Meat SPP PCR
Meat SPP PCR
Meat SPP PCR
) ( جدول التعديالت
CONTENTS
1. Purpose:
2. Scope:
3. Applicability.
4. Environment.
5. Equipment And Media.
6. Precautions.
7. Procedure.
8. Retention And Disposal.
9. Method Validation.
10. Test Report
11 Assuring the test result
12. Appendices.
13 Distribution List.
1. Purpose:
Detection of meat spp adulturation using real time pcr .
2. Scope:
A horizontal method for the detection of meat spp adulturation by real time
pcr according to : ISO ISO 20837;2006,20836:2021
3. Applicability.
This procedure shall be applied by all personnel who authorized to
Carry out this test.
4. Environment.
No air currents
No dusty atmosphere
Atmospheric confederation .22±2 and 45-50% humidity
5. Equipments and Media.
5.1. Equipments
- THERMAL CYCLER
- VORTEX
-CENTRIFUGE
-THERMAL BLOCK
-automatic pipette
5.2 kits
6. Precautions.
Avoid unnecessary talking
Wear a laboratory coat to protect your cloths
Do not put any thing in or near your mouth
Wash your hands with soap and water.
Operation should not be carried out in direct sunlight.
7.Procedure
7.1.Enrichment and sample treatment for bacteria
Food samples should be enriched according to the corresponding International
Standards or other appropriate standards. Other enrichment media found to be more
PCR compatible could be used, if they have been shown, through validation, to
have performance at least comparable to those described in International Standards.
Some enrichment media recommended in International Standards contain less PCR-
inhibitory substances than others, which should be carefully considered in
connection with the choice of sample preparation method.
For some products, special care should be taken to suppress the growth of
competing background microorganisms (e.g. by addition of selective chemicals or
antibiotics). Least destructive methods, such as a simple dilution, centrifugation,
protein digestion, filtration, density centrifugation, immunomagnetic separation,
etc. may be tried. In the case of lack of PCR response, more rigorous methods such
as boiling, the use of chelating agents or harsh chemicals, such as chloroform and
ethanol, or kits with similar actions may be tried. Simple physical methods may be
used to reduce the fat content of high-fat samples. Chelating agents may be used to
reduce the high calcium content of dairy products which can be inhibitory.
For real time PCR analysis, the detection occurs simultaneously with amplification.
Confirmation of the identity of the PCR product should be undertaken by an
appropriate method other than size determination, for example by the following:
a) by DNA sequencing of the PCR product;
b) by hybridization of the PCR product with specific DNA probes( meat spp
adulturation )
c) by carrying out restriction analysis of the PCR product; the length of the
fragments after restriction shall correspond to the expected length of the target
DNA sequence after restriction.
A positive result may also or alternatively be confirmed by using a standardized
microbiological cultural and confirmatory method as described by appropriate
International Standards.
Controls
The quality, integrity and amount of the DNA template influences the outcome of
the PCR, and hence the analytical results obtained.
Because of the risk of obtaining false positive and/or false negative results,
appropriate controls shall be included in each PCR run. The frequency of use shall
be determined as part of the laboratory quality assurance programme. An internal or
external amplification control shall be used in every PCR run.
If available and appropriate, reference materials and reference cultures should be
used a positive and negative controls.
For the purposes of this International Standard, the controls to be used are given in