ZIB

11

Electronic Resource

Thick slurry bevelling (1979)

Lederer, W. J. ; Spindler, A. J. ; Eisner, D. A.

Springer

Pflügers Archiv 381 (1979), S. 287-288

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ISSN: 1432-2013

Keywords: Microelectrodes ; Electrode bevelling ; Heart muscle voltage clamp

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract A simple, inexpensive and rapid bevelling method is described. A settled slurry of 0.05 μm alumina powder in saline is used as the grinding surface. The bevelling process is continuous and reproducible over a wide range of electrode resistances.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00583261

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12

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Propagation of excitation-contraction coupling into ventricular myocytes (1994)

Cheng, H. ; Cannell, M. B. ; Lederer, W. J.

Springer

Pflügers Archiv 428 (1994), S. 415-417

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ISSN: 1432-2013

Keywords: Heart ; Cardiac muscle ; Contraction ; E-C coupling ; Calcium channels ; Ryanodine receptors ; Intracellular calcium

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract This paper examines the [Ca2+]i transient in isolated rat heart cells using a laser scanning confocal microscope and the calcium indicator fluo-3. We find that the depolarization-evoked [Ca2+]i transient is activated synchronously near the surface and in the middle of the heart cell with similar kinetics of activation. The time of rise of the transient did not depend on whether the sarcoplasmic reticulum (SR) Ca-release was abolished (by thapsigargin and ryanodine). The synchrony of activation and the similarity of levels of [Ca2+]i at the peripheral and deeper myoplasm (regardless of the availability of SR Ca-release) shows that sarcolemmal Ca channels and SR Ca-release channels are distributed throughout the rat heart cell and that the propagation of the action potential into the interior of the cell is rapid. In addition, the activation of calcium release from the SR by CICR is rapid (≪2 ms) when compared to the time-course of calcium influx via the sarcolemmal Ca channel.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00724526

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13

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Modulation of ATP-sensitive potassium channel activity by flash-photolysis of ‘caged-ATP’ in rat heart cells (1990)

Nichols, C. G. ; Niggli, E. ; Lederer, W. J.

Springer

Pflügers Archiv 415 (1990), S. 510-512

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ISSN: 1432-2013

Keywords: Adenosine triphosphate ; Caged-adenosine triphosphate ; Potassium channel ; Metabolism ; Heart ; Cardiac ventricle

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract We have used ‘caged-ATP’ to investigate the kinetic behavior of KATP channels in ventricular cells from rat heart. In whole cells, loaded with ‘caged-ATP’, an increase of intracellular [ATP] following a UV light flash produced a decrease of KATP channel current that was too slow (τ ≈ 300 ms) to be explained by the expected timecourse of ATP release (τ ≈ 3 ms) and the time-course of channel blockade by ATP (τ ≈ 20 ms). In isolated membrane patches, caged-ATP itself caused partial blockade of KATP channels. Under these conditions, photorelease of ATP caused channel activity to decline further. The results suggest that caged-ATP can bind to the KATP channel but, on binding, decreases the open probability to a lesser extent than does ATP. Additionally, the observations indicate that for photolytically-generated ATP to bind to the channel, caged-ATP must first unbind (slowly) from the channel. We conclude that ‘caged-ATP’ is not fully caged with respect to its allosteric action on the KATP channel.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00373635

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14

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Measurement of intracellular Ca2+ concentration using Indo-1 during simultaneous flash photolysis to release Ca2+ from DM-nitrophen (1994)

Kirby, Mark S. ; Hadley, Robert W. ; Lederer, W. J.

Springer

Pflügers Archiv 427 (1994), S. 169-177

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ISSN: 1432-2013

Keywords: Indo-1 ; Flash photolysis ; DM-nitrophen ; Nd: YAG laser ; Cardiac cells ; 293 cells

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract We have constructed a modular instrument to measure intracellular [Ca2+] ([Ca2+]i) in single isolated cells while simultaneously imposing step changes in [Ca2+]i using “caged Ca2+”. By combining the outputs of a xenon arc lamp with a frequency-tripled (Nd: YAG) laser, the instrument can operate with low maintained illumination to measure [Ca2+]i using a ratiometric Ca2+-sensitive fluorophore and also activate the release of Ca2+ from a caged-Ca2+ compound with a high energy pulse of ultraviolet light. This instrument is simple to assemble, introduces little electrical noise, provides a wide range of illumination power, produces only moderate photobleaching of the Ca2+ indicator and can be readily adapted to diverse cellular preparations. We demonstrate the use of this system to measure step changes in [Ca2+]i in adult rat ventricular myocytes and a human embryonic kidney cell line (293 cells) in culture.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00585957

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15

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Excitation-contraction coupling in heart muscle (1989)

Lederer, W. J. ; Cannell, M. B. ; Cohen, N. M. ; [et al.]

Springer

Molecular and cellular biochemistry 89 (1989), S. 115-119

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ISSN: 1573-4919

Keywords: excitation-contraction coupling ; mammalian heart muscle ; calcium current ; fura-2 ; intracellular calcium ; sodium-calcium exchange

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Chemistry and Pharmacology , Medicine

Notes: Abstract We have investigated the links between electrical excitation and contraction in mammalian heart muscle. Using isolated single cells from adult rat ventricle, a whole-cell voltage-clamp technique and quantitative fluorescence microscopy, we have measured simultaneously calcium current (Ica) and [Ca2+]i (with fura-2). We find that the voltage-dependence of Ica and the [Ca 2+]i-transient and the dependence of [Ca2+]i-transient on depolarization-duration cannot both be readily explained by a simple calcium-induced Ca-release (‘CICR’) mechanism. Additionally, we find that when [Ca2+]i and [Na+]i are at their diastolic levels, activation of the Na-Ca exchange mechanism by depolarization does not measurably trigger the release of Ca2+i. Finally, measuring Ica in adult and neonatal rat heart cells and using the alkaloid ryanodine, we have carried out complementary experiments. These experiments show that there may be an action of ryanodine on Ica that is independent of [Ca2+]i and independent of a direct action of the alkaloid on the calcium channel itself. Along with experiments of others showing that ryanodine binds to the sarcoplasmic reticulum calcium-release channel/spanning protein complex, our data suggests a model to explain our findings. The model links the calcium channels responsible for Ica to the sarcoplasmic reticulum by means of one or more of the spanning protein(s). Information from the calcium channel can be communitated to the sarcoplasmic reticulum by this route and, presumably, information can move in the opposite direction from the sarcoplasmic reticulum to the calcium channel.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00220762

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16

Electronic Resource

Fluorescence lifetime imaging of intracellular calcium (1993)

Szmacinski, Henryk ; Lakowicz, Joseph R. ; Lederer, W. J. ; [et al.]

Springer

Journal of fluorescence 3 (1993), S. 161-167

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ISSN: 1573-4994

Keywords: Fluorescence lifetime imaging microscopy ; intracellular calcium ; live cells

Source: Springer Online Journal Archives 1860-2000

Topics: Physics

Notes: Abstract Fluorescence lifetime imaging microscopy (FLIM) is a new methodology for studying the spatial and temporal dynamics of macromolecule, molecules, and ions in living cells. In FLIM image contrast is derived from the mean fluorescence lifetime at each point in a two-dimensional image. In our case the lifetime was measured by the phase-modulation method. We describe our FLIM apparatus, which consists of a fluorescence microscope, high-speed gated proximity focused MCP image intensifier, and slow-scan CCD camera. To accomplish subnanosecond time-resolved imaging, the gain of the image intensifier is modulated with a high-frequency signal, resulting in stationary phase-sensitive intensity images on the image intensifier. These images are recorded using a cooled slow-scan CCD camera and stored in an image processor. The lifetime images are created from a series of phase-sensitive images at various phase shift of the gain-modulation signal. We demonstrate calcium concentration imaging in living COS cells based on Ca2+-induced lifetime changes of Quin-2. The phase-angle image is mapped to the Ca2+ concentration image using anin vitro-determined calibration curve. The Ca2+ concentration was found to be uniform throughout the cell. In contrast, the intensity image shows significant spatial differences, which likely reflect variations in the thickness and distribution of probe within the cell.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00862736

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17

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Use of thapsigargin to study Ca2+ homeostasis in cardiac cells (1995)

Rogers, Terry B. ; Inesi, Giuseppe ; Wade, Robert ; [et al.]

Springer

Bioscience reports 15 (1995), S. 341-349

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ISSN: 1573-4935

Keywords: ATPase ; calcium ; sarcoplasmic reticulum ; thapsigargin

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Chemistry and Pharmacology

Notes: Abstract Several reports have documented that thapsigargin is a potent inhibitor of the SR Ca2+ ATPase isolated from cardiac or skeletal muscle. We have characterized the specificity of this agent in intact rat cardiac myocytes using cells maintained in the whole cell voltage clamp configuration. We have shown that thapsigargin decreases the magnitude of the Ca2+ transient and the twitch by about 80% while it slows the decay rate for these responses. These changes were not accompanied by any alterations in sarcolemmal currents or in the trigger Ca2+ generated by the inward calcium current. Taken together these results reveal that the action of thapsigargin is restricted to the SR Ca2+ ATPase in intact cardiac myocytes. Furthermore, it is demonstrated unambiguously that SR intracellular Ca2+ stores are an absolute requirement for the development of contractile tension in rat heart myocytes. It is shown that thapsigargin is a valuable probe to examine the importance of SR pools of Ca2+ and the role of the Ca2+ ATPase in intact myocytes as well as in genetically altered heart cells.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01788366

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18

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A novel experimental chamber for single-cell voltage-clamp and patch-clamp applications with low electrical noise and excellent temperature and flow control (1986)

Cannell, M. B. ; Lederer, W. J.

Springer

Pflügers Archiv 406 (1986), S. 536-539

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ISSN: 1432-2013

Keywords: Chamber ; Perfusion ; Superfusion ; Bath ; Voltage-clamp ; Single cell ; Patch-clamp ; Heart

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract We describe a simple and inexpensive experimental chamber that is designed to overcome several problems encountered when doing electrical and optical studies on single cells or on isolated membrane patches. The bath is small enough to fit on the stage of a standard inverted microscope. It includes a novel solution level-detector, the output of which is used to actively control the level of solution in the experimental chamber. A Peltier-effect device is located adjacent to the flow-chamber and heats or cools the inflowing solution. Solutions can be rapidly switched using two electrically actuated microvalves. The attraction of this system is that, with appropriately quiet power supplies, not only is the bath solution-level held at a fixed height, but the temperature of the bathing solution can also be set over a wide temperature range (minimum range is 15 to 45°C), and solutions can be rapidly changed. All of the construction details are supplied as are appropriate electrical circuits. Without modification, the chamber can be used for applications as diverse as fluorescence microscopy of living cells, time-lapse photomicroscopy and single-cell motion detection as well as single cell voltage-clamp and isolated membrane patch-clamp. With simple modification the system can be adapted for use in experiments on multicellular preparations.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00583378

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