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237 results on '"CHAUHAN, D. S."'

201. Diagnostic value of real time PCR for neurotuberculosis.

Author

Dayal R, Senthilkumar P, Katoch VM, Chauhan DS, and Yadav NK

Subjects
Case-Control Studies, Child, Child, Preschool, DNA, Bacterial cerebrospinal fluid, DNA, Bacterial genetics, Humans, Infant, Mycobacterium tuberculosis genetics, Predictive Value of Tests, RNA, Ribosomal, 16S genetics, Tuberculosis, Central Nervous System cerebrospinal fluid, Mycobacterium tuberculosis isolation & purification, Polymerase Chain Reaction methods, Tuberculosis, Central Nervous System diagnosis
Published
2010

202. Potential of a metabolic gene (accA3) of M. leprae as a marker for leprosy reactions.

Author

Sharma R, Lavania M, Chauhan DS, Katoch K, Amresh, Pramod, Rakhi, Richa, and Katoch VM

Subjects
Bacterial Proteins metabolism, Biomarkers, Biopsy, Case-Control Studies, Computational Biology, Enzyme-Linked Immunosorbent Assay, Gene Expression Profiling, Humans, Leprosy immunology, Leprosy microbiology, Mycobacterium leprae isolation & purification, Mycobacterium leprae metabolism, Reverse Transcriptase Polymerase Chain Reaction methods, Bacterial Proteins genetics, Leprosy pathology, Mycobacterium leprae genetics, RNA, Bacterial genetics
Abstract

Understanding the mechanism(s) of reactions in leprosy remains a challenging task for both clinicians and basic scientists. While there is some understanding of host processes associated with different type of lepra reactions, there is very little information about bacterial factors triggering these inflammatory processes. This study is continuation of our earlier research programme on leprosy genomics in which significant transcription of 11 genes was observed during active disease and these included accA3 gene. In present study, we have investigated the potential of this gene or its gene product as molecular and or immunological marker for studying the reactions. Using quantitative Real-Time RT-PCR significant higher expression (mean log2 ratio=3.39) of accA3 was observed in specimens from leprosy reaction cases compared with cases without reactions. in silico homology model of this protein was analyzed for hydrophilic and B-cell epitope regions. Peptides with maximum antigenecity were selected, cloned, expressed and used to study sero-reactivity across the disease spectrum by indirect ELISA. While sero-reactivity was observed in leprosy cases the antibody levels did not vary significantly between the patient/s of same clinical type with and without reaction thereby indicating the limitation of this approach for this purpose. Measurement of transcription of this gene has, thus, potential as a molecular marker for monitoring the reactions.

Published
2009

203. Role of embCAB gene mutations in ethambutol resistance in Mycobacterium tuberculosis isolates from India.

Author

Jadaun GP, Das R, Upadhyay P, Chauhan DS, Sharma VD, and Katoch VM

Subjects
Culture Media, DNA, Bacterial genetics, Humans, India, Microbial Sensitivity Tests, Mycobacterium tuberculosis isolation & purification, Oxazines metabolism, Sequence Analysis, DNA, Tuberculosis microbiology, Xanthenes metabolism, Antitubercular Agents pharmacology, Bacterial Proteins genetics, Drug Resistance, Bacterial, Ethambutol pharmacology, Mutation, Missense, Mycobacterium tuberculosis drug effects, Mycobacterium tuberculosis genetics
Abstract

In the present study, ethambutol (EMB) resistance-associated mutations were characterised in the embCAB genes of clinical isolates of Mycobacterium tuberculosis (MTB) collected in India. Thirty MTB isolates were tested for their susceptibility to first-line antitubercular drugs using the Löwenstein-Jensen proportion method, and EMB minimum inhibitory concentrations of MTB isolates were determined by the resazurin microtitre assay. Sequencing of various regions of the embCAB genes was performed to identify EMB resistance-associated mutations. Mutations of embB306 were detected in 15 of 23 EMB-resistant MTB isolates. Three EMB-resistant isolates had mutations at codon 270 of the embC gene, two of which also harboured embB306 mutations. No mutation was identified in the embA gene. All seven EMB-sensitive MTB isolates had the wild-type embCAB sequence. In summary, embB306 mutations were associated with EMB resistance, and mutation at codon 270 of the embC gene may contribute to high-level EMB resistance in some MTB isolates.

Published
2009
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204. Serological diagnosis of tuberculosis.

Author

Dayal R, Singh A, Katoch VM, Joshi B, Chauhan DS, Singh P, Kumar G, and Sharma VD

Subjects
Acyltransferases immunology, Adolescent, Antigens, Bacterial immunology, Bacteriological Techniques, Child, Child, Preschool, Enzyme-Linked Immunosorbent Assay, Female, Humans, Immunoglobulin G blood, Infant, Infant, Newborn, Male, Sensitivity and Specificity, Serologic Tests methods, Tuberculosis diagnosis
Abstract

Objective: To evaluate the efficacy of ELISA for the detection of IgG antibodies against antigen 85 complex (Ag 85 complex) of Mycobacterium tuberculosis., Methods: Children of either sex, 0-18 years of age, attending the outpatient department and admitted in the casualty and wards of the Department of Pediatrics, S.N. Medical College, Agra, were included in present study. The study was carried out on children with pulmonary and CNS tuberculosis along with matching controls (83 cases and 32 controls). Informed consents of their parents or guardians were taken. They were subjected to clinical examination, relevant laboratory investigations, tuberculin test and chest radiograph. Relevant body fluids were subjected to bacteriological tests; ELISA was applied to serum samples for detection of IgG antibodies against antigen 85 complex (Ag85). The result of ELISA was compared with bacteriological tests [Ziehl Neelson (ZN) staining for acid-fast bacilli, culture on Lowenstein Jensen (LJ) medium and culture on BacT/Alert 3D system]., Results: ELISA tests showed a significantly higher sensitivity (59.1%) as compared with LJ medium culture method (19.3%), BacT/Alert 3D system (24.1%) and ZN staining (16.9%) in all patients (p<0.001). Specificity of ELISA test was 71.9%., Conclusion: In view of the convenience, low cost and good sensitivity, ELISA tests have a promising future in the diagnosis of childhood tuberculosis.

Published
2008
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205. Predominance of Mycobacterium fortuitum-chelonae complex in Ghatampur field area, endemic for leprosy.

Author

Lavania M, Katoch K, Parashar D, Sharma P, Das R, Chauhan DS, Sharma VD, and Katoch VM

Subjects
Bacterial Proteins chemistry, Bacterial Proteins genetics, Chaperonin 60 chemistry, Chaperonin 60 genetics, DNA, Bacterial chemistry, DNA, Bacterial genetics, Humans, India epidemiology, Mycobacterium Infections, Nontuberculous epidemiology, Mycobacterium chelonae genetics, Polymerase Chain Reaction, Polymorphism, Restriction Fragment Length, RNA, Ribosomal, 16S chemistry, RNA, Ribosomal, 16S genetics, Rural Population, Sequence Analysis, DNA, Endemic Diseases, Mycobacterium Infections, Nontuberculous microbiology, Mycobacterium chelonae isolation & purification, Soil Microbiology, Water Microbiology
Abstract

Non-tuberculous mycobacteria (NTM) are commonly found in the environment. As exposure to environmental mycobacteria has been reported to immunomodulatory in this study, the presence of environmental mycobacteria was investigated in soil, drinking water and drainage sample in Ghatampur, India, which is known for high endemicity for leprosy. Soil, drinking water from the hand pumps/wells and also drainage water collected in pools was collected in clean containers and cultured for environmental mycobacteria. Samples were processed according to the protocol established earlier. 69 soil, 62 drinking water and 31 drainage water samples were analysed from soil and water collected from 48 villages of this field area. After decontamination, cultures were set upon Lowenstein Jensen (LJ) medium. Mycobacteria were identified using biochemical tests and molecular techniques such as PCR-RFLP targeting hsp65 kD and rpoB region as well as 16S ribosomal sequencing in case of isolates showing variable biochemical features. NTM (non-tubercular mycobacteria) were isolated from 47.82% of soil samples, 20.69% of drinking water samples and 19.35% of the drainage water samples, overall mycobacteria could be isolated 52/162 of samples (32.09%). Among these mycobacteria, M. fortuitum-chelonae complex was predominant in this area; other species isolated were M. phlei, M. vaccae, M. terrae and M. flavescens. Relevance of exposure to these mycobacteria on endemicity needs to be studied by immunological and epidemiological parameters.

Published
2008

206. Development and evaluation of real-time RT-PCR assay for quantitative estimation of viable Mycobacterium leprae in clinical samples.

Author

Sharma R, Lavania M, Katoch K, Chauhan DS, Gupta AK, Gupta UD, Yadav VS, and Katoch VM

Subjects
Biopsy, Humans, Leprosy, Lepromatous pathology, RNA, Bacterial chemistry, Sensitivity and Specificity, Statistics, Nonparametric, Leprosy, Lepromatous microbiology, Mycobacterium leprae genetics, Mycobacterium leprae isolation & purification, RNA, Bacterial genetics, Reverse Transcriptase Polymerase Chain Reaction methods
Abstract

Detection of live organisms by molecular methods has special significance in leprosy where causative organism can not be cultivated in vitro. Such techniques would be especially important for monitoring the progress of the disease. While real-time RT- PCR technology will be appropriate for this purpose, there is very little experience of use of such tools in leprosy. This study describes the development of a quantitative RT-PCR targeting 16S rRNA based on primers used in a semi quantitative RT-PCR and its application on clinical samples including slit scraping and biopsies. RNA was extracted from biopsies from 3 lepromatous leprosy (LL) cases and standard curve was generated by plotting crossing over point against the dilutions of input RNA quantity (number of bacilli used for RNA extraction). Real-time RT-PCR was performed for quantitative detection of live M. leprae in 28 slit (13/28 smear positive) scrappings and 32 biopsies (22/32 smear positive). Number of viable bacteria as estimated by solid stained bacilli and real-time PCR correlated (no difference p>0.05). The test achieved a theoretical analytical sensitivity limit of up to single live bacillus even considering 11.3% efficiency of RNA preparation which was calculated by spiking of known number of leprosy bacilli in non leprosy skin biopsies (PCR negative). All smear positive cases were positive by this assay. This assay appears to be a promising tool for detection and quantification of viable bacilli in selected clinical situations and should be of use even in smear negative cases also.

Published
2008

207. Potential of Mw as a prophylactic vaccine against pulmonary tuberculosis.

Author

Katoch K, Singh P, Adhikari T, Benara SK, Singh HB, Chauhan DS, Sharma VD, Lavania M, Sachan AS, and Katoch VM

Subjects
Bacterial Vaccines administration & dosage, Double-Blind Method, Humans, Incidence, India epidemiology, Leprosy epidemiology, Leprosy immunology, Leprosy prevention & control, Prevalence, Rural Population, Sputum microbiology, Treatment Outcome, Tuberculosis, Pulmonary diagnosis, Tuberculosis, Pulmonary epidemiology, Vaccination standards, Bacterial Vaccines therapeutic use, Mycobacterium immunology, Tuberculosis, Pulmonary immunology, Tuberculosis, Pulmonary prevention & control
Abstract

Mycobacterium w (Mw), is a cultivable, non-pathogenic mycobacterium and has been tried extensively as an immunomodulator in leprosy. This has been found to be safe and has shown beneficial immunoprophylactic effect in population based, double blind placebo controlled trials in North India. These effects were also observed in the vaccine trials in South India. Keeping in view these beneficial effects and its earlier reported protective effect against tuberculosis in animals, its protective efficacy was evaluated in a rural population of about 28,948 people belonging to 272 villages in Ghatampur, Kanpur (India). The population was vaccinated with two doses (1st dose of 1x10(9) heat killed organisms followed 6 months later with a 2nd dose of 5x10(8) organisms) of Mw 10-13 years ago originally to investigate its effect against leprosy. The vaccine/placebo was given to healthy contacts of leprosy patients who had no evidence of suffering from tuberculosis. Incidence and prevalence of pulmonary tuberculosis in the present study was assessed in a blind manner by an active field survey and also retrospectively by history of anti tuberculosis treatment received by the patient in the intervening period (since vaccination), which was also corroborated by scrutinizing the medical records. Diagnosis was confirmed by standard clinical and bacteriological criteria. A total of 69 patients were diagnosed to be suffering from pulmonary tuberculosis during the survey which included 17 new sputum smear positive cases and 52 previously partially treated but still active pulmonary tuberculosis cases. The difference in the new sputum positive cases between the vaccinated (5/17) and placebo groups (12/17) was significant at 5% level of significance for 1 tailed test (Z>1.64). As 75% (52/69) of the cases had been diagnosed as suffering from pulmonary tuberculosis but had not taken adequate therapy all the cases diagnosed during the intervening period were recorded and re-analysis done. The differences are more significant at 1% level of significance for 1 tail test (Z>2.59) when all cases were analysed as a group. A small proportion 12.85% (total number=3036) of the contacts in the study population had BCG scars. On analysis of results on protection against tuberculosis in this group, BCG did provide protection against tuberculosis (p<0.01). In the placebo group the prevalence of tuberculosis was 1.11% which reduced to 0.70% for those who received Mw vaccine (p<0.01) which further decreased to 0.53% in those who had BCG scars and received Mw. These results thus provide evidence suggesting protective efficacy of Mw against pulmonary tuberculosis and that Mw merits investigation in future prospective immunoprophylactic trials along with other candidates for protection against pulmonary tuberculosis.

Published
2008
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210. Molecular typing of Mycobacterium tuberculosis isolates from different parts of India based on IS6110 element polymorphism using RFLP analysis.

Author

Chauhan DS, Sharma VD, Parashar D, Chauhan A, Singh D, Singh HB, Das R, Aggarwal BM, Malhotra B, Jain A, Sharma M, Kataria VK, Aggarwal JK, Hanif M, Shahani A, and Katoch VM

Subjects
Bacterial Typing Techniques, Gene Dosage, Humans, India epidemiology, Tuberculosis epidemiology, Mycobacterium tuberculosis classification, Mycobacterium tuberculosis genetics, Polymorphism, Genetic, Polymorphism, Restriction Fragment Length
Abstract

Background & Objective: IS 6110 based typing remains the internationally accepted standard and continues to provide new insights into the epidemiology of Mycobacterium tuberculosis. The aim of the study was to characterize M. tuberculosis isolates obtained from different parts of India based on IS6110 element polymorphism using restriction fragment length polymorphism (RFLP) analysis., Methods: RFLP was analyzed among 308 isolates of M. tuberculosis deposited in the Mycobacterial Repository Centre, Agra, from different parts of India. DNAs isolated from these strains were restricted with Pvu II, transferred on to nylon membrane and hybridized with a PCR amplified DIG-labeled 245 bp IS6110 probe., Results: Based on the copy number, M. tuberculosis isolates were classified into four groups, (i) lacking IS6110 element; (ii) low copy number (1-2); (iii) intermediate copy number (3-5); and (iv) high copy number (6-19). Copy number higher than 19 however was not observed in any of the isolates studied. At the national level, 56 per cent of the isolates showed high copy number of IS6110, 13 per cent showed intermediate copy number, 20 per cent showed low copy number, whereas 11 per cent isolates lacked IS6110 element. At the regional level, there was not much difference in the RFLP profiles of isolates (IS6110 copy numbers/patterns) from different parts of the country., Interpretation & Conclusion: IS6110 DNA based fingerprinting could be a potentially useful tool for investigating the epidemiology of tuberculosis in India.

Published
2007

211. Recent advances in molecular biology of leprosy.

Author

Katoch VM, Lavania M, Chauhan DS, Sharma R, Hirawati, and Katoch K

Subjects
Drug Design, Drug Resistance, Bacterial, Genome, Bacterial, Humans, Leprosy epidemiology, Polymerase Chain Reaction, RNA, Ribosomal genetics, Leprosy diagnosis, Mycobacterium leprae genetics
Abstract

The last three decades have witnessed rapid progress in understanding the molecular biology of Mycobacterium leprae. Following the availability of complete genome sequence of leprosy bacillus in 2001, things have drastically changed. With the information about genetic structure, several techniques have been developed for diagnosis, molecular epidemiology and also detection of drug resistance. With the decline in the prevalence of leprosy globally, there has been some reduction in interest in the molecular methods for diagnosis, yet molecular techniques for studying the transmission dynamics and detection of drug resistance continue to be relevant. Knowledge about complete genome sequence has made it possible to undertake studies that can improve our understanding of the structure and function of this enigmatic organism. Newer information emerging about biology of M. leprae would provide insight into mechanisms of its survival and persistence in host and is likely to lead to better diagnostics and also therapeutics for mycobacterial infections in general.

Published
2007

212. Rapid identification of mycobacteria by gene amplification restriction analysis technique targeting 16S-23S ribosomal RNA internal transcribed spacer & flanking region.

Author

Katoch VM, Parashar D, Chauhan DS, Singh D, Sharma VD, and Ghosh S

Subjects
Nucleic Acid Amplification Techniques, RNA, Ribosomal, 16S genetics, RNA, Ribosomal, 23S genetics, Restriction Mapping, Bacterial Typing Techniques methods, Mycobacterium genetics
Abstract

Background & Objective: Conventional identification of a clinical isolate of mycobacteria primarily based on culture characteristics and biochemical tests needs several weeks and may remain inconclusive. This study was undertaken to develop a new rapid method to identify the mycobacterial isolates at species level by gene amplification restriction analysis using primers encoding 16S-23S rRNA internal transcribed spacer (ITS) region and flanking parts of the 16S as well as 23S rRNA gene., Methods: This system is based on the amplification of approximately 1.8 kb fragment encoding 16S-23S rRNA spacer region and flanking parts of the 16S as well as 23S rRNA gene. This assay was applied on 13 reference strains and 480 clinical isolates of mycobacteria to validate the technique. Restriction was carried out with three restriction endonucleases Hha I, Hinf I and Rsa I., Results: Distinct gene amplification restriction analysis patterns were obtained by restriction of amplicons with three distinct restriction endonucleases (Hha I, Hinf I and Rsa I) which could differentiate various mycobacterial species., Interpretation & Conclusion: Restriction patterns with the enzymes used in this study could clearly distinguish Mycobacterium tuberculosis complex from other non chromogenic clinically important species M. avium and M. intracellulare. Results indicated this assay to be a simple, rapid and reproducible method to identify clinically relevant mycobacteria.

Published
2007

213. Applications of real-time PCR technology to mycobacterial research.

Author

Parashar D, Chauhan DS, Sharma VD, and Katoch VM

Subjects
Colony Count, Microbial, Drug Resistance, Bacterial genetics, Humans, Mycobacterium classification, Mycobacterium drug effects, Mycobacterium isolation & purification, Mycobacterium Infections diagnosis, Mycobacterium Infections drug therapy, Mycobacterium Infections microbiology, Mycobacterium tuberculosis genetics, Polymerase Chain Reaction trends, Species Specificity, Mycobacterium genetics, Polymerase Chain Reaction methods
Abstract

Real-time polymerase chain reaction (PCR) is being used worldwide for various research purposes. In this review we discuss the principles of real-time PCR, different methodologies and chemistries available and their applications in mycobacterial research. This technology allows for the direct detection of PCR product during the exponential phase of the reaction. Being a very powerful, accurate, rapid and sensitive method, this technique holds immense promise for detection of mycobacteria, differentiation of mycobacterial species, quantification of mycobacterial load and detection of drug resistance in mycobacterial infection.

Published
2006

214. Detection of Mycobacterium leprae DNA from soil samples by PCR targeting RLEP sequences.

Author

Lavania M, Katoch K, Sachan P, Dubey A, Kapoor S, Kashyap M, Chauhan DS, Singh HB, Sharma VD, Jadhav RS, and Katoch VM

Subjects
DNA, Bacterial analysis, Environmental Monitoring, Humans, India, Leprosy microbiology, Leprosy transmission, Mycobacterium leprae genetics, Polymorphism, Restriction Fragment Length, Mycobacterium leprae isolation & purification, Soil Microbiology
Abstract

Despite near elimination of leprosy as a public health problem, several problems in leprosy still remain. These include early detection, determining efficacy of the treatment and differentiating relapses from re-infection. These aspects have important impact on the patients undergoing treatment and also have a bearing on understanding transmission dynamics in the community. While early diagnosis and management do not need major technological inputs, various reports have suggested that M. leprae is found in the environment and may have a role in continued transmission of disease. In earlier studies from other parts of world the presence of M. leprae DNA in the environment has been investigated both by microbiological and molecular studies. In the present study, an attempt was made to extract M. leprae DNA from soil samples, which were collected from eighteen different locations including 3 from our Institute area and 15 from different villages of Ghatampur area. We optimized a protocol for the extraction of DNA and amplified a fragment of M. leprae using specific primers targeting RLEP sequences. It was found that 33.3% of these soil samples collected from areas inhabited by leprosy cases gave positive result for M. leprae specific DNA. The utility of this method needs to be explored on a larger scale to establish the presence of M.leprae in the environment, and its role in the spread of the disease.

Published
2006

215. Detection of M. leprae by reverse transcription- PCR in biopsy specimens from leprosy cases: a preliminary study.

Author

Hirawati, Katoch K, Chauhan DS, Singh HB, Sharma VD, Singh M, Kashyap M, and Katoch VM

Subjects
Biopsy, Humans, Leprosy microbiology, Mycobacterium leprae genetics, RNA, Ribosomal, 16S classification, Reverse Transcriptase Polymerase Chain Reaction, Sensitivity and Specificity, Leprosy diagnosis, Mycobacterium leprae isolation & purification, RNA, Ribosomal, 16S isolation & purification, Skin microbiology
Abstract

A reverse transcription (RT)-PCR assay targeting 16S rRNA of Mycobacterium leprae has been used to detect M.leprae specific nucleic acids. This study has been initiated to gain experience about detection of RNA from seven biopsy specimens by RT-PCR assay using species- specific primers described earlier. These biopsy specimens were from clinically confirmed and untreated leprosy cases belonging to BB and BL types. The earlier reported method was established in our laboratory. 171 bp fragment by RT-PCR was amplified from 4/7 cases. The positives results by RT-PCR were from the biopsies from fresh or short term treated cases whereas negative results were from specimens from long term treated cases showing clinical features of relapse. DNA targeting PCR (36 KDa) showed positivity in both groups. These results suggest that RT-PCR positivity possibly reflect the presence of viable organisms. Thus as earlier predicted RT-PCR assay may be useful for viability determinations for assessing the response to chemotherapy as well as presence of persisters in relapse cases.

Published
2006

216. Simultaneous use of two PCR systems targeting IS6110 and MPB64 for confirmation of diagnosis of tuberculous lymphadenitis.

Author

Singh HB, Singh P, Jadaun GP, Srivastava K, Sharma VD, Chauhan DS, Sharma SK, and Katoch VM

Subjects
False Negative Reactions, Humans, Mycobacterium tuberculosis genetics, Polymerase Chain Reaction methods, Sensitivity and Specificity, Tuberculosis, Lymph Node microbiology, DNA Transposable Elements genetics, DNA, Bacterial isolation & purification, Lymph Nodes microbiology, Mycobacterium tuberculosis isolation & purification, Tuberculosis, Lymph Node diagnosis
Abstract

PCR has emerged as a powerful technique for detection of various pathogens including Mycobacterium tuberculosis. In present study, eighty one samples of lymph node biopsies from clinically suspected cases of tuberculous lymphadenitis were examined for AFB, culture on Löwenstein Jensen medium and simultaneous use of two PCRs targeting IS6110 and MPB64. Positivity with M. tuberculosis culture and AFB was 13.6% and 28.4% respectively. All samples culture positive for nontuberculous mycobacteria were negative by both PCR systems. Higher proportion of positive results were observed with PCR targeting IS6110 by which 56 of 81 (69.1%) samples showed positive results as compared to PCR targeting MPB64 by which 39 of 81 (48.2 %) samples showed positive results. When combined, 63 out of 81 (77.8%) samples were detected positive for M. tuberculosis DNA. However, 7/81 (8.6 %) samples remained negative by IS6110 but positive by MPB64 method. Thus our data suggest that the use of one additional PCR (other than IS6110 system) can reduce false negativity of PCR results in the samples harboring zero copy of IS6110 element which is known to exist in Indian population.

Published
2006

217. The paradox of pyrazinamide: an update on the molecular mechanisms of pyrazinamide resistance in Mycobacteria.

Author

Singh P, Mishra AK, Malonia SK, Chauhan DS, Sharma VD, Venkatesan K, and Katoch VM

Subjects
Amidohydrolases genetics, Drug Resistance, Bacterial genetics, Humans, Mycobacterium tuberculosis enzymology, Mycobacterium tuberculosis genetics, Tuberculosis drug therapy, Antitubercular Agents pharmacology, Drug Resistance, Bacterial drug effects, Mycobacterium tuberculosis drug effects, Pyrazinamide pharmacology
Abstract

Pyrazinamide (PZA) is an important front line anti-tuberculosis drug because of its sterilizing activity against semi-dormant tubercle bacilli. In spite of its remarkable role in shortening the treatment duration from 9 months to 6 months when used in combination with Rifampicin and Isoniazid, PZA remains a difficult paradox because of its incompletely understood mode of action and mechanism of resistance. PZA is a nicotinamide analog prodrug which is converted into the active bactericidal form pyrazinoic acid by the bacterial enzyme pyrazinamidase (PZase). PZA does not appear to have a specific cellular target and instead, exerts its bactericidal effect by disrupting the membrane energetics and acidification of cytoplasm. Majority (72-97%) of PZA-resistant isolates of M. tuberculosis exhibit mutations in their pncA gene or upstream area leading to loss of PZase activity. A wide diversity of pncA mutations scattered along the entire length of pncA gene is unique to PZA resistance. However, PZA resistant isolates with normal PZase activity and wild type pncA sequences have also been reported in several studies which indicate that alternate mechanisms of PZA resistance exist. Investigations into these mechanisms would be useful in developing alternative diagnostic/therapeutic measures. This review presents the update of various mechanisms of PZA resistance in different mycobacteria with special emphasis on mode of action of PZA and mechanisms of resistance in Mycobacterium tuberculosis.

Published
2006

218. Characterization of mycobacteria isolated from bovines by PRA-targetting hsp 65 gene region.

Author

Parashar D, Srivastava RK, Chauhan DS, Sharma VD, Singh M, Lavania M, Chauhan A, Bhatia AK, and Katoch VM

Subjects
Animals, Bacterial Proteins genetics, Cattle, Chaperonin 60, Chaperonins genetics, DNA, Bacterial analysis, Mycobacterium phlei genetics, Mycobacterium tuberculosis genetics, Nontuberculous Mycobacteria genetics, Polymerase Chain Reaction methods, Bacterial Proteins classification, Chaperonins classification, Mycobacterium phlei classification, Mycobacterium tuberculosis classification, Nontuberculous Mycobacteria classification, Polymorphism, Restriction Fragment Length, Tuberculosis, Bovine classification
Abstract

Bovine tuberculosis caused by the bacterium Mycobacterium bovis is a major infectious disease of animals and has zoonotic importance for humans. Even though the incidence is believed to be very low in India, human tuberculosis caused by M. bovis has been increasingly recognized in many other countries of the world. As differentiation of mycobacterial species take long time, a method for the rapid identification of mycobacteria isolated from bovine samples to the species level was used, which is based on polymerase chain reaction (PCR) of the gene encoding for the 65-kD protein followed by restriction analysis. The method involves restriction enzyme analysis of PCR products obtained with primers common to all mycobacteria and generate M. tuberculosis complex specific pattern. PRA was performed on 33 bovine isolates of which 90.9% (30/33) isolates were identified clearly as M. tuberculosis complex, M. fortuitum, M. phlei and M. smegmatis using restriction enzyme Hae III.

Published
2006

219. Estimation of efflux mediated multi-drug resistance and its correlation with expression levels of two major efflux pumps in mycobacteria.

Author

Gupta AK, Chauhan DS, Srivastava K, Das R, Batra S, Mittal M, Goswami P, Singhal N, Sharma VD, Venkatesan K, Hasnain SE, and Katoch VM

Subjects
ATP-Binding Cassette Transporters genetics, ATP-Binding Cassette Transporters metabolism, Adenosine Triphosphatases genetics, Adenosine Triphosphatases metabolism, Bacterial Proteins genetics, Bacterial Proteins metabolism, Drug Resistance, Multiple, Bacterial genetics, Humans, Microbial Sensitivity Tests, Multidrug Resistance-Associated Proteins genetics, Multidrug Resistance-Associated Proteins metabolism, Mycobacterium phlei genetics, Mycobacterium phlei physiology, Mycobacterium tuberculosis genetics, Nontuberculous Mycobacteria genetics, Reverse Transcriptase Polymerase Chain Reaction, Tuberculosis, Multidrug-Resistant genetics, ATP-Binding Cassette Transporters drug effects, Adenosine Triphosphatases drug effects, Bacterial Proteins drug effects, Multidrug Resistance-Associated Proteins drug effects, Mycobacterium phlei drug effects, Mycobacterium tuberculosis drug effects, Nontuberculous Mycobacteria drug effects, Tuberculosis, Multidrug-Resistant metabolism
Abstract

Multidrug resistance has been posing an increasing problem in the treatment of tuberculosis. Mutations in the genomic targets of drugs have been identified as the major mechanism behind this resistance. However, high degree of resistance in some isolates towards major drugs like rifampicin, isoniazid, ethambutol and streptomycin can not be explained solely on the basis of mutations. Besides this, certain other mechanisms like efflux pumps have also been considered as alternative mechanisms in the drug resistant isolates where there is no mutation and these mechanisms are specially important for drug resistance in non-tuberculous mycobacteria (NTM). In this study, we have estimated efflux pump mediated drug resistance in different mycobacterial species with the help of efflux pump inhibitors. All major anti-tuberculous drugs have been shown to be extruded by efflux pumps and the degree to which these drugs are extruded, vary in different mycobacterial species and isolates. The correlation of this resistance with functional activity of two major efflux pump genes pstB and Rv1258c was also assessed by reverse transcription PCR. Besides the significant role of these pumps observed, other efflux pumps, present in mycobacteria, may also be involved in drug resistance and need to be investigated.

Published
2006

220. Simultaneous ethambutol & isoniazid resistance in clinical isolates of Mycobacterium tuberculosis.

Author

Gupta P, Jadaun GP, Das R, Gupta UD, Srivastava K, Chauhan A, Sharma VD, Chauhan DS, and Katoch VM

Subjects
Humans, Microbial Sensitivity Tests, Antitubercular Agents pharmacology, Drug Resistance, Multiple, Bacterial, Ethambutol pharmacology, Isoniazid pharmacology, Mycobacterium tuberculosis drug effects
Abstract

Background & Objective: There is a need to understand the nature of drug resistance patterns and predictors of emergence of drug resistance in Mycobacterium tuberculosis. There could be common factors/mechanisms for resistance to the drugs, isoniazid and ethambutol, both acting on cell wall. The present study was conducted to analyze the antimycobacterial susceptibility patterns of M. tuberculosis isolates to determine the minimum inhibitory concentrations (MICs) of ethambutol for M. tuberculosis; and to find out possible association of ethambutol resistance with isoniazid resistance., Methods: A total of 380 M. tuberculosis isolates were tested for their susceptibilities to ethambutol at 2, 4, 6 microg/ml, isoniazid at 1 microg/ml and rifampicin at 64 microg/ml using MIC method., Results: 44.21, 24.73 and 14.21 per cent isolates were resistant to ethambutol at concentrations of 2, 4 and 6 microg/ml respectively. At 6 microg/ml of ethambutol concentration, 85.18 per cent ethambutol resistant isolates were resistant to isoniazid also. At the same ethambutol concentration a fraction of 28.75 per cent isoniazid resistant isolates were ethambutol resistant., Interpretation & Conclusion: Ethambutol resistance was accompanied with isoniazid resistance in a large percentage of isolates whereas ethambutol resistance was weakly linked with multidrug resistance. On the other hand, association between isoniazid and ethambutol resistance was weak showing one way linkage.

Published
2006

221. Optical coherence tomography of intraocular lens implants and their relationship to the posterior capsule: a pilot study comparing a hydrophobic acrylic to a plate-haptic silicone type.

Author

Elgohary MA, Chauhan DS, and Dowler JG

Subjects
Aged, Female, Humans, Hydrophobic and Hydrophilic Interactions, Lens Implantation, Intraocular, Male, Middle Aged, Phacoemulsification, Pilot Projects, Prospective Studies, Prosthesis Design, Retrospective Studies, Acrylic Resins, Cataract diagnosis, Lens Capsule, Crystalline pathology, Lenses, Intraocular, Postoperative Complications diagnosis, Silicone Elastomers, Tomography, Optical Coherence
Abstract

Background: Optical coherence tomography (OCT) has been used to examine the anterior as well as the posterior segment and can be used to examine the intraocular lens (IOL) and their relationship to the posterior capsule in vivo., Objectives: To use OCT to examine two of the IOLs and some of the features related to the development of posterior capsular opacification (PCO)., Methods: This is a pilot study of a prospective (n = 12) and a retrospective (n = 14) series of patients who had uneventful phacoemulsification and IOL implantation of either hydrophobic acrylic (Acrysof; Alcon) or plate-haptic (PH) silicone (C11UB; Chiron, Bausch & Lomb) IOLs. The outcome of interest was the ability of OCT to clearly delineate the outline of the IOL optics and their appositional relationship to the posterior capsule., Results: OCT showed that hydrophobic acrylic IOLs had a better defined outline than PH silicone IOLs. It also showed close apposition between hydrophobic acrylic optics and the mid-peripheral part of the posterior capsule and the absence thereof with PH silicone IOLs., Conclusions: Hydrophobic acrylic implants have better definition on the OCT scans than PH silicone and they develop close apposition to the posterior capsule. The latter feature is consistent with the 'no space, no cell, no PCO' concept and what is known about the effect of the implant material and design on the rate of PCO., (Copyright (c) 2006 S. Karger AG, Basel.)

Published
2006
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222. Direct detection and identification of Mycobacterium tuberculosis and Mycobacterium bovis in bovine samples by a novel nested PCR assay: correlation with conventional techniques.

Author

Mishra A, Singhal A, Chauhan DS, Katoch VM, Srivastava K, Thakral SS, Bharadwaj SS, Sreenivas V, and Prasad HK

Subjects
Animals, Base Sequence, Cattle, DNA Primers, Genes, Bacterial, Molecular Sequence Data, Mycobacterium bovis genetics, Mycobacterium tuberculosis genetics, Sensitivity and Specificity, Sequence Alignment, Species Specificity, Tuberculosis diagnosis, Cattle Diseases diagnosis, Mycobacterium bovis isolation & purification, Mycobacterium tuberculosis isolation & purification, Polymerase Chain Reaction methods, Tuberculosis veterinary, Tuberculosis, Bovine diagnosis
Abstract

Mycobacterium tuberculosis and M. bovis infect animals and humans. Their epidemiology in developed and developing countries differs, owing to differences in the implementation of preventive measures (World Health Organization, 1999). Identification and differentiation of these closely related mycobacterial species would help to determine the source, reservoirs of infection, and disease burden due to diverse mycobacterial pathogens. The utility of the hupB gene (Rv2986c in M. tuberculosis, or Mb3010c in M. bovis) to differentiate M. tuberculosis and M. bovis was evaluated by a PCR-restriction fragment length polymorphism (RFLP) assay with 56 characterized bovine isolates. The degree of concordance between the PCR-RFLP assay and the microbiological characterization was 99.0% (P < 0.001). A nested PCR (N-PCR) assay was developed, replacing the PCR-RFLP assay for direct detection of M. tuberculosis and M. bovis in bovine samples. The N-PCR products of M. tuberculosis and M. bovis corresponded to 116 and 89 bp, respectively. The detection limit of mycobacterial DNA by N-PCR was 50 fg, equivalent to five tubercle bacilli. M. tuberculosis and/or M. bovis was detected in 55.5% (105/189) of the samples by N-PCR, compared to 9.4% (18/189) by culture. The sensitivities of N-PCR and culture were 97.3 and 29.7, respectively, and their specificities were 22.2 and 77.7%, respectively. The percentages of animals or samples identified as infected with M. tuberculosis or M. bovis by N-PCR and culture reflected the clinical categorizations of the cattle (P of <0.05 to <0.01). Mixed infection by N-PCR was detected in 22 animals, whereas by culture mixed infection was detected in 1 animal.

Published
2005
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224. DNA fingerprinting of Mycobacterium tuberculosis isolates from Agra region by IS 6110 probe.

Author

Chauhan A, Chauhan DS, Parashar D, Gupta P, Sharma VD, Sachan AS, Gupta R, Agarawal BM, and Katoch VM

Abstract

DNA fingerprinting using IS 6110 probe has been used all over the world quite successfully to characterize M. tuberculosis strains. The present study has been carried out to study the polymorphism among isolates of M. tuberculosis from Agra region from patients attending the clinics at SN Medical College and TBDTC, Agra. Sputa were collected in sterilized containers and brought to CJIL, Agra. Samples were processed and cultured on Lowenstein Jensen (LJ) slants. M. tuberculosis isolates were identified by standard biochemical tests. DNA from these isolates were purified by a physicochemical procedure, restricted with Pvu II enzyme and hybridized with PCR amplified and DIG labeled 245 bp IS 6110 probe. With a view to study IS 6110 polymorphism, M. tuberculosis isolates obtained from different geographical areas of Agra region were analyzed. Among the 60 isolates taken in study, 5 had no copy of IS 6110, 8 had 1-4 copies and 47 had multiple copies of IS 6110. DNA fingerprinting using this probe was found to be quite discriminating for typing of most of the strains (80%) which had multiple copies. RFLP profiles did not correlate with geographical areas, contacts or the resistance pattern of the strains. While this data shows the potential of IS 6110 based RFLP for strain characterization of M. tuberculosis in Agra, to understand the molecular epidemiology of tuberculosis in this region, a larger number of isolates from defined geographical areas need to be studied.

Published
2004

225. Correlation of mutations detected by INNO-LiPA with levels of rifampicin resistance in Mycobacterium tuberculosis.

Author

Srivastava K, Das R, Jakhmola P, Gupta P, Chauhan DS, Sharma VD, Singh HB, Sachan AS, and Katoch VM

Subjects
Humans, India, Mutation, Mycobacterium tuberculosis genetics, Mycobacterium tuberculosis physiology, Statistics as Topic, Antibiotics, Antitubercular pharmacology, DNA-Directed RNA Polymerases genetics, Drug Resistance, Bacterial physiology, Microbial Sensitivity Tests, Mycobacterium tuberculosis drug effects, Rifampin pharmacology
Abstract

Background & Objectives: Due to emergence of drug resistance in Mycobacterium tuberculosis, there is a need to have accurate and rapid methods for detection of drug resistance to important drugs like rifampicin. The present study was aimed at evaluation of a commercially available INNO-LiPA assay, for the detection of mutation in rpoB gene region of M. tuberculosis and correlate these mutations with levels of rifampicin resistance for assessing their clinical relevance., Methods: Fifty five well-characterized isolates of M. tuberculosis deposited from various regions of India in Mycobacterial Repository Centre at the CJILOMD, Agra were subjected to susceptibility testing for rifampicin at various concentrations of drug viz., 10, 40, 64, 128 microg/ml on Lowenstein- Jensen (LJ) medium. rpoB gene fragment (260 bp) was amplified using Rif-TB amplification kit and after hybridization, detection was done by using INNO-LiPA Rif TB kit., Results: The rpoB gene could be amplified from DNA extracted from all the 55 culture isolates and showed clear hybridization pattern with M. tuberculosis complex specific probes on LiPA strips. Mutations detected were correlated with degree of rifampicin resistance. All the sensitive isolates (identified by MIC) were identified as rifampicin sensitive (100%) by INNO-LiPA as they exhibit positive for wild type 'S' probes and negative for 'R' probes. Two of the 5 isolates, resistant at 10 microg/ml and 40 microg/ml had either D516V, H526Y mutations or unknown mutations. Thirty (85.71%) isolates resistant at clinically relevant levels (64,128microg/ml) exhibited double, triple or more 'R' type mutations (R(2(D516V)), R(4a(H526Y)), R(4b(H526D)), R(5(S531L))) as well as unknown mutations present at 'S' probes region whereas remaining isolates did not show any mutation by this method. This method could identify with definitiveness 60 per cent ( 21/35) isolates as rifampicin resistant as mutations observed in others were also present in isolates with low levels of resistance., Interpretation & Conclusion: The results indicate that INNO-LiPA Rif TB test is a rapid and easy to use method for detection of mutations associated with rifampicin resistance in M. tuberculosis. However, as some of these mutations are also present in isolates with low degree of resistance which are still microbiologically sensitive to rifampicin, there is a need to improve this assay by exclusion of some of the current probes and inclusion of more probes.

Published
2004

226. A preliminary report on characterization and identification of non tuberculous mycobacteria (NTM) on the basis of biochemical tests and protein / isoenzyme electrophoretic patterns.

Author

Gupta P, Katoch VM, Gupta UD, Chauhan DS, Das R, Singh D, Srivastava K, Singh HB, and Sharma VD

Abstract

Purpose: To assess the usefulness of protein electrophorograms and protein zymodemes in the identification and characterization of non tuberculous mycobacteria (NTM)., Methods: Cell free extracts (CFEs) from 22 mycobacterial isolates belonging to slow growing and other clinically relevant species were included in the study. The strains isolated from the environment were identified on the basis of their standard biochemical tests; pigmentation and growth characters. The CFEs were electrophoresed and stained for proteins and esterases., Results: Most of the isolates identified on the basis of biochemical tests exhibited characteristic protein and esterase pattern for M. scrofulaceum, M. avium and M. xenopi. Others showed variations in their proteins and esterase pattern though they were identified as M. scrofulaceum, M. avium and M. xenopi., Conclusions: Based on these studies it appears that because of variability in the protein and isoenzyme patterns of NTM, it may be advisable to use them along with biochemical tests and other tests for identifying and characterizing the different mycobacterial species belonging to slow growers.

Published
2002

227. Drug susceptibility profiles of Mycobacterium tuberculosis isolates at Jaipur.

Author

Malhotra B, Pathak S, Vyas L, Katoch VM, Srivastava K, Chauhan DS, Singh D, Sharma VD, Das R, and Singh HB

Abstract

Purpose: To find prevalence of drug resistance in Mycobacterium tuberculosis isolated from patients attending SMS Medical College, Jaipur during 1997-99., Methods: Sputum samples from 164 patients with pulmonary tuberculosis were processed and cultured on Lowenstein Jensen medium and M. tuberculosis isolates were tested for drug sensitivity., Results: M. tuberculosis was isolated in 122/164 (74.3%) samples and comprised 97.6% (122/125) of mycobacterial isolates. There were only three isolates of nontuberculous mycobacteria -one each of M. kansasii, M. avium and M. fortutium. Primary drug resistance in M. tuberculosis was estimated to be 3/44 (6.8%) to rifampicin, 6/44 (13.6%) to isoniazid and 2 strains (4.5%) were multi drug resistant i.e. resistant to both rifampicin and isoniazid. Among the isolates from cases with previous history of treatment of varying duration (acquired drug resistance) resistance to rifampicin was estimated to be 28.2% and for isoniazid to be 39.7%. 24.3% strains of these drug resistant isolates were multi drug resistant., Conclusions: While this information may not reflect true prevalence of drug resistance in the region this may help in further planning long term surveillance studies to know the trend of drug resistance in this area.

Published
2002

228. Rapid discrimination of Indian isolates of M. tuberculosis by random amplified polymorphic DNA (RAPD) analysis - a preliminary report.

Author

Singh HB, Chauhan DS, Singh D, Das R, Srivastava K, Yadav VS, Kumar A, Katoch VM, and Sharma VD

Abstract

Purpose: Due to relatively complex nature of molecular typing systems for M. tuberculosis as well as lack of applicability of some of the probes, there is a need for alternate procedures for molecular epidemiology. In this study the usefulness of RAPD analysis for typing of Indian strains of M.tuberculosis was investigated., Methods: One hundred and three coded isolates from different parts of the country were analysed by Random amplified polymorphic DNA (RAPD) technique. Purified and amplified DNA from cultures were analysed by ethidium bromide staining after electrophoresis. The bands were confirmed by densitometry and the patterns were analysed by hierarchical cluster analysis., Results: The patterns elicited by the analysis appeared to be quite discriminatory and characteristic., Conclusions: Clustering observed among isolates attending the same hospital indicates future application potential of RAPD analysis for molecular epidemiology of tuberculosis in India.

Published
2002

229. Analysis of quantitative relationship between viability determination in leprosy by MFP, ATP bioluminescence and gene amplification assay.

Author

Gupta UD, Katoch K, Sharma RK, Singh HB, Natragan M, Singh D, Sharma VD, Chauhan DS, Das R, Srivastava K, and Katoch VM

Subjects
Animals, Bacterial Proteins genetics, Humans, Immunotherapy methods, Leprostatic Agents therapeutic use, Leprosy microbiology, Luminescent Measurements, Mice, Mice, Inbred BALB C, Mycobacterium leprae drug effects, Polymerase Chain Reaction, Time Factors, Treatment Outcome, Adenosine Triphosphate metabolism, Foot microbiology, Leprosy drug therapy, Mycobacterium leprae growth & development, Nucleic Acid Amplification Techniques
Abstract

Two hundred twenty-one untreated, borderline lepromatous/lepromatous (BL/LL) leprosy patients have been investigated for viability by the mouse foot pad method (MFP), adenosine triphosphate (ATP) and polymerase chain reaction (PCR). The biopsies were collected at the beginning of and 12/24 months after treatment. The patient group was treated with a) immunotherapy (BCG/Mw) + MDT; b) MDT + pyrazinamide; c) control MDT; d) MDT + minocycline 100 mg once a month supervised + ofloxacin 400 mg once a month supervised. Biopsies were divided in three parts for use in the mouse foot pad, molecular and ATP investigations. In untreated and treated patients (at 12 and 24 months), there was a general agreement among all three techniques, and PCR and ATP showed higher positivity as compared to MFP. Further, there was good correlation among the viable biomass estimated by bacillary ATP levels, PCR assay and growth in mouse foot pads. The positivity was observed by MFP as well as PCR assay (18-kDa and 36-kDa) from all of the specimens when the ATP content was more than 3.6 pg/million. When the ATP content was below 3.5 pg/million, the positive takes in MFP decreased but the PCR positivity correlated with ATP bioluminescence up to 0.04 pg/million. When the ATP content was even lower, the uptake in the MFP was possibly a matter of chance, while PCR positivity was observed in 96% of the cases. For specimens with undetectable ATP, positivity was seen in 1% of the cases, showing the inability of ATP bioluminescence method to detect low background due to host ATP. PCR signals in some cases could be due to the higher sensitivity of the method or persistence of DNA after bacterial death in some cases. On the whole, the PCR methods even though targeting DNA have shown good correlations with biomass which confirm their usefulness in monitoring therapeutic responses in leprosy.

Published
2001

230. Typing of drug resistant isolates of Mycobacterium tuberculosis from India using the IS6110 element reveals substantive polymorphism.

Author

Siddiqi N, Shamim M, Amin A, Chauhan DS, Das R, Srivastava K, Singh D, Sharma VD, Katoch VM, Sharma SK, Hanief M, and Hasnain SE

Subjects
DNA Fingerprinting, Evolution, Molecular, Humans, India, Mycobacterium tuberculosis drug effects, Phenotype, Phylogeny, Polymorphism, Restriction Fragment Length, Antitubercular Agents pharmacology, DNA Transposable Elements genetics, Drug Resistance, Multiple, Bacterial genetics, Mycobacterium tuberculosis classification, Mycobacterium tuberculosis genetics, Polymorphism, Genetic genetics, Tuberculosis microbiology
Abstract

We investigated IS6110 polymorphism in clinical isolates of Mycobacterium tuberculosis from patients attending the outpatient department at various hospitals in northern India. DNA fingerprinting of 126 clinical isolates of M. tuberculosis was carried out using restriction fragment length polymorphism (RFLP) associated with the IS6110 element in M. tuberculosis genomes. A substantive degree of polymorphism was evident in the MDR M. tuberculosis isolates. The number of bands in the fingerprints varied from 0 to 19. However, the lack of common bands made it difficult to cluster the majority of these isolates. We were also unable to associate drug resistance with IS6110 copy number. Specific regions of the gyrA and katG genes from a representative number of these isolates were sequenced to determine the genotype. The majority of the isolates analyzed were found to belong to Group 1, indicating that these strains were evolutionarily older. We find no evidence of the W strain, prevalent in the US, in our study. The epidemiological patterns of the various strains in India seem to be very complex, as reflected by the presence of a large number of different strains (types) within north India.

Published
2001
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231. Optical coherence tomography of the vitreoretinal interface in macular hole formation.

Author

Tanner V, Chauhan DS, Jackson TL, and Williamson TH

Subjects
Aged, Aged, 80 and over, Female, Fovea Centralis pathology, Humans, Male, Middle Aged, Prospective Studies, Retinal Perforations etiology, Retinal Perforations physiopathology, Visual Acuity, Retinal Perforations pathology, Tomography, Vitreous Body pathology
Abstract

Aims: To image the vitreoretinal interface and provide further information on the pathogenesis of idiopathic macular hole formation., Methods: Prospective recruitment of 80 eyes of 41 consecutive patients referred with a diagnosis of idiopathic full thickness macular hole (FTMH) to a teaching hospital retinal clinic. Both eyes of each patient underwent optical coherence tomography (OCT) imaging with vertical and horizontal scans centred on the fovea., Results: A total of 30 eyes had stage 2 or 3 FTMHs and, of these, 21 had persistent vitreofoveal attachment and associated prefoveal opacities. 18 prefoveal opacities were identified by Goldmann contact lens examination and confirmed on OCT examination. Three prefoveal opacities were identified only on OCT examination. 10 eyes had stage 4 FTMHs and four cases were identified in whom the OCT appearance was consistent with impending, aborted, or lamellar macular holes., Conclusions: The wide range in OCT appearance of macular holes and associated prefoveal opacities suggests that, in at least some cases, a significant amount of retinal tissue is torn from the foveal area during macular hole formation. OCT imaging provides additional information on macular hole pathogenesis and is valuable in the planning of surgical intervention.

Published
2001
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232. Comparison between optical coherence tomography and fundus fluorescein angiography for the detection of cystoid macular edema in patients with uveitis.

Author

Antcliff RJ, Stanford MR, Chauhan DS, Graham EM, Spalton DJ, Shilling JS, Ffytche TJ, and Marshall J

Subjects
Exudates and Transudates, Humans, Interferometry, Light, Prospective Studies, Fluorescein Angiography methods, Fundus Oculi, Macular Edema diagnosis, Tomography methods, Uveitis complications
Abstract

Purpose: To compare optical coherence tomography (OCT) with fundus fluorescein angiography (FFA) for the detection of cystoid macular edema (CME) in patients with uveitis., Design: Prospective comparative observational series., Participants: One hundred twenty-one eyes of 58 patients with uveitis of varied causes (seven patients were studied twice)., Testing: Patients with suspected CME underwent OCT scanning followed by FFA at the same visit., Main Outcome Measures: Detection and distribution of macular edema., Results: One hundred eight eyes had similar results on both OCT and FFA in that 67 eyes had CME and 41 eyes had no CME. In 10 eyes subretinal fluid was detected on OCT but not FFA. Five of these eyes had CME on FFA but not OCT. Three other eyes had CME that was detected by FFA but not by OCT. Compared with FFA, the OCT sensitivity for detecting CME was 96% (including the eyes with subretinal fluid), and the OCT specificity was 100%., Conclusions: OCT is as effective at detecting CME as is FFA but is superior in demonstrating axial distribution of fluid.

Published
2000
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233. Papillofoveal traction in macular hole formation: the role of optical coherence tomography.

Author

Chauhan DS, Antcliff RJ, Rai PA, Williamson TH, and Marshall J

Subjects
Humans, Middle Aged, Retinal Perforations diagnosis, Saccades, Tissue Adhesions, Vitreous Detachment diagnosis, Fovea Centralis pathology, Optic Disk pathology, Retinal Perforations etiology, Tomography methods, Vitreous Detachment complications
Abstract

Objectives: To determine the validity of the assumption that optical coherence tomographic scans of macular holes have a discrete linear signal (DLS) that represents a detached posterior vitreous face, and to analyze the DLS in macular hole pathogenesis., Methods: Optical coherence tomographic scans were taken of 3 situations in which the vitreous conditions were known: (1) dissected intact vitreous, (2) clinically evident Weiss rings, and (3) maculae before and after saccades in eyes without a biomicroscopic posterior vitreous detachment. In addition, 70 eyes of 35 patients with macular holes underwent clinical examination and optical coherence tomographic scanning that passed through the optic disc and the fovea or macular hole., Results: Spatial properties of the DLS matched those of the posterior vitreous face in the situations examined. Of the 70 eyes, 16 (23%) had a biomicroscopic posterior vitreous detachment, whereas a DLS was demonstrated in 40 (57%). Of the 54 eyes without a biomicroscopic posterior vitreous detachment, 18 (33%) had a DLS attached focally to the optic disc margin and the fovea or macular hole. All 7 of the "can opener" holes examined had a nasally "hinged" central flap, 6 with a focally attached DLS., Conclusions: The DLS corresponds to the posterior vitreous face. Anteronasal papillofoveal traction may generate some macular holes.

Published
2000
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234. The interpretation of optical coherence tomography images of the retina.

Author

Chauhan DS and Marshall J

Subjects
Adult, Aged, Animals, Cattle, Cockayne Syndrome surgery, Humans, Laser Coagulation, Middle Aged, Nerve Fibers pathology, Retina cytology, Retina surgery, Retinitis Pigmentosa surgery, Cockayne Syndrome pathology, Retina pathology, Retinitis Pigmentosa pathology, Tomography methods
Abstract

Purpose: To determine the relationship between optical coherence tomography (OCT) images of the retina and retinal substructure in vitro and in vivo., Methods: In vitro, OCT images of human and bovine retina were acquired after sequential excimer laser ablation of the inner retinal layers. Measurements of bands in the OCT images were compared with measurements of retinal layers on histology of the ablated specimens. In vivo, OCT images were acquired of retinal lesions in which there was a displacement of pigmented retinal pigment epithelial (RPE) cells: retinitis pigmentosa and laser photocoagulation (eight eyes each)., Results: The mean thickness of human inner OCT bands (131 microm; 95% confidence interval [CI], 122-140 microm) was 7.3 times that of the retinal nerve fiber layer (RNFL). This band persisted despite ablation greater than 140 microm. The inner aspect of the outer OCT band corresponded to the apical RPE, but the mean thickness of this band in human tissue (55 microm; 95% CI, 48-62 microm) was 2.6 times the thickness of the RPE-choriocapillaris complex. OCT measurement of total retinal thickness was accurate (coefficient of variance, 0.05) and precise (coefficient of correlation with light microscopy, 0.98). Hyperpigmented lesions gave rise to high signal, attenuating deeper signal; hypopigmented lesions had the opposite effect on deeper signal., Conclusions: The inner band is not RNFL specific, partly consisting of a surface-related signal. The location, not thickness, of the outer band corresponds to RPE melanin. Given the additional effect of polarization settings, precise OCT measurement of specific retinal layers is currently precluded.

Published
1999

235. Effect of treatment on PCR positivity in multibacillary leprosy patients treated with conventional and newer drugs ofloxacin and minocycline.

Author

Singh HB, Katoch K, Natrajan M, Sharma RK, Gupta UD, Sharma VD, Singh D, Chauhan DS, Srivastava K, and Katoch VM

Subjects
Adenosine Triphosphate analysis, Biopsy, Clofazimine therapeutic use, Dapsone therapeutic use, Drug Evaluation, Humans, Leprosy microbiology, Mycobacterium leprae genetics, Polymerase Chain Reaction, Rifampin administration & dosage, Rifampin therapeutic use, Sensitivity and Specificity, Treatment Outcome, DNA, Bacterial analysis, Drug Therapy, Combination therapeutic use, Leprostatic Agents therapeutic use, Leprosy drug therapy, Minocycline therapeutic use, Mycobacterium leprae isolation & purification, Ofloxacin therapeutic use
Abstract

In order to develop objective criteria to monitor trends of therapeutic responses positivity of PCR signals and ATP assay methods has been compared in multibacillary (MB) leprosy patients. Biopsies from lesions of 95 BL/LL patients before and after one year of treatment with a new drug regimen comprising of conventional and newer drugs ofloxacin and minocycline have been studied. These biopsies were processed for bacillary ATP assay and PCR positivity for a 36 kDa gene target by earlier published methods. In the untreated patients bacillary ATP levels were detectable in all specimens and ranged from 0.02 to more than 36 pg/millions organisms. After one year of treatment ATP levels were not detectable in any of the 57 biopsies specimens available for analysis. However, PCR signals were detectable in 3 out of 57 biopsies. In two specimens signals were very weak detectable only by hybridization. It may be concluded that DNA based PCR assay may be useful in monitoring the trends of therapeutic responses in MB patients under treatment.

Published
1999

236. Pulmonary hypertension and diffuse macular edema responsive to acetazolamide.

Author

Hammond CJ, Chauhan DS, and Stanford MS

Subjects
Adult, Blood Pressure, Edema etiology, Edema pathology, Female, Fluorescein Angiography, Fundus Oculi, Humans, Hypertension, Pulmonary complications, Intraocular Pressure, Retinal Detachment drug therapy, Retinal Detachment etiology, Retinal Detachment pathology, Retinal Diseases etiology, Retinal Diseases pathology, Tomography, Uveal Diseases drug therapy, Uveal Diseases etiology, Uveal Diseases pathology, Acetazolamide therapeutic use, Edema drug therapy, Hypertension, Pulmonary drug therapy, Macula Lutea pathology, Retinal Diseases drug therapy
Published
1998

237. Trichophytobezoars in a neonatal calf.

Author

Kumar A, Tanwar RK, Gahlot TK, and Chauhan DS

Subjects
Animals, Bezoars diagnostic imaging, Male, Radiography, Bezoars veterinary, Cattle, Reticulum, Rumen
Published
1982

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