Piglet small intestine epithelial cell classification and separation method
A technology for intestinal epithelial cells and epithelial cells is applied in the field of piglet intestinal epithelial cell fractionation, which can solve the problems of inability to realize high-throughput research on physiological processes and metabolic changes, and achieve the effects of low cost and simple operation.
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Embodiment 1
[0025] The method for fractionating piglet intestinal epithelial cells comprises the following steps:
[0026] (1) Six 0-day-old suckling piglets were selected. After slaughtering, the small intestines of piglets with a length of 60 cm were cut, and 100 mL of preheated oxygenated phosphate buffer solution at 37 ° C was perfused into the intestinal cavity, and both ends were clamped with hemostatic forceps. Incubate in a water bath shaker at ℃ for 30 minutes at a shaking speed of 70 rpm;
[0027] Among them, the phosphate buffer solution is composed of: sodium chloride 150mM, sodium dihydrogen phosphate 4mM, disodium hydrogen phosphate 4mM, phenylmethylsulfonyl fluoride 0.1mM, dithiothreitol 0.4mM, pH 7.4.
[0028] (2) Discard the phosphate buffer, perfuse 100mL of cell separation solution, and continue to incubate in a water bath shaker at 37°C for 2.5 hours at a shaking speed of 70 rpm. Minutes, 120 minutes and 150 minutes to collect cell separation fluid and perfuse new cel...
Embodiment 2
[0033] The method for fractionating piglet intestinal epithelial cells comprises the following steps:
[0034] (1) Six 25-day-old weaned piglets were selected. After slaughtering, the piglets’ small intestines with a length of 80 cm were cut, and 110 mL of preheated oxygenated phosphate buffer solution at 37 ° C was perfused into the intestinal cavity, and both ends were clamped with hemostatic forceps. Incubate in a water bath shaker at ℃ for 30 minutes at a shaking speed of 70 rpm;
[0035] Among them, the phosphate buffer solution is composed of: sodium chloride 142mM, sodium dihydrogen phosphate 5mM, disodium hydrogen phosphate 5mM, phenylmethylsulfonyl fluoride 0.2mM, dithiothreitol 0.5mM, pH 7.4.
[0036] (2) Discard the phosphate buffer, perfuse 110mL of cell separation solution, and continue to incubate in a water bath shaker at 37°C for 2.5 hours at a shaking speed of 70 rpm. Minutes, 115 minutes and 150 minutes to collect cell separation fluid and perfuse new cell s...
Embodiment 3
[0041] The method for fractionating piglet intestinal epithelial cells comprises the following steps:
[0042] (1) Select 6 70-day-old piglets, cut the small intestine section with a length of 90cm after slaughtering, perfuse 150mL of preheated oxygenated phosphate buffer solution at 37°C in the intestinal cavity, clamp both ends with hemostatic forceps, and incubate at 37°C Incubate in a water bath shaker for 30 minutes at a shaking speed of 70 rpm;
[0043] Among them, the phosphate buffer solution is composed of: sodium chloride 135mM, sodium dihydrogen phosphate 6mM, disodium hydrogen phosphate 6mM, phenylmethylsulfonyl fluoride 0.3mM, dithiothreitol 0.6mM.
[0044] (2) Discard the phosphate buffer, perfuse 150mL of the cell separation solution, and continue to incubate in a water bath shaker at 37°C for 2.5 hours at a shaking speed of 70 rpm, and collect the cells at 40 minutes, 90 minutes and 150 minutes after incubation. Separation fluid and perfuse new cell separation f...
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Abstract
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