10 research outputs found
An Improved Method for High Quality Metagenomics DNA Extraction from Human and Environmental Samples
To explore the natural microbial community of any ecosystems by high-resolution molecular approaches including next generation sequencing, it is extremely important to develop a sensitive and reproducible DNA extraction method that facilitate isolation of microbial DNA of sufficient purity and quantity from culturable and uncultured microbial species living in that environment. Proper lysis of heterogeneous community microbial cells without damaging their genomes is a major challenge. In this study, we have developed an improved method for extraction of community DNA from different environmental and human origin samples. We introduced a combination of physical, chemical and mechanical lysis methods for proper lysis of microbial inhabitants. The community microbial DNA was precipitated by using salt and organic solvent. Both the quality and quantity of isolated DNA was compared with the existing methodologies and the supremacy of our method was confirmed. Maximum recovery of genomic DNA in the absence of substantial amount of impurities made the method convenient for nucleic acid extraction. The nucleic acids obtained using this method are suitable for different downstream applications. This improved method has been named as the THSTI method to depict the Institute where the method was developed
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Genomic plasticity associated with antimicrobial resistance in Vibrio cholerae.
The Bay of Bengal is known as the epicenter for seeding several devastating cholera outbreaks across the globe. Vibrio cholerae, the etiological agent of cholera, has extraordinary competency to acquire exogenous DNA by horizontal gene transfer (HGT) and adapt them into its genome for structuring metabolic processes, developing drug resistance, and colonizing the human intestine. Antimicrobial resistance (AMR) in V. cholerae has become a global concern. However, little is known about the identity of the resistance traits, source of AMR genes, acquisition process, and stability of the genetic elements linked with resistance genes in V. cholerae Here we present details of AMR profiles of 443 V. cholerae strains isolated from the stool samples of diarrheal patients from two regions of India. We sequenced the whole genome of multidrug-resistant (MDR) and extensively drug-resistant (XDR) V. cholerae to identify AMR genes and genomic elements that harbor the resistance traits. Our genomic findings were further confirmed by proteome analysis. We also engineered the genome of V. cholerae to monitor the importance of the autonomously replicating plasmid and core genome in the resistance profile. Our findings provided insights into the genomes of recent cholera isolates and identified several acquired traits including plasmids, transposons, integrative conjugative elements (ICEs), pathogenicity islands (PIs), prophages, and gene cassettes that confer fitness to the pathogen. The knowledge generated from this study would help in better understanding of V. cholerae evolution and management of cholera disease by providing clinical guidance on preferred treatment regimens.DBT Indi
Molecular characterizations of rel and rellike genes of Mycobacterium tuberculosis
Mycobacterium tuberculosis (Mtb) is a highly pathogenic bacterium belonging to the Mycobacteriaceae family and the causative agent of tuberculosis (TB), also known as „white plague‟. Robert Koch (Fig. 1) first discovered the pathogen in 1882. Mtb has an unusual, waxy coating on its cell surface (primarily mycolic acid), which makes the cells impervious to Gram staining, therefore, acid-fast detection techniques are used. Mtb is highly aerobic and requires high levels of oxygen. Mtb typically attacks the lungs, but can also affect other tissues of the body. It is transmitted through person to person via aerosols. In healthy people, infection with Mtb often causes no symptoms, since the person's immune system acts to “wall off” the bacteria. The symptoms of active TB of the lung are coughing, sometimes sputum may contain frank blood, chest pains, weakness, weight loss, fever and night sweats. The most frequently used diagnostic methods for TB are the tuberculin skin test, acid-fast stain and chest radiograph
Functional Characterization of the Stringent Response Regulatory Gene dksA of Vibrio cholerae and Its Role in Modulation of Virulence Phenotypes
In bacteria, nutrient deprivation evokes the stringent response, which is mediated by the small intracellular signaling molecule
ppGpp. In Gram negatives, the RelA enzyme synthesizes and SpoT hydrolyzes ppGpp, although the latter protein also has weak
synthetase activity. DksA, a recently identified RNA polymerase binding transcription factor, acts as a coregulator along with
ppGpp for controlling the stringent response. Recently, we have shown that three genes, relA, spoT, and relV, govern cellular levels
of ppGpp during various starvation stresses in the Gram-negative cholera pathogen Vibrio cholerae. Here we report functional
characterization of the dksA gene of V. cholerae (dksAVc), coding for the protein DksAVc. Extensive genetic analyses of the
�dksAVc mutants suggest that DksAVc is an important component involved in the stringent response in V. cholerae. Further
analysis of mutants revealed that DksAVc positively regulates various virulence-related processes, namely, motility, expression of
the major secretory protease, called hemagglutinin protease (HAP), and production of cholera toxin (CT), under in vitro conditions.
We found that DksAVc upregulates expression of the sigma factor FliA (�28), a critical regulator of motility in V. cholerae.
Altogether, it appears that apart from stringent-response regulation, DksAVc also has important roles in fine regulation of virulence-
related phenotypes of V. cholera
Genetic and mutational characterization of the small alarmone synthetase gene relV of Vibrio cholerae
Rugose atypical Vibrio cholerae O1 El Tor responsible for 2009 cholera outbreak in India
Vibrio cholerae causes cholera outbreaks in endemic regions where the water quality and sanitation facilities remain poor. Apart from biotype and serotype changes, V. cholerae
undergoes phase variation, which results in the generation of two morphologically different variants termed smooth and rugose. In this study, 12 rugose (R-VC) and 6 smooth (S-VC) V. cholerae O1 Ogawa isolates were identified in a cholera outbreak that occurred in Hyderabad, India. Antimicrobial susceptibility results showed that all the isolates were resistant to ampicillin, furazolidone and nalidixic acid. In addition, R-VC isolates were resistant to ciprofloxacin (92 %), streptomycin (92 %), erythromycin (83 %), trimethoprim-sulfamethoxazole (75 %) and tetracycline
(75 %). Based on the ctxB gene analysis, all the isolates were identified as El Tor variant with mutation in two positions of ctxB, similar to the classical biotype. The R-VC isolates specifically showed excessive biofilm formation and were comparatively less motile. In addition, the majority of these isolates (~83 %) displayed random mutations in the hapR gene, which encodes haemagglutinin protease regulatory protein. In the PFGE analysis, R-VC and S-VC were placed in distinct clusters but remained clonally related. In the ribotyping analysis, all the R-VC isolates
exhibited R-III pattern, which is a prevailing type among the current El Tor isolates. A hapR deletion mutant generated using an S-VC isolate expressed rugose phenotype. To our knowledge, this is the first report on the association of rugose V. cholerae O1 in a large cholera
outbreak with extended antimicrobial resistance and random mutations in the haemagglutinin protease regulatory protein encoding gene (hapR)