243 research outputs found

    The multidimensional analysis of cell behaviour

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    The cell motility assays became an important step for trial of new developed anti-tumor drugs and compounds [1, 2]. Set of experiments was performed with microtubule affecting drugs on a model population of 3T3 cells. This study is focused on the complex analysis of cell population behavior that can be further used to develop method for evaluation of drugs in preclinical trials

    A substorm in midnight auroral precipitation

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    International audienceDMSP F7 spacecraft observations for the whole of 1986 were used to construct the empirical model of the midnight auroral precipitation during a substorm. The model includes the dynamics of different auroral precipitation boundaries and simultaneous changes in average electron precipitation energy and energy flux in different precipitation regions during all substorm phases, as well as the IMF and solar wind plasma signatures during a substorm. The analysis of the model shows a few important features of precipitation. (1) During the magnetic quietness and just before the beginning of the substorm expansive phase the latitudinal width of the auroral precipitation in the nightside sector is about 5 ? 6° CGL, while that of the auroral oval is about 2 ? 3° CGL during such periods. (2) For about 5 min before the substorm onset a decrease in the average precipitating electron energy in the equatorward part of auroral zone was observed simultaneously, with an increase in both the average electron energy and energy flux of electron precipitation in the poleward part of the auroral zone. (3) The isotropy boundary position in the beginning of the substorm expansive phase coincides well with the inner edge of the central plasma sheet. The analysis of interplanetary medium parameters shows that, on average, during the substorm development, the solar wind dynamic pressure was about 1.5 times that of the magnetic quietness period. Substorms occurred predominantly during the southward IMF orientation, suggesting that substorm onset often was not associated with the northern turn or decrease in the southward interplanetary Bz . The Northern Hemisphere's substorms occurred generally during the positive interplanetary By in winter, and they were observed when the interplanetary By was negative in summer

    Analysis of microtubule targeting drugs and mitotic slippage

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    New nucleic dyes for pico-and nanoplankton cytometric analysis

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    Flow cytometry (FCM) is a promising tool in the field of aquatic phytoplankton ecology because it allows for multi-parameter assessment of the physiological state of individual cells in an algal population. It can help to elucidate major questions such as phytoplankton taxa identification, the evaluation of cell quantity and viability, and the measuring of phytoplankton and general microbial metabolic activities. Traditionally, microalgal characterization is performed by microscopic analysis using UV-excited nuclear dyes (e.g. Hoechst and DAPI) or dyes that are excited in the blue-green part of the spectrum such as propidium iodide and eosin. The development of multi-laser cytometric systems has widened the possibilities for multi-parametric analysis and cell sorting of phytoplankton populations. Notwithstanding, significant algae autofluorescence originating from different types of chlorophyll and accessory pigments may overlap with propidium iodide and/or eosin staining and affect the resolution of algae clusters and cell sorting

    New nucleic dyes for pico-and nanoplankton cytometric analysis

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    Flow cytometry (FCM) is a promising tool in the field of aquatic phytoplankton ecology because it allows for multi-parameter assessment of the physiological state of individual cells in an algal population. It can help to elucidate major questions such as phytoplankton taxa identification, the evaluation of cell quantity and viability, and the measuring of phytoplankton and general microbial metabolic activities. Traditionally, microalgal characterization is performed by microscopic analysis using UV-excited nuclear dyes (e.g. Hoechst and DAPI) or dyes that are excited in the blue-green part of the spectrum such as propidium iodide and eosin. The development of multi-laser cytometric systems has widened the possibilities for multi-parametric analysis and cell sorting of phytoplankton populations. Notwithstanding, significant algae autofluorescence originating from different types of chlorophyll and accessory pigments may overlap with propidium iodide and/or eosin staining and affect the resolution of algae clusters and cell sorting

    BCL-XL ACTIVITY INFLUENCES OUTCOME OF THE MITOTIC ARREST

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    Microtubule-targeting (MT) drugs taxanes and vinca alkaloids are widely used as chemotherapeutic agents against different tumors for more than 30 years because of their ability to block mitotic progression by disrupting the mitotic spindle and activating the spindle assembly checkpoint (SAC) for a prolonged period of time. However, responses to mitotic arrest are different—some cells die during mitotic arrest, whereas others undergo mitotic slippage and survive becoming able for proliferation. Using normal fibroblasts and several cancer cell types we determined two critical doses, T1 and T2, of mitotic inhibitors (nocodazole, Taxol, and vinorelbine). T1 is the maximal dose cells can tolerate undergoing normal division, and T2 is the minimal mitostatic dose, wherein > 90% of mitotic cells are arrested in mitosis. In all studied cell lines after treatment with mitotic inhibitors in a dose above T2 cells had entered mitosis either die or undergo mitotic slippage. We show that for all three drugs used cell death during mitotic arrest and after slippage proceeded via mitochondriadependent apoptosis. We determined two types of cancer cells: sensitive to mitotic arrest, that is, undergoing death in mitosis (DiM) frequently, and resistant to mitotic arrest, that is, undergoing mitotic slippage followed by prolonged survival. We then determined that inhibition of Bcl-xL, but not other antiapoptotic proteins of the Bcl-2 group that regulate MOMP, make resistant cells susceptible to DiM induced by mitotic inhibitors. Combined treatment with MT drugs and highly specific Bcl-xL inhibitors A-1155643 or A-1331852 allows achieving 100% DiM in a time significantly shorter than maximal duration of mitotic arrest in all types of cultured cells tested. We further examined efficacy of sequential treatment of cultured cells using mitotic inhibitors followed by inhibitors of Bcl-xL anti-apoptotic protein and for the first time show that sensitivity to Bcl-xL inhibitors rapidly declines after mitotic slippage. Thus sequential use of mitotic inhibitors and inhibitors of Bcl-xL anti-apoptotic protein will be efficient only if the Bcl-xL inhibitor will be added before mitotic slippage occurs or soon afterward. The combined treatment proposed might be an efficient approach to anti-cancer therapy

    The use of HaloTag-based technology in flow and laser scanning cytometry analysis of live and fixed cells

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    <p>Abstract</p> <p>Background</p> <p>Combining the technologies of protein tag labeling and optical microscopy allows sensitive analysis of protein function in cells.</p> <p>Findings</p> <p>Here, we describe development of applications using protein tag technology (HaloTag (HT)-based) for flow and laser scanning cytometry (LSC). Cell lines, expressing recombinant surface β1-integrin-HT and HT-p65 fusion protein, and a CD4 T cell line (Jurkat) infected with human immunodeficiency virus type 1 (HIV-1) reporter virus expressing the unfused HT (HIV-1<sub>Lai-Halo</sub>), were stained with different HT ligands and successfully detected by flow cytometers equipped with 488 and 561 nm lasers as well as a laser scanning cytometer (equipped with 488 and 405 nm lasers) alone or combined with cell cycle and viability markers.</p> <p>Conclusions</p> <p>Use of HT technology for cytometric applications has advantages over its use in microscopy as it allows for the statistical measurement of protein expression levels in individual cells within a heterogeneous cell population in combination with cell cycle analysis. Another advantage is the ability of the HaloTag to withstand long fixation and high concentration of fixative, which can be useful in research of infectious agents like HIV and/or mycobacteria.</p
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