5) and heating for 30 min at 37 °C (Richardson & Loomis, 1992) T

5) and heating for 30 min at 37 °C (Richardson & Loomis, 1992). The number of viable spores present after heating was counted under the microscope. Two independent developmental expression selleck chemicals llc profiles of stlA obtained by RT-PCR have

been reported previously. These two reports used different primers and showed different expression patterns, leading to the re-examination of the expression pattern (Austin et al., 2006; Ghosh et al., 2008). Figure 1 shows the expression profiles obtained with two different primer sets. Primer set 1 included the primers stlA-KSf and stlA-KSr and was designed based on the keto-synthase domain, which has 119 bp of intron between the positions of these primers. Primer set 2 was identical to that used in a previous report (Ghosh et al., 2008). We obtained identical results with the two different primer sets. The expression of stlA peaked around the early stage of development and declined as development progressed. However, in the last stage of development, it showed a weak peak. These results were in accordance with the previously obtained results. Recently, a database of RNA sequences obtained from developmental stages (dictyExpress) was published (Rot et al., 2009), and our expression profile was in accordance with that shown in the dictyExpress database. Two Selleckchem AZD6244 previously reported studies used the same Ax2 strain and allowed the

cells to grow in an axenic medium. Ribose-5-phosphate isomerase On the other

hand, the dictyExpress database used a different strain Ax4 grown in the association with Klebsiella aerogenes. We found that stlA expression in the vegetative stage was induced by the presence of Klebsiella (Akabane et al., in preparation). Despite these differences, the present expression pattern was in accordance with that shown in the dictyExpress database. Two different gene products have been reported for SteelyA. MPBD was the main in vitro product according to one report, but another report identified pyrone as the gene product (Austin et al., 2006; Ghosh et al., 2008). Because the structure of MPBD has been examined thoroughly (Saito et al., 2006), we first focused on MPBD. To test whether MPBD is the product of SteelyA, we compared the materials released from mature fruiting bodies of the stlA null strain and Ax2, wild-type strain. Nonpolar compounds released from the cells were collected using the Amberlite XAD-2 resin. After the elution of bound compounds from the resin, extracted materials were dissolved in 40% methanol and separated by reverse-phase HPLC. This method was used in a previous study in which MPBD was purified and identified as a differentiation-inducing factor (Saito et al., 2006). We detected the HPLC peak from the Ax2 sample, but not from the stlA null sample. To confirm that the stlA mutant lacked MPBD, we further analyzed the HPLC fractions by GC–MS.

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