Improved experimental buffer solution and application thereof
A buffer solution and experimental technology, applied in the field of biological detection, can solve problems such as false positives, achieve the effects of reducing electrostatic force, reducing non-specific binding, and improving detection resolution
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Embodiment 1
[0029] An embodiment of the improved experimental buffer of the present invention comprises the following components: Tris-HCl buffer, sodium chloride, 8-anilinonaphthalene-1-sulfonate, thimerosal, calf serum, casein, Na 2 EDTA and Procline300;
[0030] The mass volume ratio of the sodium chloride is 2.55%; the mass volume ratio of 8-anilinonaphthalene-1-sulfonate is 0.08%; the mass volume ratio of thimerosal is 0.02‰; the volume ratio of calf serum is 10% ; The mass volume ratio of casein is 0.2%; Na 2 The mass volume ratio of EDTA is 0.001%; the volume ratio of Procline300 is 0.1%.
[0031] The preparation method of the improved experimental buffer is as follows: prepare according to the preparation amount of 1L, accurately weigh 6.06g Tris, 0.01g Na 2 Add EDTA, 2.0g casein, 25.50g sodium chloride, 0.8g 8-anilinonaphthalene-1-sulfonate, 0.02g thimerosal into a clean container, add 300mL purified water to fully dissolve the solid reagent, slowly add 3.0mL Mix well with H...
Embodiment 2
[0033] An embodiment of the improved experimental buffer of the present invention comprises the following components: PB buffer, sodium chloride, 8-anilinonaphthalene-1-sulfonate, calf serum, bovine serum albumin, Na 2 EDTA and Procline300;
[0034] The mass volume ratio of the sodium chloride is 10.00%; the mass volume ratio of 8-anilinonaphthalene-1-sulfonate is 0.2%; the volume ratio of calf serum is 10%; the mass volume ratio of bovine serum albumin 0.2%; Na 2 The mass volume ratio of EDTA is 0.001%; the volume ratio of Procline300 is 0.1%.
[0035] The preparation method of the improved experimental buffer is as follows: prepare according to the preparation amount of 1L, accurately weigh 2.32g disodium hydrogen phosphate dodecahydrate, 0.44g sodium dihydrogen phosphate dihydrate, 0.01g Na 2 Add EDTA, 2.0g bovine serum albumin, 100.0g sodium chloride, 2.0g 8-anilinonaphthalene-1-sulfonate into a clean container, add 300mL purified water to fully dissolve the solid reag...
Embodiment 3
[0037] An embodiment of the improved experimental buffer of the present invention comprises the following components: MOPS buffer, sodium chloride, sodium salicylate, mouse serum, tryptone, Na 2 EDTA and Procline300;
[0038] The mass volume ratio of described sodium chloride is 1.60%; The mass volume ratio of sodium salicylate is 0.5%; The volume ratio of mouse serum is 10%; The mass volume ratio of tryptone is 0.2%; 2 The mass volume ratio of EDTA is 0.001%; the volume ratio of Procline300 is 0.1%.
[0039] The preparation method of the improved experimental buffer is as follows: prepare according to the preparation amount of 1L, accurately weigh 10.46g 3-(N-morpholine)propanesulfonic acid, 8.50ml triethanolamine, 0.01g Na 2 Add EDTA, 2.0g tryptone, 16.0g sodium chloride, 5.0g sodium salicylate into a clean container, add 300mL purified water to fully dissolve the solid reagent, then add 100mL mouse serum and 1.0mL Procline300 to make up the purified water to 1000mL, mix...
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