SIST EN ISO 21570:2006

SLOVENSKI STANDARD
SIST EN ISO 21570:2006
01-marec-2006
Živila – Analitske metode za odkrivanje gensko spremenjenih organizmov in
njihovih produktov – Kvantitativne metode na osnovi nukleinske kisline (ISO
21570:2005)
Foodstuffs - Methods of analysis for the detection of genetically modified organisms and
derived products - Quantitative nucleic acid based methods (ISO 21570:2005)
Lebensmittel - Verfahren zum Nachweis von gentechnisch modifizierten Organismen und
ihren Produkten - Quantitative auf Nukleinsäuren basierende Verfahren (ISO
21570:2005)
Produits alimentaires - Méthodes d'analyse pour la détection des organismes
génétiquement modifiés et des produits dérivés - Méthodes quantitatives basées sur
l'utilisation des acides nucléiques (ISO 21570:2005)
Ta slovenski standard je istoveten z: EN ISO 21570:2005
ICS:
67.050 Splošne preskusne in General methods of tests and
analizne metode za živilske analysis for food products
proizvode
SIST EN ISO 21570:2006 en
2003-01.Slovenski inštitut za standardizacijo. Razmnoževanje celote ali delov tega standarda ni dovoljeno.

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SIST EN ISO 21570:2006

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SIST EN ISO 21570:2006
EUROPEAN STANDARD
EN ISO 21570
NORME EUROPÉENNE
EUROPÄISCHE NORM
November 2005
ICS 67.050

English Version
Foodstuffs - Methods of analysis for the detection of genetically
modified organisms and derived products - Quantitative nucleic
acid based methods (ISO 21570:2005)
Produits alimentaires - Méthodes d'analyse pour la Lebensmittel - Verfahren zum Nachweis von gentechnisch
détection des organismes génétiquement modifiés et des modifizierten Organismen und ihren Produkten -
produits dérivés - Méthodes quantitatives basées sur Quantitative auf Nukleinsäuren basierende Verfahren (ISO
l'utilisation des acides nucléiques (ISO 21570:2005) 21570:2005)
This European Standard was approved by CEN on 26 October 2005.
CEN members are bound to comply with the CEN/CENELEC Internal Regulations which stipulate the conditions for giving this European
Standard the status of a national standard without any alteration. Up-to-date lists and bibliographical references concerning such national
standards may be obtained on application to the Central Secretariat or to any CEN member.
This European Standard exists in three official versions (English, French, German). A version in any other language made by translation
under the responsibility of a CEN member into its own language and notified to the Central Secretariat has the same status as the official
versions.
CEN members are the national standards bodies of Austria, Belgium, Cyprus, Czech Republic, Denmark, Estonia, Finland, France,
Germany, Greece, Hungary, Iceland, Ireland, Italy, Latvia, Lithuania, Luxembourg, Malta, Netherlands, Norway, Poland, Portugal, Slovakia,
Slovenia, Spain, Sweden, Switzerland and United Kingdom.
EUROPEAN COMMITTEE FOR STANDARDIZATION
COMITÉ EUROPÉEN DE NORMALISATION
EUROPÄISCHES KOMITEE FÜR NORMUNG
Management Centre: rue de Stassart, 36  B-1050 Brussels
© 2005 CEN All rights of exploitation in any form and by any means reserved Ref. No. EN ISO 21570:2005: E
worldwide for CEN national Members.

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SIST EN ISO 21570:2006
EN ISO 21570:2005 (E)




Foreword



This document (EN ISO 21570:2005) has been prepared by Technical Committee CEN/TC 275 "Food
analysis - Horizontal methods", the secretariat of which is held by DIN, in collaboration with Technical
Committee ISO/TC 34 "Agricultural food products".

This European Standard shall be given the status of a national standard, either by publication of an identical
text or by endorsement, at the latest by May 2006, and conflicting national standards shall be withdrawn at
the latest by May 2006.

According to the CEN/CENELEC Internal Regulations, the national standards organizations of the following
countries are bound to implement this European Standard: Austria, Belgium, Cyprus, Czech Republic,
Denmark, Estonia, Finland, France, Germany, Greece, Hungary, Iceland, Ireland, Italy, Latvia, Lithuania,
Luxembourg, Malta, Netherlands, Norway, Poland, Portugal, Slovakia, Slovenia, Spain, Sweden, Switzerland
and United Kingdom.

2

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SIST EN ISO 21570:2006


INTERNATIONAL ISO
STANDARD 21570
First edition
2005-11-01

Foodstuffs — Methods of analysis for the
detection of genetically modified
organisms and derived products —
Quantitative nucleic acid based methods
Produits alimentaires — Méthodes d'analyse pour la détection des
organismes génétiquement modifiés et des produits dérivés —
Méthodes quantitatives basées sur l'utilisation des acides nucléiques




Reference number
ISO 21570:2005(E)
©
ISO 2005

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SIST EN ISO 21570:2006
ISO 21570:2005(E)
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©  ISO 2005
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SIST EN ISO 21570:2006
ISO 21570:2005(E)
Contents Page
Foreword. v
Introduction . vi
1 Scope . 1
2 Normative references . 1
3 Terms and definitions. 1
4 Principle. 2
4.1 General. 2
4.2 Amplification, detection and confirmation of PCR products . 2
4.3 Quantitation of PCR products . 2
5 Reagents. 2
6 Apparatus and equipment . 2
7 Guidelines concerning the procedure. 3
7.1 General. 3
7.2 Target sequence stability. 3
7.3 Calibration of the analysis . 3
7.4 Quantitation considerations . 3
7.5 Quality assurance requirements . 3
8 Interpretation. 4
9 Expression of results . 4
10 Test report . 5
Annex A (informative) Target taxon-specific methods. 6
A.1 Target taxon-specific method for the absolute quantitation of the adh1 gene DNA of
maize using real-time PCR. 6
Annex B (informative) Screening methods. 12
B.1 Screening method for the relative quantitation of the 35S-promoter DNA of soya bean line
GTS 40-3-2 using real-time PCR. 12
Annex C (informative) Construct-specific methods . 20
C.1 Construct-specific method for the quantitation of soya bean line GTS 40-3-2 DNA using
real-time PCR (Method 1) . 20
C.2 Construct-specific method for the quantitation of soya bean line GTS 40-3-2 DNA using
real-time PCR (Method 2) . 27
C.3 Construct-specific method for the quantitation of Event176 maize DNA using real-time
PCR. 34
C.4 Construct-specific method for the quantitation of soya bean line GTS 40-3-2 DNA using
real-time PCR . 41
C.5 Construct-specific method for the quantitation of maize line MON 810 DNA using
real-time PCR . 49
C.6 Construct-specific method for the quantitation of maize line Event176 DNA using
real-time PCR . 56
C.7 Construct-specific method for the quantitation of maize line Bt11 DNA using real-time
PCR. 63
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SIST EN ISO 21570:2006
ISO 21570:2005(E)
C.8 Construct-specific method for the quantitation of maize line GA21 DNA using real-time
PCR. 71
C.9 Construct-specific method for the quantitation of maize line T25 DNA using real-time PCR . 78
Annex D (informative) Event-specific methods . 87
D.1 Event-specific method for the absolute and relative quantitation of maize line Bt11 DNA
based on real-time PCR. 87
D.2 Event-specific method for the relative quantitation of maize line MON 810 DNA using
real-time PCR. 93
Bibliography . 100

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SIST EN ISO 21570:2006
ISO 21570:2005(E)
Foreword
ISO (the International Organization for Standardization) is a worldwide federation of national standards bodies
(ISO member bodies). The work of preparing International Standards is normally carried out through ISO
technical committees. Each member body interested in a subject for which a technical committee has been
established has the right to be represented on that committee. International organizations, governmental and
non-governmental, in liaison with ISO, also take part in the work. ISO collaborates closely with the
International Electrotechnical Commission (IEC) on all matters of electrotechnical standardization.
International Standards are drafted in accordance with the rules given in the ISO/IEC Directives, Part 2.
The main task of technical committees is to prepare International Standards. Draft International Standards
adopted by the technical committees are circulated to the member bodies for voting. Publication as an
International Standard requires approval by at least 75 % of the member bodies casting a vote.
Attention is drawn to the possibility that some of the elements of this document may be the subject of patent
rights. ISO shall not be held responsible for identifying any or all such patent rights.
ISO 21570 was prepared by the European Committee for Standardization (CEN) Technical Committee
CEN/TC 275, Food Analysis — Horizontal methods, in collaboration with Technical Committee ISO/TC 34,
Food products, in accordance with the Agreement on technical cooperation between ISO and CEN (Vienna
Agreement).
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SIST EN ISO 21570:2006
ISO 21570:2005(E)
Introduction
The search for ingredients of genetically modified origin is performed by means of the following successive (or
simultaneous) steps. After sample collection, nucleic acids are extracted from the test portion. Extracted
nucleic acids can be further purified, simultaneously or after the extraction process. Afterwards, they are
quantified (if necessary), diluted (if necessary) and subjected to analytical procedures (such as PCR). These
steps are detailed in the present and in the following International Standards:
ISO 21569, Foodstuffs — Methods of analysis for the detection of genetically modified organisms and derived
products — Qualitative nucleic acid based methods
ISO 21570, Foodstuffs — Methods of analysis for the detection of genetically modified organisms and derived
products — Quantitative nucleic acid based methods
Further information about definitions and general items involving the steps cited above are collected in:
ISO 24276, Foodstuffs — Methods of analysis for the detection of genetically modified organisms and derived
products — General requirements and definitions.
The International Organization for Standardization (ISO) draws attention to the fact that it is claimed that
compliance with this document may involve the use of a patent concerning the PCR technology.
ISO takes no position concerning the evidence, validity and scope of these patent rights.
ISO has been informed that Applied Biosystems, Roche Molecular Systems, Inc. and Hoffman-La Roche hold
patent rights concerning PCR technology. The companies have assured the ISO that they are willing to
negotiate licences under reasonable and non-discriminatory terms and conditions with applicants throughout
the world. In this respect, the statements of the holders of these patent rights are registered with ISO.
Information may be obtained from:
Licensing Department
Applied Biosystems
850 Lincoln Centre Drive
Foster City, CA 94404,
USA
and
Roche Molecular Systems, Inc.
Licensing Department
1145 Atlantic Avenue
Alameda, CA 94501,
USA
Attention is drawn to the possibility that some of the elements of this document may be subject of patent rights
other than those identified above. ISO shall not be held responsible for identifying any or all such patent rights.

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SIST EN ISO 21570:2006
INTERNATIONAL STANDARD ISO 21570:2005(E)

Foodstuffs — Methods of analysis for the detection of
genetically modified organisms and derived products —
Quantitative nucleic acid based methods
1 Scope
This International Standard provides the overall framework of quantitative methods for the detection of
genetically modified organisms (GMOs) in foodstuffs, using the polymerase chain reaction (PCR).
It defines general requirements for the specific amplification of DNA target sequences, in order to quantify the
relative GMO-derived DNA content and to confirm the identity of the amplified DNA sequence.
Guidelines, minimum requirements and performance criteria laid down in this International Standard are
intended to ensure that comparable, accurate and reproducible results are obtained in different laboratories.
This International Standard has been established for food matrices, but is also applicable to other matrices,
e.g. feed and plant samples from the environment.
Specific examples of methods are provided in Annexes A to D.
2 Normative references
The following referenced documents are indispensable for the application of this document. For dated
references, only the edition cited applies. For undated references, the latest edition of the referenced
document (including any amendments) applies.
ISO 21569:2005, Foodstuffs — Methods of analysis for the detection of genetically modified organisms and
derived products — Qualitative nucleic acid based methods
ISO 21571, Foodstuffs — Methods of analysis for the detection of genetically modified organisms and derived
products — Nucleic acid extraction
1)
ISO 24276:— , Foodstuffs — Methods of analysis for the detection of genetically modified organisms and
derived products — General requirements and definitions
ISO Guide 32, Calibration in analytical chemistry and use of certified reference materials
3 Terms and definitions
For the purposes of this document, the terms and definitions given in ISO 24276 apply.

1) To be published.
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SIST EN ISO 21570:2006
ISO 21570:2005(E)
4 Principle
4.1 General
Quantitative analysis consists of the quantitation of target DNA sequences in the test samples. Each method
specifies the target sequences(s).
[1],[2] [3],[4]
Quantitation may be performed using competitive or real-time PCR .
A quantitative analysis should clearly express the quantity of the target genetic element, relative to the
quantity of a specific reference, appropriate calibrants and controls, and be within the dynamic range of the
analytical method used and the test portion analysed.
The analysis generally consists of
⎯ amplification of one or more specific target sequences,
⎯ detection and confirmation of the specificity of the PCR product(s), and
⎯ quantitation of the amplified fragments relative to calibrants.
NOTE In the case of real-time PCR analysis, amplification, detection and confirmation occur simultaneously.
4.2 Amplification, detection and confirmation of PCR products
See ISO 21569 for the principles of amplification, detection and confirmation of the DNA sequences.
4.3 Quantitation of PCR products
The principle of quantitation is usually to determine the ratio (expressed as a percent) of two DNA target
sequences; i.e. a sequence representing the genetically modified organism of interest and an (endogenous)
target taxon-specific sequence. However, in some cases, quantitation can also be carried out relative to a
specified amount of food matrix (e.g. when detecting GM microorganisms in foods).
Calibrants (calibration materials) used for quantitation should be traceable to certified reference materials
(CRMs), if available. If not available, other suitable reference material should be used. Example guidance is
provided in Reference [5]. Information on validation studies and measurement uncertainty has been gathered
[6],[7],[8],[9]
from international studies .
5 Reagents
All reagents and materials used in the analysis should be identical, or equivalent, to those specified in the
method. Otherwise, all reagents and materials should be of molecular biology grade. These reagents shall be
stored and used as recommended by the supplier or according to the laboratory quality assurance
specifications. For a list of reagents, see the specific annex.
6 Apparatus and equipment
See Annexes A to D and ISO 24276.
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SIST EN ISO 21570:2006
ISO 21570:2005(E)
7 Guidelines concerning the procedure
7.1 General
General considerations relevant to PCR amplification for the detection of GMOs are described in ISO 21569.
Annexes A to D specify PCR detection methods together with details of their scope of application. The
demonstrated performance characteristics for each method are detailed.
The concentration of the DNA sequence of interest should be within the dynamic range of the method.
NOTE A target taxon specific monitor run can be undertaken to determine whether the template DNA is of sufficient
quality (length and structural integrity), purity and quantity to allow the detection and quantitation of a GMO belonging to
the target taxon. This may be of particular relevance when DNA is extracted from composite or highly processed matrices.
The DNA extracted from each test portion should be analysed at least in duplicate.
Appropriate controls shall be included (see ISO 24276:—, Table 1).
7.2 Target sequence stability
The allelic and copy number stability of the target sequence should be considered for cultivars of different
geographic and phylogenic origins.
7.3 Calibration of the analysis
An appropriate number of calibration points and replicates covering the range of quantitation shall be applied
[e.g. four calibration points with two replicates (altogether 4 × 2 values) or six calibration points with one
measurement at each point (altogether 6 values)]. The quality of the calibration influences the measurement
[9]
uncertainty .
As an alternative to genomic DNA calibration reference materials, for example, a dilution series of a plasmid
or synthetic dsDNA containing the target sequence may be used, provided that it is demonstrated to perform
in an equivalent way to the genomic DNA reference material and the genomic DNA extracted from the sample.
7.4 Quantitation considerations
PCR methods should be appropriately designed to minimize the variability.
NOTE Depending on the method used and/or the material analysed, the presence of stacked genes can lead to
overestimation of the true GMO content.
For the determination of the limit of quantitation (LOQ), see ISO 24276.
Calculation of the GMO content based on copy numbers of target sequences per haploid genome is
influenced by the homo- and heterozygosity of the species under investigation. For details, see Annexes A to
D.
Use of the ∆∆C (cycle of threshold) method is only valid if the amplification efficiencies of the target
t
taxon-specific assay and the GMO-specific assay are very similar.
7.5 Quality assurance requirements
Consistency between measurements is desirable to obtain reliable estimates of target sequence quantities.
However, knowledge of the relative standard deviation of repeatability of the method is required to establish

whether the measurements are consistent (see the ISO 5725 series for details). To calculate the relative
standard deviation of repeatability, the number of separate measurements per laboratory sample may exceed
what is feasible in practice in terms of acceptable costs. Consequently, if a specified GMO-derived DNA is to
be reported (in percent), a feasible solution should require the following as a minimum:
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SIST EN ISO 21570:2006
ISO 21570:2005(E)
a) within test portion consistency:
⎯ through rejection of measurements ⎯ through maximum deviation observed between dilutions and individual measurements equals the
value expected from the corresponding dilution factor ± 33 %;
b) between test portion consistency:
⎯ estimated relative GMO-derived DNA concentrations obtained under a) for each test portion should
not differ by values greater than −50 % to +100 % of the estimated quantity value (equal to a ∆C of 1
t
in real-time PCR) (i.e. for two test portions, measurements of 1,0 % and 2,0 % are acceptable,
measurements of 0,9 % and 2,1 % are not).
In order to guarantee accuracy of the measurements, a reference material (RM), preferably certified (CRM),
for the quantity of the event concerned, with an appropriate level of metrological reliability and with reasonable
similarity of matrix shall be selected and analysed. In the absence of a CRM, in-house RM may be prepared
by a procedure demonstrating stability, homogeneity and traceability, and ensuring the absence of bias. The
quantified uncertainty shall fulfil the required uncertainty for the calibration (see ISO Guide 32).
8 Interpretation
The PCR result will be either
a) fit for quantitation of the target sequence provided
⎯ the result is positive according to ISO 21569:2005, 8.1,
⎯ the observable inhibition of the reaction is negligible,
⎯ the analysis produces an unambiguous measurement value,
⎯ the target sequence content is within the dynamic range of the method, and
⎯ the analysis is calibrated in an acceptable way (see 7.3), or
b) not fit for quantitation of the target sequence if any of the conditions listed above are not fulfilled.
The measurement uncertainty shall be sufficiently small to enable the laboratory to draw the relevant
conclusions.
Annexes A to D describe the measurement of the target DNA quantities. These quantities can be used to
calculate the GMO content. These calculations usually take into consideration relevant biological factors, such
as the homo- or heterozygosity of the target sequences.
If the GM target sequence content or the taxon-specific target sequence content is below the limit of
quantitation, the result shall only be expressed qualitatively.
NOTE Stating that the GMO-derived DNA content is below the practical LOQ accompanied by a specification of that
LOQ is considered to be a qualitative expression of the result.
9 Expression of results
The results shall clearly state the quantity of the GM target sequence relative to the target taxon-specific
sequence. The results should also provide values for the measurement uncertainty, such as the standard
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SIST EN ISO 21570:2006
ISO 21570:2005(E)
deviation or relative standard deviation. Furthermore, the LOD and LOQ of the method and the practical LOD
and LOQ should be reported.
The target sequences may or may not be detected, or the quantity of at least one of them may be below the
limit of quantitation. Table 1 describes the four alternative cases and the corresponding expression of the
result to be included into the test report.
Table 1 — Expression of results
Result Expression of the result
Target taxon-specific sequence is not See ISO 21569.
detected.
“For species x, DNA was not detected.”
Target taxon-specific sequence is According to ISO 21569.
detected but GM target sequence is not
“For species x, GMO-derived DNA was not detected.”
detected.
In addition, if applicable, add: “The practical limit of detection is X %.”
(Specify unit used.)
The target taxon-specific sequence and For each GMO, state:
the GM target sequence are both detected
“GMO (specify the GMO) derived DNA as determined by detection of
but the quantity is below the LOQ of at
(specify target sequence) derived from (specify species) was detected.”
least one of the target sequences.
In addition, if applicable: “The practical limit of quantitation is X %.” (Specify
unit used.)
The target taxon-specific sequence and For each GMO, state:
the GM target sequence are both detected
“The content of GMO (specify the GMO) derived DN
...