Patent ID: 7332340

Claim:
A process for identifying a novel target for use for the development of therapeutic modalities and drugs effective against tuberculosis comprising: I) disrupting devR (Rv 3133C) gene located in a ˜3.3 kb EcoRI-HindIII insert of plasmid pJT53.34, II) constructing pJQ200Skdev::kan from the disrupted devR gene, III) introducing said plasmid into M. tuberculosis H37Rv, IV) selecting single crossover transformants indicative of plasmid integration on Middlebrook 7H10 agar plates containing kanamycin, V) analyzing said single crossover transformants by polymerase chain reaction (PCR) for the presence of devR, Km R and sucrose resistance (SacB) gene sequences, VI) subjecting said sequences to the step of Southern analysis with devR probe, devS probe kanamycin resistant gene probe so as to designate M. tuberculosis Dup devR containing wild-type and the disrupted copies of the devR locus, VII) growing M. tuberculosis Dup devR in Middlebrook 7HP medium containing kanamycin and sucrose, VIII) subjecting said grown M. tuberculosis Dup devR strain into a plurality of plates having Middlebrook 7H10 medium containing kanamycin and sucrose therein so as to obtain kanamycin resistant transformants, thereby obtaining devR mutant strain of M. tuberculosis, IX) subjecting said grown M. tuberculosis devR to the step of Southern hybridization followed by polymerase chain reaction process for the confirmation of said allelic exchange, X) subjecting said transformants to the step of polymerase chain reaction analysis for devR::kan disrupted gene, XI) subjecting said devR::kan disrupted gene to the step of Western blotting and immuno electron microscopy for the confirmation of functional disruption of said gene, XII) evaluating the viability of growth of the strain M. tuberculosis devR mutant under conditions of oxygen limitation for devR and devS gene expression, XIII) evaluating the viability of growth of said strain M. tuberculosis devR under conditions of oxygen limitation in aerobic conditions for devR and devS gene expression, XIV) subjecting said grown strain to the step of RT-PCR analysis for transcripts obtained from the Rv3134c-devR-devS operon, XV) scanning said transcripts by using the Ultra-Violet products gel documentation system and subjecting the same to the step of densiometric analysis by using a computer software, XVI) testing M. tuberculosis devR mutant strain for virulence in guinea pigs comprising (a) histopathological analysis of the infected organs (lung and liver) from guinea pigs infected with devR mutant and wild-type strains of M. tuberculosis and (b) recovery of M. tuberculosis from spleen of infected animals and quantification of bacterial load.