Your search keyword '"H. V. Batra"' showing total 13 results

1. Functional characterization of a broad and potent neutralizing monoclonal antibody directed against outer membrane protein (OMP) of Salmonella typhimurium

Author

Urmil Tuteja, Rohini Krishna Kota, Radhika Madam Urs, Shivakiran Makam, Prakash Narayana Reddy, Gyati Yatung, and H. V. Batra

Subjects

Monoclonal antibody, Salmonella typhimurium, Salmonella, Cross Reactions, medicine.disease_cause, Applied Microbiology and Biotechnology, Bacterial Adhesion, Epitope, Microbiology, Mice, 03 medical and health sciences, Enterobacteriaceae, Antigen, parasitic diseases, Escherichia coli, medicine, Animals, Humans, Bactericidal assay, Neutralizing antibody, 030304 developmental biology, Antigens, Bacterial, Mice, Inbred BALB C, 0303 health sciences, biology, 030306 microbiology, Chemistry, Cross-reactivity, Antibodies, Monoclonal, Complement System Proteins, General Medicine, biology.organism_classification, Antibodies, Neutralizing, Proteus mirabilis, Applied Microbial and Cell Physiology, Bacteriostatic, A549 Cells, biology.protein, Female, Bacterial outer membrane, Bacterial Outer Membrane Proteins, Biotechnology

Abstract

In the present study, we have generated a murine monoclonal antibody (mAb) named Sal-06 by using the crude outer membrane protein preparation of Salmonella enteric subsp. enterica serovar Typhimurium ATCC 14028 strain as antigen. Sal-06mAb belonging to IgG1 isotype demonstrated broad cross-reactivity to standard and isolated strains of genus Salmonella and others such as Escherichia coli, Klebsiella pneumonia, and Proteus mirabilis. Cross-reactivity across several bacterial genera indicated that the epitopes reactive to Sal-06mAb are conserved among these members. Neutralizing effects of Sal-06mAb on Salmonella growth and survival was evaluated in vitro using bacteriostatic and bactericidal activity with and without complement and bacterial invasion inhibition assay. Sal-06mAb demonstrated a bacteriostatic effect on the growth of S. typhimurium ATCC 14028 strain which is both time and concentration (of mAb) dependent. It was also found that the bacterial growth inhibition was complement independent. When the bacterial cells were preincubated with Sal-06mAb, it reduced the adherence and invasion of bacterial cells into A549 epithelial cell line. This was confirmed by CFU count analysis, phase contrast, and fluorescence microscopy. Scanning electron microscope (SEM) imaging confirmed the antimicrobial effects of Sal-06mAb on S. typhimurium ATCC 14028. The development of broadly reactive and cross protective Sal-06mAb opens new possibilities for immunotherapy of sepsis caused by Gram-negative Enterobacteriaceae members.

Published

2020

2. Nisin based stabilization of novel fruit and vegetable functional juices containing bacterial cellulose at ambient temperature

Author

Manoranjan Kumar, A. Jagannath, P. S. Raju, and H. V. Batra

Subjects

Microbial cellulose, chemistry.chemical_classification, Short Communication, Beetroot Juice, Sensory analysis, Lycopene, chemistry.chemical_compound, chemistry, Bacterial cellulose, Food science, Carotenoid, Nisin, Food Science, Betanin

Abstract

The current study reports the preparation and stabilization of novel functional drinks based on fruit and vegetable juices incorporating bacterial cellulose from Acetobacter xylinum. Pineapple, musk melon, carrot, tomato, beet root and a blend juice containing 20 % each of carrot and tomato juice with 60 % beet root juice has been studied. These juices have been stabilized over a storage period of 90 days at 28 °C, by the use of nisin and maintaining a low pH circumventing the need for any chemical preservatives or refrigeration. Instrumental color values have been correlated with the pigment concentrations present in the fresh as well as stored juices. There was 36, 72 and 60 % loss of total carotenoids in the case of carrot, pineapple and musk melon juices respectively while the lycopene content remained unchanged after 90 days of storage. The betanin content decreased 37 % in the case of beetroot juice and 25 % in the case of beetroot juice blended with carrot and tomato juices. Sensory analysis has revealed a clear preference for the beetroot blended mixed juice.

Published

2014

3. Development and evaluation of a multiplex PCR assay for simultaneous detection of major mycotoxigenic fungi from cereals

Author

K. Balakrishna, H. V. Batra, M. Venkataramana, S. R. Priyanka, and H. S. Murali

Subjects

Fusarium, Ochratoxin A, Aflatoxin, biology, Trichothecene, food and beverages, biology.organism_classification, Microbiology, chemistry.chemical_compound, chemistry, Multiplex polymerase chain reaction, Fumonisin, Mycotoxin, Zearalenone, Food Science

Abstract

The aim of the present study was to develop a multiplex PCR (mPCR) assay for the simultaneous detection of five major metabolic pathway genes viz. aflr (Aflatoxin), pks (Ochratoxin A), tri5 (Trichothecene), pks13 (Zearalenone) and fum13 (Fumonisin), producing Aspergillus, Penicillium and Fusarium species. The mPCR assay with competitive internal amplification control to eliminate false negative results employing specific primers for each of the above mentioned five genes was optimized and validated using standard strains. The standardized mPCR assay detected all five major mycotoxin metabolic genes along with artificially inoculated maize seeds with mycotoxigenic Fusarium, Penicillium and Aspergillus spores. The detection limit of this mPCR assay was 1 × 103 spores per gram of artificially inoculated samples upon 48 h of incubation at room temperature. When the developed mPCR assay was applied on to 177 contaminated maize, paddy and sorghum, many of the samples (100 out of 177) were contaminated with either one or more mycotoxins. The mPCR results were further evaluated with high performance liquid chromatography and in general both the methods provided unequivocal results. The developed mPCR based assay was found to be rapid, cost effective and user friendly and can be used for diagnosis of major mycotoxigenic fungi.

Published

2013

4. Detection of toxigenic strains of Aeromonas species in foods by a multiplex PCR assay

Author

H. V. Batra, H.S. Murali, and K. Balakrishna

Subjects

biology, Aerolysin, biology.organism_classification, 16S ribosomal RNA, Microbiology, law.invention, Aeromonas hydrophila, Aeromonas, law, Ampicillin, Multiplex polymerase chain reaction, medicine, Original Article, Polymerase chain reaction, Food contaminant, medicine.drug

Abstract

Aeromonas hydrophila and other aeromonads are ubiquitous organisms found in meat, vegetables, drinking water and various other food items. They cause diarrhea and extra-intestinal infections in normal and immunocompromised patients. The aim of the study was to develop a multiplex PCR assay for the detection of virulence-associated genes of Aeromonas including hemolysin (hlyA), aerolysin (aerA), glycerophospholipid-cholesterol acyl transferase (GCAT) alongwith a 16S rRNA gene. Internal amplification control (IAC), which was coamplified with aerA primers, was also included in this study. The results showed that all cultures of Aeromonas were accurately identified by the assay without showing non-specificity. A. hydrophila could be detected at a range of 10-50 CFU ml(-1) from experimentally spiked fish, chicken and milk samples following overnight enrichment in alkaline peptone water supplemented with 10 μg/ml ampicillin (APW-A) by this multiplex PCR (mPCR). When evaluated on a total of 74 naturally occurring food samples, four samples were identified to contain Aeromonas by mPCR. All these results were compared to the conventional culture, isolation and biochemical identification procedures. The high throughput and cost-effective mPCR method developed in this study could provide a powerful tool for detection of pathogenic Aeromonas spp. from food and environmental samples and in addition, the method has advantages in terms of specificity, sensitivity and ease of use compared to other reported PCR methods and DNA hybridization assays.

Published

2010

5. Molecular characterization of lactic acid bacteria recovered from natural fermentation of beet root and carrot Kanji

Author

H.S. Murali, P. T. Roshini, Joseph J. Kingston, H. V. Batra, M. Radhika, and M. A. Raksha

Subjects

food and beverages, Biology, biology.organism_classification, 16S ribosomal RNA, Microbiology, Amplified Ribosomal DNA Restriction Analysis, DNA profiling, Genotype, Original Article, Fermentation, Fermentation in food processing, Genotyping, Bacteria

Abstract

The lactic acid bacteria (LAB) play an important role in the fermentation of vegetables to improve nutritive value, palatability, acceptability, microbial quality and shelf life of the fermented produce. The LAB associated with beetroot and carrot fermentation were identified and characterized using different molecular tools. Amplified ribosomal DNA restriction analysis (ARDRA) provided similar DNA profile for the 16 LAB strains isolated from beetroot and carrot fermentation while repetitive extragenic palindromic PCR (rep-PCR) genotyping could differentiate the LAB strains into eight genotypes. Thirteen strains represented by five genotypes could be clustered in five distinct groups while three LAB strains exhibiting distinct genotypes remained ungrouped. These genotypes could be identified to be belonging to L. plantarum group by 16S rDNA sequencing. The recAnested multiplex PCR employing species-specific primers for the L. plantarum group members identified the LAB strains of six genotypes to be L. paraplantarum and the other two genotypes to be L. pentosus. Three genotypes of L. paraplantarum were consistently found on the third and sixth day of beetroot fermentation whereas a distinct genotype of L. paraplantarum and L. pentosus appeared predominant on the tenth day. From carrot Kanji two distinct genotypes of L. paraplantarum and one genotype of L. pentosus were identified. REP-PCR DNA fingerprinting coupled with 16S rDNA sequencing and recA-nested multiplex PCR could clearly identify as well as differentiate the diverse L. plantarum group strains involved in the fermentation.

Published

2010

6. Multiplex PCR assay for the detection of enterotoxic Bacillus cereus group strains and its application in food matrices

Author

H. V. Batra, T. D. Kalyan Kumar, and H.S. Murali

Subjects

biology, Toxin, Bacillus cereus, biology.organism_classification, medicine.disease_cause, Microbiology, law.invention, Bacillus anthracis, Plasmid, Cereus, law, Bacillus thuringiensis, Multiplex polymerase chain reaction, medicine, Original Article, Polymerase chain reaction

Abstract

Bacillus cereus, Bacillus thuringiensis and Bacillus anthracis are the major concerns for the food safety in terms of frequency and/or seriousness of the disease. Being members of the same group and sharing DNA homology to a larger extent, they do create problems when their specific detection/identification is attempted from different food and environmental sources. Numerous individual polymerase chain reaction (PCR) and few multiplex PCR (mPCR) methods have been employed to detect these organisms by targeting toxin genes but with lack of internal amplification control (IAC). Therefore, we attempted a mPCR with IAC for the detection of enterotoxic B. cereus group strains by selecting hbl A, nhe A and cyt K genes from B. cereus, indicative of the diarrheal potential and cry I A and pag genes, the plasmid borne phenotypic markers specific to B. thuringiensis and B. anthracis strains, respectively. Multiplex PCR assay validation was performed by simultaneous comparison with the results of single-target PCR assays and correlated to the classical conventional and biochemical identification of the organisms. The mPCR was able to detect as low as 10(1)-10(2) organisms per ml following overnight enrichment of spiked food samples (vegetable biriyani and milk) in buffered peptone water (BPW). The presence of these organisms could also be detected by mPCR in naturally contaminated samples of rice based dishes and milk. The high throughput and cost-effective mPCR method described could provide a powerful tool for simultaneous, rapid and reliable detection of enterotoxic B. cereus group organisms.

Published

2010

7. Simultaneous detection of pathogenic B. cereus, S. aureus and L. monocytogenes by multiplex PCR

Author

T. D. Kalyan Kumar, H. V. Batra, and H.S. Murali

Subjects

Food poisoning, biology, business.industry, Bacillus cereus, Virulence, biology.organism_classification, Food safety, medicine.disease, medicine.disease_cause, Microbiology, Cereus, Listeria monocytogenes, Staphylococcus aureus, Multiplex polymerase chain reaction, medicine, Original Article, business

Abstract

Three important foodborne pathogens, Bacillus cereus, Listeria monocytogenes and Staphylococcus aureus are of major concern for food safety in terms of frequency and seriousness of the disease. The occurrence these three important pathogens and their coexistence in food matrices are predominant. Moreover, symptoms associated with B. cereus and S. aureus food poisoning not only closely resembles each other but can also be overlapping with other foodborne infections. In this context, detection of these three pathogens simultaneously in food samples by a single multiplex PCR (mPCR) would have advantages in terms of rapidity and cost saving, when compared with single organism specific PCRs. mPCR has been standardized by targeting three major diarrheal enterotoxin genes hbl A, cyt K and nhe A of B. cereus, virulence associated nuc and Ent B genes of S. aureus and virulence associated hly and iap genes of L. monocytogenes along with internal amplification control (IAC). The results showed that mPCR accurately identified all the three organisms individually or in combination without non-specificity. The mPCR was able to detect as low as 10 to 100 organisms per ml of growth following overnight enrichment of spiked food samples (vegetable biriyani and milk) and their presence in naturally contaminated samples also. The high throughput and cost effective multiplex PCR method developed in this study could provide a powerful tool for simultaneous, rapid and reliable detection of B. cereus, S. aureus and L. monocytogenes in food samples.

Published

2009

8. Detection of Salmonella enterica serovar Typhimurium by selective amplification of fliC, fljB, iroB, invA, rfbJ, STM2755, STM4497 genes by polymerase chain reaction in a monoplex and multiplex format

Author

M. Radhika, H. V. Batra, Mahesh Shanmugasundaram, and H.S. Murali

Subjects

Serotype, Salmonella, biology, Physiology, General Medicine, biology.organism_classification, medicine.disease_cause, Applied Microbiology and Biotechnology, Enterobacteriaceae, law.invention, Microbiology, law, Salmonella enterica, Multiplex polymerase chain reaction, medicine, Multiplex, Polymerase chain reaction, Bacteria, Biotechnology

Abstract

The aim of the work was to specifically differentiate S. typhimurium from other closely related Salmonella serovars by monoplex or multiplex PCR and to detect it from water and food samples. Genes targeted were invA, iroB, STM4497, STM2755, fliC, fljB and rfbJ and evaluated on 58 Salmonella standard serovars/strains including 9 S. typhimurium strains, 7 suspected Salmonella isolates and 8 other organisms as negative controls. Both invA and iroB showed a uniform amplification with all serovars of S. enterica group. STM2755 and STM4497 gene based PCR’s specifically exhibited amplification in all the nine confirmed S. typhimurium strains. The rfbJ PCR produced amplification with confirmed S. typhimurium strains, in addition showed reaction with S. abony. Both STM4497, STM2755 PCR’s and rfbJ could identify two of the seven biochemically suspected Salmonella isolates that were later confirmed to be S. typhimurium on the basis of sequence data. PCR for fliC genes had amplification exhibited by a large number of serovars of the S. enterica group, including S. typhimurium strains but not to S. brunei,S. newporti, S. abony and S. weltevreden. fljB was detected in all strains of S. enterica and E. coli with the exception of S. typhi. fljB and fliC were amplified in 6/7 and 5/7 presumptive Salmonella isolates. The same PCR’s were converted into two multiplex formats for simultaneous identification of the Salmonella genus, S. enterica group and S. typhimurium as a species. The first multiplex set comprised on invA, iroB, STM4497, STM2755 and the IAC. The second multiplex set comprised of invA, iroB, fljB, fliC, rfbJ along with IAC. The detection limit for S. typhimurium in the two multiplex PCR sets was in the range of 350–400 cfu/PCR reaction and that of DNA around 2 pg. The multiplex PCR (format 1) was first evaluated on spiked water, chicken and mutton samples and the detection limit for S. typhimurium was in the range of 100 cfu/100 ml

Published

2009

9. Antimicrobial susceptibility and molecular characterization of Vibrio cholerae from cholera outbreaks in Chennai

Author

K. Thavachelvam, Urmil Tuteja, H. V. Batra, T. James, B. Janardhanan, and Joseph J. Kingston

Subjects

biology, Tetracycline, medicine.disease, biology.organism_classification, medicine.disease_cause, Microbiology, Cholera, El Tor, Virology, Multiple drug resistance, Antibiotic resistance, Vibrio cholerae, Genotype, Multiplex polymerase chain reaction, medicine, Original Article, medicine.drug

Abstract

The genotype and antibiotic resistance pattern of the toxigenic Vibrio cholerae strains associated with cholera outbreaks vary frequently. Fifty-one V. cholerae strains isolated from cholera outbreaks in Chennai (2002–2005) were screened for the presence of virulence and regulatory genes by multiplex polymerase chain reaction (PCR) assay. Genotyping of the isolates was done by VC1 primers derived from enterobacterial repetitive intergenic consensus (ERIC)-related sequence in V. cholerae. All the isolates possessed toxigenic genes, such as ctxA, ctxB, tcpA, ace, ompU, toxR and zot. Two different El Tor genotypes and one O139 genotype could be delineated by VC1-PCR. One of the El Tor genotypes was similar to the El Tor strains isolated from Bhind district and Delhi during 2004. Antibiotic susceptibility testing revealed greater variability among the isolates tested. All the isolates were found to be susceptible to norfloxacin, ciprofloxacin and tetracycline. Thiry-three per cent of the isolates were found to be resistant to more than 4 antibiotics and could be termed as multiple antibiotic resistant. Coexistence of O139 serogroup along with the El Tor biotype could be identified among the strains recovered during the period 2002–2004. The O139 isolates were found to be more susceptible to the antibiotics tested when compared to the El Tor isolates.

Published

2009

10. Generation and characterization of a lipopolysaccharide-specific murine monoclonal antibody to Proteus vulgaris OX19

Author

H. V. Batra, Diprabhanu Bakshi, Urmil Tuteja, and Reena Jain

Subjects

biology, Physiology, medicine.drug_class, Proteus vulgaris, General Medicine, biology.organism_classification, Monoclonal antibody, Applied Microbiology and Biotechnology, Molecular biology, Proteus mirabilis, Enterobacteriaceae, Epitope, Microbiology, Proteus, Antigen, medicine, Hybridoma technology, Biotechnology

Abstract

The three strains of non-pathogenic Proteus species namely, Proteus vulgaris OX2, P. vulgaris OX19 and Proteus mirabilis OXK used in the Weil-Felix test are the group-specific cross-reactive antigens for Rickettsia and Orientia species. Earlier studies have revealed that the group specific and cross-reactive antigens responsible for the Weil-Felix test lie mostly in the lipopolysaccharide (LPS) moiety of the bacterial cell wall [Amano et al. (1993a) Infect Immun 61:4350-4355, (1993b) Microbiol Immunol 37:927-933, (1998) Infect Immun 66:923-926]. The three Proteus strains (OX2, OX19 and OXK) were used to raise murine monoclonal antibodies (MAbs) by hybridoma technology. Several MAb-producing hybridomas could be stabilized following limiting dilution. Affinity and specificity of these MAbs were checked by indirect ELISA using a battery of homologous and heterologous antigens including LPS. Amongst these, one MAb was found to be specific for P. vulgaris OX19 LPS. Since the Weil-Felix reaction is based on the cross-reactivity between the LPS based epitopes, this MAb could be of potential use in mapping of epitopes on the cross-reactive LPS and may also be useful as a potential diagnostic reagent.

Published

2006

11. Generation and Characterization of Murine Monoclonal Antibodies to Recombinant YopM, YopB and LcrV Proteins of Yersinia pestis

Author

Rekha Khushiramani, H. V. Batra, Jyoti Shukla, Urmil Tuteja, and Anupama Panikkar

Subjects

biology, medicine.diagnostic_test, Physiology, medicine.drug_class, General Medicine, Monoclonal antibody, biology.organism_classification, Applied Microbiology and Biotechnology, Enterobacteriaceae, Type three secretion system, Microbiology, law.invention, Antigen, Western blot, Yersinia pestis, law, medicine, Recombinant DNA, LcrV, Biotechnology

Abstract

YopM, an effector, YopB, a translator, and LcrV, a regulator, are proteins forming important componants of type III secretion system of Yersinia pestis. Recombinant truncated YopM of 32 kDa, YopB of 28 kDa and LcrV of 31 kDa sizes were utilized for priming BALB/c mice for the generation of monoclonal antibodies following standard poly-ethylene glycol (PEG) fusion protocol. Nine, 10 and 6 stabilized hybridoma cell lines could be generated against YopM, YopB and LcrV proteins, respectively. All these monoclonal antibodies were found reactive to Y. pestis strain A1122 and did not show any cross-reactivity to Y. enterocolitica, Y. pseudotuberculosis, Y. kristensenii, Y. frederiksenii, Y. intermedia, Klebsiella pneumoniae, Escherichia coli, Salmonella typhi, Salmonella abortus-equi and Staphylococcus aureus tested by ELISA and Western blotting. Monoclonal antibodies also exhibited reactivity to their corressponding native protein antigens in Y. pestis i.e. 42 kDa for YopM, 41 kDa for YopB and 37 kDa for LcrV in immunoblotting. Reactivity of monoclonal antibodies was further assessed on 26 Y. pestis isolates including 18 from 1994 plague outbreak regions (11 from pneumonic patients, 7 from rodents) and 8 from rodents of Deccan plateau of Southern India by Western blotting as well as by sandwich ELISA. The monoclonal antibodies could specifically locate the expression of yopM, yopB and lcrV genes among these Indian Y. pestis strains as well. Results obtained with sandwich ELISA and Western blot were identical to those observed by PCR. Monoclonal antibodies to Yops, therefore, can be employed for an early and reliable identification of virulent Y. pestis strains.

Published

2005

12. Rapid detection of Salmonella typhi in foods by combination of immunomagnetic separation and polymerase chain reaction

Author

Subodh Kumar, G.P. Singh, K. Balakrishna, and H. V. Batra

Subjects

Salmonella, biology, Physiology, General Medicine, biology.organism_classification, medicine.disease_cause, Salmonella typhi, Immunomagnetic separation, Applied Microbiology and Biotechnology, Enterobacteriaceae, Rapid detection, Microbiology, law.invention, law, medicine, Bacteria, Polymerase chain reaction, Biotechnology

Abstract

A combination of immunomagnetic separation and polymerase chain reaction (IMS-PCR) was used to detect Salmonella typhi in food and water samples. IMS was found to be an effective method for specific capture of S. typhi from artificially inoculated meat rinse samples. The bacteria could be detected within 6 h by IMS-PCR with a sensitivity of 105 cells. However, when tested in milk samples, the method was less effective. In comparison to conventional culture method, IMS-PCR is a rapid and specific method for detection of S. typhi and could be useful in outbreak situations for tracing the source of infection.

Published

2005

13. Serodiagnostic value of the 19 kilodalton antigen ofMycobacterium tuberculosis in indian patients

Author

H. V. Batra, V. Ramesh, Juraj Ivanyi, A. Chandramui, and G. Bothamley

Subjects

Microbiology (medical), medicine.medical_specialty, Tuberculosis, India, Sensitivity and Specificity, Epitope, Serology, Kilodalton, Mycobacterium tuberculosis, Epitopes, Medical microbiology, Antigen, medicine, Humans, Serologic Tests, Tuberculosis, Cutaneous, Tuberculosis, Pulmonary, Antigens, Bacterial, Chi-Square Distribution, biology, business.industry, Antibodies, Monoclonal, General Medicine, medicine.disease, biology.organism_classification, Antibodies, Bacterial, Virology, United Kingdom, Infectious Diseases, Tuberculosis, Meningeal, Immunology, biology.protein, Antibody, business

Abstract

Previous studies in UK subjects suggested that the 19 kDa protein antigen of Mycobacterium tuberculosis might be valuable in the serodiagnosis of paucibacillary tuberculosis. In this study, antibody titres for the 19 kDa antigen were higher in healthy controls in India than in the UK. Consequently, the diagnostic sensitivity of this antigen and its TB23 epitope was negligible in Indian patients with tuberculosis. However, a diagnostic sensitivity of 50% was achieved in patients with skin tuberculosis on the basis of a high ratio between antibody titres for the whole antigen and its TB23 epitope.

Published

1992