126 lines
6.2 KiB
Plaintext
126 lines
6.2 KiB
Plaintext
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Here in alt.drugs have been lot of talk about LSD synthesis lately.
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I guess as an conclusion it can be said that the synthesis can be
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carried out with good chemistry knowledge and laboratory. Then the
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problem is where to get lysergic acid derivative for the synthesis.
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The full synthesis of the lysergic acid is too difficult. Lysergic
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acid amides can be extracted from the seeds of morning glory or
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hawaiian baby wood rose, but it is not practical, because the huge
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amount of seeds needed to get enough lysergic acid amides for
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the LSD synthesis. To my opinion the only feasible possibility is
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to cultivate ergot.
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What I would like to know is how difficult it is to cultivate
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Claviceps purpurea for example. Is it harder than growing psychedelic
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mushrooms? Is the following procedure any good and how hard it is
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to carry out? Any constructive comments?
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Michael Valentine Smith: Psychedelic Chemistry
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From pages 105-107:
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The Culture and Extraction of Ergot Alkaloids
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Make up a culture medium by combining the following ingredients in about
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500 milliliters of distilled water in a 2 liter, small-neck flask:
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Sucrose .......................................... 100 grams
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Chick pea meal .................................... 50 grams
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Calcium nitrate ..................................... 1 gram
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Monopotassium phosphate ......................... 0.25 grams
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Magnesium sulphate .............................. 0.25 grams
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Potassium chloride ............................. 0.125 grams
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Ferrous sulphate heptahydrate ................... 8.34 milligrams
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Zinc sulphate heptahydrate ...................... 3.44 milligrams
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Add water to make up one liter, adjust pH 4 with ammonia solution and
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citric acid. Sterile by autoclaving.
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Inoculate the sterilized medium with Claviceps purpurea under sterile
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conditions, stopper with sterilized cotton and incubate for two weeks
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periodically testing and maintaining pH 4. After two weeks a surface
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culture will be seen on the medium. Large-scale production of the
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fungus can now begin.
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Obtain several ordinary 1 gallon jugs. Place a two-hole stopper in
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the necks of the jugs. Fit a short (6 inch) glass tube in one hole,
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leaving 2 inches above the stopper. Fit a short rubber tube to this.
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Fill a small (500 milliliter) Erlenmeyer flask with a dilute solution
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of sodium hypochlorite, and extend a glass tube from the rubber tube
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so the end is immersed in the hypochlorite. Fit a long, glass tube in
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the other stopper hole. It must reach near the bottom of the jug and
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have about two inches showing above the stopper. Attach a rubber tube
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to the glass tube as short or as long as desired, and fit a short glass
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tube to the end of the rubber tube. Fill a large, glass tube (1 inch x
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6 inches) with sterile cotton and fit 1-hole stoppers in the ends.
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Fit the small, glass tube in end of the rubber tube into 1 stopper of
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the large tube. Fit another small glass tube in the other stopper.
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A rubber tube is connected to this and attached to a small air pump
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obtained from a tropical fish supply store. You now have a set-up for
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pumping air from the pump, through the cotton filter, down the long
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glass tube in the jug, through the solution to the air space in the top
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of the jug, through the short glass tube, down to the bottom of the
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Erlenmeyer flask and up through the sodium hypochlorite solution into
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the atmosphere. With this aeration equipment you can assure a supply
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of clean air to the Claviceps purpurea fungus while maintaining a
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sterile atmosphere inside the solution.
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Dismantle the aerators. Place all the glass tubes, rubber tubes,
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stoppers and cotton in a paper bag, seal tight with wire staples
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and sterilize in an autoclave.
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Fill the 1-gallon jugs 2/3 to 3/4 full with the culture medium and
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autoclave.
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While these things are being sterilized, homogenize in a blender the
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culture already obtained and use it to inoculate the media in the
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gallon jugs. The blender must be sterile. Everything must be sterile.
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Assemble the aerators. Start the pumps. A slow bubbling in each jug
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will provide enough oxygen to the cultures. A single pump can, of
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course, be connected to several filters.
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Let everything sit a room temperature (25 C) in a fairly dark place
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(never expose ergot alkaloids to bright light - they decompose) for
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a period of ten days.
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After ten days adjust the culture to 1% ethanol using 95% ethanol
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under sterile conditions. Maintain growth for another two weeks.
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After total of 24 days growth period the culture should be considered
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mature. Make the culture acidic with tartaric acid and homogenize in
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a blender for one hour.
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Adjust to pH 9 with ammonium hydroxide and extract with benzene or
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chloroform/iso-butanol mixture.
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Extract again with alcoholic tartaric acid and evaporate in a vacuum
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to dryness. The dry material in the salt (i.e., the tartaric acid salt,
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the tartrate) of the ergot alkaloids, and is stored in this form because
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the free basic material is too unstable and decomposes readily in the
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presence of light, heat, moisture and air.
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To recover the free base for extraction of the amide of synthesis to
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LSD, make the tartrate basic with ammonia to pH 9, extract with chloroform
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and evaporate in vacuo.
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If no source of pure Claviceps purpurea fungus can be found, it may be
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necessary to make a field trip to obtain the ergot growths from rye or
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other cereal grasses. Rye grass is by far the best choice. The ergot will
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appear as a blackish growth on the tops of the rye where the seeds are
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and are referred to as "heads of ergot." From these heads of ergot sprout
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the Claviceps purpurea fungi. They have long steams with bulbous heads when
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seen under a strong glass or microscope. It is these that must be removed
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from the ergot, free from contamination, and used to inoculate the culture
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media. The need for absolute sterility cannot be overstressed. Consult any
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elementary text on bacteriology for the correct equipment and procedures.
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Avoid prolonged contact with ergot compounds, as they are poisonous and
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can be fatal.
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