲和层析柱的制备及其应用

本文介绍用加工成颗粒性的硝酸纤维素作为固相配体支持物,制备一种新的免疫吸附亲和层析柱,用于纯化AFP。该法制备简单,固相支持物连接抗体之前不需活化处理和使用化学交联剂。实验结果表明,纯化的AFP纯度较高,收获量也大,是一种实用的柱层析技术。     

苦瓜植株不同构件层次对支持物直径变化的行为反应

 采用实验生态学的方法,在提供不同直径支持物的情况下,对攀援植物苦瓜(Momordica charantia)不同构件层次的形态可塑性反应、生物量积累和生物量配置的变化进行了研究。结果表明：1)支持物直径对植株分枝出现的时机无明显影响,但分枝数量和分枝在主茎上的着生位置受支持物直径影响较大;2)植株个体水平比分枝水平对支持物直径的变化有更灵敏的反应,当支持物直径较大时,植株个体表现出对支持物较强的寻觅能力：主茎伸长受阻,比茎长变大,分枝数量和分枝率增大,分枝长度增加,比叶柄长度增加,根冠比减小;3)分枝形态特征和生物量特征对支持物直径的变化均无显著反应;4)苦瓜植株个体水平上的形态特征变化、生物量配置格局的改变以及分枝行为的变化是植株对支持物有效性变化的响应,有利于增强植株“寻觅”支持物的能力。     

压电免疫传感器固定方法

抗原抗体在石英晶体电极表面固定而不丧失其活性是压电免疫传感器成功的关键,直接影响到它的灵敏度和可重复性等性质。介绍了压电免疫传感器传统的表面固定方法:主要有戊二醛交联法、自组装单分子膜法(SAM)、蛋白A固定法;以及国内外最新研究的不需通常固定化步骤的方法,主要是压电凝胶免疫分析法(LEPIA)和PEG压电凝胶分析法,并对这些方法的发展前景做了展望 。     

支持物对攀援葎草分枝形态塑性和繁殖对策影响的性别差异

葎草(Humulus scandens)为草本雌雄异株攀援植物,采用野生种群人为控制的方法,设置单株觅到乔木(高度(3±0.5)m)、灌木(高度(1±0.5)m)和无支持物3种生长方式,测定分枝的生物量分配、形态特征和繁殖特征等指标,分析支持物对分枝形态可塑性和繁殖对策的影响,探讨雌(♀)、雄(♂)株分枝利用支持物的性别差异。结果表明:(1)支持物对葎草的茎、叶、花穗性状具有极强的可塑性,且表现出显著的性别差异,♀株的茎性状与花性状、♂株叶性状易受支持物的影响。(2)支持物对分枝生物量分配的影响呈显著的性别差异,♀株的分枝生物量分配差异性显著高于♂株;随支持物增高,♀株的茎分配比显著降低,而花分配比增加,但♂株的茎、花分配比均未受支持物的影响。(3)支持物对♀株分枝的繁殖指数和繁殖比率有极显著的影响(P0.05),对繁殖效率指数影响较小,而♂株则采用了相反的繁殖策略。     

检测特异性抗体分泌细胞(ASCs)的固相酶联免疫斑(ELISPOT)技术的建立

ＥＬＩＳＰＯＴ技术是目前国外评价疫苗免疫原性和免疫应答机理研究中最常使用的方法。本文用自制的ＮＣ膜２４孔板为固相支持物,建立了检测小鼠脾细胞中特异性ＡＳＣｓ的ＥＬＩＳＰＯＴ技术,在检测方法的特异性、结果的稳定性上均取得了满意的效果。并对该方法的某些实验条件进行了摸索。     

5-羟色胺在豚鼠胰腺分布的免疫组织化学研究

本研究用ABC免疫染色法,结合葡萄糖氧化酶-DAB-硫酸镍铵(Glucose oxidase-DAB-Nickle,GDN)显色技术,在Bouin液固定的常规石蜡切片上,研究了5-羟色胺(5-hydroxytryptamin,5-HT)在豚鼠胰腺内的定位和分布,并用相邻切片免疫双标记,观察了它与胰岛素的共存关系,结果发现,在豚鼠胰腺内,外分泌部均有5-HT免疫反应细胞分布。在胰腺内分泌部(胰岛)5-HT免疫反应细胞分布均匀,大部分胰岛细胞呈阳性5-HT样免疫反应,用相邻薄切片免疫双标记技术证明,胰岛内的5-HT免疫反应细胞主要是B细胞。在胰腺外分泌部,5-HT免疫反应细胞呈单个分散或聚集分布,主要位于腺泡和导管等处,偶见于结缔组织间隔中。本文对研究5-HT在胰腺的生理作用及其机制提供了形态学依据。     

基因工程

聚丙烯经改良可用寡核酸合成的新型固相支持物。这种物质溶剂抗性好,经久耐用。先将此塑料制品暴露于射     

用免疫点试验检测未浓缩的杂交瘤培养上清液中的同型和轻链型鼠单克隆抗体

<正>长期以来生物化学家们在核酸的工作中就广泛利用硝酸纤维素滤膜作为一种固相支持物以吸附和固定核酸。Towbin等(1979)首先证实它在从聚丙烯酰胺胶转移或贴印蛋白的用途,随后又用于检测抗体。Sharon等(1979)和Hawkes等(1982)介绍了一种点-免疫结合试验,直接应用硝酸纤维膜中的抗原点来筛选单克隆抗体和其它抗体。 单克隆抗体技术的广泛应用,在许多实验室就产生了一种需要,即从大量的单克隆蛋白中简便地检查鼠免疫球蛋白同型物(isotype)和轻链类。生产抗同型血清既费力又费钱。如果将抗体固定在硝酸纤维膜上     

Immobilization of proteins on oxidized crosslinked Sepharose preparations by reductive amination

Mild periodate oxidation of certain commercially available crosslinked agarose beads (Sepharose CL-4B and CL-6B) results in the generation of aldehydo groups which were useful for immobilization of amino compounds by reductive amination using pyridine borane. Consumption of periodate ion and production of formaldehyde were only observed with crosslinked Sepharose preparations and were correlated with a binding capacity much greater than that of uncross-linked gels when subjected to the reductive amination reaction. Up to 50 mg (approximately 0.73 mumol) of bovine serum albumin and 30 mumol of glycylglycine were coupled per gram of moist oxidized Sepharose CL-6B. The immobilization reaction was shown to proceed at neutral pH requiring about 12 h for completion and to be relatively insensitive to temperature and pyridine borane concentration. The oxidized gel was shown to be stable for at least 2 months upon storage in 0.1 M acetic acid. This method has proven to be useful for the preparation of a variety of affinity matrices and immobilized enzymes.     

Detergent-solubilized proteoglycans in rat testicular Sertoli cells

Rat Sertoli cells were cultured for 48 h in the presence of [35S]sulfate and extracted with 4 M guanidine chloride. In this extract, a Sepharose CL-2B Kav 0.10 proteoheparan appeared lipid associated, since after addition of detergent it emerged at Kav = 0.65 on Sepharose CL-2B. Treatment of cells with 0.2% Triton X-100 released 35S-labeled material which was purified by ion-exchange chromatography and hydrophobic interaction chromatography on octyl-Sepharose. Proteoglycan with affinity for octyl-Sepharose (Kav = 0.30 and 0.12 on Sepharose CL-4B and CL-6B, respectively) mostly carried heparan sulfate chains with Kav = 0.38 and minor proportion of heparan chains with Kav = 0.77 on Sepharose CL-6B. An association with lipids was confirmed by intercalation into liposomes of this proteoheparan which might be anchored in the plasma membrane, via an hydrophobic segment and/or covalently linked to an inositol-containing phospholipid. Non-hydrophobic material consisted of: (i) proteoheparan slightly smaller in size than lipophilic proteoheparan and possibly deriving from this one and (ii) two heparan sulfate glycosaminoglycan populations (Kav = 0.38 and 0.86 on Sepharose CL-6B) corresponding to single glycosaminoglycan chains and their degradation products.     

羊栖菜褐藻糖胶抗凝血活性的研究

本文研究了羊栖菜褐藻糖胶的化学组成和抗凝血活性之间的关系。采用热水提取得羊栖菜粗多糖,CaCl2纯化得褐藻糖胶,DEAE Sepharose CL-6B柱层析与Sepharose CL-6B柱层析对褐藻糖胶进行分级,得到F1、F2、F31、F32和F33五个级分,均为岩藻糖、半乳糖和甘露糖等糖基组成的杂多糖,并含有硫酸酯和糖醛酸以及少量的蛋白质,相对分子质量范围2．5万～95万。采用活化部分凝血活酶时间(APTT)和凝血酶时间(TT)检测了这5个级分的抗凝血活性,结果显示,羊栖菜褐藻糖胶能显著延长APTT的凝血时间,而对TT的影响不明显。F1、F31和F32对APTT的影响比较显著,而F2、F33和羊栖菜粗多糖的影响较小。研究表明,羊栖菜褐藻糖胶主要是通过抑制内源凝血途径而达到抗凝血的效果,其抗凝血活性与褐藻糖胶的硫酸基含量成正相关,而与相对分子质量和糖醛酸含量无关。     

Hyaluronate-Binding Proteins of Murine Brain

The distribution of hyaluronate-binding activity was determined in the soluble and membrane fractions derived from adult mouse brain by sonication in low-ionic-strength buffer. Approximately 60% of the total activity was recovered in the soluble fraction and 33% in membrane fractions. In both cases, the hyaluronate-binding activities were found to be of high affinity (KD = 10(-9) M), specific for hyaluronate, and glycoprotein in nature. Most of the hyaluronate-binding activity from the soluble fraction chromatographed in the void volume of Sepharose CL-4B and CL-6B. Approximately 50% of this activity was highly negatively charged, eluting from diethylaminoethyl (DEAE)-cellulose in 0.5 M NaCl, and contained chondroitin sulfate chains. This latter material also reacted with antibodies raised against cartilage link protein and the core protein of cartilage proteoglycan. Thus, the binding and physical characteristics of this hyaluronate-binding activity are consistent with those of a chondroitin sulfate proteoglycan aggregate similar to that found in cartilage. A 500-fold purification of this proteoglycan-like, hyaluronate-binding material was achieved by wheat germ agglutinin affinity chromatography, molecular sieve chromatography on Sepharose CL-6B, and ion exchange chromatography on DEAE-cellulose. Another class of hyaluronate-binding material (25-50% of that recovered) eluted from DEAE with 0.24 M NaCl; this material had the properties of a complex glycoprotein, did not contain chondroitin sulfate, and did not react with the antibodies against cartilage link protein and proteoglycan. Thus, adult mouse brain contains at least three different forms of hyaluronate-binding macromolecules. Two of these have properties similar to the link protein and proteoglycan of cartilage proteoglycan aggregates; the third is distinguishable from these entities.     

Partial characterization of proteoglycans synthesized by human glomerular epithelial cells in culture

Confluent adult and fetal human glomerular epithelial cells were incubated for 24 h in the presence of [3H]-amino acids and [35S]sulfate. Two heparan-35SO4 proteoglycans were released into the culture medium. These 35S-labeled proteoglycans eluted as a single peak from anion exchange chromatographic columns, but were separable by gel filtration on Sepharose CL-6B columns. The larger heparan-35SO4 proteoglycan eluted with the column void volume and at a Kav of 0.26 from Sepharose CL-4B columns. The most abundant medium heparan-35SO4 proteoglycan was a high buoyant density proteoglycan similar in hydrodynamic size (Sepharose CL-6B Kav 0.23) to those previously described in glomerular basement membranes and isolated glomeruli. Heparan-35SO4 chains from both proteoglycans were 36 kDa. A smaller proportion of Sepharose CL-6B excluded dermatan-35SO4 proteoglycan was also synthesized by these cells. The predominant protein cores of both medium heparan-35SO4 proteoglycans were approximately 230 and 180 kDa. A hybrid chondroitin/dermatan-heparan-35SO4 proteoglycan with an 80-kDa protein core copurified with the smaller medium heparan-35SO4 proteoglycan. This 35S-labeled proteoglycan appeared as a diffuse, chondroitinase ABC sensitive 155-kDa fluorographic band in sodium dodecyl sulfate-polyacrylamide gels after the Sepharose CL-6B Kav 0.23 35S-labeled proteoglycan fraction was digested with heparitinase. The heparitinase generated heparan sulfate proteoglycan protein cores and the 155-kDa hybrid proteoglycan fragment had molecular weights similar to those previously identified in rat glomerular basement membrane and glomeruli using antibodies against a basement membrane tumor proteoglycan precursor (Klein et al. J. Cell Biol. 106, 963-970, 1988). Thus, human glomerular epithelial cells in culture are capable of synthesizing, processing, and releasing heparan sulfate proteoglycans which are similar to those synthesized in vivo and found in the glomerular basement membrane. These proteoglycans may belong to a family of related basement membrane proteoglycans.     

Human alfa-fetoprotein: isolation and production of monoclonal antibodies.

Alfa-fetoprotein from human cord serum was purified in a single step by hydrophobic interaction chromatography on Phenyl Sepharose CL-4B with a final recovery of alfa-fetoprotein of about 90% and a purification factor of 900. The purified preparation was homogeneous on SDS-PAGE and native PAGE running with a relative molecular weight of 72,000. Monoclonal antibodies against this purified preparation were raised by hybridoma technology using Sp2/0 myeloma cells as a fusion partner. 50% of culture wells exhibited hybrid growth and 7% of these wells contained anti-AFP secreting hybrids. Positive hybrid cells were cloned twice by the limiting dilution method and 8 clones were obtained that secreted monoclonal antibodies. Five of these cell lines (3F6H10, 3F6H4, 3F6H1, 3F6G5 and 3F6G10) were selected at random for purification and characterization purposes. All 5 cell lines secreted monoclonal antibodies of IgG1 subclass which were purified by affinity chromatography on Protein A- Sepharose CL-4B column with a final recovery of 80% and a purification factor of about 13. The purified preparations were homogeneous on SDS-PAGE, native PAGE and IEF. The monoclonal antibodies were highly specific for human alfa-fetoprotein as determined by Western blotting. The affinity constants (K) of these Mab ranged from 10(6) to 10(9) l/mol.     

Aggregated proteoglycan synthesis in organ cultures of human nucleus pulposus.

Proteoglycans isolated under associative conditions in the presence of protease inhibitors from human nucleus pulposus contained 17% aggregate and 83% non-aggregating monomer (Kav = 0.5 on Sepharose CL-2B). Isolated aggregate after reduction and alkylation was resolved into two components (Kav = 0.15 and 0.43) on Sepharose CL-2B. Labeled proteoglycans isolated from parallel samples pulsed with [35S]sulfate and chased for up to 18 h were present largely as aggregated material (up to 78%). Reduction and alkylation of the labeled samples gave a labeled proteoglycan monomer with Kav = 0.15. Both the labeled and unlabeled chondroitin sulfate chains had the same distribution on Sepharose CL-6B and equivalent molecular weights (Mr = 2.0 x 10(3)). After chondroitinase ABC digestion, the unlabeled keratan sulfate-protein core was polydisperse with a Kav = 0.38 on Sepharose CL-4B while the labeled keratan sulfate-protein core had a Kav = 0.05. This indicates that the newly synthesized proteoglycan had a large core protein and suggests that the proteoglycans present in nucleus pulposus are originally synthesized as large molecular weight, aggregating proteoglycans.     

An affinity gel for the inhibition, binding, and isolation of serine proteases

A preparation procedure for gels for the specific binding and inhibition of serine proteases is described. Phosphoryl trifluoride was synthesized and reacted with two different types of agarose gels, a crosslinked agarose (Sepharose CL-4B) and an agarose containing spacer arms with terminal vicinal-diol groups (a hydrolyzed epoxy-activated Sepharose 6B). The phosphoryl difluoride groups coupled to the gels were, in both cases, further modified by treatment with isopropanol to obtain isopropyl fluorophosphate groups covalently bound to the matrix. It was found that both modified gels absorbed and inhibited plasmin, but that the modified gel with spacer arms was markedly more efficient.     

Characterization of immunosuppressive substances in the basic protein fraction of uterine secretions from pregnant ewes

The basic protein fraction of ovine uterine secretions collected late in pregnancy (Days 125-140) contains a substance capable of inhibiting in vitro blastogenic responses of lymphocytes to phytohemagglutinin (PHA) or mixed lymphocyte reactions. In this study, the immunosuppressive substance in the basic protein fraction of uterine secretions was further defined by gel filtration. The immunosuppressive activity resided in a group of high molecular weight proteins eluting at the void volume of Sephacryl S-200 and Sepharose CL-6B columns. For example, incorporation of thymidine by PHA-stimulated lymphocytes incubated with 20, 40, 80, and 120 micrograms/ml of protein from the void volume of Sepharose CL-6B was 65, 28, 2, and 0 percent of control lymphocytes, respectively. Based on polyacrylamide-gel electrophoresis in the presence of sodium dodeylsulfate (SDS), the immunosuppressive fraction from Sepharose CL-6B chromatography contained aggregates of uterine milk proteins (UTM-proteins) and a pair of proteins running at the top of a 5% (w/v) polyacrylamide gel. Other protein peaks resolved by Sephacryl S-200 and Sepharose CL-6B contained aggregates of UTM-proteins but were not immunosuppressive. The substance inhibiting in vitro lymphocyte function was not of conceptus origin, because it was found in fluid from the ligated uterine horn of unilaterally pregnant ewes and from the uterus of an ovariectomized ewe treated for 60 days with progesterone and estrone.     

A general method for purification of deoxycytidine kinase.

Deoxycytidine kinase from a variety of animal tissues binds to Cibacron Blue 3G-A coupled to Sepharose CL-6B. The enzyme can be selectively eluted with ATP to yield single-step purifications of 17-89-fold. The affinity adsorbent is re-usable.