EN ISO 15216-1:2017
Superseded
A superseded Standard is one, which is fully replaced by another Standard, which is a new edition of the same Standard.
Microbiology of the food chain - Horizontal method for determination of hepatitis A virus and norovirus using real-time RT-PCR - Part 1: Method for quantification (ISO 15216-1:2017)
30-04-2021
29-03-2017
European foreword
Foreword
Introduction
1 Scope
2 Normative references
3 Terms and definitions
4 Principle
5 Reagents
6 Equipment and consumables
7 Sampling
8 Procedure
9 Interpretation of results
10 Expression of results
11 Precision
12 Test report
Annex A (normative) - Diagram of procedure
Annex B (normative) - Composition and preparation of reagents
and buffers
Annex C (informative) - Real-time RT-PCR mastermixes and
cycling parameters
Annex D (informative) - Real-time RT-PCR primers and
hydrolysis probes for the detection of HAV, norovirus
GI and GII and mengo virus (process control)
Annex E (informative) - Growth of mengo virus strain MC[0]
for use as a process control
Annex F (informative) - RNA extraction using the NucliSENS[R]
system
Annex G (informative) - Generation of dsDNA control stocks
Annex H (informative) - Generation of EC RNA stocks
Annex I (informative) - Typical optical plate layout
Annex J (informative) - Method validation studies and
performance characteristics
Bibliography
ISO 15216-1:2017 specifies a method for the quantification of levels of HAV and norovirus genogroup I (GI) and II (GII) RNA, from test samples of foodstuffs (soft fruit, leaf, stem and bulb vegetables, bottled water, BMS) or food surfaces. Following liberation of viruses from the test sample, viral RNA is then extracted by lysis with guanidine thiocyanate and adsorption on silica. Target sequences within the viral RNA are amplified and detected by real-time RT-PCR.This method is not validated for detection of the target viruses in other foodstuffs (including multi-component foodstuffs), or any other matrices, nor for the detection of other viruses in foodstuffs, food surfaces or other matrices.
Committee |
CEN/TC 463
|
DevelopmentNote |
Supersedes CEN ISO/TS 15216-1. (04/2017)
|
DocumentType |
Standard
|
PublisherName |
Comite Europeen de Normalisation
|
Status |
Superseded
|
Supersedes |
Standards | Relationship |
ONORM EN ISO 15216-1 : 2017 | Identical |
DIN EN ISO 15216-1:2017-07 | Identical |
SN EN ISO 15216-1 : 2017 | Identical |
DIN EN ISO 15216-1:2015-09 (Draft) | Identical |
SS-EN ISO 15216-1 : 2017 | Identical |
NF EN ISO 15216-1 : 2017 | Identical |
UNI EN ISO 15216-1 : 2017 | Identical |
NEN EN ISO 15216-1 : 2017 | Identical |
UNE-EN ISO 15216-1:2017 | Identical |
ISO 15216-1:2017 | Identical |
NS EN ISO 15216-1 : 2017 | Identical |
PN EN ISO 15216-1 : 2017 | Identical |
BS EN ISO 15216-1:2017 | Identical |
I.S. EN ISO 15216-1:2017 | Identical |
ISO 22174:2005 | Microbiology of food and animal feeding stuffs — Polymerase chain reaction (PCR) for the detection of food-borne pathogens — General requirements and definitions |
ISO 7218:2007 | Microbiology of food and animal feeding stuffs — General requirements and guidance for microbiological examinations |
ISO 20838:2006 | Microbiology of food and animal feeding stuffs — Polymerase chain reaction (PCR) for the detection of food-borne pathogens — Requirements for amplification and detection for qualitative methods |
ISO 5725-2:1994 | Accuracy (trueness and precision) of measurement methods and results Part 2: Basic method for the determination of repeatability and reproducibility of a standard measurement method |
ISO 17468:2016 | Microbiology of the food chain — Technical requirements and guidance on establishment or revision of a standardized reference method |
ISO 22119:2011 | Microbiology of food and animal feeding stuffs — Real-time polymerase chain reaction (PCR) for the detection of food-borne pathogens — General requirements and definitions |
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