| CPC G01N 33/57438 (2013.01) [G01N 33/5304 (2013.01); G01N 2333/75 (2013.01)] | 2 Claims |
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1. A detection method of dot immunoblotting detection, comprising:
connecting a portable sputum aspirator with a hole plate through a hose, cutting a nitrocellulose membrane into a size which is the same as the size of an upper-layer supporting plate on the upper end surface of the hole plate, placing the nitrocellulose membrane onto the hole plate having a plurality of through holes, turning on the portable sputum aspirator, setting a negative pressure value of the portable sputum aspirator to be 0.06 MPa, and forming a plurality of sample injection grooves in the surface of the nitrocellulose membrane;
dividing the plurality of sample injection grooves into reference substance holes and sample holes, each repeated for three times, separately adding a reference substance and 1 μL of a sample to be tested into each reference substance hole and each sample hole, and naturally air drying the nitrocellulose membrane for 30 minutes at the end of the sample injection;
placing the nitrocellulose membrane into a skim milk powder solution with a concentration of 5%, placing the skim milk powder solution onto a shaking table for blocking at room temperature for 1.5 hours, abandoning the blocking liquid, and rinsing the membrane with Tris Buffered Saline and Polysorbate-20 (TBS-T), wherein the skim milk powder solution with the concentration of 5% is obtained by diluting a skim milk powder solution with a TBS-T solution until the concentration is 5%;
diluting a primary antibody with a bovine serum albumin solution with a concentration of 5% in a ratio of 1:500, uniformly and completely immersing the nitrocellulose membrane into the diluted primary antibody, placing the mixture onto the shaking table, carrying out constant temperature incubation at 37° Celsius for 4 hours, and placing the nitrocellulose membrane into the TBS-T at the end of the incubation for washing on the shaking table, for 5 minutes at each time, wherein the bovine serum albumin solution with the concentration of 5% is obtained by diluting a bovine serum albumin solution with the TBS-T solution until the concentration is 5%;
diluting a secondary antibody with a skim milk powder solution with a concentration of 1% in a ratio of 1:5000, uniformly and completely immersing the nitrocellulose membrane into the diluted secondary antibody, placing the mixture onto the shaking table, carrying out incubation at room temperature for 1.5 hours, and placing the nitrocellulose membrane into the TBS-T at the end of the incubation for washing, for 15 minutes at each time, wherein the skim milk powder solution with the concentration of 1% is obtained by diluting a skim milk powder solution with the TBS-T solution until the concentration is 1%;
laying the washed nitrocellulose membrane at a proper position of a developing device, uniformly adding dropwise a developer onto the nitrocellulose membrane, and using a gel imaging system to carry out exposure and development, and saving an image; and
scanning and analyzing, by means of Image J software, a gray value of an image obtained by the development, and expressing a relative concentration of a target protein of each sample by using a gray value of a reference sample;
wherein the TBS-T solution comprises Tris, NaCl, Polysorbate-20 and ddH2O; wherein, a mass of the Tris is 2.42 g; a mass of the NaCl is 8.0 g; a volume of the Polysorbate-20 is 1 mL; and a volume of the TBS-T solution is supplemented to 1000 ml by using the ddH2O; and
wherein the secondary antibody is labeled by horse radish peroxidase.
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