In Situ Calibration of Nucleoplasmic versus Cytoplasmic Ca2+ Concentration in Adult Cardiomyocytes

Ljubojevic, Senka; Walther, Stefanie; Asgarzoei, M.; Sedej, Simon; Pieske, Burkert; Kockskämper, Jens

doi:10.1016/j.bpj.2011.03.060

Cited by 53 publications

(65 citation statements)

References 39 publications

(54 reference statements)

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“…The higher apparent K d of Lyn-D3cpv is not due to the use of ␣-toxin for membrane permeabilization because K d values of the nucleoplasmictargeted 3NLS-D3cpv are similar when calibrated using digitonin or ␣-toxin. Our finding is congruent with previous observations that the same cameleon may show different K d values in different subcellular compartments (14,32). One potential limitation of D3cpv is the slower kinetics compared with the Ca 2ϩ fluorescent dyes (19), so it may miss the detection of very rapid transient events.…”

Section: Et-1 and Ang II Preferentially Triggered Subsarcolemmal Ca 2supporting

confidence: 92%

Detection of differentially regulated subsarcolemmal calcium signals activated by vasoactive agonists in rat pulmonary artery smooth muscle cells

Subedi

Paudel

Sham

2014

American Journal of Physiology-Cell Physiology

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Section: Et-1 and Ang II Preferentially Triggered Subsarcolemmal Ca 2supporting

confidence: 92%

Detection of differentially regulated subsarcolemmal calcium signals activated by vasoactive agonists in rat pulmonary artery smooth muscle cells

Subedi

Paudel

Sham

2014

American Journal of Physiology-Cell Physiology

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“…This is about 1.7 times larger than the measured in vitro K D,t value. The only available in situ K D values for ACR so far were published by Ljubojević et al [44]. In that study, K D,i values were determined in rat ventricular cardiomyocytes at 2183 nM in nucleoplasm and 1336 nM in cytoplasm, respectively.…”

Section: Resultsmentioning

confidence: 99%

Asante Calcium Green and Asante Calcium Red—Novel Calcium Indicators for Two-Photon Fluorescence Lifetime Imaging

Jahn

Hille

2014

PLoS ONE

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For a comprehensive understanding of cellular processes and potential dysfunctions therein, an analysis of the ubiquitous intracellular second messenger calcium is of particular interest. This study examined the suitability of the novel Ca2+-sensitive fluorescent dyes Asante Calcium Red (ACR) and Asante Calcium Green (ACG) for two-photon (2P)-excited time-resolved fluorescence measurements. Both dyes displayed sufficient 2P fluorescence excitation in a range of 720–900 nm. In vitro, ACR and ACG exhibited a biexponential fluorescence decay behavior and the two decay time components in the ns-range could be attributed to the Ca2+-free and Ca2+-bound dye species. The amplitude-weighted average fluorescence decay time changed in a Ca2+-dependent way, unraveling in vitro dissociation constants K D of 114 nM and 15 nM for ACR and ACG, respectively. In the presence of bovine serum albumin, the absorption and steady-state fluorescence behavior of ACR was altered and its biexponential fluorescence decay showed about 5-times longer decay time components indicating dye-protein interactions. Since no ester derivative of ACG was commercially available, only ACR was evaluated for 2P-excited fluorescence lifetime imaging microscopy (2P-FLIM) in living cells of American cockroach salivary glands. In living cells, ACR also exhibited a biexponential fluorescence decay with clearly resolvable short (0.56 ns) and long (2.44 ns) decay time components attributable to the Ca2+-free and Ca2+-bound ACR species. From the amplitude-weighted average fluorescence decay times, an in situ K D of 180 nM was determined. Thus, quantitative [Ca2+]i recordings were realized, unraveling a reversible dopamine-induced [Ca2+]i elevation from 21 nM to 590 nM in salivary duct cells. It was concluded that ACR is a promising new Ca2+ indicator dye for 2P-FLIM recordings applicable in diverse biological systems.

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“…Other components of the calcium handling machinery are present on the nuclear envelope such as the Serca pump, and Ryr2 [43]. The presence of IP 3 receptors on the nuclear envelope, if localized facing the nuclear matrix, suggests that IP 3 can regulate nuclear calcium levels.…”

Section: Role Of Canonical Pip2 Hydrolysis In Cardiac Myocytesmentioning

confidence: 99%

Regulation of Phosphatidylinositol-specific Phospholipase C at the Nuclear Envelope in Cardiac Myocytes

Smrcka¹

2015

Journal of Cardiovascular Pharmacology

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Phosphatidylinositol 4,5 bisphosphate hydrolysis at the plasma membrane by phospholipase C is one of the major hormone regulated intracellular signaling systems. The system generates the diffusible second messenger IP3 and the membrane bound messenger diacylglycerol. Spatial regulation of this system has been thought to be through specific subcellular distributions of the IP3 receptor or PKC. As is becoming increasingly apparent, receptor-stimulated signaling systems are also found at intracellular membranes. As discussed in this issue, GPCRs have been identified at the nuclear envelope implying intracellular localization of the signaling systems that respond to GPCRs. Here we discuss the evidence for the existence of PLC signals that regulate nuclear processes, as well as the evidence for nuclear and nuclear envelope localization of PLC signaling components, and their implications for cardiac physiology and disease.

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In Situ Calibration of Nucleoplasmic versus Cytoplasmic Ca2+ Concentration in Adult Cardiomyocytes

Cited by 53 publications

References 39 publications

Detection of differentially regulated subsarcolemmal calcium signals activated by vasoactive agonists in rat pulmonary artery smooth muscle cells

Detection of differentially regulated subsarcolemmal calcium signals activated by vasoactive agonists in rat pulmonary artery smooth muscle cells

Asante Calcium Green and Asante Calcium Red—Novel Calcium Indicators for Two-Photon Fluorescence Lifetime Imaging

Regulation of Phosphatidylinositol-specific Phospholipase C at the Nuclear Envelope in Cardiac Myocytes

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