An optimized method for RNA extraction from the polyurethane oligomer degrading strain Pseudomonas capeferrum TDA1 growing on aromatic substrates such as phenol and 2,4-diaminotoluene

doi:10.1371/journal.pone.0260002

Fig 1.

Optimized RNA extraction method from Pseudomonas capeferrum TDA1.

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Table 1.

Total RNA quantity (ng/μL) and purity (A₂₆₀/A₂₈₀ and A₂₆₀/A₂₃₀) for different RNA isolation methods applied on cells from Pseudomonas capeferrum TDA1 growing on different carbon sources (succinate, phenol and 2,4-TDA).

Values represent mean ± SD.

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Fig 2.

Bioanalyzer results.

Electropherograms of total RNA extracted from Pseudomonas capeferrum TDA1 grown on: A) phenol (with TriFast method), B) phenol (with modified RNAzol RT method) and C) 2,4-TDA (with modified RNAzol RT method). The main peaks correspond to ribosomal RNA (16S and 23S).

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