Chlorella sorokiniana CS-01 and culture method thereof for producing grease
A cultivation method and technology of chlorella, applied in the field of fermentation, can solve problems such as shortage of land resources and rising crop prices, and achieve the effects of good application potential, good growth and high yield
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Embodiment 1
[0028] Under sterile conditions, single algae were picked from a solid plate and dropped into a small test tube containing 5 mL of sterilized culture solution, placed in an illuminated incubator for static culture, and grown to the end of the exponential phase with an inoculation ratio of 1:10 to expand the culture.
[0029] Inoculate the algae liquid into 3L sterilized BG11 medium with a final concentration of 1×10 6 A / mL~3×10 6 per mL, the culture temperature was 30°C, the pH of the medium was 8.1, the nitrogen source was sodium nitrate with a concentration of 0.5 g / L, and the concentration of EDTA-Fe(III) after adding was 1×10 -4 mol / L, nitrogen source and EDTA-Fe(III) were all added at one time, the light intensity was 10000LX, the light-dark ratio was 14:10, and the culture method was static culture for 30 days.
[0030] The algae cells were collected by centrifugation, freeze-dried in vacuum, weighed the dry weight of the algae powder and calculated the output of the al...
Embodiment 2
[0032] Under sterile conditions, single algae were picked from a solid plate and dropped into a small test tube containing 5 mL of sterilized culture solution, placed in an illuminated incubator for static culture, and grown to the end of the exponential phase with an inoculation ratio of 1:10 to expand the culture.
[0033] Inoculate the algae liquid into 3L sterilized BG11 medium with a final concentration of 1×10 6 A / mL~3×10 6 per mL, the culture temperature was 30°C, the pH of the medium was 11, the nitrogen source was sodium nitrate with a concentration of 0.5 g / L, and the concentration of EDTA-Fe(III) after adding was 1×10 -4 mol / L, the addition method is one-time addition, the light intensity is 10000LX, the light-to-dark ratio is 14:10, and the cultivation method is static cultivation for 30 days.
[0034] The algae cells were collected by centrifugation, freeze-dried in vacuum, weighed the dry weight of the algae powder and calculated the output of the algae powder t...
Embodiment 3
[0036] Under sterile conditions, single algae were picked from a solid plate and dropped into a small test tube containing 5 mL of sterilized culture solution, placed in an illuminated incubator for static culture, and grown to the end of the exponential phase with an inoculation ratio of 1:10 to expand the culture.
[0037] Inoculate the algae liquid into 3L sterilized BG11 medium, and the final concentration after inoculation is 1×10 6 A / mL~3×10 6 per mL, the culture temperature was 30°C, the pH of the medium was 8.1, the nitrogen source was sodium nitrate with a concentration of 0.2 g / L, and the concentration of EDTA-Fe(III) after adding was 1×10-4 mol / L, EDTA-Fe(III) is added in one time. On the seventh day of cultivation, sodium nitrate was fed (the original nitrogen source was basically completely consumed), the feeding amount was 0.2 g / L culture solution, the light intensity was 10000 Lx light-dark ratio was 14:10, and the culture method was aeration culture for 20 days...
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