The strains clearly synthesized unsaturated fatty acids when grown at all of the different temperatures. However, the level of unsaturated fatty acids synthesized was lower than that seen in K1060 carrying a plasmid (pCY9) that encoded E. coli fabB and the amount of cis-vaccenate decreased with increased growth temperature. Moreover, despite the differing copy numbers, the two plasmids that encoded C. acetobutylicium FabF1 gave similar levels of unsaturated fatty acids. These
results provide an explanation for lack of complementation of the fabB(Ts) phenotype at 42°C by the fabF1-encoding plasmids. At 42°C the low activity of FabF1 did not allow enough unsaturated fatty acid see more synthesis to support growth. To test whether or not C. acetobutylicium FabF1 has FabB function at learn more 42°C we assayed unsaturated fatty acid synthesis in strain
CY242 carrying the fabF1 plasmid pHW36 (growth was supported by cyclopropane fatty acid supplementation) (Fig. 3). Under these conditions [14C] acetate labeling showed low levels of unsaturated fatty acids synthesis upon arabinose induction of FabF1 expression (Fig. 3). Therefore, FabF1 has the ability to replace FabB in E. coli unsaturated fatty acid synthesis but its expression allows growth only when the host FabF is present to perform the bulk of the chain elongation reactions. Phosphoprotein phosphatase Table 2 Fatty acid compositions (% by weight)of fabB strain K1060 transformed with plasmids encoding either C. acetobutylicium fabF1 or E. coli PLX4032 order fabB. 30°C 37°C 42°C Fatty acid pHW33 pHW36 pCY9 pHW33 pHW36 pCY9 pHW33 pHW36 pCY9 C14:0 4.9 9.2 2.2 11.1 7.7 4 11.1 9.9 2.5 C16:1 12.8 8.1 16.8 17.5 18 20 19.7 13.5 20.3 C16:0 22.1 21.6 10.8 25.9 23.6 13.8 32.6 42.7 19.7 C18:1 43.1 43.1 67.1 31.8 34.4 58.1 17.7 22.4 51 C18:0 17 18 3.2 13.7 16.3 3.7 18.9 11.5 6.5 Figure 3 Expression of C. acetobutylicium FabF1 restores UFA synthesis to E. coli fabB strains. The methyl esters of fatty acids were obtained from the phospholipids as described in Methods. Lane 1 is
the esters of the wild type E. coli strain MG1655. Lane 2 is the esters of strain CY242 carrying pHW36 (fabF1) in presence of arabinose induction. Lane 3 is the esters of strain CY242 carrying pHW36 (fabF1) in the absence of induction. Lane 4 is the esters of strain CY242 carrying vector pBAD24. The migration positions of the methyl esters of the fatty acid species are shown. The designations are: Sat, saturated fatty acid esterss; Δ9C16:1, methyl ester of cis-9-hexadecenoic; Δ11C18:1, methyl ester of cis-11-octadecenoic. Functional analysis of C. acetobutylicium FabZ in vivo The sole fabZ homologue in the C. acetobutylicium genome is located within a large cluster of putative fab genes [10].