Preparation method and application of lotus leaf cell secondary metabolite freeze-dried powder
A technology of secondary metabolites and freeze-dried powder, which is applied in the field of plant cell culture and cosmetics, can solve the problems of limited lotus leaf growth season, complex production process, and impact on the output of finished products, and achieve reduced damage, high safety, and simplified production. The effect of the production process
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Embodiment 1
[0031] 1. Obtain lotus leaf cell lines
[0032] 1) Take 1 kg of fresh lotus leaves for cleaning and disinfection, and soak in 10 L of 15% sodium hypochlorite for 20 minutes. Under aseptic conditions, pour out the lotus leaves gently, wash each time with 2 L of sterile deionized water, a total of three times, and gently stir during each washing process.
[0033] 2) Under sterile conditions, cut the sterilized lotus leaves into pieces with sterilized scissors, and the size of each piece is ≤1mm 2 .
[0034] Transfer the lotus leaf fragments to a sterile clean beaker, add 10ml of MS (Murashige and Skoog) medium for every 1.0g of fragments, first grade 0.05ml mass fraction of 0.2 cellulase and 0.05ml mass fraction of 0.2 pectinase, Digest for 3 hours.
[0035] 3) Filter the digestive juice with a 200-mesh sterile mesh sieve to remove impurities, extract 20ul lotus leaf cell filtrate, add it to the Countstar cell counter, centrifuge the filtrate for 10min under a centrifugal for...
Embodiment 2
[0065] 1. Obtain lotus leaf cell lines
[0066] 1) Take 1 kg of fresh lotus leaves for cleaning and disinfection, and soak in 10 L of 20% sodium hypochlorite for 20 minutes. Under aseptic conditions, pour out the lotus leaves gently, wash each time with 2 L of sterile deionized water, a total of three times, and gently stir during each washing process.
[0067] 2) Under sterile conditions, cut the sterilized lotus leaves into pieces with sterilized scissors, and the size of each piece is ≤1mm 2 .
[0068] Transfer the lotus leaf fragments to a sterile clean beaker, add 10ml of MS (Murashige and Skoog) medium per 1.0g of fragments, first grade 0.05ml mass fraction of 0.3% cellulase and 0.05ml mass fraction of 0.3% pectin Enzyme, digested for 3 hours.
[0069] 3) Filter the digestive juice with a 200-mesh sterile mesh sieve to remove impurities, extract 20ul lotus leaf cell filtrate, add it to the Countstar cell counter, centrifuge the filtrate under 250g centrifugal force fo...
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