Commission Regulation (EC) No 796/2004 (repealed)Show full title

ANNEX ICOMMUNITY METHOD FOR THE QUANTITATIVE DETERMINATION OF Δ⁹-TETRAHYDROCANNABINOL CONTENT IN HEMP VARIETIES

1.Scope and area of application

This method seeks to determine the Δ⁹-tetrahydrocannabinol (hereinafter referred to as ‘THC’) content of varieties of hemp (Cannabis sativa L.) As appropriate, the method involves applying procedure A or B herein described.

The method is based on the quantitative determination of Δ⁹-THC by gas chromatography (GC) after extraction with a suitable solvent.

1.1.Procedure A

Procedure A shall be used for checks on production as provided for in Article 52(1) of Regulation (EC) No 1782/2003 and Article 26(2)(a) of this Regulation.

1.2.Procedure B

Procedure B shall be used in cases as referred to in Article 52(2) of Regulation (EC) No 1782/2003 and Article 33(4) of this Regulation.

2.Sampling

2.1.Samples

2.2.Sample size

Procedure A: the sample shall comprise parts of 50 plants per field.

Procedure B: the sample shall comprise parts of 200 plants per field.

Each sample shall be placed in a fabric or paper bag, without crushing it, and be sent to the laboratory for analysis.

The Member State may provide for a second sample to be collected for counteranalysis, if required, to be kept either by the producer or by the body responsible for the analysis.

2.3.Drying and storage of the sample

Drying of the samples shall begin as soon as possible and, in any case, within 48 hours using any method below 70 ^oC. Samples should be dried to a constant weight and to a moisture content of between 8 % and 13 %.

After drying, the samples shall be stored without crushing them at below 25 ^oC in a dark place.

3.Determination of THC content

3.1.Preparation of the test sample

Stems and seeds over 2 mm in size shall be removed from the dried samples.

The dried samples shall be grinded to obtain a semi-fine powder (passing through a 1 mm mesh sieve).

The powder may be stored for 10 weeks at below 25 ^oC in a dark, dry place.

3.2.Reagents and extraction solution

Reagents

• Δ⁹-tetrahydrocannabinol, pure for chromatographic purposes,

• Squalane, pure for chromatographic purposes, as an internal standard.

Extraction solution

• 35 mg of squalane per 100 ml hexane.

3.3.Extraction of Δ⁹-THC

100 mg of the powdered test sample shall be weighed, be placed in a centrifuge tube and 5 ml of extraction solution shall be added containing the internal standard.

Place in an ultrasound bath and leave for 20 minutes. Centrifuge for five minutes at 3000 r.p.m. and then remove the supernatant THC solution. Inject the solution into the chromatograph and carry out a quantitative analysis.

3.4.Gas chromatography

4.Results

The findings shall be expressed to two decimal places in grams of Δ⁹-THC per 100 grams of analytical sample dried to constant weight. A tolerance of 0.03 g per 100 g shall apply.

• Procedure A: one determination per test sample.

  However, where the result obtained is above the limit laid down in Article 52(1) of Regulation (EC) No 1782/2003, a second determination shall be carried out per analysis sample and the mean value of the two determinations shall be taken as the result.

• Procedure B: the result corresponds to the mean value of two determinations per test sample.

ANNEX IIVARIETIES OF HEMP GROWN FOR FIBRE ELIGIBLE FOR DIRECT PAYMENTS

a.Hemp grown for fibre

• Carmagnola

• Beniko

• Chamaeleon

• Cs

• Delta-Ilosa

• Delta 405

• Dioica 88

• Epsilon 68

• Fedora 17

• Felina 32

• Ferimon – Férimon

• Fibranova

• Fibrimon 24

• Futura 75

• Juso 14

• Red Petiole

• Santhica 23

• Santhica 27

• Uso 31

b.Hemp grown for fibre authorised in the 2004/2005 marketing year

• Bialobrzeskie

• Cannacomp(1)

• Fasamo

• Felina 34 – Félina 34

• Fibriko TC

• Finola

• Lipko(2)

• Silesia(3)

• Tiborszállási(2)

• UNIKO-B

ANNEX IIICORRELATION TABLE