44 results about "Microcystin-LR" patented technology

The invention discloses an alga lysing / algal toxin degradation double-effect engineering strain Y1 and a construction method thereof, belonging to the field of microbiology for treatment of blue-green algae. Fusion is performed on parent strains with alga lysing and algal toxin degradation functions by utilizing a protoplast fusion technology to construct the double-effect engineering strain with excellent traits of parents, namely Bacillussphaericus with the collection number of CGMCCNO. 7519. The alga lysing and the derived algal toxin pollution problem are synchronously solved. The protoplast fusion rate can achieve 31.97% under optimal conditions, and the double-effect engineering strain has certain guide effects on solving the problems of blue-green alga bloom and the derived MC-LR (microcystin-LR) pollution and constructing the engineering strain integrating the MC-LR degradation function and the alga lysing property into a whole by performing a protoplast fusion technology, thereby providing reference for achieving the effect on treating both the root course and the symptoms for solving the large-area blue-green alga bloom problem.

The invention discloses a method for detecting microcystin-LR by self-assembly based on the end face of a gold nano-rod, belonging to the technical field of chemical immunoassay. In the invention, the end face of the gold nano-rod is respectively coupled with microcystin coating antigen and anti-microcystin antibody to form a probe of the gold nano-rod; and the synthesized probe of the gold nano-rod performs immunological reaction with the microcystin-LR so as to achieve the detection of the microcystin-LR through the change of the grain diameter of a nano-chain which is formed by the antigenantibody reaction of the end face of the gold nano-rod. The invention performs reaction in a liquid environment, only one step of reaction is needed without washing step, which simplifies the condition of the reaction, reduces labour intensity and improves the detection sensitivity.

The invention relates to a microcystic toxin-LR electrochemical detection method with amplified graphene signals. The method comprises the following steps: (1) dropwise adding a mixed solution with a ratio of an endonuclease reaction buffer solution: a graphene-aptamer compound: a microcystic toxin-LR solution to be detected: an endonuclease solution of (9-11):(4-6):(2-4):(1-3) on the surface of an MCH / Au NPs / Au electrode; (2) culturing the MCH / Au NPs / Au electrode for 1 to 2 hours at a temperature of 25 to 35 DEG C, slightly washing the electrode surface by ethanol and ultrapure water to remove weakly combined graphene, drying the electrode in nitrogen gas, taking the electrode out, carrying out electrochemical detection to measure the concentration of the microcystic toxin-LR solution. According to the provided method, a high sensitive electrochemical analysis technology and an aptamer with a high specific recognition performance are effectively combined to detect trace microcystic toxin-LR in the environment, the detection is highly sensitive and highly specific, moreover, the instruments are cheap and portable, the method is simple and easy to perform, and the results can be obtained quickly.

The invention relates to a method for detecting microcystin-LR through a palladium-gold alloy nanoscale cage immune chromatography test strip, and belongs to the technical field of immunity chromatography chemistry. The method comprises the following steps: preparing a Pd-Au bimetal nanoscale cage with a hollow structure by taking Pd nano-particles as seed crystals; spraying a monoclonal antibody for labeling the microcystin-LR to a combined pad; spraying BSA (Bovine Serum Albumin) coupling microcystin-LR on a detection line; spraying goat anti-rat IgG on a control line to prepare the immune chromatography test strip for fast detecting the microcystin-LR in a water body; and carrying out quantitative analysis on the microcystin-LR contained in a test sample by a competition immune chromatography and by reading the grey value of gold nanoscale cage-microcystin antibody mixture remained on the detection line. According to the method, because the adhesion of sulfhydryl and amido in a protein molecule of a Pd-Au alloy is higher than the binding force of a single-metal gold nanoscale cage by virtue of the synergistic action of two metal elements in the alloy, a microcystin antibody is easier to label by that Pd-Au alloy nanoscale cage than by the gold nanoscale cage, and the formed Pd-Au alloy nanoscale cage-microcystin antibody mixture is more stable.