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Figure 4 | Genome Biology

Figure 4

From: Identification of cyanobacterial non-coding RNAs by comparative genome analysis

Figure 4

Test of transcript accumulation of Yfr1-7 from MED4 (MED) under different conditions. The left side shows the Northern hybridizations for which the following conditions were used: nutrient depletion (phosphate (P-), nitrogen (N-), iron (Fe-)); blue light for three hours (3 h); controls under blue (Blue), white (White) and no light (Dark); oxidative stress mediated by the application of 3-(3,4-dichlorophenyl)-1,1-N-N'-dimethylurea (DCMU); low (15°C) and high (30°C) temperatures; and high light intensity (50 μE). For comparison, 5S rRNA was hybridized as an internal standard and the mRNA of gene PMM3822n which, with a length of approximately 250 nucleotides, was taken as an example for a small mRNA. Additional controls by quantitative RT-PCR for the genes isiB (Fe), glnA (N), pstS (P) and hli8 (high light) [data not shown] were carried out to confirm the effects of nutrient depletion or high light. The amounts of these mRNAs were enhanced by a factor of 79.7 (isiB), 5.8 (glnA), 2.8 (hli8) and 4.0 (pstS) under the respective treatment compared to standard conditions (data not shown). Yfr6 shows an inconstant signal; for example, at cold, blue/white light, N-, Yfr2 to Yfr5 were hybridized with the consensus oligonucleotide y_gen (Figure 5). The band intensities were quantified and normalized to the amount of 5S rRNA as an internal standard (right).

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