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32

Orange Juice

FDA/BAM

2

UPB

BAX

®

MP Media

1 http://origin-www.fsis.usda.gov/PDF/MLG_4_05.pdf 2 http://www.fda.gov/downloads/Food/ScienceResearch/LaboratoryMethods/BacteriologicalAn alyticalManualBAM/UCM244774.pdf

Hot Dogs (325 grams) – One test portion preparation

BAX

®

System Real-Time PCR Assay for

Salmonella

vs. USDA-FSIS MLG Reference Method Comparison –

1.0

BAX

®

System Real-Time PCR Assay for

Salmonella

and USDA/FSIS-MLG

1.1

To each 325g test portion, add one-third to one-half of 2925 mL pre-warmed

(35± 1°C) BPW (approximately 975 mL to 1450 mL). Homogenize each sample for

approximately two minutes. Add the remaining 2925 mL of BPW. Incubate for 18 - 24

hours at 35 ± 2°C.

Note: Take care when enriching samples that pre-warmed media is not allowed to

cool. Only remove as much primary enrichment as needed when preparing samples.

Allowing the BPW to cool while enriching samples may impact the integrity of the test

system.

1.2

Follow prompts in the Rack Wizard to enter identifying data on the entire rack and on

the individual samples.

1.3

Place one cluster tube per sample in a cluster tube rack. Add 200

µ

L of prepared lysis

reagent to each tube (lysis tube).

1.4

Transfer 5

µ

L of each pre-enriched sample to the corresponding lysis tube and ensure

the tubes are capped.

1.5

Incubate lysis tubes at 37ºC for 20 minutes, then at 95ºC for 10 minutes in either

individual heating blocks or the DuPont Thermal Block. Cool lysates for at least five

minutes in either a refrigerated cooling block or the automated thermal block prior to

the final transfer to PCR tubes.

1.6

Warm up the cycler/detector by selecting RUN FULL PROCESS from the menu bar of the

application window.

1.7

Place a PCR tube holder on the PCR cooling block. Insert one PCR tube per sample into

the holder and remove caps. Using a multi-channel pipette, transfer 30

µ

L of sample

lysate to a PCR tube. Cap PCR with the flat optical cap strips provided in the kit.

1.8

Follow screen prompts to load samples into the cycler/detector and begin the program.

At the completion of the PCR and detection process, follow the screen prompts to

remove samples and display results.

Test Result Confirmation

1.9

Using the primary enrichment (step 1.1 above), transfer 0.5

±

0.05 mL enriched sample

into 10 mL Tetrathionate (TT-Hajna) broth and 0.1

±

0.02 mL into 10 mL modified

Collaborative Study Approved Protocol

Expert Review Panel Use Only

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