Your search keyword '"M T, Alam"' showing total 18 results

1. Moringa oleifera seed lectin inhibits Ehrlich ascites carcinoma cell growth by inducing apoptosis through the regulation of Bak and NF-κB gene expression

Author

Ranajit Kumar Shaha, M T Alam, Aninda Chakrabortty, Sadnima Zaman, K.M. Ahsanul Kabir, Imtiaj Hasan, A.K.M. Asaduzzaman, Md. Nurujjaman, Fazle Rabbi Shakil Ahmed, Syed Rashel Kabir, Md. Belal Uddin, and Shaikh Shohidul Islam

Subjects

0301 basic medicine, Protein Denaturation, Hemagglutination, Cell, Apoptosis, Biology, Biochemistry, Ehrlich ascites carcinoma, Flow cytometry, 03 medical and health sciences, Mice, 0302 clinical medicine, Structural Biology, Cell Line, Tumor, Lectins, medicine, Animals, Carcinoma, Ehrlich Tumor, Molecular Biology, Cell Shape, Cell Proliferation, Moringa oleifera, medicine.diagnostic_test, Cell growth, NF-kappa B, Temperature, Lectin, General Medicine, Cell Cycle Checkpoints, Cell cycle, Hydrogen-Ion Concentration, Molecular biology, Caspase Inhibitors, Gene Expression Regulation, Neoplastic, 030104 developmental biology, medicine.anatomical_structure, bcl-2 Homologous Antagonist-Killer Protein, 030220 oncology & carcinogenesis, Seeds, biology.protein

Abstract

A Moringa oleifera seed lectin (MOSL) was purified by using chitin column with the molecular mass of 17±1kDa. The lectin agglutinated mouse, cow and human erythrocytes and the hemagglutination activity was inhibited by methyl-α-d-mannopyranoside, methyl-β-d-galactopyranoside, lactose and glucose. The lectin exhibited 100% hemagglutination activity at the pH range from 8.0 to 9.0 and temperature range from 30 to 60°C. Additionally, the lectin gradually lost its activity in the presence of urea but the activity abolish completely when treated with EDTA. MOSL showed mild toxicity against brine shrimp nauplii with a LC50 value of 131.0μg/ml. Antiproliferative activity was studied against Ehrlich ascites carcinoma (EAC) cells and 71.08% cell growth inhibition was observed in vitro at 200μg/ml. The lectin was injected (i.p.) into EAC mice at the doses of 2.0 and 4.0mg/kg/day for five consecutive days and 25.38% and 55% of cell growth inhibition was observed, respectively. MOSL caused the cell cycle arrest at G2/M phase as determined by FACS flow cytometry. The cell growth inhibition was due to the induction of apoptosis in the EAC cells which was confirmed by cell morphological study, caspase-3 inhibitor and activation of Bak and suppression of Bcl-2 and NF-κB genes expression.

Published

2017

2. Chemical investigation and microbial activity of Tinospora cordifolia miers

Author

AH Molla, M T Alam, Mth Molla, M G Zakaria, and Ahsan

Subjects

biology, Traditional medicine, medicine.drug_class, Antibiotics, Forestry, Context (language use), Brine shrimp, Plant Science, Aquatic Science, Tinospora cordifolia, biology.organism_classification, Antimicrobial, Microbiology, Minimum inhibitory concentration, Insect Science, medicine, Animal Science and Zoology, Antibacterial activity, Ecology, Evolution, Behavior and Systematics, Bacillus megaterium

Abstract

Context: Plants have been used in treating human diseases for thousands of years. Medicinal plant drug discovery continues to provide new and important leads against various pharmacological targets including cancer, malaria, HIV/AIDS, Alzheimer's, and pain. Objectives: The chemical investigation, antimicrobial activity and toxicity of the active principles isolated from the plant. Materials and Methods: The rectified spirit extract of the fresh stem of the plant Tinospora cordifolia was fractionated using standard chromatographic techniques to afford several fractions. The fraction TC-1 was purified by crystallization and screened. FTIR, 1 H NMR, 13 C NMR spectral analyses were performed to characterize the compound. The antibacterial and antifungal activities of TC-1 were observed by “Disc diffusion method” against a number of pathogenic bacteria and fungi. Standard antibiotics “Kanamycin” (30?g/disc) and “Fluconasol” (500 ?g/disc) were used respectively for comparison. The minimum inhibitory concentration (MIC) of the compound TC-1 was carried out by the “Serial Dilution Technique”. The compound also showed significant activity against the brine shrimp nauplii. Results: The compound TC-1 showed promising antibacterial and antifungal activities against all tested organisms.The minimum inhibitory concentration (MIC) of TC-1 against Bacillus megaterium and Salmonella typhi-A was found to be 128?g/ml in nutrient broth medium. The value of medium lethal concentration, LC 50 (9.34 ?g/ml) indicated the high toxic effect of the compound TC-1. Conclusion: It may be concluded that the compound TC-1 is an alkaloid having significant activities. DOI: http://dx.doi.org/10.3329/jbs.v20i0.17737 J. bio-sci. 20: 153-160, 2012

Published

2014

3. Effect of raised extracellular calcium on cell spread area in quail medullary bone osteoclasts

Author

A. S. M. T. Alam, Z. A. Bascal, C. G. Dacke, and Mone Zaidi

Subjects

medicine.medical_specialty, Time Factors, Medullary cavity, Cell, Osteoclasts, chemistry.chemical_element, Motility, Coturnix, Calcium, chemistry.chemical_compound, Cell Movement, Osteoclast, Internal medicine, biology.animal, medicine, Extracellular, Animals, Cells, Cultured, biology, Ionomycin, General Medicine, Quail, Endocrinology, medicine.anatomical_structure, chemistry, Female

Abstract

The present study reports on the effects of extracellular calcium ([Ca2+]o) elevation and ionomycin on cell spread area of medullary bone osteoclasts freshly isolated from egg-laying Japanese quail. The responses were compared with those demonstrated in osteoclasts cultured for periods of 5-8 days and also to those previously demonstrated in neonatal rat osteoclasts. Freshly isolated medullary bone osteoclasts, unlike rat osteoclasts, were refractory to 20 mM [Ca2+]o, in that they showed no change in cell spread area. They did, however, show a modest (15%) reduction in cell spread area to ionomycin (7-50 microM), applied for 15-30 min. When medullary bone osteoclasts were precultured for 5-8 days, they exhibited a well-developed response to 20 mM [Ca2+]o with a 46% reduction in cell spread area. They also showed a similar reduction in cell spread area in response to ionomycin (4 microM). It is concluded that, unlike freshly isolated neonatal rat osteoclasts, those obtained from quail medullary bone appear refractory to inhibitory factors such as [Ca2+]o. However, when the avian cells are cultured for a few days they appear to recover their ability to respond to [Ca2+]o.

Published

1994

4. Amylin inhibits bone resorption by a direct effect on the motility of rat osteoclasts

Author

P. J. R. Bevis, Mone Zaidi, A. S. M. T. Alam, Christopher L.-H. Huang, and Baljit S. Moonga

Subjects

Calcitonin, Amyloid, endocrine system, medicine.medical_specialty, endocrine system diseases, Calcitonin Gene-Related Peptide, Osteoclasts, Motility, Amylin, macromolecular substances, In Vitro Techniques, Calcitonin gene-related peptide, Biology, Bone resorption, chemistry.chemical_compound, Cytosol, Cell Movement, Osteoclast, Internal medicine, Cyclic AMP, medicine, Animals, Bone Resorption, Rats, Wistar, Forskolin, Colforsin, General Medicine, Islet Amyloid Polypeptide, Rats, Resorption, Endocrinology, medicine.anatomical_structure, chemistry, Calcium

Abstract

We have performed a set of independent studies on the effects of the circulating pancreatic polypeptide, amylin, on rat osteoclast function, in vitro. Time-lapse video observations, measuring cell protrusions and retraction, showed that 250 nmol l-1 amylin or 250 nmol l-1 beta-calcitonin gene-related peptide (beta-CGRP) inhibited osteoclast motility (quiescence or Q effect). Both amylin and beta-CGRP produced inhibitory responses with a significant first-order regression over time (half-times, 19 and 28 min respectively). In contrast, 250 nmol l-1 amylin or 250 nmol l-1 beta-CGRP produced no change of osteoclast spread area, whilst 300 pmol l-1 calcitonin (CT) application resulted in cell retraction (R effect). Forskolin (10 mumol l-1) mimicked amylin and CGRP in inhibiting osteoclast motility (half-time, 8.6 min), and similarly lacked an effect on cell spread area. Neither amylin nor beta-CGRP (62.5–1250 nmol l-1) elevated cytosolic free calcium levels ([Ca2+]i) in single osteoclasts whilst 300 pmol l-1 salmon calcitonin (sCT) produced a rapid phasic elevation of [Ca2+]i, confirming previous results with asusuberic (1-7) eel calcitonin. The osteoclast-bone resorption assay revealed the following potency difference in direct comparison of the area of resorption per bone slice: beta-CGRP/amylin, 0.1; sCT/amylin, 800 and human CT/amylin, 12. The potency of deamidated amylin approached that of beta-CGRP. Assay precision ranged between 0.3 and 0.8. Amylin (250 nmol l-1) also significantly (P < 0.05) reduced supernatant (tartrate-resistant) acid phosphatase in the bone-osteoclast cultures. These measures independently indicate an effect of amylin on osteoclast motility through mechanisms distinct from those of calcitonin, possibly through different selectivities for receptor subtypes, the cyclic AMP-linked 'amylin subtype' and the [Ca2+]i-linked 'calcitonin subtype'.

Published

1993

5. Osteoclastic inhibition: an action of nitric oxide not mediated by cyclic GMP

Author

Harish K. Datta, Baljit S. Moonga, Mone Zaidi, P S Lidbury, John R. Vane, Markus Hecker, Iain MacIntyre, and A. S. M. T. Alam

Subjects

Calcitonin, musculoskeletal diseases, medicine.medical_specialty, Vasodilator Agents, Osteoclasts, Nitric Oxide, Calcium in biology, Bone resorption, Nitric oxide, chemistry.chemical_compound, Cytosol, Osteoclast, Internal medicine, Dibutyryl Cyclic GMP, medicine, Animals, Bone Resorption, Mode of action, Cyclic GMP, Cells, Cultured, Multidisciplinary, Ionomycin, Cell Membrane, Rats, Inbred Strains, Rats, Resorption, Kinetics, Endocrinology, medicine.anatomical_structure, Animals, Newborn, chemistry, Molsidomine, Calcium, Bone marrow, Research Article

Abstract

The osteoclast is unique in its ability to resorb bone, and excessive osteoclastic activity has been implicated in osteoporosis, Paget disease of bone, rheumatoid arthritis, and the growth of metastases in bone. The activity of this cell is controlled by the main circulating inhibitor, calcitonin, in association with locally produced modulators. We show that nitric oxide (NO) may be an important member of the latter group. NO is produced by the vascular endothelium and nervous system and is involved in both neurotransmission and the regulation of blood pressure. However, our results show that the autocoid is also a potent inhibitor of osteoclast function. NO (30 microM) produced a decrease to approximately 50% of the original osteoclast spread area. Similar effects were also produced by 3-morpholinosydnonimine or sodium nitroprusside, reagents that spontaneously release NO. These shape changes were associated with a reduction of bone resorption after a 24-hr incubation of isolated osteoclasts on devitalized bone slices. NO is thought to act by stimulating guanylate cyclase, with a consequent increase in cyclic GMP, but a different mode of action is likely in the osteoclast since dibutyryl or 8-bromo cyclic GMP have no effect. It should be noted that calcitonin can produce similar changes in shape and activity but is associated with an increase in osteoclast intracellular calcium and cessation of membrane movement; neither of these is produced by NO, suggesting that its mode of action is different. The abundance of NO-producing endothelial cells in bone marrow and their proximity to osteoclasts suggests that marrow endothelial cells may play a physiological role in the regulation of osteoclastic activity.

Published

1991

6. Nano-mechanical methods in biochemistry using atomic force microscopy

Author

Rehana Afrin, Atsushi Ikai, M T Alam, Shuhei Nishida, Hiroshi Sekiguchi, and Takaharu Okajima

Subjects

Globular protein, Biochemical Phenomena, Atomic force acoustic microscopy, Nanotechnology, Receptors, Cell Surface, macromolecular substances, Ligands, Microscopy, Atomic Force, Biochemistry, Quantitative Biology::Cell Behavior, Quantitative Biology::Subcellular Processes, Antigen-Antibody Reactions, Indentation, Microscopy, medicine, Cell Adhesion, Animals, Humans, Composite material, Molecular Biology, chemistry.chemical_classification, Chemistry, Cell Membrane, technology, industry, and agriculture, Stiffness, Cell Biology, General Medicine, Conductive atomic force microscopy, DNA, Elasticity (physics), Elasticity, Biomechanical Phenomena, Nucleic Acid Conformation, Adhesive, medicine.symptom

Abstract

The atomic force microscope has been extensively used not only to image nanometer-sized biological samples but also to measure their mechanical properties by using the force curve mode of the instrument. When the analysis based on the Hertz model of indentation is applied to the approach part of the force curve, one obtains information on the stiffness of the sample in terms of Young's modulus. Mapping of local stiffness over a single living cell is possible by this method. The retraction part of the force curve provides information on the adhesive interaction between the sample and the AFM tip. It is possible to functionalize the AFM tip with specific ligands so that one can target the adhesive interaction to specific pairs of ligands and receptors. The presence of specific receptors on the living cell surface has been mapped by this method. The force to break the co-operative 3D structure of globular proteins or to separate a double stranded DNA into single strands has been measured. Extension of the method for harvesting functional molecules from the cytosol or the cell surface for biochemical analysis has been reported. There is a need for the development of biochemical nano-analysis based on AFM technology.

Published

2003

7. Extracellular Ca2+ sensing by the osteoclast

Author

C. L.-H. Huang, Bridget E. Bax, V.S. Shankar, A. S. M. T. Alam, Mone Zaidi, Michael Pazianas, Christopher M.R. Bax, Peter J.R. Bevis, and Baljit S. Moonga

Subjects

Membrane potential, Physiology, Osteoclasts, Cell Biology, Biology, Feedback, Membrane Potentials, Cytosol, medicine.anatomical_structure, Biochemistry, Osteoclast, Extracellular fluid, medicine, Extracellular, Biophysics, Plasma membrane Ca2+ ATPase, Humans, Calcium, Calcium Channels, Receptor, Molecular Biology, Intracellular

Abstract

An increasing number of cell types appear to detect changes in the extracellular Ca2+ concentration and and accordingly modify their function. We review recent evidence for the existence and function of such a mechanism in the osteoclast. Elevated external [Ca2+] in the mM range reduces bone resorption and results in motile changes in the cells. These changes may partly result from elevations of cytosolic [Ca2+] triggered through activation of a surface Ca2+ receptor. Closer analyses of the increases in cytosolic [Ca2+] associated with receptor activation are hindered by the action of this ion both as extracellular agonist and intracellular second messenger. Variations in the peak cytosolic [Ca2+] response to external Ca2+ with changes in cell membrane potential by K+ and valinomycin establish a contribution from extracellular Ca2+. Use of CIO4-, Ni2+ and Cd2+ as surrogate activators in low extracellular [Ca2+] indicate a contribution from Ca2+ release from intracellular stores as well. Such agonists also modify Ca2+ redistribution in other systems, such as skeletal muscle. Thus, we may gain insights into osteoclast extracellular Ca2+ detection and transduction from known features of more well-characterised cell systems.

Published

1993

8. Role of the endothelial cell in osteoclast control: new perspectives

Author

Baljit S. Moonga, A. S. M. T. Alam, V.S. Shankar, D R Blake, J. S. Gill, T. Sahinoglu, Michael Pazianas, Mone Zaidi, C.R. Stevens, Christopher M.R. Bax, Bridget E. Bax, and C. L.-H. Huang

Subjects

musculoskeletal diseases, medicine.hormone, Calcitonin, medicine.medical_specialty, Histology, Endothelium, Physiology, Endocrinology, Diabetes and Metabolism, Osteoclasts, Nitric Oxide, Bone resorption, Nitric oxide, Bone remodeling, Endothelins, chemistry.chemical_compound, Osteoclast, Internal medicine, medicine, Cyclic AMP, Humans, Cyclic guanosine monophosphate, Osteoblasts, Cell biology, Endothelial stem cell, medicine.anatomical_structure, Endocrinology, chemistry, Bone Remodeling, Reactive Oxygen Species

Abstract

The osteoclast is of central importance in the process of bone remodeling. Its function is regulated by hormones and locally produced factors. Endothelial cells occur in close proximity to the osteoclast. Some endothelial cell-derived products, including endothelins, nitric oxide, and reactive oxygen species, have been recently implicated as modulators of osteoclast function. Endothelins inhibit bone resorption and osteoclast margin ruffling (quiescence or Q effect) at concentrations similar to those effective for their primary vasoconstrictive action. Contrary to expectations, however, it has been shown that endothelin action on the osteoclast is not mediated through an elevation of cytosolic Ca2+. Nitric oxide (NO) produces marked cell retraction (retraction or R effect), but its detailed mode of action is unknown. However, it is clear that the effects of this autocoid are not due to enhanced cyclic guanosine monophosphate (cGMP) production, a transduction system commonly used by NO. Finally, the reactive oxygen species H2O2 has been shown recently to enhance osteoclastic activity. Thus, the reported effects of the endothelial cell-derived products on the osteoclast are generally consistent with a regulatory role for endothelial cells in osteoclast control and suggest the existence of unique activation pathways, well worth exploring further. Unravelling the responsible mechanisms may also help understand the pathophysiology of a range of bone and joint diseases. For example, in rheumatoid arthritis, there is increased H2O2 production from activated neutrophils, and bone resorption is a major pathophysiological feature.

Published

1993

9. Stimulation of a Gs-like G protein in the osteoclast inhibits bone resorption but enhances tartrate-resistant acid phosphatase secretion

Author

V.S. Shankar, Mone Zaidi, Michael Pazianas, Baljit S. Moonga, A. S. M. T. Alam, and C. L.-H. Huang

Subjects

Anions, Calcitonin, medicine.medical_specialty, Cholera Toxin, G protein, Acid Phosphatase, Biophysics, Osteoclasts, medicine.disease_cause, Pertussis toxin, Biochemistry, Bone resorption, Fluorides, Osteoclast, GTP-Binding Proteins, Internal medicine, medicine, Animals, Virulence Factors, Bordetella, Bone Resorption, Aluminum Compounds, Molecular Biology, Tartrates, Tartrate-resistant acid phosphatase, biology, Cell Death, Cholera toxin, Acid phosphatase, Cell Biology, Fluorine, Resorption, Rats, Endocrinology, medicine.anatomical_structure, Pertussis Toxin, biology.protein, Aluminum

Abstract

Previous studies have demonstrated that G-protein agonists induce quiescence (Q effect) or retraction (R effect) in isolated osteoclasts. We now report the functional effects of such agonists on osteoclastic bone resorption and enzyme release. Exposure of osteoclasts to tetrafluoro-aluminate anions (AlF 4 − ), a universal G protein stimulator, resulted in a marked concentration-dependent inhibition of bone resorption. This was associated with a dramatic increase in the secretion of the osteoclast-specific enzyme, tartrate-resistant acid phosphatase (TRAP). Cholera toxin, a G s stimulator and a selective Q effect agonist, similarly abolished bone resorption and enhanced TRAP secretion. In contrast, pertussis toxin, a G i inhibitor and a selective R effect agonist, inhibited bone resorption significantly, but slightly reduced enzyme release. The results suggest an involvement of a G s -like G protein in TRAP secretion from the osteoclast, possibly through a cyclic AMP-dependent mechanism.

Published

1993

10. A quantitative description of components of in vitro morphometric change in the rat osteoclast model: relationships with cellular function

Author

Christopher L.-H. Huang, Michael Pazianas, V.S. Shankar, Baljit S. Moonga, Mone Zaidi, A. S. M. T. Alam, Peter J.R. Bevis, and Bridget E. Bax

Subjects

Calcitonin, Amyloid, Time Factors, Cell, Biophysics, Osteoclasts, Motility, Amylin, Biology, Cell Movement, Osteoclast, Extracellular, medicine, Animals, Rats, Wistar, Receptor, Cells, Cultured, General Medicine, In vitro, Islet Amyloid Polypeptide, Rats, Models, Structural, Kinetics, medicine.anatomical_structure, Animals, Newborn, Immunology, Calcium, sense organs, Function (biology)

Abstract

We describe the in vitro morphometric changes shown by rat osteoclasts that accompany their functional responses to the application of a range of regulatory agents of known physiological importance. We introduce a cellular motility parameter, mu, which was defined through a quantification of retraction-protrusion behaviour. This was used in conjunction with a net cell retraction, rho, which is derived from the change in total cell area following the application of an agent. These terms were used together for the description of cellular motility changes in response to specific cellular regulatory agents. The definition of retraction-protrusion was normalised against control cell area, to give a dimensionless variable independent of the net cell retraction. Thus, mutual terms present in either descriptor cancelled when the complementary parameter was held constant. Furthermore, the descriptor, mu remained time-invariant for extended intervals (around 20 min) even when rho was varying following cell introduction into culture. Interventions also with substances known to modify osteoclast function, were capable of altering each descriptor, to different extents. Thus elevation of the extracellular Ca2+ concentration ([Ca2+]e) at the osteoclast calcium "receptor" altered rho without changes in mu. In contrast, the polypeptide amylin (250 nM), within 20 minutes of application, elicited a marked change in mu, but only a relatively small change in rho. Finally, human calcitonin treatment (300 pM) influenced both descriptors. When combined together, these morphometric findings accordingly offer complementary descriptions of visible cellular changes in response to added agents of physiological relevance.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1992

11. Endothelin inhibits osteoclastic bone resorption by a direct effect on cell motility: implications for the vascular control of bone resorption

Author

T.J. Chambers, V.S. Shankar, A Gallagher, A. S. M. T. Alam, H K Datta, Baljit S. Moonga, Mone Zaidi, S R Bloom, C. L.-H. Huang, and M A Ghatei

Subjects

musculoskeletal diseases, medicine.medical_specialty, Acid Phosphatase, Osteoclasts, Biology, Bone resorption, Endocrinology, Osteoclast, Cell Movement, Internal medicine, medicine, Animals, Bone Resorption, Cells, Cultured, Dose-Response Relationship, Drug, Endothelins, Cell Membrane, Acid phosphatase, Rats, Inbred Strains, Smooth muscle contraction, Resorption, Rats, Endothelial stem cell, medicine.anatomical_structure, Animals, Newborn, biology.protein, Cortical bone, Calcium, Bone marrow, Endothelium, Vascular

Abstract

The abundance of endothelin (ET)-producing endothelial cells in bone marrow and the proximity of these cells to bone-resorbing osteoclasts prompted us to evaluate the action of ET-1 on osteoclast function. Osteoclasts disaggregated from neonatal rat long bones were settled onto devitalized cortical bone substrate, and resorption was quantified by morphometry. The supernatant tartrate-resistant acid phosphatase activity was determined by a spectrophotometric method using paranitrophenol phosphate as substrate. Cell motility was quantified by time lapse video- and computer-assisted image processing using an empirical procedure for morphometric analysis. Cytosolic free calcium levels ([Ca2+]i) were measured in single cells by an indo 1-based microspectrofluorimetric method. Using the area of bone resorbed per slice as response, we found that ET-1 caused a significant (P = 0.011) concentration-dependent inhibition of osteoclastic bone resorption (EC50 = 2.5 nM) without inhibiting acid phosphatase secretion. Exposure of isolated osteoclasts to ET-1 also led to a marked concentration-dependent inhibition of osteoclast motility (EC50 = 7.9 nM; P = 0.013; t1/2 = 18 min) without significant effects on cell spread area. These effects of ET-1 were reversible after removing the peptide, and the cells remained viable during the experiments. In addition, ET-1 did not elevate [Ca2+]i at the concentrations tested. The results suggest that ET-1 specifically interacts with an osteoclast receptor to inhibit osteoclastic bone resorption and cell motility. As the concentration of ET-1 required for osteoclast inhibition was similar to that reported for smooth muscle contraction, it is possible that ET-1, produced locally from the bone marrow endothelial cell, might play a primary role in osteoclast regulation.

Published

1992

12. Regulation of cytosolic free calcium in isolated rat osteoclasts by calcitonin

Author

P. J. R. Bevis, F. Avaldi, Baljit S. Moonga, R. Soncini, Christopher L.-H. Huang, A. S. M. T. Alam, and Mone Zaidi

Subjects

Calcitonin, medicine.medical_specialty, Cytoplasm, Endocrinology, Diabetes and Metabolism, Cell, chemistry.chemical_element, Osteoclasts, Cytosolic free calcium, Calcium, Rats, Endocrinology, medicine.anatomical_structure, Spectrometry, Fluorescence, chemistry, Osteoclast, Internal medicine, Second messenger system, medicine, Extracellular, Animals, Calcitonin receptor, Cells, Cultured

Abstract

It is now established that calcium is a second messenger mediating the action of calcitonin on the osteoclast. We have demonstrated that an increase in the concentration of intracellular free calcium ([Ca2+]i) is associated with (and possibly mediates) the functional effects of calcitonin, including an acute reduction of cell spread area (the R effect) and, in the longer term, a reduction in enzyme release. The present study addresses questions relating to mechanisms of calcitonin action on osteoclast [Ca2+]i. We have used asusuberic(1–7) eel and human calcitonin as agonists, and an indo-1-based dual-emission microspectrofluorimetric method for the measurement of [Ca2+]i in single osteoclasts. Whilst asusuberic(1–7) eel calcitonin caused a biphasic increase in [Ca2+]i, human calcitonin produced only a monophasic [Ca2+]i response of a much lower magnitude. Each biphasic response consisted of a rapid initial transient increase, occurring within seconds of exposure, followed by a sustained increase in [Ca2+]i. The magnitude of the latter response was more variable, but was consistently below the peak value of [Ca2+]i. The sustained phase of the calcitonin effect was abolished in extracellular Ca2+-free medium. This phase is therefore dependent on extracellular [Ca2+] ([Ca2+]e) whilst the rapid transient increase appeared to be dependent on Ca2+i redistribution. The effects of calcitonin on [Ca2+]i were concentration-dependent, with neither latency nor oscillations. Repetitive 30-s exposures to calcitonin failed to produce subsequent responses. There was a marked concentration-dependent correlation between changes in osteoclast [Ca2+]i and the magnitude of the R effect. Thus the likely components of the biphasic [Ca2+]i response are a rapid redistribution followed by the transmembrane flux of Ca2+. We suggest that the increase in [Ca2+]i may mediate, in part, the inhibitory effect of calcitonin. Journal of Endocrinology (1992) 132, 241–249

Published

1992

13. Whoosh test 2 and confirmation of lumbar epidural space

Author

J. Chabra, M. T. Alam, Divya Jain, R. M. Khan, and M. Ashraf

Subjects

medicine.medical_specialty, Anesthesiology and Pain Medicine, medicine.anatomical_structure, Lumbar, business.industry, medicine, Radiology, business, Epidural space, Test (assessment)

Published

2003

14. CYTOLOGICAL EFFECTS OF MICROWAVE RADIATION IN CHINESE HAMSTER CELLS IN VITRO

Author

M. T. Alam, N. G. Lambert, N. Barthakur, and S. S. Kasatiya

Subjects

Genetics, biology, Cell, TEMPERATURE ELEVATION, Dose-Response Relationship, Radiation, Cell Biology, Plant Science, Vacuole, biology.organism_classification, Molecular biology, Chromosomes, Chinese hamster, In vitro, Chromosomal Breakages, Cell Line, Cold Temperature, medicine.anatomical_structure, Cell culture, medicine, Microwaves, Microwave

Abstract

Cytological effects were investigated in the Chinese hamster cell line (CHO-K1) exposed to microwave radiation of 2450 MHz frequency and incident power of 25 to 200 W for a period of 30 min. Nuclear vacuoles, pycnotic and decondensed chromosomes were observed in cells exposed to 25 W under elevated temperature conditions (uncontrolled temp). In addition a significant increase in chromosomal breakages/cell was observed. Cells exposed to relatively higher power, 75-200 W, under hypothermic conditions (29 °C) revealed no significant increase in either nuclear vacuoles or other chromosomal anomalies over control cells. Radiation-induced temperature elevation appears to be an essential factor in the cytological effects of microwave.

Published

1978

15. Investigation on antimicrobial activities of the plant Swertia chirata Ham

Author

M T Alam, Fazle Rabbi Shakil Ahmed, Tamzid Hossain Molla, and Mst. Jesmin Sultana

Subjects

Gentianaceae, biology, Kanamycin, Brine shrimp, Pathogenic bacteria, Bacillus subtilis, biology.organism_classification, Antimicrobial, medicine.disease_cause, Microbiology, medicine, Food science, Artemia salina, medicine.drug, Bacillus megaterium

Abstract

Biological activities of fresh stem of the plant Swertia chirata Ham. (F. Gentianaceae) extracted in rectified spirit is reported here. The crude rectified spirit extract was fractionated by using standard chromatographic techniques on alumina, which gave six fractions (A, B, C, D, E & F). When subjected to column chromatographic analysis on neutral alumina, fraction D yielded a pure compound tentatively known as AJ-1 that have melting point of 178° C. AJ-1 was screened for its antibacterial activities against 12 pathogenic bacteria, 6 Gram positive and 6 Gram negative, by disc diffusion method at a concentration of 200 μg/disc. The results obtained were compared with those for a standard antibiotic Kanamycin. AJ-1 showed significant activity against Bacillus megaterium (11 mm), Bacillus subtilis (9 mm), Salmonella typhi-A (10 mm), Shigella flexeneriae (10 mm) and Klebsiella sp (11 mm) but a little activity against Staphylococcus aureus . The Minimum Inhibitory Concentrations (MIC) of AJ-1 determined against Bacillus megaterium and Salmonella typhi-A were 128 μg/ml and 128 μg/ml, respectively when tested in a nutrient broth medium. AJ-1 also showed significant activity against the brine shrimp ( Artemia salina ) nauplii (LC50 value of 9.34 μg/ml), in which the mortality rate increased with the increasing concentration of the compound, suggesting a positive correlation between brine shrimp toxicity and cytotoxicity. Key words : Biological activity; Swertia chirata; Gentianaceae; pathogenic bacteria DOI: 10.3329/jles.v2i2.7494 J. Life Earth Sci., Vol. 2(2) 31-34, 2007

Published

1970

16. Chromosomal anomalies induced by the organic phosphate pesticide guthion in Chinese hamster cells

Author

S. S. Kasatiya, M. Corbeil, A. Chagnon, and M. T. Alam

Subjects

Insecticides, Secondary constriction, Mutant, Cell, Mitosis, Chromatids, In Vitro Techniques, Chromosomes, Chinese hamster, Dicentric chromosome, chemistry.chemical_compound, Cricetinae, Genetics, medicine, Animals, Genetics (clinical), Chromosome Aberrations, biology, Organothiophosphorus Compounds, biology.organism_classification, Phosphate, Molecular biology, medicine.anatomical_structure, chemistry, Chromatid

Abstract

Chromosomal anomalies associated with the use of the organic phosphate pesticide guthion were investigated in Chinese hamster cells (line CHO-K1). Most commonly observed were chromatid breaks and exchanges. Infrequently, mild failure of condensation, despiralization, secondary constriction, gaps, pulverization, ring and dicentric chromosomes were noted. The mean number of chromosome breaks per cell was significantly higher in treated cells than in control cells. Autoradiographic studies revealed that while higher dosages of the chemical (80–120 μg/ml) arrested cells and prevented their movement out of S phase, a lower dosage (60 μg/ml) caused a progression delay. In relation to the relative length of no. 1 and no. 2 chromosomes, no apparent difference existed in the incidence of total breaks between them. However, significant differences in the nonrandom distribution of breaks in no. 1 and no. 2 chromosomes indicated linear differentiation of breakage susceptibility along the chromosomes. An increased concentration of breaks was observed in the long arms of both no. 1 and no. 2 chromosomes. The experimental results suggest that guthion, as well as inducing chromosomal anomalies, may produce a viable mutant.

Published

1974

17. The XYY syndrome in an adolescent male exhibiting prominent behavioral problems

Author

R. Deschamps, M. T. Alam, S. S. Kasatiya, W. F. Grant, and E. Gaba

Subjects

Male, medicine.medical_specialty, Pediatrics, Adolescent, Fluorescence, Pregnancy, Internal medicine, Genetics, medicine, Leukocytes, Methods, Humans, Dermatoglyphics, Genetics (clinical), Sex Chromosome Aberrations, Chromosome Aberrations, Staining and Labeling, business.industry, Learning Disabilities, Infant, Newborn, Mouth Mucosa, Social Behavior Disorders, Electroencephalography, Syndrome, medicine.disease, Body Height, Mother-Child Relations, Obstetric Labor Complications, Endocrinology, Sex Chromatin, Quinacrine, Karyotyping, XYY syndrome, Female, business, Infant, Premature

Published

1972

18. Pollen longevity in birch (Betula)

Author

M. T. Alam and W. F. Grant

Subjects

Betula populifolia, biology, Anthesis, Germination, media_common.quotation_subject, Pollen, Botany, Longevity, medicine, Plant Science, medicine.disease_cause, biology.organism_classification, media_common

Abstract

To carry out reciprocal crosses between birch species which vary by several weeks in their time of anthesis, the period of pollen viability has been determined for three species, Betula populifolia, B. cordifolia, and B. papyrifera. Pollen viability decreased from 85–95% at the time collected to 32–44% after being stored at room temperature (23–27 °C) for 30 days and to 1.0–1.5% after 60 days. In contrast, pollen germination for pollen stored at 2–5 °C for 105 days fell only to 46.0% for B. populifolia and 20.5% and 21.5% for B. cordifolia and B. papyrifera, respectively.

Published

1971