156 results about "Hemocyanin" patented technology

A method for preparing multicloning antibody includes synthesizing polypeptide, connecting the coupling agent with keyhole limpet hemocyanin for forming hapten ¿C carrier protein system, immunizing rabbit then picking up its blood for separating out serum, purifying out multicloning antibody of anti ¿C specific site amino acid phosphorylation protein and anti ¿C corresponding non phosphorylation protein after two steps of antigen affinity chromatography .

The invention relates to a preparation method and application of a miniature high-efficiency clenbuterol immuno-affinity chromatography column. The technical scheme is characterized by comprising the following steps of: preparing a high-quality antibody, synthesizing efficient prepared bromoacetyl chloride clenbuterol purified by a liquid chromatogram and thiolation hemocyanin into immunogen immune animals, and obtaining antiserum; reacting the purified bromoacetyl chloride clenbuterol with thiolation agarose to obtain clenbuterol-agarose padding, loading the padding into an antigen affinity chromatography column; and purifying a clenbuterol specific antibody in the antiserum by using the antigen affinity chromatography column. The preparation method of the clenbuterol immuno affinity chromatography column comprises the following steps of: coupling high-quality antibodies at high density to the agarose oxidized by periodic acid to prepare an antibody affinity padding, and placing 25 mul of padding in a small specially-made column to prepare the miniature immuno-affinity chromatography column. The immuno-affinity chromatography column provided by the invention can be used for specifically gathering clenbuterol in a sample to be tested at high efficiency and can increase the accuracy, reliability and sensitiveness of detection when being combined with an analytic instrument and colloidal gold test paper for use.

The invention relates to a pesticides benzoepin artificial antigen-antibody and it's preparing method and application, which specifically relates to preparing small molecular compound artificial hapten, antigen and antibody of cyclopentacliene pesticides benzoepin and application of establishing immunity analysis method. It uses benzoepin derivation as hapten to connect separately with carrier protein like hemocyanin and horse radish peroxidase so as to synthesis artificial antigen and enzyme antigen. Artificial antigen becomes antibody though animal immunity, taking-up blood, antiserum and purity.

The invention provides preparation of malachite green artificial antigen and antibody, and relates to preparation of artificial hapten, artificial antigen and antibody of a triphenylmethane chemical substance malachite green. By adopting the preparation method, the problems of complex process, high cost and low analysis speed of the traditional physical and chemical analysis method are overcome. A simple, convenient, quick, sensitive and accurate enzyme immunoassay is provided. The method comprises the following steps: taking 4-[bi(4-dimethylamino)phenyl]methyl benzoic acid and 5-{4-[bi-(4-dimethylamino)phenyl]methyl} phenyl valeric acid as haptens to be respectively connected with carrier proteins such as hemocyanin, ovalbumin and the like to synthetize artificial antigen; carrying out animal immunization, taking blood, separating out antiserum, and purifying, so as to prepare the antibody. The antibody is stable, and has good specificity and sensitivity, and a good application prospect, and can be applied to fast immunodetection of the malachite green.

The invention relates to an immunoassay kit for detecting ethopabate, and a preparation method and application thereof, belonging to the field of immunological detection. The kit comprises an ELISA plate coated with an ethopabate antigen, an ethopabate monoclonal antibody solution, an enzyme-labeled or fluorescently-labeled goat anti-mouse secondary antibody, a standard ethopabate solution, a washing solution and a diluent, wherein the ethopabate antigen is a conjugate of ethopabate semiantigen and a vector, and the vector is one or two selected from a group consisting of ovalbumin, bovine serum albumin, thyroid protein, hemocyanin, human serum albumin and polylysine. When applied to detection of ethopabate residues in animal food, the kit has the advantages of high sensitivity, precision and accuracy, good specificity, low cross-reaction rate, good stability, long storage time, easy operation, quickness and suitability for on-site primary screening of large quantities of samples, and is beneficial for simplifying residue analysis of ethopabate.