The binding sites of mAb BG11 and mAb DC10 are depicted with antibody icons. CS1, a conserved region of bacterial OppA proteins, is shown in diagonal strips, and conserved regions of mycoplasmal OppA proteins are depicted by dotted areas (CS2) and vertical strips (CS3). The ATP-binding site consists of the C-terminal localized Walker A (grid) and Walker B (horizontal strips) motifs. The deletion mutants were sign with gaps between the OppA bulks. Modified regions of the Walker A mutants were described below the OppA bulks. B. SDS-PAGE of the recombinant OppA mutants and wild type proteins P50, P60/P80, OppAwt and the
dephosphorylated OppAΔPi variant. The purified proteins were separated on a PLX3397 9.5% SDS gel followed by Coomassie staining and the wild type OppA variants in addition by ProQ- staining demonstrating phosphorylations. SeeBlue Plus 2 Pre-Stained Standard from Invitrogen was used as molecular weight marker. In the search for conserved sequence motifs in OppA proteins of different species, three regions with high homologies were detected: the region of AA179 – AA244, which is conserved in bacterial OppA proteins, thus
named CS1 (consensus sequence 1), and regions CS2 (AA365 – AA372) and CS3 (AA701 – AA729), which are conserved in mycoplasmal OppA proteins. To determine the functions of these regions, OppA mutants, OppAΔCS1, OppAΔCS2 and OppAΔCS3 were constructed (selleck products Figure 1A). With regard to the ATPase activity of OppA we analyzed five mutants. In 2004 two OppA mutants, OppAK875R (here named OppAWA1) and OppAΔP-loop this website (OppAWA2) had already been characterized. They were modified to different extent within the Walker A region (AA869 – AA876) leading to a decreased ATPase activity to 15% (OppAWA1) and 6% (OppAWA2) in relation to the wild type [14]. As L-NAME HCl computer analysis revealed a putative Walker A motif (AA411 – AA418) in the OppA protein of M. pulmonis (MYPU_6070), we constructed a third Walker A mutant (OppAWA3) by replacing the original Walker A region
of M. hominis with the putative Walker A sequence. Interestingly this putative Walker A motif of M. pulmonis OppA is located within the CS2 region. In the fourth OppA mutant, OppAΔWB the less conserved Walker B motif plus a downstream region of several hydrophobic amino acids was deleted (AA737 – AA752). In the OppAN mutant the C-terminal half of OppA (AA481- AA 961) was deleted thus missing the CS3, Walker B and Walker A motif. All OppA mutants were expressed in E. coli with an N-terminal histidine-tag instead of the 28 AA signal peptide; including the cysteine residue where signal peptidase II cleavage and lipid modification would normally take place in M. hominis. After purification the quality of the OppA mutants and wild type membrane proteins used in the following analyses was documented by SDS- PAGE. Dephosphorylation of OppA was demonstrated by ProQ staining (Figure 1B).