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The Biochemical Analysis of Coexpressed and Copurified XpsE/MBP-XpsLN Complex
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|摘要:||T2SS of Xanthomonas campestris pv campestris is assembled by 12 proteins. XpsE is the only cytoplasmic component and the likely energy supplier of the system, whereas XpsL is a bitopic membrane protein with a single transmembrane segment. The role of XpsL in T2SS is not so clear. It has been previously observed that the hexameric XpsE, whose formation is nucleotide-dependent, interacts in vitro directly with the cytoplasmic domain of XpsL as MBP-XpsLN. We thus speculated that XpsE may form complex with XpsLN in vivo. In this study, we attempted the complex isolation by coexpressing XpsE and MBP- XpsLN in E. coli. Copurification of MBP-XpsLN and Strep-tagged XpsE was observed on the SDS-PAGE when purified using double-affinity chromatography, indicating that a stable XpsE/MBP-XpsLN complex was formed as a consequence of their coexpression in E. coli. The molecular size of such a complex was estimated to be 800 kDa as revealed by size-exclusion chromatography. We thus postulated that the complex may be constituted of 6 molecules each component. The protein complex purified from size-exclusion chromatography exhibited an ATPase activity sixfold that of the singly expressed XpsE. In addition, the ATPase activity of the complex was stimulated by cardiolipin by threefold. The XpsE/MBP-XpsLN complex resulted from the coexpression strategy employed here might resemble an intermediate stage during secretion process in vivo, thus enabling us to study in the future the mechanistic events driven by the interaction between XpsE and XpsL.|
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