8 daltons. Because these two values are similar, we consider that
the purified protein is the product of the gene whose nucleotide sequence was determined in this experiment. The lipase of A. sobria is biosynthesized Selleck CX-4945 as a precursor form consisting of a pre-region (from the first to 18th amino acid residue) and mature region (from the 19th amino acid residue to the carboxy terminal end). The pre-region functions as a signal peptide in translocation across the inner membrane and is cleaved off during translocation. As shown in Figure 1, we confirmed that the mature form of the lipase exists in the culture supernatant; however, there is a possibility that the majority of lipase remains in cells, some lipase appearing outside the cells due to cell destruction. To examine the location of the lipase, the cells were cultured in NB (0.5). At 6, 12, and 24 hrs, a portion of the culture fluid (20 mL) was removed. Three fractions, the culture supernatant, periplasmic, and outer membrane
fractions, were made from each culture and the existence of lipase in each fraction was examined by immunoblotting. As shown in Figure 7, lipase was detected in the periplasm and culture supernatant fractions. In particular, the density of the band in lane 9 (sample prepared from the culture supernatant fraction after Galunisertib concentration 24 hr culture) is high. This band was not detected in any samples prepared from the outer membrane fraction throughout the cultivation period, indicating that the lipase is an exoprotein. Because the lipase synthesized
in the cytoplasm translocated across the inner membrane with the help of the pre-region and remained for a while in the periplasm, samples prepared IKBKE from the periplasmic fraction reacted with the antiserum (Fig. 7) and the lipase crossed the outer membrane without remaining in it. As shown in Figure 1, production of lipase was suppressed when A. sobria 288 (asp−, amp−) was cultured in NB (3.0). To elucidate how NaCl suppressed lipase production, we examined the effect of NaCl in medium on gene transcription by A. sobria for the lipase. A. sobria 288 (asp−, amp−) were cultured in NB (0.5) and NB (3.0) and the cells recovered 3, 6, 9, 12, and 24 hrs after initiation of the culture. The RNAs of these cells were extracted and the amounts of RNA indicated in Figure 8 fixed to the membrane and reacted with the probe for the lipase gene. As shown in Figure 8, the densities of the dots in the samples from the culture in NB (3.0) at 3, 6, and 9 hrs were slightly higher than those from culture of the strain in NB (0.5). Next, we examined the transcriptional level of lipase gene by quantitative RT-PCR. The cDNAs were prepared from the RNA samples obtained from the cells cultured in NB (0.5) and NB (3.0) for 6 hrs by treatment with reverse transcriptase. The DNA fragment of lipase was amplified from these cDNAs. However, amplification did not occur in the sample which was not treated with reverse transcriptase.