Antisera Raised Against the Drug Imipramine

Antisera against 2-aminoimipramine covalently coupled to albumin have been raised in two rabbits. Both antisera bind imipramine and related tricyclic compounds as if to a single class of sites with high affinity and high titres. Displacement/inhibition assays showed that the affinities of various tricyclic compounds for the antisera showed a good correlation with the affinities of these drugs for the tricyclic antidepressant inhibitory sites on plasma-membrane 5-hydroxytryptamine carriers of human platelets and rat brain cortex. 5-Hydroxytryptamine and 5-hydroxytryptamine-uptake-selective drugs did not inhibit [3H]imipramine binding to antisera. The anti-imipramine antibodies were purified using imipramine-Sepharose affinity chromatography and were shown to be IgG class by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and protein A-Sepharose precipitation.     

Antisera for radioimmunoassay of 17alpha-ethynylestradiol and mestranol

Antisera for 17α-ethynylestradiol and mestranol have been prepared by immunizing rabbits with 6-(O-carboxymethyl) oxime-bovine serum albumin conjugates prepared from 6-oxo-17α-ethynylestradiol and 6-oxomestranol, respectively. These antisera showed little cross-reaction with known metabolites of these steroids. A comparison is made between our antisera and some prepared by others, where coupling to the steroid is effected through the C-7 position.     

Mechanism for Inhibition of Deoxyribonuclease Activity by Antisera

The activity of bovine DNase, but not that of porcine DNase, is inhibited by antisera against bovine DNase, and vice versa. Inhibition of DNase is found in the immunoglobulin G-containing fractions, as shown by ion exchange chromatography. Inactive DNase, carboxymethylated specifically at the active site His¹³⁴, competes with active DNase and reverses the antisera inhibition of DNase, suggesting that the epitode responsible for inhibition does not contain the active site His¹³⁴. Alignment of the sequences of DNase of these two species shows that the greatest variation occurs between residues 153 and 163, within which are three consecutive peptide bonds, Lys-Trp-His-Leu, that are readily cleaved by trypsin, chymotrypsin, or thermolysin. The 8-hr digest of DNase by each of these three proteases has lost the ability to reverse antisera inhibition. The degree of antisera inhibition varies with the metal ion used as the activator for DNase-catalyzed reactions. When Mn²⁺, Co²⁺, or Mg²⁺ plus Ca²⁺ are used as activators, inhibition is approximately 50%. When pBR322 plasmid is used as substrate, gel electrophoresis shows that the DNase-catalyzed DNA hydrolysis produces a significant amount of double-strand cuts with Mn²⁺, Co²⁺, or Mg²⁺ plus Ca²⁺ as activators and antisera inhibit DNase action only on double-strand cuts. With only Mg²⁺ as the activator no double-strand cuts are observed, either in the presence or absence of antisera, and the DNase activity is not significantly inhibited. We conclude that antisera inhibition is due to antibody binding of the DNase polypeptide chain within residues 153 and 163. These residues are not crucial for catalysis, but are required for DNA binding, which results in double-strand cuts.     

Simultaneous Detection of Several Nepoviruses Infecting Grapevine in a Single DAS-ELISA Test Using Mixed Antisera

Single and mixed antisera have been compared in DAS-ELISA for the routine diagnosis of nepoviruses infecting grapevine. The use of mixed polyclonal antibodies allowed in a single test the simultaneous detection of several nepoviruses (ArMV + GFLV) or serotypes of nepoviruses (TBRV serotypes G + S and RRV serotypes E + G) whatever the nature of the antigens, e.g. purified virions, diseased grapevine leaves or grapevine wood shavings. The detection was as reliable and efficient as with simple antibodies. The plant samples which were positively diagnosed by mixed antisera often showed an increase of their absorbance values, in comparison with the detection using simple antisera, while the background level was unchanged. The origin of this enhancement remains unclear, but it seems to be closely related to the mixing of the conjugated antibodies.     

Antisera to the secretory component recognize the murine Fc receptor for IgA

Studies were undertaken to determine a possible structural relationship between the secretory component (SC) and the receptor for IgA (Fc alpha R). An IgA-mediated rosetting technique was used to assess the presence of Fc alpha R+ cells in various lymphoid tissues from normal BALB/c mice and mice bearing an IgA plasmacytoma (MOPC 315). Tissues from the MOPC 315-bearing BALB/c mice were found to have a significantly higher percentage of Fc alpha R+ cells; thus, nonadherent spleen cells from MOPC 315-bearing mice were used as a source of Fc alpha R+ cells in these studies. The cells were preincubated with anti-SC and then assayed for the ability of IgA to bind to the Fc alpha R. Antisera to SC from various species inhibited the formation of IgA-mediated rosettes, although preincubation of the Fc alpha R+ cells with antisera directed against other cell surface molecules (e.g., Thy1.2, Lyt1, Lyt2, Fc gamma R, MHC class I and II) or preimmune sera had no significant effect on IgA-mediated rosette formation. Preabsorption of the anti-SC with secretory IgA or with free SC removed the inhibitory effect; preabsorption with myeloma IgA had no effect. These data suggest that SC and Fc alpha R are related serologically and may be structurally related, possible in the IgA-binding region.     

水仙病毒血清学研究Ⅰ．水仙花叶病毒抗血清的制备及其应用

经人工接种分离纯化的水仙花叶病毒（NMV）,以表现局斑的苋色藜叶片为提纯材料,经聚乙二醇（PEG600）沉淀、差速离心和蔗糖密度梯度离心提纯后,进行6次家兔免疫注射制备抗血清。结果表明注射后3周左右效价最高,经毛细管沉淀方法测定可达1：5,000。用琼脂双扩散方法将此NMV抗血清与来自荷兰的NMV抗血清进行比较,结果发现二者的抗体性相同。应用此法制成的NMV抗血清,以琼脂双扩散、ELISA方法分别对30份水仙组培脱毒试管苗样本进行带毒率检测。结果表明所测得的平均带毒率分别为33．3％和80．0％,并用IEM测定方法验证了ELISA结果的可靠性和准确性。     

Antisera against small neurotransmitter-like molecules

Antisera were produced against three types of small neurotransmitter-like molecules: indolealkylamines, catecholamines and amino acid derivatives such as GABA. The specificity of the antisera were evaluated using radioimmunological or immunoenzymatic competition tests between a radiolabelled ligand or conjugated hapten, and analog molecules from the same metabolic pathway. The antibody site was characterized by the ratios of cross-reactivity and the affinity constants. On the basis of these in vitro studies, each immune response was found to be specific for the target molecule.     

Antisera specificities to beta-D-galactopyranoside cluster ligands

Mono-, di-, and tri-beta-D-galactopyranosides of 2-(5-hydrazinocarbonylpentanamido)-2-(hydroxymethyl)-1,3-propan edi ol [(Gal)n-TA] have been conjugated to bovine serum albumin (BSA), and used to study the binding specificities to the Gal receptors of liver parenchymal cells. In this study, rabbit antisera produced to the (Gal)n-TA-BSA were characterized by using an enzyme-linked, immunosorbent assay under conditions that allow only the antibodies directed to the carbohydrate part of the antigen to react with the solid-phase (Gal)n-TA-BSA antigens. Inhibition assays using (Gal)n-TA-BSA conjugates showed a relative specificity of the antisera for the number of Gal residues on the TA bridging group to the BSA carrier-protein, indicating that antibodies having specificities to oligosaccharide branch points can be produced. Inhibition assays with (Gal)n-TA haptens, Gal, and methyl beta-D-Gal indicated that the antibody combining-sites interact mainly with the Gal units; no inhibition was observed with the TA bridging group used as a hapten inhibitor. The spatial distances of the Gal units were apparently important for interaction with the anti-(Gal)n-TA-BSA antibody-combining-sites, as (Lac)3-TA-BSA and (Lac)3-TA exhibited relatively little inhibitory activity.     

大鼠精核蛋白抗血清的制备

用大鼠精核蛋白（Ｒａｔ　Ｐｒｏｔａｍｉｎｅ,ＲＰ）－核糖核酸（ＲＮＡ）复合物（ＲＰ－ＲＮＡ　Ｃｏｍｐｌｅｘｅｓ）免疫大鼠,得到了特异的抗ＲＰ抗血清,并用Ｉｍｍｕｎｏｄｏｔｔｉｎｇ和Ｉｍｍｕｎｏｂｌｏｔｔｉｎｇ方法验证了其特异性。该抗血清和ＲＰ有特异的反应,并和哺乳动物小鼠和羊的精核蛋白有一定程度交叉反应,而与体细胞类型核蛋白（Ｈ１,Ｈ２ａ,Ｈ２ｂ,Ｈ３,Ｈ４）无交叉反应。并对制备该抗血清的意义予以讨论。     

Anti-theta Antisera may Contain Anti-allotype Contamination

THETA (θ) is a tissue-specific mouse allo-antigen present in the highest concentrations in thymus and brain^1–3. Anti-θ allo-antisera are produced after multiple injections of thymus cell suspensions into hosts differing at the θ locus, but not at the principal histocompatibility locus (H-2). Anti-θ antisera have been used by many investigators^3–9 to differentiate thymus derived lymphocytes from non-thymus derived lymphocytes and to describe the relative role of each class of cells in various immunological functions. Because it is possible that some thymocytes bear immunoglobulins bound to the cell surface, we tested the hypothesis that anti-θ allo-antisera contain antibodies directed against immunoglobulin allotype specificities of the donor, as well as antibodies to the donor θ allo-antigens.     

The Production of Antisera to the Klebsiella Capsular Antigens

Three methods of antiserum production have been compared. One of these consistently gave rise to greater homologous quellung titres and was used routinely. A modification of this method using vaccines consisting of washed, killed suspensions of type strains resulted in no significant increase in titres or decrease in cross-reactions. Considerable differences were found between the homologous quellung titres and cross-reactions of antisera prepared in the same laboratory on different occasions.     

Comparison of Immunization Methods for Producing Reference Adenovirus Antisera in Horses

Horses were immunized by a variety of inoculation procedures designed to determine the most efficient method of producing antisera to adenovirus types 25 to 31. The procedures evaluated included immunization by (i) direct intravenous (iv) injection, (ii) iv infusion, (iii) intramuscular (im) injection of virus with and without Freund's incomplete adjuvant, (iv) combined iv and im injections, and (v) combined iv infusion and im injection. The im schedule (no. 3) was superior to the others in terms of immunizing antigen and time required, and hemagglutination-inhibition (HI) and serum-neutralizing (SN) antibody levels produced. HI and SN tests performed with sera before and after heating at 56 C for 30 min showed that heat-inactivation was not necessary for tests with equine antisera.     

Method for Typing Antisera to Herpesvirus hominis by Indirect Hemagglutination Inhibition

A test for typing antisera to Herpesvirus hominis that uses the method of indirect hemagglutination inhibition is described. The test, which is based upon the differential absorption of herpes antisera by preparations of type 1 and type 2 antigens, is rapidly and easily performed. The results permit some conclusions to be drawn regarding the antigenic relationships between the two virus types. Some of the practical limitations of the test are discussed.