Regulation of Expression of the TIR-Containing Protein C Gene of the Uropathogenic Escherichia coli Strain CFT073

Abstract: The uropathogenic Escherichia coli strain CFT073 causes kidney abscesses in mice Toll/interleukin-1 receptor domain-containing protein C (TcpC) dependently and the corresponding gene is present in around 40% of E. coli isolates of pyelonephritis patients. It impairs the Toll-like receptor (TLR) signaling chain and the NACHT leucin-rich repeat PYD protein 3 inflammasome (NLRP3) by binding to TLR4 and myeloid differentiation factor 88 as well as to NLRP3 and caspase-1, respectively. Overexpression of the tcpC ge… Show more

“…The phenotype of the CFT073 ∆hns strain was weaker after 24 h of culture (Figure 8B). As we reported earlier, high pH values stimulated the P2 promoter [12]. We therefore compared the P2 promoter activity of the three different gene-deficient P2 reporter strains upon stimulation with increasing pH.…”

“…We repeated the experiment with the reporter construct pPc2397-Pc2398:gfpmut:KAN containing, in addition to the promoter P2, the promoter P1, which may generate a polycistronic mRNA encompassing c2397 and tcpC (c2398). While we described earlier the transcription start of P2 in the 5 UTR of the gene c2397 [12], we now determined the transcription start of P1 using a 5 RACE PCR approach and found two different transcription start sites, one 57 and the other one 13 bp before a putative start codon of c2397 (Figure S4). Increasing potassium chloride concentration also stimulated the pPc2397-Pc2398:gfpmut:KAN (P1 + P2) reporter construct (Figure 5C,D) with no real difference to pPc2398:gfpmut:KAN (P2).…”

“…We therefore tested the ability of the uroepithelial cell line T24/83 to activate the tcpC promoter. We transformed CFT073 with the reporter plasmid Pc2398:gfpmut2 containing the P2 promoter fused to the green fluorescent protein mut2 (gfpmut2), described above, to generate the plasmid-based reporter strain CFT073 pPc2398:gfpmut2:KAN [12]. We then co-incubated the CFT073 pPc2398:gfpmut2:KAN reporter strain for 4 and 24 h with titrated amounts of T24/83 cells in McCoy medium and measured its fluorescence intensity by flow cytometry.…”

“…The former is located in the 5 UTR of the gene c2397, the latter in the 5 UTR of c2398, which encodes TcpC. We found that P2 responded much more strongly than P1 to stimuli such as high pH, glucose concentration of 3 mmol/l or more, and urine [12]. These stimuli not only activated the plasmid-based reporter constructs transformed into CFT073 on plasmids but also stimulated a chromosomal reporter strain where we replaced tcpC by gfpmut2.…”

“…These stimuli not only activated the plasmid-based reporter constructs transformed into CFT073 on plasmids but also stimulated a chromosomal reporter strain where we replaced tcpC by gfpmut2. We mapped the transcription start of P2 44 bp 5 of a putative start codon of the c2398 RNA [12].…”

The Promoter of the Immune-Modulating Gene TIR-Containing Protein C of the Uropathogenic Escherichia coli Strain CFT073 Reacts to the Pathogen’s Environment

“…The phenotype of the CFT073 ∆hns strain was weaker after 24 h of culture (Figure 8B). As we reported earlier, high pH values stimulated the P2 promoter [12]. We therefore compared the P2 promoter activity of the three different gene-deficient P2 reporter strains upon stimulation with increasing pH.…”

“…We repeated the experiment with the reporter construct pPc2397-Pc2398:gfpmut:KAN containing, in addition to the promoter P2, the promoter P1, which may generate a polycistronic mRNA encompassing c2397 and tcpC (c2398). While we described earlier the transcription start of P2 in the 5 UTR of the gene c2397 [12], we now determined the transcription start of P1 using a 5 RACE PCR approach and found two different transcription start sites, one 57 and the other one 13 bp before a putative start codon of c2397 (Figure S4). Increasing potassium chloride concentration also stimulated the pPc2397-Pc2398:gfpmut:KAN (P1 + P2) reporter construct (Figure 5C,D) with no real difference to pPc2398:gfpmut:KAN (P2).…”

“…We therefore tested the ability of the uroepithelial cell line T24/83 to activate the tcpC promoter. We transformed CFT073 with the reporter plasmid Pc2398:gfpmut2 containing the P2 promoter fused to the green fluorescent protein mut2 (gfpmut2), described above, to generate the plasmid-based reporter strain CFT073 pPc2398:gfpmut2:KAN [12]. We then co-incubated the CFT073 pPc2398:gfpmut2:KAN reporter strain for 4 and 24 h with titrated amounts of T24/83 cells in McCoy medium and measured its fluorescence intensity by flow cytometry.…”

“…The former is located in the 5 UTR of the gene c2397, the latter in the 5 UTR of c2398, which encodes TcpC. We found that P2 responded much more strongly than P1 to stimuli such as high pH, glucose concentration of 3 mmol/l or more, and urine [12]. These stimuli not only activated the plasmid-based reporter constructs transformed into CFT073 on plasmids but also stimulated a chromosomal reporter strain where we replaced tcpC by gfpmut2.…”

“…These stimuli not only activated the plasmid-based reporter constructs transformed into CFT073 on plasmids but also stimulated a chromosomal reporter strain where we replaced tcpC by gfpmut2. We mapped the transcription start of P2 44 bp 5 of a putative start codon of the c2398 RNA [12].…”

The Promoter of the Immune-Modulating Gene TIR-Containing Protein C of the Uropathogenic Escherichia coli Strain CFT073 Reacts to the Pathogen’s Environment