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TrueNAT Sample Processing: Other Body Fluids
Learning ObjectivesTrueNAT Sample Processing: Other Body Fluids
The extra-pulmonary samples (Non-sputum) can also be processed and used for MTB and Rif diagnosis using Truenat. The processing of various extra-pulmonary samples is described below.
Reagents required:
Trueprep AUTO MTB Sample Pre-treatment Pack for sample processing
- Reagents stable for two years (2-40°C) or one month (temperatures up to 45°C)
- Avoid exposure to light or elevated temperatures
- Do not freeze
Steps in processing of non-sputum samples
Non-sputum samples like tissue biopsy should not be processed at the Designated Microscopy Centre (DMC), but should be transferred to a higher centre.
General Instructions
- Disinfect work surfaces with freshly prepared 1% bleach, followed by 70% alcohol.
- Process fresh specimens immediately or store frozen at -20oC. Avoid more than three freeze thaws.
- Bring frozen samples and refrigerated reagents to room temperature (20-30°C).
- Open the Trueprep AUTO MTB sample pre-treatment pack that contains:
- Liquefaction buffer bottle
- Lysis buffer bottle
- Graduated 1 ml transfer pipette.
- Processing is to be done as instructed for each sample type.
- Non-sputum sample is stable for 3 days at up to 40°C and 1 week at 30°C in the lysis buffer.
A. Processing for Bronchoalveolar Lavage (BAL), Pleural fluid, Peritoneal fluid
Equipment: Centrifuge and centrifuge tubes (10-15 ml volume)
- Add 5-10 ml specimen in a centrifuge tube.
- Centrifuge at 4000x for 5 minutes to concentrate the sample.
- Discard the supernatant until 500 μl remains.
- Add two drops of the liquefaction buffer to the concentrated sample (500 μl).
- Transfer the contents to a labelled lysis buffer tube.
- Incubate for five minutes and proceed for DNA extraction.
B. Processing for Pus, Abscess, Lymph node aspirate, Cerebrospinal Fluid (CSF)
Equipment: Centrifuge tubes (1.5 ml volume)
- Add 0.5 ml specimen in a 1.5 ml tube.
- Add two drops of liquefaction buffer.
- Transfer the contents to a labelled lysis buffer tube.
- Incubate for 5 minutes and proceed for DNA extraction.
C. Processing for Tissue/ Biopsy Samples
Equipment: Mortar and pestle (for tissue homogenization)
- Homogenize sample by using 100 μl lysis buffer in mortar and pestle.
- Add two drops of liquefaction buffer.
- Transfer the contents to a labelled lysis buffer tube.
- Incubate for five minutes.
- Use only clear fluid for DNA extraction.
The processed samples will be used for DNA extraction and PCR amplification for diagnosis of MTB and Rif resistance.
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