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. 1999 Oct 26;96(22):12844-8.
doi: 10.1073/pnas.96.22.12844.

Attenuation of virulence in Mycobacterium tuberculosis expressing a constitutively active iron repressor (V体育安卓版)

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Attenuation of virulence in Mycobacterium tuberculosis expressing a constitutively active iron repressor (VSports在线直播)

Y C Manabe et al. Proc Natl Acad Sci U S A. .

Abstract

Iron is an essential nutrient for the survival of most organisms and has played a central role in the virulence of many infectious disease pathogens. Mycobacterial IdeR is an iron-dependent repressor that shows 80% identity in the functional domains with its corynebacterial homologue, DtxR (diphtheria toxin repressor). We have transformed Mycobacterium tuberculosis with a vector expressing an iron-independent, positive dominant, corynebacterial dtxR hyperrepressor, DtxR(E175K) VSports手机版. Western blots of whole-cell lysates of M. tuberculosis expressing the dtxR(E175K) gene revealed the stable expression of the mutant protein in mycobacteria. BALB/c mice were infected by tail vein injection with 2 x 10(5) organisms of wild type or M. tuberculosis transformed with the dtxR mutant. At 16 weeks, there was a 1. 2 log reduction in bacterial survivors in both spleen (P = 0. 0002) and lungs (P = 0. 006) with M. tuberculosis DtxR(E175K). A phenotypic difference in colonial morphology between the two strains also was noted. A computerized search of the M. tuberculosis genome for the palindromic consensus sequence to which DtxR and IdeR bind revealed six putative "iron boxes" within 200 bp of an ORF. Using a gel-shift assay we showed that purified DtxR binds to the operator region of five of these boxes. Attenuation of M. tuberculosis can be achieved by the insertion of a plasmid containing a constitutively active, iron-insensitive repressor, DtxR(E175K), which is a homologue of IdeR. Our results strongly suggest that IdeR controls genes essential for virulence in M. tuberculosis. .

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Figure 1
Figure 1
Western blot of cell lysates incubated with polyclonal antibody against DtxR. Lane 1, purified DtxR (25.3 kDa). Lanes 3 and 5, lysates from wild-type M. smegmatis and M. tuberculosis, respectively, expressing native IdeR (25.2 kDa.). Lane 4, lysate from the M. smegmatis heterodiploid harboring pNBV1/SAD expressing both DtxR(E175K) and IdeR. The molecular masses, determined by size standards, are shown at left.
Figure 2
Figure 2
Virulence comparison of wild-type M. tuberculosis and M. tuberculosis DtxR(E175K) mutant. (A) The log cfu of the homogenized spleens of mice sacrificed at 4-week intervals. (B) The log cfu of homogenized lungs at 4-week intervals. Each point represents the mean log cfu of 5–6 mice ± 1 SD (error bars). * denote statistically significant differences between groups at a given time point.
Figure 3
Figure 3
(A) A 10-week-old representative colony of M. tuberculosis DtxR(E175K) on 7H10 agar. (B) A 10-week-old representative colony of wild-type M. tuberculosis (strain CDC1551) on 7H10 agar.
Figure 4
Figure 4
Alignment of the iron box consensus sequence, known DtxR binding sites, and putative M. tuberculosis DtxR/IdeR binding sites identified by an in silico genome search. The consensus sequence at the top represents the compilation of the nine aligned sequences shown. The published consensus is drawn from the literature. Gene homologues of the downstream ORFs are shown on the right.
Figure 5
Figure 5
Autoradiographs of gel-binding assay between DtxR and putative M. tuberculosis DtxR/IdeR binding sites. Shown are 100-bp 32P-end-labeled DNA fragments containing toxO (lanes 1 and 2), IB-1 (lanes 3 and 4), IB-2 (lanes 5 and 6), IB-3 (lanes 7 and 8), IB-4 (lanes 9 and 10), and IB-5 (lanes 11 and 12) separated in a nondenaturing 6% polyacrylamide gel. Odd-numbered lanes contain DNA only (unbound), and even-numbered lanes contain DNA preincubated with purified DtxR (bound).

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