ENZYMATIC METHOD FOR EXTRACTION AND PURIFICATION OF PHYTOCANNABINOIDS

Abstract

An example method of extracting phytocannabinoids from plants includes obtaining plant parts from at least one plant, the at least one plant including one or more of Cannabis, Turmeric, Ginseng, Ginkgo, Ginger, Vinca, and Bacopa. The plant parts are cooled, and are incubated in an incubation mixture of cellulose, pectinase, amylase, and proteinase dissolved in a buffer. The incubation mixture is evaporated in an evaporation chamber to obtain a phytocannabinoid extract.

Description

BACKGROUND

The present disclosure relates to phytocannabinoids, and more particularly to an enzymatic method for extraction and purification of phytocannabinoids using plant cell wall and cell content digesting enzymes.

Plant cells are bounded by rigid cell walls made of cellulose along with other minor polymers. Individual cells are held together with adjacent cells by pectin. This presents challenges for extracting phytocannabinoids from plants.

SUMMARY

An example method of extracting phytocannabinoids from plants includes obtaining plant parts from at least one plant, the at least one plant including one or more of Cannabis, Turmeric, Ginseng, Ginkgo, Ginger, Vinca, and Bacopa. The plant parts are cooled, and are incubated in an incubation mixture of cellulose, pectinase, amylase, and proteinase dissolved in a buffer. The incubation mixture is evaporated in an evaporation chamber to obtain a phytocannabinoid extract.

The embodiments, examples, and alternatives of the preceding paragraph, the claims, or the following description and drawings, including any of their various aspects or respective individual features, may be taken independently or in any combination. Features described in connection with one embodiment are applicable to all embodiments, unless such features are incompatible.

DETAILED DESCRIPTION

The present disclosure describes a novel method for extraction and purification of phytochemicals from Cannabis sativa and its sub species, varieties, hybrids, bio and ecotypes, by enzymatic digestion of cell walls, membranes and contents of cells, which results in the release of phytocannabinoids into the medium. The cannabinoid oil, which is insoluble in aqueous media, is extracted by, e.g., microwave assisted solvent extraction or super critical CO₂ extraction. The protocol makes use of the known structural features of plant cells which are held together by cellulose, pectin and other polymers.

When plant parts are chopped up or powdered and incubated in cellulase, pectinase, amylase and proteinases by vacuum infiltration, the cell walls, membranes, protein, and starch are digested and the contents are released into the incubating medium. Microwave assisted extraction in the presence of solvents aids efficient, rapid extraction of the released phytochemicals.

In an example embodiment, the method includes gathering plant organs such as leaves, flowers, roots and other plant parts. Those parts are sanitized by being washed, exposed to UV radiation or ozonolysis and then cut into small pieces or powdered. When cut, a preferred size of the pieces is about 1 square inch. If the sanitized plant organs are powdered, it is preferably done in the presence of dry ice (solid CO₂).

The next step involves incubating the pieces or powder in a mixture of cellulose, pectinase, amylase and proteinase, dissolved in a neutral buffer containing no more than 0.1 percent surfactant after vacuum infiltration of the plant tissue into the incubation medium. The mixture of the plant tissue and the incubation medium is incubated for up to 24 hours on a shaker platform that vigorously shakes the mixture. The incubated mixture is heated at a temperature around 45-50 degrees Celsius in an evaporation chamber to evaporate water from the mixture without causing evaporation of volatile oils. The resulting residue is extracted using ethanol, olive oil, coconut oil or hemp oil. Microwave assisted extraction is used in some embodiments to maximize cannabinoid extraction from cannabis or other phytochemicals even in situations where the cannabinoids are present in low concentrations. In other embodiments, the cell digested incubation mixture is directly subjected to super critical CO₂ extraction without using microwave assisted rapid extraction.

The extract resulting from the disclosed technique may be a starting point for industrial-type vacuum distillation or preparative chromatographic separations, such as high performance liquid chromatography (HPLC) for purifying and separating individual, different cannabinoid fractions.

Although example embodiments have been disclosed, a worker of ordinary skill in this art would recognize that certain modifications would come within the scope of this disclosure. For that reason, the following claims should be studied to determine the scope and content of this disclosure.

Claims

1. A method of extracting phytocannabinoids from plants, comprising: obtaining plant parts from at least one plant, the at least one plant including one or more of Cannabis, Turmeric, Ginseng, Ginkgo, Ginger, Vinca, and Bacopa;cooling the plant parts;incubating the plant parts in an incubation mixture of cellulose, pectinase, amylase, and proteinase dissolved in a buffer; andevaporating the incubation mixture in an evaporation chamber to obtain a phytocannabinoid extract.

2. The method of claim 1, wherein the buffer is a neutral buffer that contains no more than 0.1% surfactant.

3. The method of claim 1, comprising sanitizing the plant parts, said sanitizing comprising performing at least one of washing the plant parts, subjecting the plant parts to ultraviolet irradiation, and subjecting the plant parts to ozonolysis.

4. The method of claim 1, comprising shaking the incubation mixture during said incubating.

5. The method of claim 1, wherein said cooling the plant parts comprises freezing the plant parts using dry ice.

6. The method of claim 1, comprising, during said cooling and prior to said incubating, cutting the plant parts into pieces of not more than 1 inch in length in any direction.

7. The method of claim 1, comprising, during said cooling and prior to said incubating, reducing plant parts to a plant powder.

8. The method of claim 1, wherein the plant parts are plant organs including one or more of leaves, flowers, and roots.

9. The method of claim 1, wherein said evaporating the incubation mixture in an evaporation chamber comprises heating the incubation mixture at 45-50° Celsius in the evaporation chamber to evaporate water from the incubation mixture.

10. The method of claim 9, comprising: extracting residue from the evaporated incubation mixture using ethanol, olive oil, coconut oil, or hemp oil.

11. The method of claim 10, comprising subjecting the incubation mixture to super critical CO2 extraction.

12. The method of claim 11, comprising: filtering the extracted residue through at least one filter, thereby removing sediment and cellular debris from the phytocannabinoid extract, and adsorbing plant pigments of the phytocannabinoid extract.

13. The method of claim 12, comprising: performing vacuum distillation on the phytocannabinoid extract; orpurifying the phytocannabinoid extract using preparative column chromatography.

14. The method of claim 13, wherein the preparative column chromatography comprises high pressure liquid column chromatography.

15. The method of claim 10, comprising: filtering the extract through at least one filter, thereby removing sediment and cellular debris from the phytocannabinoid extract, and adsorbing plant pigments of the phytocannabinoid extract.

16. The method of claim 10, comprising subjecting the incubation mixture to microwave assisted extraction.

17. The method of claim 16, comprising: performing vacuum distillation on the phytocannabinoid extract; orpurifying the phytocannabinoid extract using preparative column chromatography.

18. The method of claim 16, comprising: filtering the extract through at least one filter, thereby removing sediment and cellular debris from the phytocannabinoid extract, and adsorbing plant pigments of the phytocannabinoid extract.

19. The method of claim 16, comprising: subjecting the incubation mixture to super critical CO2 extraction; orperforming vacuum distillation on the phytocannabinoid extract; orpurifying the phytocannabinoid extract using high pressure liquid column chromatography.

20. The method of claim 18, wherein said filtering comprises: removing sediment and cellular debris from the phytocannabinoid extract using a first filter; andadsorbing plant pigments of the phytocannabinoid extract using a second filter that is separate from the first filter, the second filter including charcoal.