Your search keyword '"Chakrabarti, S. K."' showing total 53 results

1. Development and application of reverse transcription-loop mediated isothermal amplification assay for sensitive detection of groundnut bud necrosis virus infecting potato.

Author

Raigond B, Pathania S, Verma G, Bhardwaj P, Kochhar T, and Chakrabarti SK

Subjects

Reverse Transcription, Nucleic Acid Amplification Techniques, Sensitivity and Specificity, Solanum tuberosum, Viruses

Abstract

Reverse-transcription loop-mediated isothermal amplification (RT-LAMP) assay was developed for detection of groundnut bud necrosis virus (GBNV) causing potato stem necrosis disease. The isothermal temperatures, reaction periods and concentrations of reaction mixture were optimized where, the assay worked well at 65 °C for 50 min, 6 U of WarmStart Bst 2.0 DNA polymerase, 1.4 mM dNTPs and 2.0 mM MgSO 4. The optimized assay proved to be specific to GBNV with no cross reactivity to other viruses infecting potato in India. The specificity of RT-LAMP assay was found to be 100 fold more sensitive than that of RT-PCR. The developed assay was applied for the detection of GBNV from 80 potato leaf samples where 24 samples were found infected which was confirmed by RT-PCR. It was concluded that the RT-LAMP assay developed for detection of GBNV was specific, sensitive and suitable for its use in virus indexing under potato seed production programme., Competing Interests: Declaration of competing interest The authors declare that they have no conflict of interest., (Copyright © 2023 Elsevier Inc. All rights reserved.)

Published

2023

2. Spraying of dsRNA molecules derived from Phytophthora infestans, along with nanoclay carriers as a proof of concept for developing novel protection strategy for potato late blight.

Author

S S, Sharma S, Bairwa A, Tomar M, Kumar R, Bhardwaj V, Jeevalatha A, Bakade R, Salaria N, Thakur K, Singh BP, and Chakrabarti SK

Subjects

Disease Resistance genetics, Plant Diseases prevention & control, RNA, Double-Stranded genetics, Fungicides, Industrial pharmacology, Phytophthora infestans genetics, Solanum tuberosum genetics

Abstract

Background: Phytophthora infestans is a late blight-causing oomycetes pathogen. It rapidly evolves and adapts to the host background and new fungicide molecules within a few years of their release, most likely because of the predominance of transposable elements in its genome. Frequent applications of fungicides cause environmental concerns. Here, we developed target-specific RNA interference (RNAi)-based molecules, along with nanoclay carriers, that when sprayed on plants are capable of effectively reducing late blight infection., Results: Targeted the genes unique to sporulation, early satge infection and the metabolism pathway stages based on in an our own microarray data. We used nanoclay as a carrier for sorbitol dehydrogenase, heat shock protein 90, translation elongation factor 1-α, phospholipase-D like 3 and glycosylphosphatidylinositol-anchored acidic serine-threonine-rich HAM34-like protein double-stranded (ds)RNAs, which were assessed by culture bioassay, detached leaf assay and spray methods, and revealed a reduction in growth, sporulation and symptom expression. Plants sprayed with multigene targeted dsRNA-nanoclay showed enhanced disease resistance (4% disease severity) and less sporulation (<1 × 10 3 ) compared with plants sprayed with dsRNA alone., Conclusion: The use of nanoclay with multigene targeted dsRNA was assumed to be involved in effective delivery, protection and boosting the action of RNAi as a spray-induced gene silencing approach (SIGS). A significant reduction in growth, sporulation, disease severity and decreased gene expression authenticates the effects of SIGS on late blight progression. This study demonstrated as a proof of concept the dsRNA-nanoclay SIGS approach, which could be used as an alternative to chemical fungicides and transgenic approaches to develop an environmentally friendly novel plant protection strategy for late blight. © 2022 Society of Chemical Industry., (© 2022 Society of Chemical Industry.)

Published

2022

3. Genetic diversity studies based on morpho-pathological and molecular variability of the Sclerotinia sclerotiorum population infecting potato (Solanum tuberosum L.).

Author

Chaudhary S, Lal M, Sagar S, Tyagi H, Kumar M, Sharma S, and Chakrabarti SK

Subjects

Ascomycota genetics, Evolution, Molecular, India, Phenotype, Phylogeny, Phylogeography, Sequence Analysis, DNA, Virulence, Ascomycota classification, Ascomycota pathogenicity, Genetic Variation, Plant Diseases microbiology, Solanum tuberosum microbiology

Abstract

White mould or stem rot, caused by Sclerotinia sclerotiorum (Lib.) de Bary, is a devastating fungal disease found in major potato cultivation areas worldwide. The aim of this study was to characterize genetic diversity in the S. sclerotiorum population from the main potato producing regions of India by means of morphological (mycelial growth, colony colour, number and distribution pattern of sclerotia) and molecular characteristics, as well as to evaluate the virulence of S. sclerotiorum isolates in potato for the first time. Among the S. sclerotiorum population analyzed, high phenotypic and genotypic diversity were observed. Using all the morphological characteristics, a dendrogram was constructed based on Gower's similarity coefficient that distributed all the isolates into three clusters at the 0.62 similarity coefficient. Carpogenic germination of apothecia revealed that larger sclerotia produced a greater number of apothecia while smaller sclerotia produced fewer apothecia. Pathogenicity test results revealed that out of 25 isolates, seven were highly aggressive, 14 were moderate and four had low aggressiveness, whilst isolates from Punjab were more pathogenic than those of Uttar Pradesh. Phylogenetic analysis of universal rice primer polymorphism showed high genetic variability within the isolates that grouped all the isolates in three evolutionary lineages in the resulting dendrogram and showed partial relationship with geographical locations of the isolates. Further, the findings suggest the occurrence of higher heterogeneity and genetic diversity among the S. sclerotiorum isolates that indicates the existence of both clonal and sexual reproduction in the pathogen population of potato producing areas in India.

Published

2020

4. Development of a visual detection method for Potato virus S by reverse transcription loop-mediated isothermal amplification.

Author

Kumar R, Kaundal P, Arjunan J, Sharma S, and Chakrabarti SK

Abstract

A reverse transcription-loop mediated isothermal amplification (RT-LAMP) assay was developed to detect the Potato virus S (PVS) in potato. Two sets of six novel primers that recognize the coat protein gene sequence of the PVS were designed and RT-LAMP assay was optimized for the parameters such as different concentrations of primers, MgSO 4 , betaine, dNTPs, Bst DNA polymerase, temperature and duration. The RT-LAMP was carried out under isothermal conditions without the thermal cycler using PVS infected leaf and tuber samples, LAMP specific primers with amplification at 65 °C for 60 min, and 80 °C for 5 min. The results were assessed by gel electrophoresis and visual observation of colour change using SYBR Green I dye. The detection limit of the developed RT-LAMP assay was determined and compared with a conventional reverse transcription-polymerase chain reaction (RT-PCR). RT-LAMP was found 100 times more sensitive than RT-PCR. The optimized RT-LAMP assay is robust, reliable, sensitive and convenient for the detection of the PVS in infected potato tubers including asymptomatic plants. No cross-reactions were observed with healthy plants and other potato viruses. The assay is economical and can be employed in large scale testing of potato plants against PVS under healthy seed potato production programme., Competing Interests: Conflict of interestThere is no conflict of interest by the co-authors., (© King Abdulaziz City for Science and Technology 2020.)

Published

2020

5. Complete mitogenome mapping of potato late blight pathogen, Phytophthora infestans A 2 mating type.

Author

Patil VU, Vanishree G, Pattanayak D, Sharma S, Bhardwaj V, Singh BP, and Chakrabarti SK

Abstract

Complete mitochondrial genome of Phytophthora infestans , A 2 mating type (MT) with a size of ≅37,767 bp was sequenced. A total of 53 protein-coding genes are predicted on both strands, including 25 tRNA , 2 rRNA , and 18 respiratory proteins. Gene order of A 2 MT was consistent with that established in A 1 , despite high level of polymorphism in both coding and non-coding regions. The mtDNA of A 2 MT was found to have 99.5% and 99.4% homology with Ia and Ib, whereas 94.7% and 94.3% with IIa and IIb, respectively. Study of repeats revealed a dinucleotide (AT) 9 specific to A 1 and homology of cox1 gene sequence revealed the relationship among 50 Phytophthora species., Competing Interests: None of the authors report any conflict of interest. The authors alone are responsible for the content and writing of the paper., (© 2017 ICAR - Central Potato Research Institute, India. Published by Informa UK Limited, trading as Taylor & Francis Group.)

Published

2017

6. Bardet-Biedl syndrome in two siblings: a rare entity revisited.

Author

Chakravarti HN, Ray S, Chakrabarti SK, Biswas D, Ghosh S, Mukhopadhyay S, and Chowdhury S

Subjects

Child, Developmental Disabilities etiology, Diagnosis, Differential, Disease Management, Female, Humans, Hypogonadism etiology, Male, Pediatric Obesity etiology, Retinitis Pigmentosa etiology, Symptom Assessment, Bardet-Biedl Syndrome complications, Bardet-Biedl Syndrome diagnosis, Bardet-Biedl Syndrome physiopathology, Bardet-Biedl Syndrome therapy, Developmental Disabilities diagnosis, Hypogonadism diagnosis, Pediatric Obesity diagnosis, Retinitis Pigmentosa diagnosis, Siblings

Published

2016

7. Uniplex and duplex PCR detection of geminivirus associated with potato apical leaf curl disease in India.

Author

Jeevalatha A, Kaundal P, Venkatasalam EP, Chakrabarti SK, and Singh BP

Subjects

Capsid Proteins genetics, DNA Primers genetics, India, Plant Proteins genetics, Polymerase Chain Reaction standards, Reference Standards, Sensitivity and Specificity, Urease genetics, Virology standards, Begomovirus isolation & purification, Plant Diseases virology, Polymerase Chain Reaction methods, Solanum tuberosum virology, Virology methods

Abstract

Apical leaf curl disease has emerged as a new disease in potato during the last decade in India due to a change in planting date and an increased whitefly population. Its incidence is on the rise threatening the cultivation of potato across the country. Hence, a PCR assay was developed for the detection of Tomato leaf curl New Delhi virus-potato (ToLCNDV-Potato) which is the causal agent of apical leaf curl disease in potato. Primers specific to the coat protein (AV1) and replicase (AC1) gene regions were designed and used for standardization of the PCR. Some of the primers (LCVCPF1/LCVCPR1, LCVREPF2/LCVREPR2, LCrep1F/LCrep2R) could detect the virus in 2.4-0.24pg of total DNA of infected plant. A duplex PCR assay was optimized with the selected coat protein gene specific primers and primers specific to potato urease gene, a housekeeping gene served as an internal check. The suitability of these primers was examined for detection of the virus in 80 potato apical leaf curl disease samples from 11 different potato growing states of India and also from micro-plants grown in tissue culture. The selected coat protein primer pair (LCVCPF1/LCVCPR1) was found to be conserved in all 80 isolates except for a few isolates, which had a single nucleotide substitution in the forward primer sequence. These substitutions did not interfere with amplification of the coat protein gene. The primers could detect the virus using a print-capture PCR assay both in the presence and absence of an internal control. These results indicate the robustness of the PCR assay for virus indexing of mother stocks in the seed production system., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2013

8. Complete Genome Sequence of Potato leafroll virus Isolates Infecting Potato in the Different Geographical Areas of India Shows Low Level Genetic Diversity.

Author

Jeevalatha A, Kaundal P, Shandil RK, Sharma NN, Chakrabarti SK, and Singh BP

Abstract

Five Potato leafroll virus (PLRV) isolates were collected from five states representing different potato growing parts of India. The ssRNA genome sequences of these isolates were determined. The genome comprised of 5,883 nucleotides and deduced genome organization resembled other PLRV isolates. About 97.6-98.7 % similarities was observed within the Indian isolates and were more close to European, Canadian, African, American and Czech isolates (95.8-98.6 %) than to an Australian isolate (92.9-93.4 %). These isolates were 43.7-53.1 % similar to other poleroviruses and 29.1-29.3 % to Barley yellow dwarf virus, a luteovirus. Out of five isolates, the isolate PBI-6 was recombinant one as detected by RDP3 software. Multiple sequence alignment of nucleotide and amino acid sequences of different ORFs indicated that the ORF 3 and ORF 4, corresponding to coat protein and movement proteins are more conserved than other ORFs. Amino acid changes specific to Indian isolates were observed and it was more in ORF 2 than in ORF 0, ORF 3 and ORF 4. This is the first report of complete genome sequence of PLRV isolates from India, which reveals low level genetic diversity.

Published

2013

9. Influence of drying of biosludge on organochlorine compounds from pulp and paper industry.

Author

Gupta S, Purwar M, Chakrabarti SK, and Singh S

Subjects

Industrial Waste, Temperature, Environmental Pollutants chemistry, Hydrocarbons, Chlorinated chemistry, Paper, Sewage, Water chemistry

Abstract

Pulp and paper industry is one of the major sources of man-made generation of organochlorine compounds. During biological treatment of wastewater, part of organochlorine compounds is discharged with treated effluent and part is retained on biomass and disposed of as waste activated sludge. Due to presence of these compounds, the disposal of biosludge from pulp and paper industry has become an issue. The estimation of adsorbable organic halogen (AOX) compounds after drying and grinding resulted in 49% lower concentration of AOX due to stripping of purgeable compounds. These purgeable compounds are not released at 60 degrees C in aqueous medium during estimation of purgeable organic halogen (POX) compounds. Dispersion of sludge by sonication overcomes the loss of POX compounds and results in higher concentration ofAOX compounds. The drying of biosludge samples at 45, 100 degrees C and in presence of sun light resulted in 20.1, 49.0 and 29.6% removal of purgeable AOX compounds, respectively. The lab scale sorption study using dichloromethane (as volatile organochlorine compound) reveal that biosludge from pulp and paper industry is a good adsorbent of volatile organochlorine compounds and results in poor release of these compounds during estimation of POX compounds.

Published

2012

10. Genome sequence and analysis of the tuber crop potato.

Author

Xu X, Pan S, Cheng S, Zhang B, Mu D, Ni P, Zhang G, Yang S, Li R, Wang J, Orjeda G, Guzman F, Torres M, Lozano R, Ponce O, Martinez D, De la Cruz G, Chakrabarti SK, Patil VU, Skryabin KG, Kuznetsov BB, Ravin NV, Kolganova TV, Beletsky AV, Mardanov AV, Di Genova A, Bolser DM, Martin DM, Li G, Yang Y, Kuang H, Hu Q, Xiong X, Bishop GJ, Sagredo B, Mejía N, Zagorski W, Gromadka R, Gawor J, Szczesny P, Huang S, Zhang Z, Liang C, He J, Li Y, He Y, Xu J, Zhang Y, Xie B, Du Y, Qu D, Bonierbale M, Ghislain M, Herrera Mdel R, Giuliano G, Pietrella M, Perrotta G, Facella P, O'Brien K, Feingold SE, Barreiro LE, Massa GA, Diambra L, Whitty BR, Vaillancourt B, Lin H, Massa AN, Geoffroy M, Lundback S, DellaPenna D, Buell CR, Sharma SK, Marshall DF, Waugh R, Bryan GJ, Destefanis M, Nagy I, Milbourne D, Thomson SJ, Fiers M, Jacobs JM, Nielsen KL, Sønderkær M, Iovene M, Torres GA, Jiang J, Veilleux RE, Bachem CW, de Boer J, Borm T, Kloosterman B, van Eck H, Datema E, Hekkert Bt, Goverse A, van Ham RC, and Visser RG

Subjects

Evolution, Molecular, Gene Duplication, Gene Expression Regulation, Plant, Genes, Plant genetics, Genetic Variation, Haplotypes genetics, Heterozygote, Homozygote, Immunity, Innate, Inbreeding, Molecular Sequence Annotation, Molecular Sequence Data, Plant Diseases genetics, Ploidies, Solanum tuberosum physiology, Genome, Plant genetics, Genomics, Solanum tuberosum genetics

Abstract

Potato (Solanum tuberosum L.) is the world's most important non-grain food crop and is central to global food security. It is clonally propagated, highly heterozygous, autotetraploid, and suffers acute inbreeding depression. Here we use a homozygous doubled-monoploid potato clone to sequence and assemble 86% of the 844-megabase genome. We predict 39,031 protein-coding genes and present evidence for at least two genome duplication events indicative of a palaeopolyploid origin. As the first genome sequence of an asterid, the potato genome reveals 2,642 genes specific to this large angiosperm clade. We also sequenced a heterozygous diploid clone and show that gene presence/absence variants and other potentially deleterious mutations occur frequently and are a likely cause of inbreeding depression. Gene family expansion, tissue-specific expression and recruitment of genes to new pathways contributed to the evolution of tuber development. The potato genome sequence provides a platform for genetic improvement of this vital crop., (©2011 Macmillan Publishers Limited. All rights reserved)

Published

2011

11. Degradation of pentachlorophenol by Kocuria sp. CL2 isolated from secondary sludge of pulp and paper mill.

Author

Karn SK, Chakrabarti SK, and Reddy MS

Subjects

Biodegradation, Environmental, Environmental Pollutants metabolism, Industrial Waste analysis, Micrococcaceae classification, Micrococcaceae genetics, Molecular Sequence Data, Phylogeny, Sewage analysis, Micrococcaceae isolation & purification, Micrococcaceae metabolism, Pentachlorophenol metabolism, Sewage microbiology

Abstract

A pentachlorophenol (PCP) degrading bacterium was isolated and characterized from sludge of pulp and paper mill. This isolate used PCP as its sole source of carbon and energy and was capable of degrading this compound, as indicated by stoichiometric release of chloride and biomass formation. Based on morphology, biochemical tests, and 16S rRNA gene sequence analysis this strain was identified as Kocuria sp. CL2. High Performance Liquid Chromatography (HPLC) analysis revealed that this strain was able to degrade PCP up to a concentration of 600 mg/l. This is first time we are reporting the degradation of PCP by the Kocuria species. This isolate was also able to remove 58.64% of PCP from the sludge within two weeks. This study showed that the removal efficiency of PCP by CL2 was found to be very effective and can be used in degradation of PCP containing pulp paper mill waste in the environment.

Published

2011

12. 12-Lipoxygenase Products Reduce Insulin Secretion and {beta}-Cell Viability in Human Islets.

Author

Ma K, Nunemaker CS, Wu R, Chakrabarti SK, Taylor-Fishwick DA, and Nadler JL

Subjects

12-Hydroxy-5,8,10,14-eicosatetraenoic Acid pharmacology, Animals, Apoptosis drug effects, Cell Survival drug effects, Humans, Insulin Secretion, Insulin-Secreting Cells cytology, Male, Mice, Mice, Inbred C57BL, Pentoxifylline analogs & derivatives, Pentoxifylline pharmacology, Phosphorylation, p38 Mitogen-Activated Protein Kinases metabolism, Arachidonate 12-Lipoxygenase physiology, Insulin metabolism, Insulin-Secreting Cells drug effects

Abstract

Context: Inflammation is increasingly recognized as an important contributing factor in diabetes mellitus. Lipoxygenases (LOs) produce active lipids that promote inflammatory damage by catalyzing the oxidation of linoleic and arachidonic acid, and LO is expressed in rodent and human islets. Little is known about the differential effect of the various hydroxyeicosatetraenoic acids (HETEs) that result from LO activity in human islets., Objective: We compared the effects of 12-LO products on human islet viability and function., Design: Human islets were treated with stable compounds derived from LOs: 12(S)-HETE, 15HETE, 12HPETE, and 12RHETE and then examined for insulin secretion and islet viability. The p38-MAPK (p38) and JNK stress-activated pathways were investigated as mechanisms of 12-LO-mediated islet inhibition in rodent and human islets., Results: Insulin secretion was consistently reduced by 12(S)-HETE and 12HPETE. 12(S)-HETE at 1 nm reduced viability activity by 32% measured by MTT assay and increased cell death by 50% at 100 nm in human islets. These effects were partially reversed with lisofylline, a small-molecule antiinflammatory compound that protects mitochondrial function. 12(S)-HETE increased phosphorylated p38-MAPK (pp38) protein activity in human islets. Injecting 12-LO siRNA into C57BL/6 mice reduced 12-LO and pp38-MAPK protein levels in mouse islets. The addition of proinflammatory cytokines increased pp38 levels in normal mouse islets but not in siRNA-treated islets., Conclusions: These data suggest that 12(S)-HETE reduces insulin secretion and increases cell death in human islets. The 12-LO pathway is present in human islets, and expression is up-regulated by inflammatory cytokines. Reduction of 12-LO activity could thus provide a new therapeutic approach to protect human beta-cells from inflammatory injury.

Published

2010

13. Effect of ozonation on activated sludge from pulp and paper industry.

Author

Gupta S, Chakrabarti SK, and Singh S

Subjects

Paper, Industrial Waste, Ozone, Waste Management methods

Abstract

Aerobic biological treatment with activated sludge is the predominant process all over the world for treatment of pulp and paper industry wastewater. 50-70% of the biodegradable organic material is oxidized to CO₂ and the rest is converted to bacterial biomass, typically termed as excess sludge or waste activated sludge (WAS). Handling and disposal of WAS in general and in particular from the pulp and paper industry face different processing difficulties, regulatory stringency due to organochlorine contamination and reluctance of people for reuse. With an objective of reducing the net disposable biomass, ozonation of WAS from a pulp and paper mill and from a laboratory scale batch activated sludge process operated with the wastewater and bacterial seed of the same pulp and paper mill have been carried out. With the mill sludge having predominant filamentous organisms 18% MLSS was reduced at an ozone dosage of 55 mg O₃/g dry MLSS solid (DS) resulting in 2.5 times COD increase. With the laboratory sludge which is well structured and flocculating, only 6% MLSS was reduced at an ozone dosage of 55 mg O₃/g DS. Ozonation mineralizes 26% and 20% AOX compounds embedded in the secondary sludge in the mill and laboratory sludge respectively at an ozone dosage of 55 mg O₃/g DS. During ozonation, absorbed/adsorbed lignin on biomass was released which resulted in increased colour concentration. Ozonation can be a potential oxidative pretreatment process for reducing the WAS and paving the way for cost effective overall treatment of WAS.

Published

2010

14. Assessment of genetic fidelity of micropropagated apple rootstock plants, EMLA 111, using RAPD markers.

Author

Gupta R, Modgil M, and Chakrabarti SK

Subjects

DNA, Plant genetics, Genes, Plant, Malus genetics, Random Amplified Polymorphic DNA Technique

Abstract

EMLA 111(East Malling Long Ashton), a clonal rootstock of apple (Malus pumila Mill.) was micropropagated using axillary bud and shoot apices. The present work was carried out to assess the genetic fidelity of micropropagated plants using random amplified polymorphic DNA (RAPD). Ten arbitrary decamer primers have been used to amplify genomic DNA from in vitro raised field material and mother plant. A total of 57 amplified products were obtained, out of which 53 were monomorphic across the mother tree and its tissue culture raised progenies. Of the ten primers used, 8 showed RAPD profiles which were identical to the mother plant. Similarity matrix based on Jaccard's coefficient revealed that pairwise value between the mother plant and its tissue cultured plants ranged from 0.93 to 1.00 and among tissue cultured plants, it was 0.92 to 1.00, thus indicating a high degree of genetic fidelity.

Published

2009

15. Multiple displacement amplification as a pre-polymerase chain reaction (pre-PCR) to detect ultra low population of Ralstonia solanacearum (Smith 1896) Yabuchi et al. (1996).

Author

Grover A, Azmi W, Paul Khurana SM, and Chakrabarti SK

Subjects

DNA Primers genetics, DNA, Bacterial genetics, DNA, Bacterial isolation & purification, Plant Diseases microbiology, Ralstonia solanacearum genetics, Soil Microbiology, Solanum tuberosum microbiology, Polymerase Chain Reaction methods, Ralstonia solanacearum isolation & purification

Abstract

Aims: To develop a reliable and sensitive protocol for detection of Ralstonia solanacearum using MDA-PCR (Multiple displacement amplification-PCR amplification)., Methods and Results: MDA-PCR technique was performed on pure cell lysates as well as soil samples. Pure cell lysate as well as that of soil DNA was used as template in MDA reaction. MDA of template DNA was carried out in the presence of sample buffer, reaction buffer and enzyme mix (Phi 29 DNA polymerase and random hexamers). The MDA amplified DNA was used for PCR amplification using R. solanacearum -specific PCR primers. MDA-PCR could detect as low as 1 colony forming unit (CFU ml(-1)) of bacteria within 8 h including DNA isolation., Conclusion: MDA followed by standard PCR facilitated the detection of pathogen from very low count samples. The method is of great importance in managing the brown rot disease of potato., Significance and Impact of Study: The ultrasensitive detection technique developed in the present study is sensitive and speedy enough to be included into integrated wilt disease control programmes.

Published

2009

16. Genotypic diversity in a localized population of Ralstonia solanacearum as revealed by random amplified polymorphic DNA markers.

Author

Grover A, Azmi W, Gadewar AV, Pattanayak D, Naik PS, Shekhawat GS, and Chakrabarti SK

Subjects

DNA, Bacterial genetics, Ecosystem, Genetic Markers, Genome, Bacterial, Polymerase Chain Reaction methods, Random Amplified Polymorphic DNA Technique, DNA, Bacterial analysis, Genetic Variation genetics, Plant Diseases microbiology, Ralstonia solanacearum genetics

Abstract

Aims: To assess genotypic diversity within Ralstonia solanacearum isolates of a single field., Methods and Results: A total of 44 field isolates and 22 in vitro generated clones of R. solanacearum were studied for genotypic diversity by random amplified polymorphic DNA (RAPD) technique. Genomic DNA of these isolates and clones was extracted by proteinase-K-SDS lysis mini-prep method. RAPD analysis was done with 30 decamer primers. The data were analysed using NTSYSpc 2.02h software. Forty-two out of 44 field isolates and all the clonal isolates were identified as distinct genotypes at 70% similarity level., Conclusion: Very high level of genome variability was observed within the field and clonal isolates of R. solanacearum. This might be a reason for the wide host range of this bacterium and for quick breakdown of wilt resistance in host plants., Significance and Impact of the Study: The results suggest that it would be difficult to design specific diagnostic protocol for R. solanacearum even for a localized population and to breed cultivars with broad-spectrum resistance.

Published

2006

17. Genetic diversity and differentiation of Indian isolates of Phytophthora infestans as revealed by RAPD analysis.

Author

Atheya I, Singh BP, Chakrabarti SK, and Pattanayak D

Subjects

DNA metabolism, DNA Primers chemistry, Genetic Markers, Models, Statistical, Phylogeny, Polymerase Chain Reaction, Polymorphism, Genetic, Random Amplified Polymorphic DNA Technique, Genetic Variation, Phytophthora genetics

Abstract

Sixty-seven isolates of Phytophthora infestans collected from Himalayan hill regions and subtropical planes of India were characterized by RAPD markers to assess diversity and differentiation based on location of origin. Ten random decamer primers generated 161 polymorphic fragments. Association of P. infestans isolates on the dendrogram and PCO plot revealed two clear grouping based on geographical location of origin-hill isolates and plane isolates. Quantification of diversity by Shannon index of diversity analysis demonstrated that most of the diversity was present with a particular population (hill or plane) of P. infestans isolates, with 85% variation being within and 15% being between hill and plane isolates. Subtropical plane isolates of P. infestans exhibited higher variability compared to hill isolates and they were more dispersed on the PCO plot. No clear differentiation of isolates based on mating type was reflected on the dendrogram and PCO plot.

Published

2005

18. Phylogenetic analysis of 5'-UTR and P1 protein of Indian common strain of potato virus Y reveals its possible introduction in India.

Author

Mukherjee K, Verma Y, Chakrabarti SK, and Khurana SM

Subjects

Amino Acid Sequence, Base Sequence, Cloning, Molecular, India, Nuclear Localization Signals, Phosphorylation, Potyvirus classification, Potyvirus genetics, Potyvirus physiology, Sequence Alignment, Sequence Analysis, DNA, Viral Proteins chemistry, Viral Proteins metabolism, Virus Replication, 5' Untranslated Regions genetics, Phylogeny, Viral Proteins genetics

Abstract

The 5' untranslated region (UTR) and P1 region of the Indian strain of potato virus Y ordinary strain (PVYO) was cloned and sequenced for the first time. Database searches and multiple sequence alignment showed the highest sequence similarity with the PVYO strains of European origin. Based on the phylogenetic analysis and multiple sequence alignment, the possible evolution of PVYN from PVYO is predicted. PVYO strains from China and India were perhaps introduced into these countries from a similar geographical location. All major PVY strains available in the database can be classified into two major subgroups of North American and European origin. The Chinese and Indian PVYO strains fall within the European union subgroup suggesting a long association since potato was introduced from Europe into these countries by two separate independent events. The possible function of P1 protein in plant virus replication is suggested due to in-silico prediction of nuclear localization signal (NLS) and other phosphorylation regulatory domains at the vicinity of the NLS.

Published

2004

19. Characterization of genetic diversity of some serovars of Bacillus thuringiensis by RAPD.

Author

Pattanayak D, Chakrabarti SK, Kumar PA, and Naik PS

Subjects

Bacillus thuringiensis classification, Cluster Analysis, DNA Fingerprinting, DNA Primers chemistry, Genetic Variation, Phylogeny, Polymerase Chain Reaction, Polymorphism, Genetic, Random Amplified Polymorphic DNA Technique, Serotyping, Bacillus thuringiensis genetics, DNA, Bacterial genetics

Abstract

RAPD based fingerprinting of 21 serovars of Bacillus thuringiensis (Bt) representing different serotypes was performed using 19 random decamer primers. A total of 172 polymorphic fragments, ranging in size from 161-2789 bp, were amplified from 13 of the 19 primers. Pairwise genetic similarity analysis revealed very low similarity values, ranging from 3-68%, among the serovars of Bt, indicating high genetic divergence. Nineteen serovars of Bt fell in two major clusters and remaining two formed solitary clusters in the dendogram. Clustering of Bt strains established genetic relatedness between serovars and serotypes. It has been suggested that RAPD analysis can be used for genotypic characterization of Bt to complement flagellar serotyping.

Published

2001

20. Effects of different nickel compounds on the transport of para-aminohippurate ion by rat renal cortical slices.

Author

M'Bemba Meka P and Chakrabarti SK

Subjects

Animals, Culture Techniques, Glutathione pharmacology, Kidney Cortex metabolism, L-Lactate Dehydrogenase metabolism, Male, Mannitol pharmacology, Oxidative Stress, Rats, Rats, Sprague-Dawley, Kidney Cortex drug effects, Nickel toxicity, p-Aminohippuric Acid pharmacokinetics

Abstract

In vitro rat renal cortical slice uptake of para-aminohippurate ion (PAH) expressed as tissue slice-to-medium ratio was used as a model to predict nephrotoxicity of different nickel compounds. Pretreatment with nickel compounds for a period of up to 4 h was followed by an incubation with 74 microM PAH for 2 h. The PAH uptake by renal cortical slices was reduced by nickel compounds in both concentration- and time-dependent manner. Furthermore, the extent of such reduction of PAH uptake was found to depend on the chemical form (speciation) of nickel. Thus, slice-to-medium ratios were 41, 49, 48, and 66% of control values after a 4-h pretreatment with 0.378 mM nickel carbonate hydroxide, 1.5 mM nickel subsulfide, 4 mM nickel sulfate and 2.98 mM nickel oxide, respectively. Such an inhibition of PAH transport was not due to cytotoxicity. The results suggest that the nephrotoxic potency decreases in the following order: nickel carbonate hydroxide>nickel subsulfide>nickel sulfate>nickel oxide. Treatment of renal cortical slices with high concentrations of either mannitol, a hydroxyl radical scavenger, or glutathione significantly reduced the inhibition of PAH uptake by soluble form of nickel subsulfide, with concomitant reduction of nickel ion uptake by cortical slices. But no such oxidative stress seems to be involved in nickel carbonate hydroxide-induced inhibition of PAH uptake.

Published

2001

21. Visceral afferent hypersensitivity in irritable bowel syndrome--evaluation by cerebral evoked potential after rectal stimulation.

Author

Sinhamahapatra P, Saha SP, Chowdhury A, Chakrabarti SK, Ghosh A, and Maiti B

Subjects

Adult, Colonic Diseases, Functional physiopathology, Electric Stimulation, Female, Humans, Male, Median Nerve physiopathology, Reaction Time, Rectum innervation, Sensory Thresholds, Colonic Diseases, Functional etiology, Evoked Potentials, Somatosensory, Visceral Afferents physiopathology

Abstract

Objectives: Gut hypersensitivity has been shown to be present in irritable bowel syndrome. The current study sought to determine the involvement or hypersensitivity of the gut afferents, objectively, by recording cerebral evoked potential after rectal stimulation., Methods: In 13 patients with irritable bowel syndrome and nine healthy controls, rectal perception thresholds to electrical stimulation were measured, and cerebral evoked potentials were recorded from 2 cm behind vertex (Cz') after rectal stimulation electrically (frequency 1 Hz, duration 0.5 ms) at an intensity 50% above perception threshold and with filter setting 1-250 Hz., Results: Perception thresholds to rectal electrical stimuli in patients with irritable bowel syndrome were lower than controls (p < 0.05). Rectal stimulation led to recognizable and reproducible cerebral evoked potentials. P1, N1, P2 latencies in patients with irritable bowel syndrome were shorter than that in controls (p < 0.05). P1/N1 amplitude was greater in patients with irritable bowel syndrome than in controls (p < 0.05)., Conclusions: The shorter latency and increased amplitude of cerebral evoked potential after rectal stimulation in patients with irritable bowel syndrome compared to controls provide objective evidence supporting visceral afferent hypersensitivity as the underlying mechanism in irritable bowel syndrome.

Published

2001

22. DNA-protein crosslinks induced by nickel compounds in isolated rat lymphocytes: role of reactive oxygen species and specific amino acids.

Author

Chakrabarti SK, Bai C, and Subramanian KS

Subjects

Acetates toxicity, Animals, Cross-Linking Reagents toxicity, Cysteine pharmacology, DNA chemistry, Deferoxamine pharmacology, Dose-Response Relationship, Drug, Free Radical Scavengers pharmacology, Histidine pharmacology, Lymphocytes metabolism, Magnesium pharmacology, Nickel metabolism, Nickel toxicity, Occupational Exposure, Organometallic Compounds toxicity, Oxidative Stress, Proteins chemistry, Rats, DNA metabolism, DNA Damage, Lymphocytes drug effects, Proteins metabolism, Reactive Oxygen Species metabolism

Abstract

Isolated rat lymphocytes in salts-glucose medium (pH 7.2) were incubated with nickel chloride, nickel acetate, nickel sulfate, and a soluble form of nickel subsulfide (0-2 mM) at 37 degrees C for 2 h. The soluble form of nickel subsulfide induced a significant increase in DNA-protein crosslinks (DPXLs) (111%) beginning at 0.5 mM and a maximum increase of 700% from that of the control value was reached at a 2 mM concentration, whereas nickel sulfate produced only a 65% increase of such crosslinks at the 2 mM concentration only. No significant reduction in viability of rat lymphocytes (as measured by trypan blue exclusion) due to these nickel compounds was observed at any concentration used. Time-course studies of DPXLs and cellular viability due to 2 mM nickel subsulfide indicate that DPXL formation may not be due in part to cellular necrosis. Coincubation of nickel subsulfide (2 mM) with l-histidine (16 mM), l-cysteine (4 or 8 mM), or l-aspartic acid (24 mM) significantly reduced the DPXLs induced by 2 mM nickel subsulfide. But Mg(2+) even at 24 mM failed to antagonize nickel subsulfide-induced increase in DPXLs. High concentrations of these amino acids significantly decreased the accumulation of Ni(2+) from nickel subsulfide in lymphocytes, suggesting that such reduction of cellular uptake of Ni(2+) by these amino acids is partly responsible for the potent protective effects of these amino acids against such genotoxicity of nickel subsulfide. In vitro exposure of lymphocytes to nickel subsulfide (0-2 mM) increased the formation of reactive oxygen species (ROS) in a concentration-dependent manner. Furthermore, coincubation of 2 mM nickel subsulfide with catalase, dimethylthiourea, mannitol, or vitamin C at 37 degrees C for 2 h resulted in a significant decrease of nickel subsulfide-induced formation of DPXLs, suggesting that nickel subsulfide-induced DPXLs formation in isolated rat lymphocytes is caused by the formation of ROS. The amino acid treatment also abrogated Ni(3)S(2)-induced generation of ROS. Deferoxamine (a highly specific iron chelator) treatment prevented nickel subsulfide-induced DNA-protein crosslink formation, suggesting that Ni(2+)-induced DPXL formation in rat lymphocytes is caused by the induction of Fenton/Haber-Weiss reaction, generating hydroxyl radicals. The potent protective effects of these specific amino acids against nickel subsulfide-induced DPXL formation in isolated rat lymphocytes may be due in part to impaired cellular uptake of Ni(2+), inhibition of the binding of Ni(2+) to deproteinized DNA, and a reduction in reactive oxygen species., (Copyright 2001 Academic Press.)

Published

2001

23. Influence of caffeine on allyl alcohol-induced hepatotoxicity in rats. I. In vivo study.

Author

Karas M and Chakrabarti SK

Subjects

Acrolein metabolism, Alanine Transaminase blood, Alcohol Dehydrogenase antagonists & inhibitors, Animals, Chemical and Drug Induced Liver Injury blood, Drug Interactions, Enzyme Inhibitors pharmacology, Fomepizole, Glutathione metabolism, Hepatocytes drug effects, Hepatocytes metabolism, Hepatocytes pathology, Liver metabolism, Liver pathology, Male, Phenobarbital pharmacology, Propanols metabolism, Pyrazoles pharmacology, Rats, Rats, Sprague-Dawley, Sulfhydryl Compounds, Caffeine pharmacology, Chemical and Drug Induced Liver Injury etiology, Liver drug effects, Propanols toxicity

Abstract

Cotreatment of rats with a low hepatotoxic dose (30.7 mg/kg, i.p.) of allyl alcohol (AA) and a higher, but nontoxic, dose (150 mg/kg, oral) of caffeine (CF) potentiated the hepatotoxicity of AA. This was verified by significantly higher levels of plasma alanine aminotransferase (ALT) activity and histopathologically greater severity of lesions in the periportal hepatocytes than those due to AA alone. Treatment of rats with 4-methylpyrazole (4-MP) (0.5 mmol/kg, i.p.) (an inhibitor liver alcohol dehydrogenase) for 30 minutes, followed by similar cotreatment with AA and CF, completely prevented the elevation of plasma levels of ALT and histological damage induced by cotreatment with CF and AA 24 hours following their administration. Severe liver damage induced by cotreatment with CF and AA was further, markedly enhanced by phenobarbital pretreatment (80 mg/kg, i.p., 3 days). Thus, extensive necrosis of periportal hepatocytes was noted, as well as edema and accumulation of inflammatory cells in the necrotic foci caused by such pretreatment. The depression of hepatic nonprotein sulfhydryls resulting from CF plus AA was much more severe than that caused by AA or CF alone and appeared as early as 30 minutes after administration. However, much less marked depletion of protein thiols was observed following similar treatments. Significant increase in lipid peroxidation (as measured by melondialdehyde [MDA] formation) was also observed in rat liver but only 24 hours after administration. The production ofMDA in the rat liver was significantly higher after administration of AA plus CF than after administration of AA alone. Pretreatment of rats with phenobarbital further significantly enhanced the formation of 2,4-dinitrophenylhydrazine (DNP)-reactive metabolite(s) (measured as DNP-acrolein adduct equivalents) in rat liver induced by AA (30.7 mg/kg) plus CF (150 mg/kg) within 1 hour following such treatment. Cotreatment with AA and a higher dose of CF resulted in significantly higher excretion of urinary thioethers or mercapturic acids than in rats treated with AA alone. Thus, these data suggest that an increased bioactivation pathway of acrolein involving a P450 mixed-function oxidase system caused by CF may be involved in such potentiating effects of CF on AA-induced hepatotoxicity in rats.

Published

2001

24. Caffeine potentiation of allyl alcohol-induced hepatotoxicity. II. In vitro study.

Author

Karas M and Chakrabarti SK

Subjects

Acrolein metabolism, Animals, Cell Survival drug effects, Dose-Response Relationship, Drug, Drug Synergism, Fomepizole, Glutathione metabolism, Hepatocytes metabolism, Hepatocytes pathology, In Vitro Techniques, L-Lactate Dehydrogenase metabolism, Lipid Peroxidation drug effects, Liver metabolism, Liver pathology, Male, Malondialdehyde metabolism, Propanols metabolism, Pyrazoles pharmacology, Rats, Rats, Sprague-Dawley, Sulfhydryl Compounds, Time Factors, Acrolein toxicity, Caffeine pharmacology, Hepatocytes drug effects, Liver drug effects, Propanols toxicity

Abstract

We examined the effects of caffeine (C) on allyl alcohol (AA)- and acrolein (A)-induced hepatotoxicity on freshly-isolated, rat hepatocytes obtained from livers of adult, male, Sprague-Dawley rats. Isolated rat hepatocytes in suspension were incubated in each test with one of the following: 0, 1.0, or 2.5 mM of AA alone; or with 0, 2.5, or 5 mM of C alone; or a combination of AA and C at the same range of concentrations as used alone, for 15, 30, 60, 90, and 120 minutes at 37 degrees C. A dose- and time-dependent potentiation of cytotoxicity as measured by cellular viability (using trypan blue exclusion) were observed. The AA (2.5 mM)-induced lactate dehydrogenase (LDH) leakage observed after 60 minutes incubation was completely prevented when pretreated for 15 minutes with 4-methylpyrazole (MP) (0.5 mM). Such pretreatment, even with a double dose of 4-MP, only partially, and not significantly, prevented LDH leakage when the hepatocytes were incubated with a mixture of 2.5 mM AA and 5 mM C. The depletion of hepatocyte nonprotein sulfhydryl (NPSH) content caused by AA was further enhanced in the presence of C, as early as 15 minutes after their exposure. The AA-induced increase in lipid peroxidation was also potentiated by C; however, potentiation started later, and only after sufficient depletion of NPSH (mostly glutathione) occurred resulting from the presence of AA plus C. A significant loss of protein sulfhydryls in rat hepatocytes could be noted following a 60-minute incubation period with either AA (1 mM) or AA (1 mM) plus C (5 mM). Similarly, C produced a dose-and time-dependent potentiation of A-induced liver cytotoxicity, which was preceded by severe loss of NPSH content within 15 minutes of exposure, whereas the potentiation of lipid peroxidation (LPO) resulting from A plus C was found to be a relatively late event, as with AA plus C. Furthermore, combined treatment with AA and C produced a significantly higher cytotoxicity (as measured by cellular viability) than that due to the combined treatment with A plus C based on equimolar concentration. These results suggest that two increased bioactivation pathways of AA involving the P-450 mixed-function oxidase system resulting from C may be involved in the potentiation of AA hepatotoxicity.

Published

2001

25. SarA represses agr operon expression in a purified in vitro Staphylococcus aureus transcription system.

Author

Chakrabarti SK and Misra TK

Subjects

Bacterial Proteins genetics, Cloning, Molecular, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Escherichia coli genetics, Exotoxins genetics, Gene Expression Regulation, Bacterial, Genetic Complementation Test, Staphylococcus aureus growth & development, Suppression, Genetic, Bacterial Proteins metabolism, Operon, Promoter Regions, Genetic, Staphylococcus aureus genetics, Trans-Activators, Transcription, Genetic

Abstract

Mutation and genetic complementation studies suggested that two chromosomal loci, agr and sar, are involved in the upregulation of several exotoxin genes and the downregulation of a number of surface protein genes in a growth phase-dependent manner in Staphylococcus aureus. We purified recombinant T7-tagged SarA from Escherichia coli and determined its effect on transcription from several S. aureus promoters by using purified RNA polymerase reconstituted with either sigma(A) or sigma(B) from S. aureus. Of the seven sigma(A)-dependent promoters that we tested, SarA repressed transcription from agrP2, agrP3, cna, sarP1, and sea promoters and did not affect sec and znt promoters. Furthermore, SarA had no effect on transcription from the sigma(B)-dependent sarP3 promoter. In vitro experimental data presented in this report suggest that SarA expression is autoregulated.

Published

2000

26. Altered regulation of dopaminergic activity and impairment in motor function in rats after subchronic exposure to styrene.

Author

Chakrabarti SK

Subjects

Animals, Body Weight drug effects, Brain drug effects, Brain enzymology, Brain metabolism, Male, Neurotransmitter Agents metabolism, Rats, Rats, Sprague-Dawley, Tyrosine 3-Monooxygenase metabolism, Dopamine metabolism, Motor Activity drug effects, Receptors, Dopamine metabolism, Styrene pharmacology

Abstract

Animal and human studies suggest a dopamine-mediated effect of styrene neurotoxicity. However, the results reported to date are incomplete and not consistent. As such, the mechanism of its neurotoxicity is still unclear. The present study has, therefore, reexamined the central dopaminergic system in relation to some neurobehavioral effects in rats following subchronic exposure to styrene. Groups of adult male Sprague-Dawley rats received 0, 0.25, or 0.5 g styrene per kg b.wt. by gavage for 13 consecutive weeks. Twenty-four hours after cessation of such treatment with the higher dose (0.5 g/kg), the contents of dopamine (DA) and its metabolites were significantly reduced in the corpus striatum, hypothalamus, and lateral olfactory tract regions. In vitro styrene showed a significant increase in DA release from rat striatal synaptosomes similar to that of tyramine. Significant loss of motor function was observed on days 56, 70, and 84 during the styrene treatment with the higher dose, and lasted over a month after such treatment. However, the treated animals recovered their motor function within 45-60 days after cessation of such treatment, along with the recovery of normal levels of dopamine and its metabolites. Furthermore, styrene-induced initial impairments in measures of dopaminergic activity cannot be attributed to altered regulation of tyrosine hydroxylase activity. Specific [3H]-spiroperidol binding was also unaltered 7 or 15 days after subchronic treatment with styrene. These data imply that despite the dopaminergic neuronal loss due to styrene, dopaminergic transmission was not reduced to a level that would result in an overall development of dopamine receptor supersensitivity in the striatum. Collectively, these studies indicate that the subchronic neurotoxic action of styrene may be primarily presynaptic in nature and may involve impaired regulation of DA content and stimulation of DA release.

Published

2000

27. Effects of protein-deficient nutrition during rat pregnancy and development on developmental hindlimb crossing due to methylmercury intoxication.

Author

Chakrabarti SK and Bai C

Subjects

Animals, Ataxia chemically induced, Body Weight physiology, Brain metabolism, Dietary Proteins administration & dosage, Female, Hindlimb, Lactation, Mercury pharmacokinetics, Methylmercury Compounds pharmacokinetics, Nerve Tissue Proteins biosynthesis, Pregnancy, Pregnancy Complications metabolism, Pregnancy Complications physiopathology, Rats, Rats, Sprague-Dawley, Ataxia etiology, Methylmercury Compounds toxicity, Prenatal Exposure Delayed Effects, Protein-Energy Malnutrition complications

Abstract

Pregnant rats were fed either a control (20% protein) or low (3.5%) protein diet during gestation and lactation. The pups were separated from their mothers on postnatal day 21, and were given the same diet as their corresponding mothers. The groups of pups from each diet group were treated on either postnatal day 21 or postnatal day 60 with 7.5 mg methylmercury chloride (MeHgCl) per kg b.w. once daily by gavage for 10 consecutive days, and the development of ataxia (hind-limb crossing) was monitored. The offspring from mothers on the protein-deficient diet were found to be more sensitive to MeHg-induced ataxia than those on the protein-sufficient diet. The former accumulated more mercury in different brain regions than the latter. The rates of protein synthesis in different brain regions of the offspring fed the protein-deficient diet were significantly reduced compared with the rates in those fed the protein-sufficient diet. However, MeHg treatment did not significantly modify the rates of such protein synthesis further in protein-deficient rats. Thus, a significantly much higher inhibition of the intrinsic rates of protein synthesis in different brain regions due to severe protein deficiency, as observed in this study, may be partly responsible for the increased susceptibility of developing rats fed a protein-deficient diet to MeHg-induced ataxia, or hindlimb crossing, although other factor(s) might also be involved.

Published

2000

28. Purification and characterization of an extracellular alkaline serine protease from Aspergillus terreus (IJIRA 6.2).

Author

Chakrabarti SK, Matsumura N, and Ranu RS

Subjects

Centrifugation, Density Gradient, Chromatography methods, Electrophoresis, Polyacrylamide Gel methods, Gelatin, Hydrogen-Ion Concentration, Protease Inhibitors pharmacology, Serine Endopeptidases chemistry, Substrate Specificity, Temperature, X-Ray Film, Aspergillus enzymology, Serine Endopeptidases isolation & purification

Abstract

An extracellular alkaline serine protease has been purified from Aspergillus terreus (IJIRA 6.2). The purification procedure involved chromatography on DEAE-Sephadex A25, phosphocellulose, hydroxyapatite, casein-Sepharose, gel filtration on Sephacryl-S-300 and by glycerol density gradient centrifugation. The enzyme was further purified to apparent homogeneity through a combination of electrophoresis in polyacrylamide gel containing 0.1% sodium dodecyl sulfate (SDS) with or without protease substrate (gelatin) and subsequent regeneration of its activity in situ by removal of SDS. The active enzyme was visualized in a zymogram or on the basis of protease activity exhibited on an X-ray film. The protein in the unstained segment of the gel was electroeluted. The eluted protein with protease activity exhibited a molecular mass of 37,000-daltons on electrophoresis in SDS-polyacrylamide gel. A sedimentation coefficient of 3.2S was obtained by glycerol density gradient contrifugation. Maximum activity of protease was observed at pH 8.5 and at 37 degrees C. Purified protease was active between pH 5.5 and 9.5 and was found to be stable up to 60 degrees C. With Na-caseinate, the K(m) of the purified protease was found to be 0.055 mM. Antipain, phenylmethane sulfonyl fluoride, and chymostatin served as non-competitive inhibitors. Substrate specificity was determined by using a synthetic chromogenic peptide containing N-P-Tosyl-Gly-Pro-Arg-p-nitroanilide. Results showed that the protease cleaved the peptide on the -COOH end of arginine residue.

Published

2000

29. Role of oxidative stress in nickel chloride-induced cell injury in rat renal cortical slices.

Author

Chakrabarti SK and Bai C

Subjects

Animals, Antioxidants pharmacology, Free Radical Scavengers pharmacology, Glutathione metabolism, In Vitro Techniques, Ion Transport drug effects, Kidney Cortex metabolism, Kidney Cortex pathology, L-Lactate Dehydrogenase metabolism, Lipid Peroxidation drug effects, Male, Nickel metabolism, Rats, Rats, Sprague-Dawley, Reactive Oxygen Species metabolism, Sulfhydryl Compounds pharmacology, Kidney Cortex drug effects, Nickel pharmacology, Oxidative Stress physiology

Abstract

Nickel chloride (NiCl2) induced lactate dehydrogenase (LDH) release and lipid peroxidation (LPO) in rat renal cortical slices in vitro in a concentration- (0-2 mM) and time- (0-4 hr) dependent manner, with initial significant LDH release occurring as early as 1 hr, whereas significant increase in LPO started 3 hr after exposure, suggesting that LPO results from renal cell injury. Both NiCl2-induced LDH release and LPO were prevented significantly by glutathione and dithiothreitol, suggesting that NiCl2-induced renal cell injury is dependent on thiols. However, such injury is not dependent solely on thiols, because (a) these thiols failed to inhibit completely the uptake of Ni2+ by the renal cortex, and (b) diethylmaleate pretreatment failed to increase NiCl2-induced cell injury further. Superoxide dismutase partially reduced the NiCl2-induced LDH release without affecting LPO and glutathione, whereas catalase did not affect such LDH release and LPO. Dimethylthiourea and DMSO completely prevented NiCl2-induced LPO, but only partially reduced LDH release. Deferoxamine prevented NiCl2-induced renal cell injury without affecting LPO and without significantly reducing Ni2+ uptake by the renal cortex, suggesting that nickel chelation is not important in such prevention of injury. NiCl2-induced inhibition of para-aminohippurate uptake was prevented significantly by thiols, deferoxamine, and dimethylthiourea. NiCl2-induced loss of cellular glutathione content was prevented significantly by thiols and deferoxamine, but not by superoxide dismutase and dimethylthiourea. These results suggest that LPO was not related to NiCl2-induced lethal renal cell injury, whereas such injury may be caused by the induction of the Fenton reaction, generating hydroxyl radicals.

Published

1999

30. Biphasic biomethanation of wood-hydrolysate effluent.

Author

Chakrabarti SK, Roychoudhury PK, and Bajpai PK

Subjects

Animals, Biomass, Bioreactors, Carboxylic Acids metabolism, Environmental Pollution, Euryarchaeota, Hydrogen-Ion Concentration, Methanosarcina metabolism, Methanosarcinaceae metabolism, Oxidation-Reduction, Polysaccharides metabolism, Refuse Disposal economics, Solutions, Temperature, Methane metabolism, Refuse Disposal methods, Wood

Abstract

The dissolving pulp industry, spread throughout the world, is the principal source of wood-hydrolysate effluent rich in hemicelluloses. This effluent is the major source of pollution in the industry. COD and BOD5 values of the effluent range from 60,000 to 103,000 and 42,000 to 78,000 mg/l respectively. Biomethanation of this effluent is the best possible treatment option for reducing the COD load and recovering the bioenergy embedded in the effluent. This paper deals with the study on the biphasic biomethanation of the wood-hydrolysate in upflow acidogenic reactor coupled with anaerobic filter methanogenic reactor. The two reactors were operated at organic loading rates of 69.6 and 30.1 g COD/l/d respectively. The overall COD, hemicelluloses and lignin reductions, and methane generation were observed to be 88%, 92%, 82% and 6.5 l/l reactor volume/d respectively. The relative size of the biphasic, anaerobic filter (mono-phasic) and upflow anaerobic sludge blanket (mono-phasic) reactors is found to be 1:1.6:2.03 respectively.

Published

1999

31. Toxicity and bioaccumulation of nickel sulfate in Sprague-Dawley rats following 13 weeks of subchronic exposure.

Author

Obone E, Chakrabarti SK, Bai C, Malick MA, Lamontagne L, and Subramanian KS

Subjects

Analysis of Variance, Animals, Body Weight drug effects, DNA Damage, Drinking, Environmental Pollutants pharmacokinetics, Kidney drug effects, Kidney metabolism, Liver drug effects, Liver metabolism, Lung drug effects, Lung metabolism, Male, Nervous System drug effects, Nervous System metabolism, Nickel pharmacokinetics, Organ Size drug effects, Rats, Rats, Sprague-Dawley, Specific Pathogen-Free Organisms, Spleen cytology, Spleen drug effects, Spleen metabolism, T-Lymphocyte Subsets drug effects, Testis drug effects, Testis metabolism, Tissue Distribution, Environmental Pollutants toxicity, Nickel toxicity

Abstract

Adult male Sprague-Dawley rats were given 0, 0.02, 0.05, and 0.1% nickel sulfate (NiSO4-6H2O) or 0, 44.7, 111.75, and 223.5 mg Ni/L, respectively, in their drinking water for 13 wk. Twenty-four hours following the end of such treatment, all animals survived and no apparent clinical signs of toxicity were noted. The final mean body weights of various nickel sulfate-treated rats were not significantly decreased except for the 0.1% nickel sulfate treated group when compared to those in the control. The absolute and relative organ weights were either increased or decreased or remained unchanged, depending on the organ and the dose of nickel sulfate. Total plasma proteins, plasma albumin and globulins, and plasma glutamic pyruvic transaminase activity were all significantly decreased in 0.1% nickel sulfate-treated rats. Lymphocyte subpopulations (T and B cells) were induced at lower dose levels, but suppressed at the highest (0.1%) dose group. A significant decrease in urine volume and an increase in BUN were observed at the highest dose group. Biochemical analysis of bronchoalveolar lavage fluid and lung tissue showed some lung damage, whereas no damage to the testis or DNA in liver and kidneys were found. No gross or microscopic changes were seen in any of the various tissues examined. The relative order of bioaccumulation of nickel in different organs of rats when treated at 0.1% nickel sulfate (223.5 mg Ni/L) was kidneys > testes > lung = brain > spleen > heart = liver. But with regard to order of toxicity, both immune and pulmonary systems were found to be very sensitive targets, followed by kidney.

Published

1999

32. Styrene and styrene oxide affect the transport of dopamine in purified rat striatal synaptic vesicles.

Author

Chakrabarti SK

Subjects

Animals, Biological Transport drug effects, Biological Transport physiology, Humans, Rats, Synapses physiology, Dopamine physiology, Epoxy Compounds pharmacology, Mutagens pharmacology, Styrene pharmacology, Synaptic Vesicles physiology, Visual Cortex physiology

Abstract

Animal and human studies suggest a dopamine-mediated effect of styrene neurotoxicity. To date, mechanisms of cerebral membrane transport of neurotransmitter amines in the presence of styrene in relation to its neurotoxicity have not been addressed properly. So, the present study has examined to test the hypothesis that dopaminergic malfunction in vesicular transport is a critical component in styrene-induced neurotoxicity in rats. Both styrene and its intermediate reactive metabolite, styrene oxide antagonized the in vitro striatal binding of [3H] tyramine, a putative marker of the vesicular transporter for dopamine. Both styrene and styrene oxide potently inhibited the uptake of [3H] dopamine in purified synaptic vesicles prepared from rat brain striata, in a dose-related manner, with inhibitory constants (Ki) 2.5 and 2.2 microM respectively. However, neither styrene nor styrene oxide significantly increased the basal efflux of [3H] dopamine that has been preloaded into striatal vesicles in vitro. On the other hand, both styrene and styrene oxide have failed to significantly inhibit the uptake of either [3H] norepinephrine, or [3H] serotonin into striatal synaptic vesicles. It is concluded that both styrene and styrene oxide are capable of producing impairments in dopaminergic transport in purified striatal synaptic vesicles, an effect which may be a critical component in styrene-induced neurotoxicity., (Copyright 1999 Academic Press.)

Published

1999

33. DNA-Protein crosslinks induced by nickel compounds in isolated rat renal cortical cells and its antagonism by specific amino acids and magnesium ion.

Author

Chakrabarti SK, Bai C, and Subramanian KS

Subjects

Animals, Binding, Competitive, Calcium pharmacology, Cell Survival drug effects, Cells, Cultured, Cross-Linking Reagents toxicity, DNA metabolism, Dose-Response Relationship, Drug, Kidney Cortex metabolism, Male, Nickel antagonists & inhibitors, Nickel metabolism, Protein Binding drug effects, Proteins metabolism, Rats, Rats, Sprague-Dawley, Reactive Oxygen Species physiology, Amino Acids pharmacology, DNA drug effects, Kidney Cortex drug effects, Magnesium pharmacology, Nickel toxicity, Proteins drug effects

Abstract

Suspensions of isolated renal cortical cells in modified Krebs-Henseleit buffer (pH 7.4) were incubated with nickel chloride, nickel acetate, nickel sulfate, and nickel subsulfide (0-2 mM) at 37 degreesC for 2 h. A significant increase (63%) in DNA-protein crosslinks was observed at 2 mM nickel sulfate, whereas nickel subsulfide induced a significant increase in such crosslinks beginning at 0.5 mM concentration and a maximum increase of 200% of the control value reached at 2 mM concentration. No significant reduction in viability of renal cortical cells (as measured by trypan blue exclusion) was observed due to these nickel compounds at any concentration used. In the second series of experiments, coincubation of nickel subsulfide (2 mM) with l-histidine (8 or 16 mM), l-cysteine (4 or 8 mM), or l-aspartic acid (8 or 24 mM) significantly reduced the DNA-protein crosslinks induced by 2 mM nickel subsulfide. Similarly Mg2+ (24 mM), but not Ca2+ (24 mM), was able to antagonize nickel subsulfide-induced increase in DNA-protein crosslinks. High extracellular levels of Mg2+ and these amino acids significantly decreased the accumulation of Ni2+ from nickel subsulfide in renal cortical cells. Furthermore, these amino acids at high concentrations significantly inhibited the binding of Ni2+ from nickel subsulfide to deproteinized DNA from renal cortical cells, whereas such inhibition due to Mg2+ was close to significant (0.1 > p > 0.05). In vitro exposures of renal cortical cells to nickel subsulfide (0-2 mM) increased the formation of reactive oxygen species in concentration-dependent manner. Furthermore, coincubation of 2 mM nickel subsulfide with either catalase, dimethylthiourea, mannitol, or vitamin C at 37 degreesC for 2 h resulted in a significant decrease of nickel subsulfide-induced formation of DNA-protein crosslinks, suggesting that nickel subsulfide-induced DNA-protein crosslink formation in isolated rat renal cortical cells is caused by the formation of reactive oxygen species. The potent protective effects of these specific amino acids and Mg2+ against nickel subsulfide-induced DNA-protein crosslink formation in isolated renal cortical cells are due to reduction of cellular uptake of Ni2+ and inhibition of the binding of Ni2+ to deproteinized DNA., (Copyright 1999 Academic Press.)

Published

1999

34. S-[(1 and 2)-phenyl-2-hydroxyethyl]cysteine-induced alterations in renal mitochondrial function in male Fischer-344 rats.

Author

Chakrabarti SK, Denniel C, Malick MA, and Bai C

Subjects

Animals, Cysteine administration & dosage, Cysteine toxicity, Dose-Response Relationship, Drug, Enzyme Inhibitors administration & dosage, In Vitro Techniques, Injections, Intravenous, Ketoglutaric Acids pharmacology, Kidney Cortex metabolism, Kidney Cortex pathology, Malates pharmacology, Male, Mitochondria enzymology, Mitochondria pathology, Mitochondrial ADP, ATP Translocases antagonists & inhibitors, NADH Dehydrogenase antagonists & inhibitors, Oxidative Phosphorylation drug effects, Oxygen Consumption drug effects, Rats, Rats, Inbred F344, Succinate Dehydrogenase antagonists & inhibitors, Succinic Acid pharmacology, Cysteine analogs & derivatives, Enzyme Inhibitors toxicity, Kidney Cortex drug effects, Mitochondria drug effects

Abstract

Previous studies from our laboratory have shown that mitochondrial dysfunction may be an important early event in S-[(1 and 2)-phenyl-2-hydroxyethyl]cysteine (PHEC)-induced cytotoxicity in isolated rat renal proximal tubules. The present study has therefore examined in more detail PHEC-induced mitochondrial dysfunction, both in vivo and in vitro, using isolated renal cortical mitochondria. Renal cortical mitochondria isolated from PHEC-treated rats in vivo showed depressed effects on the mitochondrial respiration and oxidative phosphorylation in both a dose (0, 250, and 500 micromol/kg iv)- and time (0-24 h)-dependent manner in the presence of both succinate (Site 2) and malate plus alpha-ketoglutarate (Site 1) as respiratory substrates, with initial significant depression occurring as early as 4 h following treatment with 500 micromol PHEC/kg. Similar mitochondrial dysfunctions were observed in vitro in concentration- and time-dependent manners with both respiratory substrates. PHEC also caused a marked dose-dependent inhibition of mitochondrial succinate dehydrogenase and NADH cytochrome c reductase activities both in vivo and in vitro, with initial inhibition occurring as early as 4 h after in vivo administration and 45 min after exposure to PHEC in vitro, while the NADH dehydrogenase activity was not considerably inhibited. The mitochondrial ATPase activity was significantly decreased 4 and 24 h following treatment with PHEC (500 micromol/kg). These results suggest that PHEC exerts its inhibitory effect on the mitochondrial respiration and oxidative phosphorylation through the action on the mitochondrial electron transport chain. PHEC significantly reduced the activity of adenine nucleotide translocase as well as the net uptake of substrates by mitochondria without affecting their efflux within 2-4 h after its injection (500 micromol/kg). On the other hand, significant renal damage, as assessed by morphological study, appeared as early as 24 h following such treatment. The observation of similar effects after both in vivo and in vitro exposures may suggest that the effect on mitochondria may have a pathogenic role in PHEC-induced renal injury in rats. PHEC produces mitochondrial toxicity that results from an inactivation of mitochondrial anionic substrate transporters as well as from an inhibition of activities of adenine nucleotide translocase and dehydrogenases., (Copyright 1998 Academic Press.)

Published

1998

35. Modulation of monoamine oxidase activity in different brain regions and platelets following exposure of rats to methylmercury.

Author

Chakrabarti SK, Loua KM, Bai C, Durham H, and Panisset JC

Subjects

Animals, Blood Platelets enzymology, Brain enzymology, Male, Rats, Rats, Sprague-Dawley, Synaptosomes drug effects, Synaptosomes enzymology, Blood Platelets drug effects, Brain drug effects, Methylmercury Compounds pharmacology, Monoamine Oxidase metabolism

Abstract

Monoamine oxidase (MAO; EC 1.4.3.4) is known to have an important role in the regulation of biogenic amines in the brain and peripheral tissues. It is also known that circulating platelets represent an excellent model for an easy assessment of the effect of MAO-B inhibitors in extracerebral tissue. The present study was carried out to determine the effects of methylmercury (MeHg) on the activity of MAO in synaptosomes of different brain regions of male Sprague-Dawley rats as well as in rat blood platelets both in vitro and in vivo. MeHg pretreatment inhibited the activity of MAO in the synaptosomes of the cortex, hypothalamus, hippocampus, striatum, cerebellum, and brain stem in a concentration-dependent (0-10 microM) manner. The threshold concentration of MeHg for such inhibition in different brain synaptosomes was found to be the same (i.e., 1 microM) except for in the rat striatum it was 2.5 microM, and the IC50 value for MeHg was found to be around 2.1 microM. Significant inhibition of the MAO activity was also observed in synaptosomes of the cortex, cerebellum, hypothalamus, and hippocampus as well as in platelets of rats 24 h after treatment by gavage with a total cumulative dose of 35 mg/kg (5 mg/kg/day for 7 days). The decrease of such activity was found to be at maximum in different brain synaptosomes and platelets 24 h following treatment with a cumulative total dose of 75 mg/kg (7.5 mg/kg/day for 10 days); the treated animals showed signs of ataxia under these conditions. The data have further shown that methylmercury is capable of inhibiting the MAO activity in different brain synaptosomes to different degrees but without showing any specificity towards any specific brain region. The present in vivo results suggest that the platelet MAO activity may be used as a potential biomarker of early neurotoxicity due to repeated exposure to MeHg in rats.

Published

1998

36. S-[(1 and 2)-phenyl-2-hydroxyethyl]-cysteine-induced cytotoxicity to rat renal proximal tubules.

Author

Chakrabarti SK and Denniel C

Subjects

Animals, Cell Death drug effects, Cell Survival drug effects, Cells, Cultured, Cysteine metabolism, Cysteine toxicity, Fructose pharmacology, Glutathione metabolism, Intracellular Membranes drug effects, Intracellular Membranes physiology, Kidney Tubules, Proximal metabolism, Kidney Tubules, Proximal ultrastructure, Lipid Peroxidation drug effects, Male, Membrane Potentials drug effects, Mitochondria drug effects, Mitochondria physiology, Oxygen Consumption drug effects, Rats, Rats, Inbred F344, Cysteine analogs & derivatives, Kidney Tubules, Proximal drug effects

Abstract

S-[(1 and 2)-phenyl-2-hydroxyethyl]-glutathione is nephrotoxic in rats through its metabolic conversion to corresponding cysteine-S-conjugate, e.g., S-[(1 and 2)-phenyl-2-hydroxyethyl]-cysteine (PHEC). The present study was carried out to determine the mechanism of PHEC-induced toxicity in isolated rat renal proximal tubules. PHEC decreased tubule viability in concentration (0-2 mM)- and time (0-3 hr)-dependent manner, with initial decreases occurring 2 hr after exposure. Tubule basal and nystatin-stimulated oxygen consumption decreased before cell death following exposure to 0.5 and 1 mM PHEC. Assessment of direct mitochondrial function within the proximal tubules showed that respiration was reduced in the absence and presence of a phosphate acceptor using site II (succinate) and site I (malate/glutamate) respiratory substrates 30 and 45 min after exposure to 0.5 and 1 mM PHEC. Exposure of proximal tubules to 1 mM PHEC caused a time-dependent decline of mitochondrial membrane potential (as measured by the uptake of the cationic fluorescent dye, rhodamine 123 by the proximal tubules) and depletion of ATP content with initial decrease occurring as early as 30 min after the exposure. Glutathione depletion and lipid peroxidation occurred within 90 min clearly preceding cell death after exposure to 0.5 and 1 mM PHEC. Pretreatment with 1 mM deferoxamine prevented PHEC-induced lipid peroxidation but did not prevent PHEC-induced cytotoxicity, whereas deferoxamine pretreatment prevented lipid peroxidation, mitochondrial dysfunction, and cytotoxicity after exposure to 0.5 mM tertiary-butyl hydroperoxide, suggesting that iron-mediated lipid peroxidation does not contribute to PHEC-induced proximal tubule cell death. Pretreatment of renal proximal tubules with 10 mM fructose failed to prevent the change in mitochondrial membrane potential, the ATP depletion and cytotoxicity caused by 1 mM PHEC, indicating that the glycolytic pathway is not important in renal proximal tubule respiration and cell injury. Pretreatment of renal tubules with aminooxyacetic acid failed to prevent the mitochondrial dysfunction induced by 1 mM PHEC, indicating an absence of further metabolism of PHEC by a beta-lyase-dependent pathway. It is therefore proposed that the alteration of mitochondrial functions and the consequent loss of cellular energy supplies can represent the mechanisms by which PHEC expressed its acute cytotoxicity.

Published

1996

37. A monoclonal antibody to a cytoskeletal protein selectively recognizing malignant neuroectodermal tumors.

Author

Chakrabarti SK, Sil M, Poddar R, and Sarkar PK

Subjects

Adult, Animals, Antibody Specificity, Brain embryology, Brain immunology, Brain Neoplasms immunology, Child, Fluorescent Antibody Technique, Ganglia, Sympathetic immunology, Humans, Hybridomas immunology, Lymphoma immunology, Mice, Mice, Inbred BALB C, Neuroectodermal Tumors classification, Organ Specificity, Tumor Cells, Cultured, Viscera immunology, Antibodies, Monoclonal immunology, Antibodies, Neoplasm immunology, Antigens, Neoplasm immunology, Cytoskeletal Proteins immunology, Neoplasm Proteins immunology, Neuroectodermal Tumors immunology

Abstract

Fusion of myeloma (P3X63-Ag 8.653) cells with spleen cells from BALB/c mice immunized with human neuroblastoma (SK-N-SH) cells yielded a hybridoma clone, referred to as 3XB7, with a unique pattern of reactivity to malignant neuroectodermal tumors except gliomas of low-grade malignancy. Indirect immunofluorescence staining under different conditions and Western blot analysis indicate that the 3XB7 MAb recognizes an intracellular cytoskeletal protein of M(r) 52K. Immunohistochemical studies with cryostat and paraffin-embedded sections from tumor biopsies revealed that the 3XB7 MAb specifically recognizes malignant neuroectodermal tumors and reacts negatively with other epithelial and mesenchymal tumors, e.g., carcinomas, lymphomas, and sarcomas as well as with normal adult and fetal brain tissues. Negative reaction was also observed with other small round cell tumors of childhood. Thus the 3XB7 antigen can be used for diagnosis of all stages of neuroblastomas, and its specific expression in gliomas with high-grade malignancy (grades III and IV) confer on it additional prognostic value.

Published

1994

38. Dynamics of Flux Tubes in Thick Accretion Disks.

Author

D'Silva S and Chakrabarti SK

Published

1993

39. Effects of fasting on the diuretic response and disposition of furosemide in rats.

Author

Chakrabarti SK and Brodeur J

Subjects

Animals, Biological Transport, Active, Fatty Acids, Nonesterified blood, Furosemide blood, Furosemide metabolism, In Vitro Techniques, Kidney metabolism, Liver metabolism, Male, Natriuresis drug effects, Rats, Diuresis drug effects, Fasting, Furosemide pharmacology

Abstract

The influence of fasting on the relationship between the disposition and diuretic effect of furosemide was studied in rats. Fasting consisted of withholding solid food, but not water, for a period of 16 h before administering furosemide (10 mg/kg, sc) or a saline vehicle. Normally fed animals also received furosemide or the vehicle. Fasting did not modify the diuretic or the natriuretic effect (per 100 g body weight) of furosemide. The distribution of total furosemide in plasma or tissues was not affected by fasting. On the other hand, fasting which produced increasing amounts of endogenous free fatty acids in plasma and kidneys increased the concentration of free furosemide in fasting plasma but not in fasting kidney or liver of rats. The in vitro binding constant of furosemide to physiological concentrations of plasma proteins was decreased from the control value by a factor of 6.5 as a result of fasting. Neither unchanged furosemide nor its metabolite in the urine was affected by fasting. Incubation of kidney cortex tissue slices with furosemide both in the presence and absence of free fatty acid indicated an inhibition of furosemide uptake in a manner closely parallel to inhibition by probenecid. Thus, failure to observe a more pronounced diuretic and saluretic effects of furosemide in fasted rats, in spite of higher concentration of free plasma furosemide, might be due to the inhibitory effect of endogenous free fatty acids and (or) other endogenous substances on the uptake of furosemide by renal tubular cells although some homeostatic control mechanisms related to fasting could also be involved.

Published

1980

40. Loss of plasmid linked drug resistance after treatment with Iodo-deoxyuridine.

Author

Chakrabartty PK, Mishra AK, and Chakrabarti SK

Subjects

Escherichia coli drug effects, Escherichia coli genetics, Idoxuridine pharmacology, R Factors drug effects

Published

1984

41. Dose-dependent metabolism of trichloroethylene and its relevance to hepatotoxicity in rats.

Author

Rouisse L and Chakrabarti SK

Subjects

Aminopyrine N-Demethylase metabolism, Aniline Hydroxylase metabolism, Animals, Cytochrome P-450 Enzyme System metabolism, Glutathione metabolism, Injections, Intraperitoneal, Liver drug effects, Male, Microsomes, Liver enzymology, Rats, Rats, Inbred Strains, Transaminases blood, Trichloroethylene toxicity, Liver metabolism, Trichloroethylene metabolism

Abstract

Fasted male Sprague-Dawley rats pretreated with phenobarbital received an intraperitoneal injection of 0.00, 0.25, 0.50, 0.75, 1.00, 1.50, or 2.00 ml/kg of trichloroethylene (TRI) in corn oil. The metabolic fate of TRI was monitored by measuring its major urinary metabolites 24 hr following the dosing. The hepatotoxic response of TRI was evaluated by determination of the serum transaminase activities (SGOT and SGPT) 24 hr after dosing. Treatment of rats with TRI up to 0.5 ml/kg did not affect the transaminase responses, but significant response was manifested at 0.75 ml/kg dose. Further continuous increases in such responses were induced on exposure to higher doses. Dose-dependent urinary excretions of trichloroethanol and trichloroacetic acid were observed and reached an apparent saturation at 1-1.5 ml/kg dose of TRI. The percentage of dose excreted as trichloroethanol was decreased from 16% at 0.25 ml or 2.8 mmole/kg to 8% at 2 ml or 22.3 mmole/kg dose. The percentage of trichloroacetic acid was decreased from 5 to 2% for the same dose interval. A maximum of only 29% depletion of hepatic glutathione was observed at 2 hr following 1 ml/kg dose of TRI. Similarly, the excretion of urinary mercapturic acid of TRI or thioether was insignificant at any dose level. These results suggest that the conjugation of hepatic glutathione with the electrophilic intermediate of TRI does not seem to be an important determinant for TRI hepatotoxicity nor the major detoxification pathway of its reactive intermediate. TRI produced also a dose-dependent decrease in hepatic microsomal monooxygenase activities as well as cytochrome P-450 content. All these results, when combined, show that there exists an apparent saturable metabolism of TRI involving its activation/deactivation pathways which correspond to an apparent threshold or minimal toxic dose, about 1 ml/kg or 11.15 mmole/kg of TRI for its hepatotoxicity.

Published

1986

42. Cooperativity of warfarin binding with human serum albumin induced by free fatty acid anion.

Author

Chakrabarti SK

Subjects

Humans, Kinetics, Protein Binding drug effects, Protein Conformation, Fatty Acids, Nonesterified pharmacology, Serum Albumin metabolism, Warfarin blood

Published

1978

43. Influence of heavy metals on the in vitro interaction between human serum albumin and warfarin.

Author

Chakrabarti SK

Subjects

Cadmium pharmacology, Drug Interactions, Humans, In Vitro Techniques, Lead pharmacology, Mercury pharmacology, Protein Binding drug effects, Zinc pharmacology, Metals pharmacology, Serum Albumin metabolism, Warfarin blood

Published

1978

44. Influence of mercury of the anesthetic response to and distribution of thiopental in rats.

Author

Chakrabarti SK

Subjects

Animals, Blood Proteins metabolism, Drug Synergism, Male, Protein Binding, Rats, Sleep drug effects, Anesthesia, Mercury toxicity, Thiopental metabolism

Abstract

Pretreatment with HgCl2 (2 mg/kg sc) 24 h before administration of thiopental (35 mg/kg ip) significantly potentiated the duration of thiopental sleeping time in adult male rats but did not influence the onset time for anesthesia. The plasma concentration of free thiopental was significantly higher in the Hg-treated animals 15 and 45 min after thiopental injection (i.e., during the period of thiopental anesthesia), with a concomitant increase of the free thiopental concentration in the brain at 15 min. However, total and free brain thiopental concentrations in Hg-treated rats at the time of awakening were not different from those in saline-treated animals. Urinary thiopental remained unchanged from 0 to 2 h, but was increased in the treated urine from 0 to 27 h. In vitro studies showed a strong inhibition of thiopental binding in 24-h Hg-treated plasma. The results suggest that the prolongation of thiopental anesthesia induced by Hg pretreatment is probably related to changes in the disposition of thiopental in the plasma and brain rather than to an alteration in the sensitivity of the central nervous system.

Published

1981

45. Studies of acute nephrotoxic potential of trichloroethylene in Fischer 344 rats.

Author

Chakrabarti SK and Tuchweber B

Subjects

Administration, Oral, Animals, Injections, Intraperitoneal, Kidney metabolism, Male, Maximum Allowable Concentration, Rats, Rats, Inbred F344, Trichloroethylene administration & dosage, Trichloroethylene metabolism, Kidney drug effects, Trichloroethylene toxicity

Abstract

Group of male Fischer 344 rats, after pretreatment with phenobarbital (80 mg/kg, ip, 3 d), were treated ip in corn oil with 0, 5.5, 11.0, and 22.0 mmol trichloroethylene (TRI) per kg body weight. Urines were collected 24 h after the treatment and the animals were then sacrificed. The nephrotoxicity of TRI was then studied by measuring certain biochemical parameters characteristic of renal injury and its in vivo metabolism by quantitating the TRI principal urinary metabolites. Treatment of rats with TRI up to 11 mmol/kg did not influence any of the measured biochemical parameters of nephrotoxicity. On the other hand, significant increases in the urinary level of N-acetyl-beta-glucose-D-aminidase (NAG) and glucose as well as serum urea nitrogen were observed at 24 h only at the highest dose level (22 mmol/kg) or TRI. Urinary excretions of both trichloroethanol and trichloroacetic acid reached an apparent saturation at the highest dose level of TRI. In inhalation studies, urinary levels of gamma-glutamyltranspeptidase, NAG, glucose, proteins, and serum urea nitrogen were significantly increased at 24 h when rats were exposed to either 1000 or 2000 ppm TRI for 6 h. The capacity of renal cortical slices to accumulate p-aminohippurate was significantly reduced 24 h after the exposure to 22 mmol TRI/kg (ip), or to 1000 or 2000 ppm TRI. These results have demonstrated that TRI exerts its acute nephrotoxic potential at a very high dose level and produces nephrotoxic insult at the proximal tubular and possibly glomerular regions of the rat kidney, whether exposed by inhalation or by an ip route. These data further indicate an involvement of a capacity-limited metabolism in the expression of acute nephrotoxicity due to TRI in Fischer 344 rats.

Published

1988

46. Studies on the subchronic nephrotoxic potential of styrene in Sprague-Dawley rats.

Author

Chakrabarti SK, Labelle L, and Tuchweber B

Subjects

Animals, Kidney metabolism, Kidney pathology, Kidney Tubules, Proximal drug effects, Kidney Tubules, Proximal ultrastructure, Male, Rats, Rats, Inbred Strains, Styrene, Time Factors, Urine drug effects, Kidney drug effects, Styrenes toxicity

Abstract

The nephrotoxic potential low non-toxic dose of styrene was studied in male Sprague-Dawley rats. Groups of rats received i.p. injections of styrene in corn oil at doses 0, 2.9, and 5.8 mmol/kg once daily, 5 days/week for 6 consecutive weeks. After collection of urine for 0-24 and 24-48 h following the end of the treatment, the rats were sacrificed. A significant increase in the excreted urinary volume was noticed at 5.8 mmol styrene during 0-24 and 24-48 h, relative to control, whereas urinary concentrations of gamma-glutamyl transpeptidase and glucose were significantly elevated during the 24-48-h period. Urinary activity of N-acetyl-beta-D-glucosaminidase was increased at the higher dose of styrene during 0-24 and 24-48 h. The capacity of renal cortical slices to accumulate p-aminohippurate was significantly reduced 48 h after the exposure to any dose of styrene. Electron microscopic examination of renal cortex 48 h after the exposure to a higher dose revealed the presence of enlarged mitochondria having more electron dense matrix. The data suggest that subchronic exposure to a very low non-toxic dose of styrene may have the potential to elicit nephrotoxicity preferentially in the proximal tubular region of the rat kidney.

Published

1987

47. Subunit dissociation of mitochondrial malate dehydrogenase.

Author

Shore JD and Chakrabarti SK

Subjects

Animals, Drug Stability, Energy Transfer, Fluorescamine, Fluoresceins, Macromolecular Substances, NAD metabolism, Protein Binding, Protein Conformation, Rhodamines, Spectrometry, Fluorescence, Swine, Malate Dehydrogenase metabolism, Mitochondria, Muscle enzymology, Myocardium enzymology

Abstract

Fluorescence polarization studies of porcine mitochondrial malate dehydrogenase labeled with fluorescein isothiocyanate or fluorescamine indicated a concentration-dependent dissociation of the dimeric molecule with a KD OF 2 X 10(7) N at pH 8.0. These results were confirmed by the concentration dependence of the stability of the enzyme at elevated temperatures and the creation of hybrid molecules with fluorescein and Rhodamine B labeled subunits, in which energy transfer was observed. The binding of NADH resulted in a small shift of the subunit dissociation curve toward monomer, demonstrating that monomer has twice the affinity for reduced coenzyme. NAD+ binding prevented dissociation of the dimer, even at concentrations below 10(-8) N. These results indicate that binding of reduced or oxidized coenzymes results in different conformation changes, which are transferred to the subunit interface.

Published

1976

48. Observation on second heterotypic dengue virus infection in mice.

Author

Sarkar JK, Das BC, Mukherjee KK, and Chakrabarti SK

Subjects

Animals, Blood Cell Count, Blood Coagulation, Blood Platelets, Dengue blood, Hemorrhage pathology, Mice, Dengue pathology

Published

1976

49. Fluorometric determination of delta-aminolaevulinate dehydratase activity in human erythrocytes as an index to lead exposure.

Author

Chakrabarti SK, Brodeur J, and Tardif R

Subjects

Colorimetry, Environmental Exposure, Humans, Kinetics, Lead blood, Spectrometry, Fluorescence methods, Erythrocytes enzymology, Hydro-Lyases blood, Lead Poisoning diagnosis, Porphobilinogen Synthase blood

Abstract

We describe a fluorometric method for determining delta-aminolaevulinate dehydratase (EC 4.2.1.24) activity in human erythrocytes and compare it with the existing colorimetric method. Incubation conditions are identical. In the proposed method, the porphobilinogen formed during incubation is converted to a stable and highly fluorescent uroporphyrin by heating for 20 min at 93 degrees C in an acidic medium in the presence of air. The correlation between results by the two methods was good (r = 0.89). We found a good negative correlation between the activity of the enzyme and the concentration of circulating lead with both methods (r = -0.61 for present method and -0.59 for colorimetric method) for groups of persons subjected to various degrees of lead exposure. Our method is more sensitive and accurate, requires less sample, and the fluorescence is more stable than is the color in the colorimetric method.

Published

1975

50. Effects of various pretreatments on the acute nephrotoxic potential of styrene in Fischer-344 rats.

Author

Chakrabarti SK and Tuchweber B

Subjects

Animals, Dose-Response Relationship, Drug, Drug Synergism, Enzyme Induction drug effects, Glutathione metabolism, Kidney pathology, Maleates pharmacology, Microsomes, Liver enzymology, Microsomes, Liver metabolism, Mixed Function Oxygenases antagonists & inhibitors, Mixed Function Oxygenases metabolism, Rats, Rats, Inbred F344, Styrene, Kidney drug effects, Styrenes toxicity

Abstract

The effects of various inducers and inhibitors of hepatic microsomal mixed-function oxidase (MFO) system and diethylmaleate treatment on styrene-induced acute nephrotoxicity in male Fischer-344 rats were studied. Groups of rats were pretreated with either 3-methylcholanthrene (15 mg/kg, i.p., 3 days), or phenobarbital (80 mg/kg, i.p., 3 days), or SKF525-A (50 mg/kg, i.p., 1 h), or piperonyl butoxide (300 mg/kg, i.p., 2 h), or diethylmaleate (400 mg/kg, i.p., 90 min) prior to an i.p. administration of styrene (0, 0.6 and 0.9 g/kg) in corn oil. The uptake of p-aminohippurate (PAH) by renal cortical slices, the morphology of renal cortices, as well as urinary excretion of N-acetyl-beta-D-glucosaminidase (NAG) and gamma-glutamyl transpeptidase (gamma-GT) of control and pretreated rats were examined 24 h after styrene. The inducers and inhibitors of MFO system failed to modify further the acute nephrotoxicity of styrene. On the other hand, diethylmaleate pretreatment not only reduced further the uptake of PAH, but also produced further significant increase in the urinary excretion of NAG and gamma-GT observed at the higher dose of styrene. Similarly, ultrastructural studies showed a moderate increase in the severity of kidney damage induced at the higher dose of styrene due to pretreatment with diethylmaleate. These data suggest that tissue glutathione concentrations and hence, corresponding conjugating activity might be important determinants of styrene nephrotoxicity. The results further indicate that a metabolic activation system not involving certain cytochrome P-450 might be responsible in styrene-induced nephrotoxicity.

Published

1987